\r\n\tThe book aims to introduce the potential reader to the problems associated with aeronautics, ranging from academic research to actual application and precise work, and to be of interest to those who want to research and build their techniques in the related fields.
",isbn:"978-1-80355-301-6",printIsbn:"978-1-80355-300-9",pdfIsbn:"978-1-80355-302-3",doi:null,price:0,priceEur:0,priceUsd:0,slug:null,numberOfPages:0,isOpenForSubmission:!0,isSalesforceBook:!1,isNomenclature:!1,hash:"a6b8e86015392b400a37551116fc0c13",bookSignature:"Associate Prof. Zain Anwar Anwar Ali",publishedDate:null,coverURL:"https://cdn.intechopen.com/books/images_new/11522.jpg",keywords:"Aeronautics, Aircraft, Control System, Surveillance, Guidance, Fixed-Wing, Rotorcraft, Jet Engine, Modern Drone, Path Planning, Adaptive Control, Hybrid Control",numberOfDownloads:null,numberOfWosCitations:0,numberOfCrossrefCitations:null,numberOfDimensionsCitations:null,numberOfTotalCitations:null,isAvailableForWebshopOrdering:!0,dateEndFirstStepPublish:"February 9th 2022",dateEndSecondStepPublish:"April 12th 2022",dateEndThirdStepPublish:"June 11th 2022",dateEndFourthStepPublish:"August 30th 2022",dateEndFifthStepPublish:"October 29th 2022",dateConfirmationOfParticipation:null,remainingDaysToSecondStep:"a month",secondStepPassed:!0,areRegistrationsClosed:!1,currentStepOfPublishingProcess:3,editedByType:null,kuFlag:!1,biosketch:"Engr. Dr. Zain Anwar Ali is working as an Associate Prof. and Editor of Sir Syed University Research Journal of Engineering and Technology. He received research funding from Higher Education Commission (HEC), Pakistan, and has research collaborations with several universities in China, including Nanjing University of Aeronautics and Astronautics, Donghua University, Shanghai University, and South East University, under different research grants provided by the National Nature Science Foundation of China.",coeditorOneBiosketch:null,coeditorTwoBiosketch:null,coeditorThreeBiosketch:null,coeditorFourBiosketch:null,coeditorFiveBiosketch:null,editors:[{id:"415526",title:"Associate Prof.",name:"Zain",middleName:"Anwar",surname:"Anwar Ali",slug:"zain-anwar-ali",fullName:"Zain Anwar Ali",profilePictureURL:"https://mts.intechopen.com/storage/users/415526/images/system/415526.png",biography:"Engr. Dr. Zain Anwar Ali received his B.S. degree in Electronic Engineering from Sir Syed University of Engineering and Technology, Karachi, Pakistan, in 2009. In the same year, he joined Sir Syed UET as a Research Assistant in the Electronic Engineering department, and was soon promoted to a Junior Lecturer due to his hard work and research contributions. He completed his Master's in Industrial Control and Automation at the Hamdard University of Engineering in 2012, securing his second position and soon being promoted to a Lecturer. Later he joined Nanjing University of Aeronautics and Astronautics (NUAA) as a Ph.D. research scholar and the Nanjing Strong Flight Electronics and Machinery LTD to complete his Ph.D. experimental work there. In 2017, he completed his Ph.D. in the field of Control Theory and Control Engineering NUAA. He then rejoined Sir Syed UET as an Assistant Professor in the Electronics Engineering department. In the same year, he was selected as a highly talented foreign expert by the Ministry of China, Beijing, at Liaocheng. After seeing his research background, the vice-chancellor of SSUET gave him the extra responsibility of an Associate Editor of Sir Syed UET research journal which is indexed at various indexing agencies and published in two issues annually. In 2018-2019, he received research funding from Higher Education Commission (HEC), Pakistan, and started some different research collaborations with several universities in China, including Nanjing University of Aeronautics and Astronautics (NUAA-Nanjing), Donghua University (DU-Shanghai), Shanghai University (SU-Shanghai), and South East University (SEU-Nanjing), under different research grants provided by the National Nature Science Foundation of China (NSFC). Currently, Dr. Ali is working as an Associate Professor at the Electronic Engineering Department, Sir Syed University of Engineering and Technology, Karachi, Pakistan, and as the Editor of Sir Syed University Research Journal of Engineering and Technology.",institutionString:"Sir Syed University of Engineering and Technology",position:null,outsideEditionCount:0,totalCites:0,totalAuthoredChapters:"1",totalChapterViews:"0",totalEditedBooks:"0",institution:{name:"Sir Syed University of Engineering and Technology",institutionURL:null,country:{name:"Pakistan"}}}],coeditorOne:null,coeditorTwo:null,coeditorThree:null,coeditorFour:null,coeditorFive:null,topics:[{id:"11",title:"Engineering",slug:"engineering"}],chapters:null,productType:{id:"1",title:"Edited Volume",chapterContentType:"chapter",authoredCaption:"Edited by"},personalPublishingAssistant:{id:"347258",firstName:"Marica",lastName:"Novakovic",middleName:null,title:"Ms.",imageUrl:"//cdnintech.com/web/frontend/www/assets/author.svg",email:"marica@intechopen.com",biography:null}},relatedBooks:[{type:"book",id:"10198",title:"Response Surface Methodology in Engineering Science",subtitle:null,isOpenForSubmission:!1,hash:"1942bec30d40572f519327ca7a6d7aae",slug:"response-surface-methodology-in-engineering-science",bookSignature:"Palanikumar Kayaroganam",coverURL:"https://cdn.intechopen.com/books/images_new/10198.jpg",editedByType:"Edited by",editors:[{id:"321730",title:"Prof.",name:"Palanikumar",surname:"Kayaroganam",slug:"palanikumar-kayaroganam",fullName:"Palanikumar Kayaroganam"}],productType:{id:"1",chapterContentType:"chapter",authoredCaption:"Edited by"}},{type:"book",id:"1591",title:"Infrared Spectroscopy",subtitle:"Materials Science, Engineering and Technology",isOpenForSubmission:!1,hash:"99b4b7b71a8caeb693ed762b40b017f4",slug:"infrared-spectroscopy-materials-science-engineering-and-technology",bookSignature:"Theophile Theophanides",coverURL:"https://cdn.intechopen.com/books/images_new/1591.jpg",editedByType:"Edited by",editors:[{id:"37194",title:"Dr.",name:"Theophile",surname:"Theophanides",slug:"theophile-theophanides",fullName:"Theophile Theophanides"}],productType:{id:"1",chapterContentType:"chapter",authoredCaption:"Edited by"}},{type:"book",id:"3161",title:"Frontiers in Guided Wave Optics and Optoelectronics",subtitle:null,isOpenForSubmission:!1,hash:"deb44e9c99f82bbce1083abea743146c",slug:"frontiers-in-guided-wave-optics-and-optoelectronics",bookSignature:"Bishnu Pal",coverURL:"https://cdn.intechopen.com/books/images_new/3161.jpg",editedByType:"Edited by",editors:[{id:"4782",title:"Prof.",name:"Bishnu",surname:"Pal",slug:"bishnu-pal",fullName:"Bishnu Pal"}],productType:{id:"1",chapterContentType:"chapter",authoredCaption:"Edited by"}},{type:"book",id:"3092",title:"Anopheles mosquitoes",subtitle:"New insights into malaria vectors",isOpenForSubmission:!1,hash:"c9e622485316d5e296288bf24d2b0d64",slug:"anopheles-mosquitoes-new-insights-into-malaria-vectors",bookSignature:"Sylvie Manguin",coverURL:"https://cdn.intechopen.com/books/images_new/3092.jpg",editedByType:"Edited by",editors:[{id:"50017",title:"Prof.",name:"Sylvie",surname:"Manguin",slug:"sylvie-manguin",fullName:"Sylvie Manguin"}],productType:{id:"1",chapterContentType:"chapter",authoredCaption:"Edited by"}},{type:"book",id:"371",title:"Abiotic Stress in Plants",subtitle:"Mechanisms and Adaptations",isOpenForSubmission:!1,hash:"588466f487e307619849d72389178a74",slug:"abiotic-stress-in-plants-mechanisms-and-adaptations",bookSignature:"Arun Shanker and B. 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\n
1. Introduction
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Both single-walled nanotubes (SWNTs) and multi-walled nanotubes (MWNTs), which possess remarkable multifunctional properties such as high Young’s modulus of 1 TPa [1], ultrahigh thermal conductivity of 2000–3500 W/mK [2,3], and outstanding electrical conductivity of 3×104 S/cm [4], have attracted much attention over the past decades [5]. Carbon nanotubes (CNTs) have been considered promising effective additives for developing high-performance composites. Currently, in the widely-used approaches for fabrication of CNT-based composites, CNTs are randomly dispersed into the matrix. This approach, however, typically results in low volume fraction, poor dispersion and random orientation of CNTs in matrices, inducing very limited enhancements and much lower properties than expected. To overcome these limitations, various CNT Structures such as buckypapers [6], CNT arrays [7–9], and CNT yarns [10] have been developed to pre-arrange the CNTs prior to fabricating composites.
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Among those CNT post-treatments, assembling CNTs into CNT fibers has attracted tremendous attention. In general, there are three major methods for production of CNT fibers: (1) wet-spinning from CNT/acid or polymer solutions [11–13]; (2) dry-spinning from vertically aligned CNT arrays [10,14–17]; and (3) direct-assembling from CNT aerogels formed in chemical vapor deposition (CVD) [5,18–24]. The first method is also known as the wet-spinning method, while the others are known as dry-spinning methods.
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The obtained CNT fibers commonly possess satisfactory mechanical and electrical properties [5], and even higher strength and better flexibility than commercial carbon fibers and polymer fibers [25]. In order to further improve their properties (mechanical strength in particular), polymer infiltration is usually performed on the CNT fibers to obtain CNT fiber/polymer composites. The polymer can greatly enhance the inter-tube load transfer, inducing high mechanical strength of the composites.
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2. Methods for assembling CNTs into CNT fibers
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2.1. Spinning from CNT Solution
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In 2000, Vigolo et al. [11] first fabricated CNT ribbons and fibers via the coagulation spinning approach that was widely used to synthesize polymer fibers. Figure 1(a) shows the schematic of the experimental setup used to make nanotube ribbons. In this method, SWNTs are homogeneously dispersed in a solution of sodium dodecyl sulfate (SDS), which helps prevent CNTs from agglomeration. The CNT dispersion is then injected into the co-flowing stream of a polymer solution that contains 5.0 wt.% of polyvinylalcohol (PVA) to form CNT ribbons, as shown in Figure 1(b). Figure 1(e) shows a typical SEM image of the as-obtained CNT ribbon, revealing a preferential orientation of the nanotubes along the ribbon’s main axis. After the ribbons are washed and dried, most of the surfactants and polymers are removed. The ribbons are collapsed into fibers due to capillary force, as shown in Figure 1(c). These fibers are more flexible than traditional carbon fibers, as shown in Figure 1(d). The diameter of CNT fibers varies from 10 to 100 μm depending on fabrication conditions. The tensile strength, modulus and electrical conductivity of the obtained fibers are 300 MPa, 40 GPa and 10 S/cm, respectively.
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Figure 1.
(a) Schematic of the experimental setup used to make nanotube ribbons. (b–d) Optical micrographs of nanotube ribbons and fibers. (b) A single folded ribbon between horizontal and vertical crossed polarizers (scale bar = 1.5 mm); (c) A freestanding nanotube fiber between two glass substrates (scale bar = 1 mm); and (d) Tying knots reveals the high flexibility and resistance to torsion of the nanotube microfibers. (e) Scanning electron micrograph shows SWNT bundles are preferentially oriented along the main axis of the ribbon (scale bar = 667 nm) [11].
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Vigolo’s technique is remarkable for further studies on fabricating continuous CNT fibers on a large scale, although this technique has some disadvantages. For example, the drawing of these as-spun gel fibers is slow (∼1 cm/min), and the solid fibers are short (∼10 cm) [26]. In addition, the fibers\' mechanical properties are low compared with those of component individual nanotubes. Moreover, mechanical performance is improved, mostly because PVA chains in a CNT fiber enhance load transfer efficiency between CNTs. However, the existence of the non-conductive PVA leads to lower electrical and thermal conductivity of the obtained CNT fibers than pure CNT sheets [27]. Thus, fibers composed solely of CNTs are desirable. In 2004, Ericson et al. [12] developed a method to fabricate well-aligned macroscopic fibers composed solely of SWNTs. In this method, purified SWNTs are dispersed in 102% sulfuric acid, which charges SWNTs and promotes their ordering into an aligned phase of individual mobile SWNTs surrounded by acid anions. This ordered dispersion is extruded into continuous lengths of macroscopic neat SWNT fibers. The obtained fibers possess a Young’s modulus of 120 ±10 GPa and a tensile strength of 116 ±10 MPa. Because these pure CNT fibers do not contain polymers, they demonstrate better electrical and thermal properties than fibers containing polymers, with an electrical conductivity of 500 S/cm and thermal conductivity of ~21 W/m K. In another method proposed by Behabtu et al. [13], high-quality CNTs are dissolved in chlorosulfonic acid and extruded into a coagulant (acetone or water) to remove the acid. The forming filament is further stretched and tensioned to ensure high CNT alignment in the structure. The resulting fibers possess a Young’s modulus of 120 ± 50 GPa and strength of 1.0 ± 0.2 GPa. The tensile strength shows a tenfold improvement over wet-spun fibers fabricated using the method developed by Ericson et al. [12]. At the same time, they display outstanding electrical conductivity (~29000 ± 3000 S/cm) and thermal conductivity (~380 ± 15 W/m K).
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2.2. Spinning from vertically aligned CNT arrays
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Just like drawing a thread from a silk cocoon, CNT fibers can be synthesized from a vertically aligned CNT array. In 2002, Jiang et al. [10] spun a 30-cm-long CNT fiber from a CNT array (~100 μm in height). In 2004, Zhang et al. [14] modified this technique by introducing twist during spinning. In this method, the nanotube arrays (~30 μm in height) are grown on an iron catalyst–coated substrate by CVD. Afterward, yarns are drawn from the array and twisted with a variable-speed motor. Figure 2(a) and (b) clearly show the SEM images of the structures formed during the spinning process. The obtained fibers have a tensile strength of ~460 MPa, modulus of ~30 GPa and electrical conductivity of 300 S/cm.
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Since then, many efforts have been made to optimize spinning processes and to improve the performance of CNT fibers. Spinning fibers from higher CNT arrays can effectively improve fiber performance. For example, Zhang et al. [15] reported the spinning of CNT fibers from relatively long CNT arrays (0.65 mm), which resulted in the strength and Young’s modulus of the CNT fibers reaching 1.91 GPa and 330 GPa, respectively. Furthermore, Li et al. [16] spun CNT fibers from 1 mm CNT arrays. Their tensile strength reached up to 3.3 GPa, which is much higher than that of CNT fibers from the 0.65 mm array. In aiming to achieve the goal of providing a continuous process for the solid-state fabrication of CNT yarns from CNT forests, Lepro et al. [17] spun fibers from CNT forests grown on both sides of highly flexible stainless steel sheets, instead of the conventionally used silicon wafers, as shown in Figure 2(c), (d) and (e). They reported that the catalyst layer is shown to be re-usable, decreasing the need for catalyst renewal during a proposed continuous process.
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Figure 2.
(a) and (b) SEM images of a carbon nanotube yarn in the process of being simultaneously drawn and twisted during spinning from a nanotube forest outside the SEM [14]; (c–e) Spinnable CNT forest grown on flexible stainless steel substrate [28].
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Studies have found that not all CNT arrays can be spun into fibers, and the degree of spinnability of CNTs is closely related to the morphology of CNT arrays [29,30]. Several research groups have made efforts to study the mechanism of spinning fibers from CNT arrays. Kuznetsov et al. [28] developed a structural model for the drawing of sheets and fibers from CNT arrays. Huynh et al. [30] studied the roles of catalyst, substrate, temperature, gas flow rates, reaction time with acetylene, etc. to identify and understand the key parameters and develop a robust, scalable process. More recently, Zhu et al. [31] pointed out that the entangled structures at the ends of CNT bundles are critical for the continuous drawing process. Further fundamental studies of this mechanism are critical for fabricating spinnable CNT arrays and improving the properties of CNT fibers.
\n\n
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2.3. Spinning from CNT aerogels
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In both of the above-mentioned methods, individual CNTs are first produced in the form of CNT powders or arrays. In this method, fibers are achieved through the post-process of spinning. Unlike the in-direct methods, CNT fibers can be assembled directly in a CVD process in which individual CNTs are synthesized. In 2000, Zhu et al. [18] first reported the direct synthesis of 20cm long ordered SWNTs with a diameter of approximately 0.3mm using a floating catalyst CVD method in a vertical furnace. In 2004, Li et al. [19] reported a method for the direct spinning of long CNT fibers from aerogels formed during CVD. Figure 3(a) is a schematic of this direct spinning process. In this method, reaction precursors are mixed and introduced into a tube furnace operated at 1200°C. In a reducing hydrogen atmosphere, the nanotubes form an aerogel in the hot zone of the furnace and are stretched into cylindrical hollow socks which are then pulled and collected continuously out of the furnace as fibers. Figure 3(b) and (c) show SEM images of the aligned CNT fibers after condensation by acetone vapor. CNT fibers, spun directly and continuously from aerogels, demonstrate both high strength (up to 357 GPa) and high stiffness (8.8 GPa), which are comparable to those of commercial fibers [20].
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Figure 3.
(a) Schematic diagram of the direct spinning process for CNT fibers [21]; (b) and (c)SEM micrographs of a fiber that consists of well-aligned MWNTs [19]; (d) Schematic diagram of the CNT fiber-spinning process using a horizontal furnace [24].
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3. Methods for enhancing CNT alignment
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The as-spun CNT fibers fabricated using the above methods usually have a porous structure, and the CNTs within the fibers have poor alignment [14,19,32]. Hence, the CNT fibers should be further densified to obtain a more closely-packed structure and better alignment of the CNTs. Since the van der Waals interaction strongly depends on the contact area between CNTs, much space and many pores between CNT bundles could lower the degree of this interaction. By applying the densification process, the densified CNT fibers can have reduced interspace between CNTs and an improved contact area, leading to an increased van der Waals interaction. As a result, these highly dense structures have a stronger van der Waals interaction between CNT bundles, hence improving fiber performance [32–34].
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3.1. Enhancing CNT alignment for fibers spun from the wet-spinning technique
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While classical composite fibers consist of CNTs embedded in a polymeric matrix, fibers fabricated by the wet-spinning technique consist of an interconnected network of polymers and CNTs. The spinning conditions, such as the flow velocity of the polymer solution and the injection rate of the CNT solution, has no measurable effect on the CNT orientation in the resulting fibers. However, when the fibers are immersed in an appropriate solvent or heated, the network of polymers and CNTs can be loosened and stretched, resulting in a significant improvement in CNT alignment. For example, Vigolo et al. [35] enhanced the CNT alignment of their SWNT/PVA fibers by re-wetting, swelling and re-drying the fibers vertically under a tensile load with a weight attached to the end of the fiber. The solvent used in the study was comprised of water, acetone and acetonitrile. Once re-wetted and swollen by the solvent, the fibers could be stretched up to 160% with significantly improved alignment, as shown in Figure 4. This indicates that the networks of CNTs and absorbed polymers form cross linked assemblies that can be elastically deformed. As a result, their strength and stiffness increased from 10 GPa and 125 MPa, to 40 GPa and 230 MPa, respectively, after the stretching.
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Separately, Miaudet et al. [36] reported an increase in tensile strength of CNT/PVA fibers from 1.4 GPa to 1.8 GPa after the hot-stretched treatment. The reduction of PVA chain alignment from ±27° to as low as 4.3°, and the nanotube alignment to as low as 9°, suggested that better alignment of the CNT and PVA chains was the main reason for the improved mechanical performance of the hot-stretched fibers.
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Figure 4.
SEM images of an as-spun fiber (a), and (b) a stretched CNT fiber [35].
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3.2. Enhancing CNT alignment for fibers spun from dry-spinning and floating catalyst techniques
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CNT fibers spun from dry-spinning and floating catalyst techniques can be densified by applying a mechanical force in their lateral direction. The densification methods can be classified into two categories: indirect approaches (such as liquid densification, twisting [32], drawing through dies [37], or an aligning and tension system [38]); and direct approaches (such as rubbing/false twisting [39] and mechanical compression [40]).
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3.2.1. Indirect approaches
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3.2.1.1. Liquid densification
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The alignment and mechanical performance of as-spun CNT fibers can be improved through liquid densification. In this method, a liquid such as acetone or ethanol is absorbed into the fibers and subsequently evaporated, resulting in a dense CNT structure. The fibers are densified due to the surface tension of the solvent and the fiber diameter is reduced accordingly. The densification process slightly improves nanotube alignment (Figure 5) and enhances load transfer between nanotubes, ensuring that most of them are fully load-bearing. Liu et al. [41] studied the mechanical properties of twisted fibers with and without acetone densification. The diameter of the yarn changed from 11.5 to 9.7 μm after shrinking. Although the maximum strain of the yarn remained unchanged (~2.3%), the Young’s modulus (~56 GPa) of the shrunk fiber was slightly greater than before shrinking (~48 GPa). Liu et al. [41] also reported a change in diameter and maximum load of twisted fibers before and after shrinking. After acetone shrinking, the diameter reduction ranged from 15% to 24%, and the load increase ranged from 15 to 40%, indicating that tensile strength was enhanced. Among common solvents (water, ethanol and acetone) used to shrink CNT yarns, acetone showed the best shrinking effect.
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Figure 5.
(a) SEM images of a twisted fiber before, and after shrinking (b) [41].
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3.2.1.2. Twisting
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The as-spun fiber is relatively loose with noticeable spaces between CNT bundles. Increasing the twist angle is an effective method for densifying CNT fibers. Since it brings CNTs into closer contact with each other, twisting improves the friction coefficient μ between CNTs, therefore contributing positively to fiber strength [15]. Zhang et al. [15] compared the tensile behaviors of twisted and untwisted CNT fibers spun from the same 650 mm height array. After twisting, the diameter of the fiber decreased from 4 to 3 μm (Figure 6), while tensile strength increased from 0.85 GPa to 1.9 GPa [15].
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Figure 6.
SEM images of as-spun CNT fiber (a), and the same fiber after post-spin twisting (b) [15].
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3.2.1.3. Drawing through dies
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The as-spun CNT fibers can be densified by being drawn through dies of different diameters. The average measured fiber diameter was determined by die size. Sugano et al. [37] densified CNT fibers spun from CNT arrays by drawing them through densifying dies with different diameters (d = 30, 35, 55, 75 μm) (Figure 7(a)). The fibers were deformed elastically after drawing CNTs through the die, and their density increased with decreasing die diameter. As CNT fibers are held together by van der Waals forces between MWNTs, these forces increased due to higher apparent density with decreasing distance between MWNTs, as shown in Figure 7(b). As a result, their strength was significantly enhanced after treatment.
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Figure 7.
(a) Schematic view of untwisted CNT yarn in the process of being drawn from the aligned MWNT array and past the sheet through a die; (b) SEM image of surface morphologies of the resulting CNT fiber.
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3.2.1.4. Aligning and tension system
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The aligning and tension system is one of the most effective methods of enhancing CNT alignment and performance of CNT fibers. Tran et al. [38] first modified the traditional dry-spinning process to improve CNT alignment of their CNT fibers (Figure 8(a)). In this modified system, a capstan effect rod system (CERS) is added to a dry-spinning system to regulate tension and torque to the fibers. As the fibers pass through a CERS, the increased tension extends and aligns the bundles (Figure 8(b) and 8(c)). This process has two effects: (i) aligning CNTs in the fibers during the initial tensioning; and (ii) condensing the CNT bundles. The first effect increases contact length between bundles, and the second effect reduces the distance between CNTs. The significant increase in fiber strength from 0.45 to 1.2 GPa after the treatment is due to better alignment of the fiber bundles and higher fiber compaction.
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Figure 8.
(a) The schematic of modified CNT yarn spinning; (b) SEM images of surface morphologies of CNT fiber spun from traditional process; and modified process (c) [38].
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Generally, the drawback of the indirect approaches is their low densifying forces. The liquid densification method, for example, employs the surface tension of volatile solvents such as acetone or ethanol to densify the CNT fibers. Its densifying force is therefore limited by the low surface tension of the solvents used [32]. Similarly, the compressive force produced by drawing CNT fibers through a die results from the drawing forces and the die size used. These drawing forces are limited by fiber strength, while a significantly smaller die could damage the fiber structure, resulting in poor strength [37]. Therefore, CNT fibers cannot be adequately densified with these methods, and their performance remains unsatisfactory.
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3.2.2. Direct approaches
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Direct approaches are considered the best solution to overcome the above limitations. As the densifying forces are applied directly to CNT fibers, the forces can condense the fibers into a much denser structure [40].
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3.2.2.1. Rubbing/false twisting
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CNT fibers can be densified using several traditional textile twistless methods such as rubbing. Miao et al. [39] used a rubbing roller system (Figure 9(a)) to densify CNT web drawn from a vertically aligned CNT forest into a compact twistless yarn. As the system used a constant rate false twisting process, there is only a temporary twist on the incoming side of the yarn, and the yarn on the outgoing side (and thus the final yarn) will be twistless. As can be seen in Figure 9(b), the resulting yarn consists of a high packing density sheath with CNTs lying straight and parallel to the yarn axis, and a low density core with many microscopic voids. With an increased contact length between CNT bundles in the high packing density sheath, the mechanical performance of the core-sheath structured, twistless carbon nanotube yarns are significantly higher than that of their corresponding twist-densified yarns.
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Figure 9.
(a) The schematic of the core-sheath, twistless CNT yarn fabricated by a rubbing roller system; and (b) SEM image of the resulting yarn.
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3.2.2.2. Mechanical compression
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Wang et al. [40] reported that CNT fibers densified by the pressurized rolling system showed highly packed structures with a densification factor of up to 10 (Figure 10(a)). Moreover, the densified fibers can reach an impressive average strength of 4.34 GPa, which is the highest extrinsic CNT fiber strength reported to date [40]. In addition, Tran et al. [24] presented a modified densification method to produce a highly packed CNT structure. As shown in Figure 10(b), CNT fibers were sandwiched between two sheets of A4 paper and pressed by a stainless-steel spatula with an applied force of approximately 100 N, at 45° to the fiber axis. The spatula was subsequently slid across the A4 paper, along the fiber axis, to compress and mechanically densify the fibers into a ribbon shape while the compressive force was maintained. The CNT ribbon in this study also showed a densification factor of up to 10, while the strength and electrical conductivity of the densified fibers approached impressive values of 2.81 GPa and 12,000 S/cm, respectively. The study showed that the mechanical densification treatment may have increased the CNT bundle size and inter-CNT contact, and induced better alignment (Figure 10(c) and (d)), resulting in improved properties of the densified CNT fiber.
\n
Figure 10.
The schematic of mechanical densification methods using (a) pressurized rolling system, and (b) spatula; SEM images of the surface morphology of the (c) as-spun CNT fiber, and (d) densified CNT ribbons [24].
\n
\n
\n
\n
\n
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4. Mechanical and physical properties of aligned CNT polymer composites
\n
The outstanding physical and mechanical properties of aligned CNT assemblies make them promising for the research and development of high-performance composites. The final properties of the composites are affected by many factors, such as, morphology of individual nanotubes and impregnating method.
\n
\n
4.1. Impregnating method
\n
Pure CNT assemblies including fibers and films have an ineffective load transfer between CNTs as the CNTs interact with each other via weak van der Waals forces. Among all methods used to enhance load transfer between CNTs, polymer impregnation is one of the most effective treatments in enhancing the mechanical properties of CNT assemblies. This reinforcement mainly stems from the enhanced inter-tube load transfer and the crystallinity of the impregnated polymer. Several impregnating methods are used to fabricate aligned CNT polymer composites.
\n
\n
4.1.1. Dip coating/soaking
\n
Dip coating or soaking is widely used to impregnate polymer into CNT assemblies. In this method, CNT assembles are immerged into polymer solution for sufficient infiltration and then taken out for curing. Liu et al. [32] reports the mechanical properties of PVA impregnated fibers spun from CNT arrays. Figure 11 shows the schematic of the CNT/polymer fiber manufacturing process and compares the tensile properties of a CNT/PVA fiber with two types of pure CNT fibers. As can be seen, the CNT/PVA composite fiber with 19 wt.% PVA possesses a tensile strength of 1.95 GPa. This result is 255% higher than that of simply twisting the CNT fiber and 103% higher than that of a CNT fiber subjected to twisting and shrinking by acetone. The greater strength of the CNT/PVA fiber stems from the decrease in fiber diameter due to the high wettability between dimethyl sulfoxide (DMSO) and CNTs, and the increase in tensile load due to improved load transfer efficiency between CNTs after PVA impregnation (Figure 11(b)).
\n
Figure 11.
(a) Schematic of the CNT/polymer fiber manufacturing process; and (b) stress-strain curves of a typical SWNT/PVA yarn and two types of pure SWNT yarns. [32]
\n
Similarly, Tran et al. [24] reported an outstanding enhancement of the electrical and mechanical performances of MWNT fibers through the combined treatments of mechanical densification and epoxy infiltration. Compared to the mechanical performances of CNT fibers produced by different post-treatments, the combined post-treatments employed in their study showed better effects, with enhancement factors of more than 13.5 for tensile strength and 63 for stiffness. After the first mechanical treatment, their condensed CNT ribbons achieved a tensile strength much greater than that of the best CNT fibers spun with wet-spinning and array-spinning methods, as shown in Figure 12. When further combined with epoxy infiltration, the CNT/epoxy ribbons reached significantly greater strength (up to 5.2 GPa) and stiffness (up to 444 GPa), which are very comparable to those of commercial PAN carbon fibers as shown in Figure 12. Furthermore, while the strength of their CNT/epoxy ribbons was comparable to that of the best double-walled CNT (DWNT) ribbons produced by the floating-catalyst method [40], their stiffness was much higher. The results suggest that by using a polymer infiltration treatment, the performance of MWNT fibers with low electrical and mechanical properties could achieve the performance of many other high-strength fibers.
\n
Figure 12.
Comparisons of mechanical properties of the best CNT fibers from array-spinning [15] and wet-spinning [13], ribbons from aerogel spinning, and PAN carbon fibers [40].
\n
Liu et al. [23] fabricated CNT/polyimide aerogel (CNT/PIA) composite fibers by dip-coating the CNT fibers in a sol solution, and then drying them using the supercritical CO2 drying process. In the CNT/PIA composite fibers, CNT fibers are tightly wrapped by porous polyimide aerogel, showing a core-shell structure. This core-shell structure resulted in the light weight, low density and high surface area of the composite fiber. Owing to the superior properties of the CNT fibers (stiffness of ~450 MPa, tensile strength of ~83 MPa and electrical conductivity of ~419 S/cm), the CNT/PIA composite fibers achieve significant enhancements in mechanical and electrical properties (stiffness of ~68.1 MPa, strength of ~11.6 MPa and electrical conductivity of ~418 S/cm), compared with the pure PIA and other CNT/PIA composite [42–46]. It was also found that the mechanical and electrical properties of CNT/PIA composite fibers decline with an increase in the diameter of CNT fibers.
\n
\n
\n
4.1.2. Resin transfer molding
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Resin transfer molding (RTM) is a very common and cost-effective method to fabricate composites in industries, in which the liquid resins are first injected to the preforms and then cured to be solid. Given its capability of making composites with large sizes and complex shapes, RTM is expected to be appropriate for preparing CNT/epoxy composites in large scale. Liu et al. [5] developed aligned CNT/epoxy composite films by combining layer-by-layer and vacuum-assisted RTM (VA-RTM) method using direct chemical vapor deposition (CVD)-spun CNT plies. The CNTs in the plies are well-condensed during the VA-RTM process (Figure 13(a)), leading to much higher mass fractions of CNTs (up to 24.4 wt.%) compared with those obtained from the conventional dispersion methods. Due to good alignment of the condensed CNTs in the plies, the CNT/epoxy composite with 24.4 wt.% CNTs achieves ~5 and ~10 times enhancements in their Young’s modulus and strength, respectively. A high tensile toughness of up to 6.39 × 103 kJ/m3 was also obtained in the composite films, making them promising candidates for protective materials, as shown in Figure 13(b). The electrical conductivity of the aligned CNT/epoxy composites reaches as high as 252.8 S/cm for the composite with 24.4 wt.% CNTs, which is ~20 times greater than that of the CNT/epoxy composites obtained using dispersion methods [47–49].
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Figure 13.
(a) Experimental set-up of the RTM process for preparing CNT/epoxy films; and (b) The CNT weight fractions and the thickness of CNT/epoxy composite films as a function of CNT plies. [5].
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\n
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4.1.3. Spray winding and layer-by-layer deposition
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The aforementioned methods are mostly regarded as off-line methods in which highly packed CNT assembles are used as preforms. Because the preforms are already tightly packed, however, these methods often have the problem of the uniformity of infiltration. As a result, the un-infiltrated part may become defects and limit the overall performance of the composites [50]. In order to control the uniformity of infiltration and avoid over-infiltration, Liu et al. [50,51] developed a one-step approach of “spray winding” to fabricate high-performance CNT composites. In this on-line infiltration method, CNT sheets, drawn out from CNT arrays, were continuously collected (wound) onto a rotating mandrel under the spray of a polymer solution, as shown in Figure 14(a). The spray-wound CNT/PVA composite films, the CNT fraction is tunable, and could be as high as 65 wt.% to reach the best mechanical properties. The best film had the tensile strength, stiffness and toughness up to 1.8 GPa, 45 GPa, and 100 J/g, respectively, much better than the fibers made by the same CNT and PVA and many other CNT/polymer composites. The high performance can be attributed to the long CNTs, highly-aligned tube morphology, and good interfacial bonding between CNT and PVA, which were obtained simultaneously. In order to control the exact layers of the composite films in large scale, Zhang et al. [52] reported a “layer-by-layer (LBL) deposition” method to produce CNT polymer composites, as shown in Figure 12(b). This on-line deposition method allowed PVA to infiltrate into the CNT film efficiently, resulting in a remarkable improvement in the mechanical property of CNT/PVA composite. The composite film possessed a tensile strength of 1.7 GPa, which is almost one order of magnitude and 20 times higher than those of the pure CNT and PVA films, respectively.
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Figure 14.
(a) Schematic view of spray winding [50]; and (b) Schematic illustration of the LBL deposition process [52].
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\n
4.2. Effect of CNT morphology
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Individual nanotube morphologies, such as length and alignment, have great influence on mechanical and physical properties of CNT polymer composites. Wang et al. [53] reported an ultrastrong and stiff CNT/composite using a stretch-winding process. The unstretched composites exhibited strength of 2.0 GPa, Young’s modulus of 130 GPa and electrical conductivity of 820 S/cm. After stretching the strength, Young’s modulus and electrical conductivity were increased to as high as 3.8GPa, 293 GPa and 1230 S/cm, respectively. These remarkable improvements can be ascribed to the enhancement of CNT alignment and decreasing of waviness. The alignment of the CNTs was characterized by polarized Raman. Specifically, the shift of the intensity ratio (IG‖/IG⊥) of G band peaks was measured. Following the stretch-winding process, the intensity ratio for the 12%-stretched sheet is increased to 7.6 from 1.6, indicating that alignment of the CNTs in the nanocomposites was significantly improve via the stretching process. Therefore, the improved CNT alignment is correlated with the observed improvements in mechanical and electrical properties of the composites.
\n
Park et al. [54] studied the effects of nanotube length and alignment on thermal conductivity of MWNT/epoxy composites. It was found that the long-MWCNT composites exhibited higher thermal conductivity than the short-MWCNT composites with the same weight percentages. At room temperature, 10 wt.% short-MWCNT/epoxy composite showed thermal conductivity of 0.35 W/mK, while the long-MWCNT composites showed 2.6 W/mK even at lower concentration of 6.38 wt.%. To improve the in-plane thermal conductivity, CNT sheets (60 wt.%) were stretched mechanically. The thermal conductivity increased up to 83 W/mK (25% stretched) and 103 W/mK (40% stretched) along the alignment direction compared to 55 W/mK of the random sample.
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5. Mesoscopic modeling of thermal conduction in aligned CNT composites
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Due to the unique morphology of aligned CNT composites, it is difficult to directly measure their thermal conductivity, especially for composites in thin film and long fiber structures. Proper computational modeling is required to accurately predict the thermal conductivity of aligned CNT composites. The widely-used effective medium theories (EMTs) can well predict the thermal conductivity of CNT composites obtained using dispersion methods. However, the EMTs generally fail to predict the thermal conductivity of aligned CNT composites, since they cannot take into account the complex morphology of CNTs and the thermal boundary resistances (TBRs) at both CNT-CNT and CNT-matrix interfaces [55]. The TBRs are the resistances to the heat flow at interfaces, which have been regarded as the bottleneck of thermal conduction in CNT composites [56].
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5.1. Thermal conduction model for two-phase aligned CNT composites
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In order to accurately predict the thermal conductivity of aligned CNT composites, Duong et al. [57] developed an off-lattice Monte Carlo (MC) approach by quantifying thermal energy through a large quantity of random thermal walkers. Thermal walkers have a random Brownian motion in the polymer matrix, which is described by the position changes of thermal walkers in each direction. The position changes take values from a normal distribution with a zero mean and a standard deviation, as expressed as below:
\n
σ=2DmΔtE1
\n
where Dm is the thermal diffusivity of polymer matrices, and ∆t is the time increment of the simulation [58]. When a walker jumps to the CNT-polymer matrix interface, it may jump into the CNT with a probability fm-CNT, or remain within the polymer matrix with a probability (1- fm-CNT). The probability is a function of the TBR between polymer and CNT, Rm-CNT, obtained using the acoustic mismatch theory (AMT) [59]:
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fm−CNT=4/ρCPvRm‐CNTE2
\n
where ρ is the density of polymer, Cp is the specific heat of polymer, and v is the sound velocity in the polymer matrix. Due to the ballistic phonon transport and ultrahigh thermal conductivity in the CNT [60], thermal walkers are assumed to travel at an infinite speed inside the SWNT [61]. The walker is allowed to exit from a CNT to the matrix by using another probability fCNT-m, which is related to fm-CNT in a way that satisfies the second thermodynamic theorem [62,63]:
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VCNTfCNT−m=Cf−CNTσmACNTfm−CNTE3
\n
wherein VCNT and ACNT are the volume and surface area of a CNT, and σm is the standard deviation of Brownian motion in the polymer matrix. Cf-CNT is the thermal equilibrium factor at the polymer-CNT interface, which is dependent on the geometry of the CNTs, and the interfacial area between the CNT and the matrix.
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By using the developed MC approach, Duong et al modeled SWNT-epoxy and SWNT-polymethyl methacrylate (PMMA) composites [64]. The thermal conductivity of SWNT-epoxy and SWNT-PMMA composites were accurately predicted. The effects of the SWNT orientation, weight fraction and TBRs on the thermal conductivity of composites were quantified. The quantitative findings showed that in SWNT-PMMA composites with 1.0wt.% of SWNT loading, aligned SWNTs achieved enhanced thermal conductivity 15 times higher than that of PMMA, whereas, the randomly dispersed SWNTs only resulted in thermal conductivity ~5 times higher than that of PMMA [64]. This indicated the superiority of aligned CNT composites.
\n
Since CNTs are normally grown into forests or spun into fibers, the contacts between CNTs may play a significant role to modify the thermal conductivity of composites. Duong et al. then modified their model to study the effect of CNT-CNT contacts on the thermal conductivity of both SWNT-epoxy and MWNT-epoxy composites [65,66]. A representative volume element (RVE) was built based on the real CNT-epoxy composites, as shown in Figure 15. In MWNT-epoxy composites with 20 vol % of MWNT loading, aligned MWNTs without contacts achieved a thermal conductivity nearly 40 times higher than that of epoxy, while, aligned MWNTs with contacts induced a thermal conductivity only 20 times higher than that of epoxy. This indicated that CNT-CNT contacts in aligned CNTs may reduce the thermal conductivity of composites. The anisotropic thermal conductivity of aligned CNT composites was also quantified. In both SWNT-epoxy and MWNT-epoxy composites, the thermal conductivity parallel to the aligned CNTs was much higher than that perpendicular to the aligned CNTs. The SWNT-epoxy composites had more significantly anisotropic thermal conduction than MWNT-epoxy composites.
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Figure 15.
Schematic drawing of CNT reinforced composites, and aligned CNTs in a polymer as a representative volume element [65].
\n
Bui et al. modified Duong’s approach to investigate the thermal behavior of the SWNT-polystyrene (PS) composites at different volume fractions and at various temperature [67]. It was found that the thermal conductivity of SWNT-PS composites increased with the temperature rise. By validating with experimental data [68], the TBRs at both SWNT-PS and SWNT-SWNT interfaces were estimated by using the MC approach. The calculations at various temperature showed that the TBR between SWNT and PS increased with the rise of temperature. A TBR value of SWNT-SWNT was estimated to be 12.15×10-8 m2K/W at 300K, which was higher than that between SWNT and PS (2.21×10-8 m2K/W). Bui et al. also conducted the comparable study between graphene-polymer composites and SWNT-polymer composites [69]. The quantitative results showed that graphene nanosheets were more effective than SWNTs to enhance the thermal conduction in polymer composites.
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5.2. Thermal conduction model for multi-phase aligned CNT composites
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Recently, multiphase polymer composites, which contain more than one type of additive in the matrix, have attracted much attention [70,71]. The multiphase composites can combine the merits of all the components, inducing advanced multifunctional properties. Diverse multiphase polymer composites have been developed, such as CNT/nanoparticle/polymer composites [70,71], CNT/graphene/polymer composites [72,73], CNT/fiber/polymer composites [74,75] and CNT-stabilized polymer blends [76]. Since there is no effective approach to study thermal properties of CNT multiphase composites, Gong et al. [77] extended Duong’s MC approach to investigate heat transfer phenomena in CNT multiphase composites. In Gong’s model, a three-phase poly(ether ether ketone) (PEEK) composite containing SWNTs and tungsten disulfide (WS2) nanoparticles was chosen as a case study, as shown in Figure 16(a) [78]. The TBRs at all interfaces (i.e. SWNT-PEEK, WS2-PEEK and SWNT-SWNT) were taken into account in their model. The results showed that the thermal conductivity of multiphase composites increased when the CNT concentration increased, and when the TBRs of CNT-PEEK and WS2-PEEK interfaces decreased. The thermal conductivity of composites with CNTs aligned parallel to the heat flux was enhanced ~2.7 times relative to that of composites with randomly-dispersed CNTs.
\n
The model could also quantitatively study the effect of the complex morphology and dispersion of SWNTs, (e.g., individual and bundled SWNTs, the number of SWNT bundles, and the number of SWNTs per bundle), on the thermal conductivity of multiphase composites. It was found that the TBR at the SWNT-SWNT interface played a significant role in the thermal conduction of the composite with SWNT bundles. As presented in Figure 16(b), the thermal conductivity of the three-phase composite decreased with the rise of SWNT-SWNT TBR. A critical SWNT-SWNT TBR was found to be 0.155×10-8 m2K/W, which dominated the heat transfer mechanism in the three-phase composite. Proper treatment may be used to reduce the SWNT-SWNT TBR, such as the condensation of SWNT fibers, to enhance the thermal conductivity of multiphase composites with aligned SWNTs [78]. Besides the CNT multiphase composites, Gong et al. also modified the MC model to study the thermal conduction mechanisms in graphene composites [79] and CNT aerogels [80], as well as the multiphase biological systems containing CNTs [77,81,82], which indicated that the MC approach may be applicable for modeling heat transfer in diverse aligned CNT composite systems.
\n
Figure 16.
(a) Schematic plot of the computational model of the SWNT/WS2/PEEK composites with SWNT bundles; (b) Effect of the SWNT-SWNT TBR on the thermal conductivity of the SWNT/WS2/PEEK composites [78].
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6. Conclusions and outlook
\n
Both the CNT fibers and their polymer composites fabricated using the methods outlined in this article attain superior mechanical, electrical and thermal properties compared with CNT composites fabricated using the conventional methods. Their advanced properties make them promising candidates for diverse applications, such as protective materials in airplanes and electrode materials in energy storage devices. For the diverse industrial applications of the aligned CNT composites, more studies should be carried out to fabricate the composites on a large scale and at low cost. New synthesis approaches can be developed to control the diameter of composite fibers and the size of composite films. To enhance their mechanical properties, cross linking should be created within CNT fibers through proper post-treatments. Chemical compositions and fabrication conditions require optimization for better polymer infiltration into the aligned CNT fibers, to achieve enhanced properties of the aligned CNT composites.
\n
\n\n',keywords:"Aligned CNT composite, CNT fiber, fiber densification, polymer infiltration, Monte Carlo model",chapterPDFUrl:"https://cdn.intechopen.com/pdfs/50178.pdf",chapterXML:"https://mts.intechopen.com/source/xml/50178.xml",downloadPdfUrl:"/chapter/pdf-download/50178",previewPdfUrl:"/chapter/pdf-preview/50178",totalDownloads:2283,totalViews:433,totalCrossrefCites:7,totalDimensionsCites:21,totalAltmetricsMentions:3,impactScore:8,impactScorePercentile:97,impactScoreQuartile:4,hasAltmetrics:1,dateSubmitted:"October 7th 2015",dateReviewed:"February 15th 2016",datePrePublished:null,datePublished:"July 20th 2016",dateFinished:"March 29th 2016",readingETA:"0",abstract:"Aligned carbon nanotube (CNT) composites have attracted a lot of interest due to their superb mechanical and physical properties. This article presents a brief overview of the synthesis approaches of aligned CNT composites. The three major methods for fabricating aligned CNT fibers are first reviewed, including wet-spinning, dry-spinning and floating catalysts. The obtained CNT fibers, however, have limited mechanical and physical properties due to their porous structure and poor CNT alignment within the fibers. Appropriate treatments are required to densify the fibers to enhance their properties. The main approaches for the densification of CNT fibers are then discussed. To further enhance load transfer within CNT fibers, polymer infiltration is always used. Typical studies on polymer infiltration of CNT fibers are reviewed, and the properties of the obtained composites indicate the superiority of this composite fabrication method over the conventional dispersion method. Since aligned CNT composites are usually obtained in structures of long fiber or thin film, it is difficult to measure the thermal conductivity of these composites. An off-lattice Monte Carlo model is developed to accurately predict the thermal conductivity of aligned CNT composites.",reviewType:"peer-reviewed",bibtexUrl:"/chapter/bibtex/50178",risUrl:"/chapter/ris/50178",book:{id:"5167",slug:"carbon-nanotubes-current-progress-of-their-polymer-composites"},signatures:"Hai M. Duong, Feng Gong, Peng Liu and Thang Q. Tran",authors:[{id:"178818",title:"Dr.",name:"Hai",middleName:null,surname:"Duong",fullName:"Hai Duong",slug:"hai-duong",email:"mpedhm@nus.edu.sg",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",institution:{name:"National University of Singapore",institutionURL:null,country:{name:"Singapore"}}}],sections:[{id:"sec_1",title:"1. Introduction",level:"1"},{id:"sec_2",title:"2. Methods for assembling CNTs into CNT fibers",level:"1"},{id:"sec_2_2",title:"2.1. Spinning from CNT Solution",level:"2"},{id:"sec_3_2",title:"2.2. Spinning from vertically aligned CNT arrays",level:"2"},{id:"sec_4_2",title:"2.3. Spinning from CNT aerogels",level:"2"},{id:"sec_6",title:"3. Methods for enhancing CNT alignment",level:"1"},{id:"sec_6_2",title:"3.1. Enhancing CNT alignment for fibers spun from the wet-spinning technique",level:"2"},{id:"sec_7_2",title:"3.2. Enhancing CNT alignment for fibers spun from dry-spinning and floating catalyst techniques",level:"2"},{id:"sec_7_3",title:"3.2.1. Indirect approaches",level:"3"},{id:"sec_7_4",title:"3.2.1.1. Liquid densification",level:"4"},{id:"sec_8_4",title:"3.2.1.2. Twisting",level:"4"},{id:"sec_9_4",title:"3.2.1.3. Drawing through dies",level:"4"},{id:"sec_10_4",title:"3.2.1.4. Aligning and tension system",level:"4"},{id:"sec_12_3",title:"3.2.2. Direct approaches",level:"3"},{id:"sec_12_4",title:"3.2.2.1. Rubbing/false twisting",level:"4"},{id:"sec_13_4",title:"3.2.2.2. Mechanical compression",level:"4"},{id:"sec_17",title:"4. Mechanical and physical properties of aligned CNT polymer composites",level:"1"},{id:"sec_17_2",title:"4.1. Impregnating method",level:"2"},{id:"sec_17_3",title:"4.1.1. Dip coating/soaking",level:"3"},{id:"sec_18_3",title:"4.1.2. Resin transfer molding",level:"3"},{id:"sec_19_3",title:"4.1.3. Spray winding and layer-by-layer deposition",level:"3"},{id:"sec_21_2",title:"4.2. Effect of CNT morphology",level:"2"},{id:"sec_23",title:"5. Mesoscopic modeling of thermal conduction in aligned CNT composites",level:"1"},{id:"sec_23_2",title:"5.1. Thermal conduction model for two-phase aligned CNT composites",level:"2"},{id:"sec_24_2",title:"5.2. Thermal conduction model for multi-phase aligned CNT composites",level:"2"},{id:"sec_26",title:"6. Conclusions and outlook",level:"1"}],chapterReferences:[{id:"B1",body:'\nDemczyk BG, Wang YM, Cumings J, Hetman M, Han W, Zettl A, et al. Direct mechanical measurement of the tensile strength and elastic modulus of multiwalled carbon nanotubes. Mater Sci Eng A. 2002;334(1–2):173-8.\n'},{id:"B2",body:'\nPop E, Mann D, Wang Q, Goodson KE, Dai HJ. 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A numerical study on the effective thermal conductivity of biological fluids containing single-walled carbon nanotubes. Int J Heat Mass Transfer. 2009;52(23-24):5591-7.\n'},{id:"B64",body:'\nDuong HM, Papavassiliou DV, Mullen KJ, Maruyama S. Computational modeling of the thermal conductivity of single-walled carbon nanotube - polymer composites. Nanotechnology. 2008;19(6):065702.\n'},{id:"B65",body:'\nDuong HM, Yamamoto N, Papavassiliou DV, Maruyama S, Wardle BL. Inter-carbon nanotube contact in thermal transport of controlled-morphology polymer nanocomposites. Nanotechnology. 2009;20(15):155702.\n'},{id:"B66",body:'\nDuong HM, Yamamoto N, Bui K, Papavassiliou DV, Maruyama S, Wardle BL. Morphology effects on nonisotropic thermal conduction of aligned single-walled and multi-walled carbon nanotubes in polymer nanocomposites. J Phys Chem C. 2010;114(19):8851-60.\n'},{id:"B67",body:'\nBui K, Grady BP, Papavassiliou DV. Heat transfer in high volume fraction CNT nanocomposites: Effects of inter-nanotube thermal resistance. Chem Phys Lett. 2011;508(4-6):248-51.\n'},{id:"B68",body:'\nPeters JE, Papavassiliou DV, Grady BP. Unique thermal conductivity behavior of single-walled carbon nanotube−polystyrene composites. Macromolecules. 2008;41(20):7274-7.\n'},{id:"B69",body:'\nBui K, Duong HM, Striolo A, Papavassiliou DV. Effective heat transfer properties of graphene sheet nanocomposites and comparison to carbon nanotube nanocomposites. J Phys Chem C. 2011;115(10):3872-80.\n'},{id:"B70",body:'\nNaffakh M, Diez-Pascual AM, Gomez-Fatou MA. New hybrid nanocomposites containing carbon nanotubes, inorganic fullerene-like WS2 nanoparticles and poly(ether ether ketone) (PEEK). J Mater Chem. 2011;21(20):7425-33.\n'},{id:"B71",body:'\nNaffakh M, Diez-Pascual AM, Marco C, Ellis G. Morphology and thermal properties of novel poly(phenylene sulfide) hybrid nanocomposites based on single-walled carbon nanotubes and inorganic fullerene-like WS2 nanoparticles. J Mater Chem. 2012;22(4):1418-25.\n'},{id:"B72",body:'\nYu AP, Ramesh P, Sun XB, Bekyarova E, Itkis ME, Haddon RC. Enhanced thermal conductivity in a hybrid graphite nanoplatelet - carbon nanotube filler for epoxy composites. Adv Mater (Weinheim, Germany). 2008;20(24):4740.\n'},{id:"B73",body:'\nGupta TK, Singh BP, Mathur RB, Dhakate SR. Multi-walled carbon nanotube–graphene–polyaniline multiphase nanocomposite with superior electromagnetic shielding'},{id:"B74",body:'\n[77] Liao WH, Tien HW, Hsiao ST, Li SM, Wang YS, Huang YL, et al. Effects of multiwalled carbon nanotubes functionalization on the morphology and mechanical and thermal properties of carbon fiber/vinyl ester composites. ACS Appl Mater Interf. 2013;5(9):3975-82.\n'},{id:"B75",body:'\nDiez-Pascual AM, Ashrafi B, Naffakh M, Gonzalez-Dominguez JM, Johnston A, Simard B, et al. Influence of carbon nanotubes on the thermal, electrical and mechanical properties of poly(ether ether ketone)/glass fiber laminates. Carbon. 2011;49(8):2817-33.\n'},{id:"B76",body:'\nCheng HKF, Basu T, Sahoo NG, Li L, Chan SH. Current advances in the carbon nanotube/thermotropic main-chain liquid crystalline polymer nanocomposites and their blends. Polymers. 2012;4(2):889-912.\n'},{id:"B77",body:'\nGong F, Papavassiliou DV, Duong HM. Off-Lattice Monte Carlo simulation of heat transfer through carbon nanotube multiphase systems taking into account thermal boundary resistances. Num Heat Transfer Part A Appl. 2014;65(11):1023-43.\n'},{id:"B78",body:'\n[81] Gong F, Duong HM, Papavassiliou DV. Inter-carbon nanotube contact and thermal resistances in heat transport of three-phase composites. J Phys Chem C. 2015;119(14):7614-20.\n'},{id:"B79",body:'\nFan Z, Gong F, Nguyen ST, Duong HM. Advanced multifunctional graphene aerogel – Poly (methyl methacrylate) composites: experiments and modeling. Carbon. 2015;81(0):396-404.\n'},{id:"B80",body:'\nGong F, Tam YS, Nguyen ST, Duong HM. Prediction of thermal resistances and heat conduction of carbon nanotube aerogels in various permeated gases. Chem Phys Lett. 2015;627:116-20.\n'},{id:"B81",body:'\nGong F, Hongyan Z, Papavassiliou DV, Bui K, Lim C, Duong HM. Mesoscopic modeling of cancer photothermal therapy using single-walled carbon nanotubes and near infrared radiation: insights through an off-lattice Monte Carlo approach. Nanotechnology. 2014;25(20):205101.\n'},{id:"B82",body:'\nFang Y, Lv Y, Gong F, Wu Z, Li X, Zhu H, et al. Interface tension-induced synthesis of monodispersed mesoporous carbon hemispheres. J Am Chem Soc. 2015;137(8):2808-11.\n'}],footnotes:[],contributors:[{corresp:"yes",contributorFullName:"Hai M. Duong",address:"mepdhm@nus.edu.sg",affiliation:'
Department of Mechanical Engineering, National University of Singapore, Singapore
Department of Mechanical Engineering, National University of Singapore, Singapore
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1. Introduction
Citrus belongs to family Rutaceae and holds an important position among fruits all around the globe. It is the most cultivated fruit in the world after grapes. Citrus is believed to be originated from southeastern Asian region [1]. Northern hemisphere accounts for about 70% of the total citrus production and approximately 80 citrus species are native to India and other tropical and sub-tropical areas of Asia [2]. Citrus being a perennial fruit tree is usually produced through vegetative propagation of scion on rootstock. Combination and compatibility of scion and rootstock can result in high yielding citrus plants. The United States, China, Brazil and the Mediterranean countries contribute two third of global citrus production and are regarded as major citrus producing countries [3]. Citrus products and by-products provide the basis for local agricultural industries, which generate employment and raise income, and in many cases, this industry constitutes an important source of foreign revenue for developed and developing countries such as Pakistan.
A number of factors and certain conditions are collectively responsible for fluctuations in citrus production. Selection of rootstock, agronomic practices and management in citrus nurseries and orchards, propagation methods and biotic and abiotic factors contribute their share to some extent in reduced citrus production. Like other commercial crops, number of diseases, insect pests and genetic problems affect the citrus production. Diseases are one of the major limiting factors for the low citrus production and gives a serious threat to citrus industry. These diseases are caused by fungi, prokaryotes, nematodes, viroids, viruses and virus-like pathogens. Among these, viruses and virus-like pathogens play a major role in citrus decline. These pathogens incur varying degree of damages to citrus plants and make their life span shorter, causing low yield and deterioration of quality and ultimately loss of economy which leads towards the citrus decline [4].
Citrus decline is the matrix of all above mentioned factors and conditions. The common diseases, playing an important role in citrus decline are citrus gummosis caused by Phytophthora sp. and Fusarium sp., citrus canker caused by Xanthomonas sp., Huánglóngbìng caused by Candidatus laberibactor sp., citrus stubborn caused by Spiroplasma citri and one of the most devastating citrus viruses i.e. citrus tristeza virus. Citrus viruses play a vital role in its decline by using the prevailing conditions and many other factors as these are bud/graft-transmissible and have systemic infections. A variety of symptoms has been observed regarding the infection of citrus viruses resulting in systemic infection. No viral diseases on citrus was under discussion or the hot issue before 1940 but during and after 60 years, thirty economically important viruses and virus-like diseases of citrus were recognized as a cause of citrus decline in different parts of the world [5, 6, 7]. Unfortunately, citrus orchards are short lived and decline within 15 years as against their potential of 50 years or more. This is mainly attributed, among other factors, to the prevalence of graft-transmissible virus and virus-like diseases, faulty nursery operations and poor orchard management. However, most of the problems originate from nurseries.
Therefore, it is the time when citrus nurseries should operate on highly technical and scientific lines and start providing disease-free and certified plants to the growers. In the first instance, nurseries should be registered and indiscriminate multiplication and sale of uncertified citrus plants must end. For this purpose, the most imperative points such as the prevalence and detection of citrus viral diseases, selection of material, production of disease-free material and streamlined screening procedures are highlighted in this bulletin. If the guidelines are properly followed and certified bud-wood becomes available for producing disease-free citrus plants, the problem of citrus decline can be minimized.
1.1 Citrus pathology
Citrus pathology is the study of citrus diseases caused by biotic (pathogens) and abiotic factors. It is now being considered as a major part in the field of plant pathology. Being a major fruit crop in the world, citrus production always remains important for the citrus industry. Physiology, morphology, biochemistry and behavior of the citrus tree towards the prevailing climatic conditions are the key areas to be kept in mind while investigating the citrus diseases. Etiology of citrus diseases and their detection methods help to manage these diseases. A plenty of information regarding the diseases of citrus and their control has been published around the world.
2. Virus and virus-like diseases of citrus
Virus, viroids and virus-like diseases, however, infecting different citrus species could not receive due attention because of the lack of laboratories with proper facilities for their proper identification. These diseases are also known as ‘graft-transmissible diseases’ (GTDs) and the term used for the casual agents is ‘citrus graft-transmissible pathogens’ (CGTPS) [8]. These are an emerging threat for citrus industry. Major viruses and virus-like pathogens include citrus tristeza virus (CTV), citrus yellow vein clearing virus (CYVCV), citrus variegation virus (CVV), concave gum, psorosis, cristacortis, ringspot, exocortis, Cachexia-xyloprosis, Candidatus liberibacter asiaticus and Spiroplasma citri [9, 10]. A brief description of these virus and virus-like pathogens is summarized below (Table 1).
Sr. No.
Citrus disease
Pathogen
Transmission
Incidence %
Host
Importance
1.
Citrus greening disease (CGD) Huánglóngbìng
Bacterium-like organism
Psyllid: Diaphorina citri
20–90
Sweet orange, grapefruit, orange jessamine
Associated with citrus decline
2.
Citrus tristeza virus (CTV)
Closterovirus
Aphid species (Aphis gossypii, Toxoptera citricida)
7–18 Up to 48
Sweet orange, lime, mandarin
Economically important
3.
Gummy bark (GB)
Virus probable
Grafting, mechanical
20–30
Mandarin, sweet orange
-do-
4.
Bud union crease (BUC)
Virus probable
Grafting, mechanical
20–30
Mandarin, sweet orange
-do-
5.
Cristacortis
Virus probable
Not known
10
All citrus species
-do-
6.
Exocortis
Viroid
Mechanical
7–10 Up to 16
Sweet lime
-do-
7.
Cachexia-xyloporosis
Viroid
Mechanical
4–10
Mandarin
-do-
8.
Citrus stubborn disease (CSD)
Prokaryote
Leaf hopper (Neoaliturus haemocops)
2–7
Sweet orange, grapefruit, periwinkle
-do-
9.
Yellow vein clearing (YVC)
Virus
Grafting, vector not known
2
Lemon, sour orange
Minor importance
10.
Ring spot/ Variegation
Virus
Not known
2–3
Sweet orange
Minor importance
Table 1.
Major virus and virus-like diseases of citrus in Pakistan, their transmission and hosts*.
The above summarized information is extracted from the work of [10, 11, 12].
Note: All diseases are graft-transmissible. No adequate information on vector transmission is available except their identity; viroids problems are favored by warm conditions.
Although plant pathologists have put their efforts for the identification and management of virus and virus-like diseases of citrus but there are some areas need to be investigated. A comprehensive book has been written by Roistacher in 1991 regarding the detection of virus and virus-like diseases of citrus. These diseases reduce the citrus yield and ultimately result in the loss of low foreign exchange. Diseases caused by viruses and virus-like pathogens are infectious, contagious and devastating due to their systemic nature. They are transmitted through different means in nature; through vegetative propagation, by insect vectors and horticultural tools used for the routine activities in citrus orchards and nurseries. These diseases have a considerable economic importance because of their involvement in the citrus decline [4]. Millions of citrus trees have been died due to CTV. The CGTPS usually have two types of effects either quick decline or long term losses. These diseases are very difficult to control or manage unless or until by the application of integrated management practices. The appropriate diagnosis or indexing method plays an important role for the management of CGTPS [8].
The major symptoms due to virus and virus-like pathogens are vein clearing, bark cracking, yellowing of leaves, leaf dropping, gummosis, mosaic, rugosity, bark scaling, stem pitting, dwarfing, chlorosis and mottling [10, 13]. The virus and virus-like diseases, infecting different citrus species in Pakistan, have been neglected for a long time due to lack of proper facilitations in the research laboratories and skilled personnel for their detection and characterization. A brief description is presented in Table 2 regarding the citrus species and viruses and virus-like diseases in Pakistan. Indexing facilities are very important for the diagnosis of plant pathogens. Similarly, unlike other pathogens viruses and virus-like pathogens are very sensitive to their indexing through different techniques. Pathogen detection system always played an important role in management of virus and virus-like pathogens. Proper indexing facilities help in the characterization and differentiation of different viruses and their isolates. Management of viruses and virus-like pathogens is only possible when appropriate indexing procedures and facilities are available.
Citrus species
Virus
Viroid
Prokaryote
Virus-like symptoms
PS
DE
CTV
IVV
RS
YUC
Ex
CX
GR
ST
BS
GB
BU
BP
Misc.
Sweet orange (Mosambi)
+
+
+
+
+
+
+
+
+
+
+
+
Sweet orange (Mosambi)
+
+
+
+
+
+
+
+
+
+
+
+
Mandarin
+
+
+
+
+
+
+
+
+
+
Sweet lime
+
+
+
+
+
+
Grapefruit
+
+
+
+
+
+
Lemon
+
+
+
+
Acid lime
+
+
+
+
Rough lemon
+
+
+
+
Sour orange
+
+
+
+
Orange jessamine
+
+
+
Table 2.
Citrus species and presence of viruses and virus-like diseases.
Note: “+” is the indication of presence of infection on the citrus varieties.
CTV = Citrus Tristeza Virus, IVV = Infection variegation, RS = Ring spot; Ex = Exocortis, CX = Cachexia xyloporsis, GR = Greening disease, ST = Stubburn Disease, BS = Bark Scaling, GB = Gummy Bark, BU = Bud Union Disease, PS = Psorosis, DE = Decline.
3. Insects as vectors of virus and virus-like pathogens
Insect pests have always been key role players in the direct or indirect transmission of plant pathogens in agricultural and horticultural crops [14, 15, 16]. Citrus tristeza, cachexia-xyloporosis, greening or Huánglóngbìng, infectious variegation, vein enation, yellow vein clearing, exocortis and stubborn are the most conspicuous viral diseases of citrus all over the world including Pakistan [11, 17]. These diseases are usually graft-transmissible and phloem-restricted. Although these diseases along with other fungal, bacterial or mycoplasmic infections of citrus are usually spread through unhealthy mechanical intrusions and by the use of infected uncertified bud, scion or rootstock in plant propagation, many type of sap-feeding insect pests play important role in the transmission of these diseases such as leafhoppers, aphids, psyllids, whiteflies and thrips [17, 18, 19, 20].
Among the vector borne viral diseases of citrus, citrus tristeza (CTV) which is caused by a Closterovirus is the most dominant and widely studied viral diseases of citrus. It is transmitted by different aphid species primarily by black citrus aphid (Toxoptera citricida Kirk.) and cotton-melon aphid (Aphis gossypii Glov.) [17, 21]. Another emerging viral disease of citrus is the yellow vein clearing (CYVCV) caused by a Mandarivirus. It was first observed in Pakistan in 1988 in the orchards of sour orange (C. aurantium L.) and lemon (C. limon L.) [22], and later on it was reported in China, India, Iran and Turkey [23, 24, 25, 26]. This CYVCV is reported to be vectored by e transmitted by whiteflies and aphids (Aphis craccivora and A. spiraecola) [25, 27]. Although not virus borne, citrus stubborn is a destructive disease being caused by a bacterium Spiroplasma citri. It is usually transmitted by many species of leafhoppers, primarily by Scaphytopius nitridus and Circulifer tenellus in citrus-growing suburbs of California and Arizona and by Circulifer haematoceps in the Mediterranean zones [17].
4. Indexing strategies
Indexing is an indispensable procedure to produce and diagnose disease-free plants. Different techniques or combination of techniques have been applied in this regard and the effectiveness of each depends upon the facilities available. Generally indexing can be divided into two types.
Field indexing; also known as biological indexing including the mechanical inoculation through direct contact or vegetative propagation and/or through insect transmission.
Laboratory indexing; also known as quick indexing including serological, molecular and chemical assays.
Commonly used indexing methods are tissue grafting, budding, insect transmission for biological indexing and enzyme-linked immunosorbent assay (ELISA) and polymerase chain reaction (PCR) for quick indexing strategies. Although all viruses and virus-like pathogens can be detected through PCR and its derivatives, polyacrylamide gel electrophoresis (PAGE) is commonly used for the detection of viroids.
4.1 Biological indexing
Biological indexing is the inoculation or introduction of virus source (infected sample) into the indicator plants for detection and purification. It involves one of the common indexing methods such as vegetative propagation of infected scion (grafting/budding) to indicator plants, mechanical inoculation of indicator plants or transmission of virus through the insect vector (e.g. aphids for CTV, psyllids for greening and leaf hoppers for prokaryotic diseases). Biological indexing is usually time consuming, require glasshouse facilities and takes about 6–12 months for results. At least 3–4 plants are required per treatment. Biological indexing of graft-transmissible pathogens, indicator plants and symptoms in the indicator plants are summarized in Table 3.
Stunted shoot, smelling of leaves, Zn deficiency like signs.
11.
Yellows (probably Aster)
5
Grapefruit, Periwinkle (C. roseus)
Warm
Chlorosis
12.
Bud union crease
5
Sweet orange
Warm
Brown line at bud union
13.
Gummy bark
5
Mandarin
Warm
Gum in the bark
Table 3.
Biological indexing of citrus graft-transmissible pathogens.
Note: The above information is extracted from the work of [10, 12] and personal communication of Dr. S.M. Mughal. (Dr. Mughal was also in the team of Dr. Catara during the surveys of citrus growing areas of Pakistan in early 1980’s).
Detailed methodology for biological indexing has been described much in literature [28, 29, 30, 31]. Followings are the generalized and simplified steps to be kept in mind during the biological indexing on the basis of available literature.
Sow the seeds of test plants (usually Mexican lime or acid lime) in the sand in germinating tray. Transplant the seedlings in pots having potting media (sand, soil and moss @ 1:1:1 ratio) after 17–28 days of germination, depending on the germinating conditions.
Inoculate the seedlings at 4–6 leaf stage.
Keep the indicator plants in insect-free chambers before and after inoculation.
Mechanical inoculation: grind the virus infected samples in phosphate buffer (pH 7.2). Dust the carborundum powder on to the indicator plants, but not too much, before inoculation (excessive dusting of carborundum will cause the necrosis and misled results).
Pass the crude virus extract from double layer muslin cloth and then apply to the indicator plants with the help of forefinger and leave for 3–4 min. Remove the excess sap from indicator plants under tap water.
Insect transmission: Do rearing of vector insects in the laboratory or collect the vector insects directly from the field and keep them in laboratory for few days to be acclimatized with the rearing conditions. Provide them with the artificial or natural diet.
Observe the fasting period according to the nature of transmission (non-persistent, persistent or semi-persistent) before allowing them to be fed on virus source to acquire the virus.
For non-persistent transmission pre-acquisition fasting time is 30–90 min. Long fasting period enhances the chances of quick acquisition of virus from the infected source.
Transfer the insects on to the young leaves with virus symptoms/virus infected plants with the help of camel brush and allow them to feed for few min.
After few min, immediately transfer the viruliferous insects on to the indicator plants and keep the plants in insect-free chamber to avoid the contamination from other insects.
Maintain the insect population on indicator plants for at least 24 hr. and eradicate them after that through insecticides.
For persistent transmission and semi-persistent transmission pre-acquisition fast has no effect. In both cases long acquisition feeding period enhances the chance of transmission.
Maintain the insect population for a week and eradicate them with insecticide in case of semi-persistent transmission while maintain the insect population through transferring them on new indicator plants till they are alive.
Vegetative propagation: Take the infected bud-wood from the virus source and graft on to the rootstock/indicator plants and keep the indicator plants in insect-free zones.
Temperature range between 65 and 95°F helps the appearance of symptoms on indicator plants for viruses and virus-like pathogens. Observation time also varies from 3 to 16 months for different viruses, virus-like pathogens and viroids.
Laboratory indexing/advanced detection methods
There are rapid methods, highly specific, routinely applicable and some of which test large number of samples. These methods are summarized in Table 4. ELISA is the main laboratory indexing method used for the detection of CTV, PAGE for viroids and PCR for all diseases. Mother plants (plants recovered by nucellar embroyony in-vivo or in-vitro, by thermotherapy or micro-grafted plants or by micro-budding may be indexed by any of the above methods. Although ‘chromatography’ is a useful in chemical indexing of certain virus and virus-like pathogens but it is less reliable than vegetative propagation indexing. Electron microscopy is also helpful for the detection of greening and stubborn diseases other than the viruses. Moreover, S. citri can be cultured on a specific medium. Now-a-days, commercial kits are available for the ELISA, PCR and other detection methods along with the instructions.
Sr. No.
Methods
Tested for
Advantages and limitations
References
1.
Immunofluorescence, tissue staining Azure A, Light microscopic observations
Advanced methods for the detection of viral diseases of citrus.
Note: Large scale screening of material is possible with any of the method(s) mentioned above. However, there are several limitations including time and availability of proper facilities and trained manpower.
4.2 Serological assays
Serology involves the quick indexing of plant viruses, based on the antibody–antigen reaction. Enzyme-linked immunosorbent assay (ELISA) is one of the widely used in detection of plant viruses. It is relatively cheap and can test large number of samples.
ELISA with its derivatives, direct (DAS-ELISA) and indirect (DAC-ELISA), is the main serological indexing tool used for most of the citrus viruses at large scale samples.
Followings are some general steps followed during the ELISA based detection or indexing [35].
For DAS-ELISA; Coat the antibodies in the ELISA plate and keep at 4°C for overnight or 37°C for 4 hr. for incubation.
Wash the plate with washing buffer for 3 times with the interval of 5 min.
Add the antigen (virus sap extracted from infected samples) into the wells of ELISA plate and incubate as above.
Repeat the washing and coat the ELISA plate with enzyme-labeled antibodies and incubate as above.
Repeat the washing step and add the substrate followed by incubation for 30 to 90 min for visual observation of color change and read the micro-plate through ELISA reader/spectrophotometer for quantitative data.
For DAC-ELISA: Add the antigen and incubate the plate as above.
Wash the ELISA plate as in DAS-ELISA.
Add the primary antibody and incubate.
Add the secondary antibody and incubate.
Add the enzyme-labeled antibodies and incubate.
Add the substrate and then observe the color change after incubation and read the plate through ELISA reader for quantitative data.
Note: Repeat the washing step after every step before adding the substrate. Stop the reaction in both types of ELISA with the help of 1 N NaOH.
4.3 Molecular assays
Molecular detection of citrus viruses and virus-like diseases has revolutionized the subject and provided the platform to detect the early stages of infection to reduce the economic losses. The molecular hybridization techniques supplemented with nucleic acid amplification methods based on PCR, in which high-throughput sequencing approaches can be adopted to identify the strains in relation to evolutionary history or phylogenetic assemblages [36, 37]. Although, nucleic acid based methods are highly sensitive and discriminatory allowing specific strain typing, but it bears the problems in reproducibility [38, 39]. Progressive efforts have been made to decrease the troubleshoots and hurdles to improve the amplification systems by improving the sensitivity and specificity of detection by limiting the high contents of plant related enzyme inhibitors. In contest, nested and multiplex PCR provides high sensitivity and make the possible to detect several targets in single assay [40]. Moreover, highly sensitive technologies by conducting the amplification of nucleic acids in an isothermal reaction, nucleic acid sequence-based amplification (NASBA) and reverse transcription loop-mediated isothermal amplification (RT-LAMP) provides specific detection of viruses and virus-like diseases.
The addition of real-time PCR for high-throughput testing allows the automation of PCR by combing the fluorimeteric approaches to detect and quantify the targets simultaneously [41, 42]. The combination of different protocols including the serological techniques and molecular approaches will increase the accuracy and reliability of virus diagnostic. Furthermore, in future prospects, nucleic acid arrays and biosensors assisted by nanotechnology will open new corridors to revolutionize the detection of plant viruses and virus-like diseases.
Citrus tristeza virus (CTV) is the most dangerous citrus disease all over the world and is also known as quick decline disease reducing the population of citrus trees significantly [43, 44, 45]. However, the utilization of advanced diagnostic methods, such as, biological indexing, electron microscopy (EM), ELISA and PCR or reverse transcriptase PCR (RT-PCR) is providing promising detection of the virus particles and leading towards the management strategies of CTV [46]. The application of conventional PCR is sensitive and specific under optimized and controlled conditions. However, sometimes, it is not possible to judge the amount of pathogens in the samples. Therefore, researchers have to employ other subsequent techniques for complete detection and quantification. Meanwhile, with real-time PCR approach, users can monitor the reaction and also the quantification of the specific pathogen in the sample. While setting up the real-time reaction for virus detection, it is the basic requirement to adapt the specific conditions of the detection system and instrument, and the characteristics of the reaction reagents and cycling procedures in which the most important are primer design, reaction components and conditions. The real-time PCR works well with small amplicons (5–200 bp), while standard PCR allows amplification of several hundred bases without sensitivity and specificity. Moreover, concentrations of MgCl2, primers, and dNTPs are usually higher than conventional PCR [47].
The new developing chemistries are setting up the protocols with different characteristics depending upon the target and assay requirements. In addition to the most widely working chemistries (SYBRGreen, TaqMan, Scorpion, Molecular Beacons), there are more novel chemicals or technologies such as Amplifluor; Locked Nucleic Acid (LNA) Probes, Sigma Proligo; Cycling Probe Technology (CPT), Takara; Light Upon eXtension (Lux) Fluorogenic Primers, Invitrogen Corporation; Plexor Technology, Promega [48, 49]. Real-time technology is being used also in multiplex formatting for the specific detection and strain identification for several viruses [50, 51, 52, 53, 54, 55]. Furthermore, real-time reaction in multiplex system is difficult to optimize due to different ratio between the targets and the reaction. The replacement of conventional PCR with real-time PCR is providing new horizons towards the multiple detection system of plant viruses especially of the citrus viruses and virus-like diseases.
5. Detection of citrus viroids
After the discovery of viroid group of pathogens as an infectious agent to the plants, new aspects in virology were come in front of researchers to be addressed. Viroids are the smallest pathogens which consist of 246 to 401 nucleotides. They are low molecular weight, circular and single stranded RNAs. Viroids exist as free RNA because they lack protein coat [56]. Since viroids do not code for protein and enzyme, they rely on host enzyme for protein synthesis system and replication. To date, 38 viroids have been identified and they are classified into 2 families i.e. Pospiviroidae and Avsunviroidae [57].
The major economic important viroids in different plants are coconut viroids (CCCVd), citrus viroids (Exocortis and cachexia and variants), Hop stunt viroid and Potato spindle tuber viroids [57]. The origin of viroids is still questionable as they do not have natural host relationship [58, 59].
Citrus production is also affected by viroids. These are the emerging threat to citrus industry. To date, seven citrus viroids have been detected so far in citrus viz. Citrus Exocortis viroid (CEVd), Citrus Bent Leaf viroid (CBLVd), Hop Stunt viroid-citrus (HPSVd-cit), Citrus Dwarfing viroid (CDVd), Citrus Bark Cracking viroid (CBCVd), Citrus viroid V (CVd V) and Citrus viroid VI (CVd VI-OS). These have been distributed in different geographical areas as shown in Table 5 [70]. Diseases caused by citrus viroids are citrus exocortis disease (CED), citrus cachexia disease (CCD), citrus leaf bending disease (CLBD), citrus bark cracking disease (CBCD) and citrus dwarfing disease (CDD). Among these, citrus exocortis and citrus cachexia-xyloporosis are the most devastating and widely distributed [57]. These diseases cause a reduction in yield, size of fruit and quality of production [8]. These are transmitted directly and through propagation [71]. Stunting, dwarfing, bark cracking, yellowing of leaves, backward leaf bent, pin holing, yield loss and ultimately tree decline are the common symptoms of citrus viroid diseases [63, 71, 72]. Citrus viroids alone or with other viruses or prokaryotes in the host contribute considerably in tree decline [73]. Exocortis and cachexia are the major viroids which are widely distributed in citrus orchards. Other citrus viroids have also been detected from citrus orchards in different parts of the world [73]. Unlike viruses, viroids do not have protein coat, therefore, these are very difficult to detect through serological methods. For this purpose, molecular techniques such as PCR, PAGE are available for the detection of citrus viroids. These are sensitive, sophisticated and rapid detection techniques. Molecular techniques not only help in the detection but also in the characterization of viroids.
5.1 Pathogen description and characterization
All citrus viroids are classified in different genus under Pospiviroidae as mentioned in Table 6.
Viroid
Geographical distribution
References
Citrus excocortis viroid (CEVd)
Australia, Argentina, Brazil, Japan, Taiwan, Corsica, China, India, Israel, Spain, Pakistan, South Africa USA, Uruguay, Iran
Hop stunt viroid-citrus (CVd-IIa) Citrus cachexia viroid (CVd-IIb)
299–302
Citrus cachexia disease.
Cocadviroid
Citrus viroid IV
284–286
Citrus bark cracking disease
Apscaviroid
Citrus bent leaf viroid (CVd-I),
318
Citrus leaf bending disease
Citrus dwarfing viroid (CVd-III)
294–297
Citrus dwarfing disease
Citrus viroid V
295
Citrus viroid VI
330
Table 6.
Classification of citrus viroids (king et al., 2011; Hammond & Owens, 2006).
Note: The above information is extracted from the work of Hammond & Owens (2006) and King et al. (2011).
5.2 Diagnostic methods for citrus viroids
Biological indexing is done through graft inoculation in indicator plants. It is very suitable to check the symptoms produced by citrus viroids and their severity. The most important host for indexing CEVd is Etrog citron (Citrus medica, Arizona 861) because of its great sensibility and rapid symptom expression [74]. According to Nakahara et al. [75], bioassay on Etrog citron is the most sensitive technique in detection of viroids although it takes more time compared to other methods. Molecular tools are now widely being used in the detection of citrus viroids. Combinations of several molecular techniques are very useful for reducing the time and to allow large numbers of samples to be examined and to identify each citrus viroid species [75, 76]. PAGE is also used to separate variation based on molecular weight. PAGE is not suitable for indexing large number of samples because it is not cost-effective. It is used to test the circularity of viroid RNA by two-dimensional denaturing PAGE (2D-PAGE) [77, 78, 79]. Sequential-PAGE is also commonly used and capable of detecting all citrus viroids [71].
Reverse transcription- polymerase chain reaction (RT-PCR) is the most commonly used method to detect citrus viroids. It is also a reliable method for quick screening and detection of citrus viroids [80]. It is known for its high specificity and ability to detect unknown viroids or variants [57]. Multiplex RT-PCR is another approach to detect simultaneously more than a viroid by using several set of primers. For instance, CEVd, CBLVd, CVd 1-LSS, CVd-II, CVd-III, CVd-IV and CVd-VI were successfully detected simultaneously via multiplex RT-PCR [69]. Real-time RT-PCR is also used to detect citrus viroid. It is a quantitative PCR technology basically same as RT-PCR but it measures and quantifies products generated during each cycle of PCR [81]. Molecular hybridization is based on the specific interaction between complementary purine and pyrimidine bases forming A-U and G-C base pairs. According to Targon et al. [82], imprint hybridization technique is fast, sensitive and economic methods to be used as a routine for citrus viroid indexing in the certification programs. However, dot-blot technique is required an appropriate amount of extracted nucleic acids [75], and it is not suitable for detection of new or unknown viroids. Another molecular approach to detect viroids is Northern blot hybridization. CEVd, CBLVd, CVd-II, CVd-III and CVd-VI were successfully detected by Northern blot hybridization using specific probes in inoculated Etrog citron [83].
5.2.1 RT-PCR for detection of citrus viroids
5.2.1.1 Samples collection
Collect the leave samples based on virus and viroids-like symptoms in the field. Bring the leaves samples to laboratory for processing and preservation until use as follows;
Collect the leave samples in sterile plastic bags and place in ice box.
In the laboratory, wash the samples first in 10% bleach followed by distilled water.
Dry the samples and put in the plastic bags.
Label the plastic bags and store them at −80°C until further use.
5.2.1.2 Nucleic acid extraction
Extract the nucleic acids from leave samples using the TESLP buffer [84] as follows;
Grind the 2-3 g of leaves (about 10–12 leaves) using mortar and pestle with liquid nitrogen. The slurry needs to be transferred to 50 ml screw cap tubes.
Add 10 ml of TESLP buffer [0.13 M Tris–HCl (pH 8.9), 0.017 M EDTA (pH 7.0), 1 M LiCl, 0.83%SDS, 5%PVP] into the tube.
Add 16 μl of 2-mercapthoethanol into the mixture.
Incubate the mixture for 30 min at room temperature in the rotary shaker.
Centrifuge the mixture at 11000 rpm for 15 min.
The supernatant needs to be transferred to a new 50 ml screw tube.
Add phenol:chloroform:iso-amyl (PCA, 25:24:1) @ 3:2 and mix well using vortex followed by centrifugation for 15 min, 11,000 rpm at room temperature.
Transfer the supernatant into a new 15 ml screw tube and add CA (24:1) @ 4:3. The mixture needs to be mixed well using vortex and repeat the step 7.
The supernatant is obtained into a new 15 ml screw tube @ 1 volume of supernatant with 0.9 volumes of 90% isopropanol.
The tube is inverted 3–4 times to mix the components. Do not vortex or centrifuge.
The mixture is incubated at −80°C for 30–40 min (or -20°C for 3–4 hr. or overnight).
The mixture is centrifuged for 15 min, 11,000 rpm at room temperature.
The isopropanol is discarded and the pellet obtained is transferred into 1.5 ml micro centrifuge tube.
The pellet is washed with 1 ml of 70% ethanol followed by washing with 1 ml absolute ethanol until the clean pallet is obtained.
The pellet is suspended in 50 μl of sterile double distilled water.
The pellet is immediately used for RT-PCR or stored in -20°C until use.
The extracted RNA is used to run RT-PCR. Reverse Transcription process is carried out in two steps to synthesis cDNA as follows;
Step 1: (1X)
Experimental RNA = 5 μl
Reverse primer = 1 μl
Double distilled water = 2.5 μl
Total Volume = 8.5 μl
The reaction is incubated at 80°C for 12 min then immediately transferred to ice for 5 min.
Step 2: (1X)
AMV-RT = 1 μl
dNTPs = 2 μl
RNAse Inhibitor = 0.5 μl
MgCL2 = 4 μl
RT buffer = 4 μl
Total volume = 11.5 μl
The reaction is incubated at 55°C for 30 min. After 30 min, the process is stopped when it reaches to 10°C. The cDNA obtained is stored in −80°C freezer until use (or it can be used immediately).
5.2.1.4 PCR protocol
The final volume of PCR should be 25 μl which consists of 12.5 μl of PCR master mix, 5 μl of cDNA, 5.5 μl of sterile double distilled water, 1 μl of forward primer and 1 μl of reverse primer.
The conditions for PCR amplification (35 cycles) are as follows:
a. Denaturation:
94°C for 10 min
94°C for 30 seconds
60°C for 1 min
b. Annealing at 60°C for 10 seconds.
c. Extension at 72°C for 10 seconds and then 5 min.
The list of specific primers used is given in Table 7.
The amplified RT-PCR product is separated using 2% agarose gel as follows [85];
2% agarose gel is prepared with 1x TBE buffer
Samples are loaded in the gel and electricity is provided at 100 volts for 50 min.
The gel is stained with Ethidium bromide for 10 min and washed with distilled water for 5 min.
The gel is visualized under Trans UV and captured with Gel Doc XR system.
5.2.1.6 PCR product purification
Positive PCR products with expected size are purified using MinElute® Gel Extraction Kit according to the standard protocol provided with Kit.
The expected size of band is excised from the agarose gel with a sterile, sharp scalpel.
The gel slice is put in a sterile 1.5 ml micro-centrifuge tube and weighed.
QC buffer, provided with the kit, is added @ 3:1 volume of gel.
The gel slice is incubated at 50°C for 10 min until the gel slice has completely dissolved.
The mixture is vortexed every 2–3 min to facilitate the dissolution of gel slices.
Then, 1 gel volume of isopropanol is added and mixed by inverting with pipette.
The MinElute spin column is placed into 2 ml collection tube.
The sample is transferred into the MinElute column and centrifuged at 13000 rpm for 1 min.
The flow-through is discarded and put back the column into the same collection tube. 750 μl of Buffer PE is added to MinElute column and let it stand for 1–2 min.
Centrifuged at 13000 rpm for 1 min and the flow-through is discarded.
The process is repeated to remove Buffer PE completely.
The ethanol residual left at the bottom of the column is discarded and MinElute column is placed into a sterile 1.5 ml micro-centrifuge tube.
30 μl of EB Buffer is added to the center of MinElute membrane to elute DNA. The mixture is let to stand for 1 min, and then is centrifuged at 13000 rpm for 1 min.
MinElute column is discarded and the tube is stored in - 20°C.
5.2.1.7 Molecular Cloning (TOPO TA cloning kit, Invitrogen)
Positive PCR samples will be cloned using the TOPO TA cloning kit according to the standard protocol provided along with the Kit as follows;
Ligation
4 μl purified PCR products.
1 μl vector (pCR2.1-TOPO).
1 μl Salt solution.
Incubate in PCR machine/ heat block at 25°C for 30 min.
Add 2 μl of ligation mixture into competent cell E. coli - do not pipette up and down, just thaw a bit/ swirl.
Put 30 min in ice.
Transformation
Put 30 sec in 42°C water bath (heat shock).
Put in ice for 5 min (immediately after heat shock).
Add 250 μl SOC medium to mixture-seal competent cell tube with parafilm.
Put at 200 rpm in 37°C incubator shaker for 1 h 30 min.
Warm the petri dish in incubator for 20–30 min.
Spread 40 μl X-gal on petri dish (LBA media).
After spread the X-gal, put the petri dish in incubator for 20–30 min.
Finally, spread the sample mix on petri dish and incubate overnight at 37°C.
Note: Strictly follow the incubation time and temperature in the protocol during cloning.
5.2.1.8 Two Dimensional poly acrylamide gel electrophoresis (2D PAGE)
2D PAGE is carried out to for the detection and to check the circularity of Viroid RNA. Following is the recipe and protocol for PAGE.
Gel Ingredients
Acrylamide (A)
Bisacrylamide (B)
40% AB in 50 ml distilled water @ 19:1 ratio
Non Denaturing Gel:
Ingredients
8% GEL
5% GEL
40% AB
6 ml
6.25 ml
10X TBE
3 ml
5 ml
dH2O
20.25 ml
37.7 8 ml
10% APS
750 μl
937.5 μl
TEMED
40 μl
43.75 μl
Total Volume
30 ml
50 ml
Mix the gel with magnetic bar.
Wash the glass with KOH and dH2O.
KOH washing buffer includes 10 g KOH + 10 ml dH2O + 90 ml and 99% ETOH.
Rinse the glass with dH2O and let it dry.
Prepare the gel and cast into electrophoresis set.
Let the gel to polymerase for 30 min.
Pre-run empty gel for 20 min at 10 mA.
Pre-run sample for 10 min at 10 mA and then run sample for 1 hr. plus at 20 mA.
5% Non-denaturing Gel
40% AB: 8.7 ml
Urea: 25.2 g
10XTBE: 5.25 ml
10% APS: 750 μl
TEMED: 45 μl
dH2O: 17.25 ml
Total volume: 52.5 ml
Fixer 1:
ETOH (10%, V/V)
10 ml
Acetic Acid (5%, V/V)
5 ml
dH2O
85 ml
Fixer 2:
ETOH (10%, V/V)
10 ml
Acetic Acid (5%, V/V)
0.5 ml
dH2O
89.5 ml
Silver Solution:
Silver Nitrate
0.3 g
dH2O
150 ml
Developer Solution:
3 mM NaBH4
0.023 g
Formaldehyde
0.75 ml
0.375 M NaOH
3 g
dH2O
200 ml
Silver Staining:
Fix the gel in fixer 1 for 10 min at room temperature in shaker.
Fix the gel in fixer 2 for 10 min at room temperature in shaker.
Dip the gel in silver stain solution for 1 hr. under dark condition.
Rinse with dH2O twice with the interval of 1 min.
Add developer solution in the end.
Stop developing by adding 5% acetic acid.
5.3 Citrus tristeza virus (Ctv): a case study
5.3.1 Introduction
CTV belongs to the genus Closterovirus of the family Clostervoiridae. Virus particle is a monopartite, positive sense, comprising of ssRNA genome of approximately 20Kb in size. It is the largest known form of a plant virus and its genome is encapsulated in a flexuous rod 2000 nm long particles composed of coat protein subunits of 25KDA [86, 87, 88, 89]. ssRNA genome comprised of 19,296 nucleotides that encode for 12 open reading frames [90]. CTV probably originated in Asia and has been spread to all citrus growing areas by infected plant material movement and now is widely distributed to all major citrus growing areas as summarized in Table 8. Over the two decades i.e. 1930–1950, millions of citrus trees were destroyed due to CTV infection and citrus orchards were almost wiped out in Brazil, Spain, and Argentina. This virus was the killer of three million citrus trees grafted on sour orange rootstock alone in south California [91, 92, 93, 94]. The tristeza disease was first reported in Florida in 1959 and by 1980s became the serious threat to citrus industry [95]. By 1991, an estimation of total world loss of 100 million trees was recorded due to CTV in Argentina, Brazil, Spain, California, Venezuela and other areas [96, 97]. Several strains of CTV have been identified primarily on the basis of their biological reaction in several citrus species and indicator plant. The major groups of strains are mild that cause barely detectable clearing of leaf veins in Mexican lime; decline–inducing strains cause death of trees when propagated on sour orange rootstock. Stem pitting strains cause mild to severe pitting of stems and branches of grapefruit and orange resulting in low yield [95, 98]. Almost all the citrus varieties and hybrids have been infected with CTV [91]. Symptom expression of CTV in citrus hosts is highly variable and depends upon host species (rootstock and scion combination), virulence of CTV isolates and soil or environmental conditions. Characteristics symptoms of CTV are vein clearing, decline, stem pitting, seedling yellows, stunting and leaf corking on different citrus hosts like sweet orange, grapefruit, grafted on sour range root stock. Severity of infection and symptoms expression on cultivars vary from mild to severe isolates [99, 100, 101]. CTV is transmitted in nature by different species of aphids in a semi-persistent manner and through grafting [102, 103]. The most efficient vector involved in semi-persistent manner is T. citricida Kirkaldy (brown or black citrus aphid) when compared with other aphids.
Regions
Countries
Status
EPPO
Israel, Spain, Turkey
Present
France
Found but not established
Algeria, Cyprus, Egypt, Italy, Morocco, Tunisia
Scattered infection
Asia
Brunei, China, Georgia
Present
India
Widespread
Indonesia. Iran, Japan
Present
Jordan
Unconfirmed
Korea, Malaysia, Nepal
Present
Pakistan
Present (Scarce Information available)
Philippines, KSA, Sri Lanka, Taiwan, Thailand, Viet Nam, Yemen
Antigua, Barbuda, Bahamas, Belize, Costa Rica, El Salvador, Guatemala, Honduras, Jamaica, Netherlands Antilles, Nicaragua, Puerto Rico, St. Lucia, Trinidad, Tobago
Present
Dominica
Unconfirmed
South America
Argentina, Bolivia, Brazil
Present (wide spread)
Chile
Found, not established
Colombia, Ecuador, Guyana, Peru, Paraguay, Suriname, Uruguay
Present
Oceania
American Samoa, Australia, Fiji, New Zealand
Present
Table 8.
Geographical Distribution of Citrus tristeza closterovirus.
Source: Anonymous, 2004.
5.3.2 Indexing
Serological and biological indexing: Indexing includes biological, serological and molecular methods, which are the common procedures according to their reliability, sensitivity and duration to detect the CTV. During a survey in Spain, 22 CTV isolates were collected on the basis of geographical information, source tree and symptomology and then were characterized by biological indexing. Diversified symptoms were produced on 9 indicator species. Mexican lime was found to be a good indicator host [104].
In Morocco, 14 diverse isolates were selected from samples during survey and then characterized on the basis of reaction pattern. Among these 14 isolates, four were severe and two were mild isolates. Isolates were also indexed against a series of monoclonal antibodies [105]. DAS-ELISA was used to detect the CTV from the samples collected during a survey in Western and Midwestern development regions of Nepal [106]. One hundred and eighty-eight samples were analyzed through biological indexing and DAS- ELISA to detect tristeza, psorosis and similar diseases like-symptoms including viroids in orange varieties in all the regions and the cachexia was detected as the most important and widespread disease [107]. Biological indexing is still considered as an important tool using for the characterization of CTV isolates. Different strains were identified through symptoms expression on differential hosts, including Mexican lime and sweet orange. Moreover, they observed visual symptoms of different strains on Mexican lime and sweet orange through biological indexing followed by ELISA [108]. Detection of CTV in Spain was compared by indexing using monoclonal and polyclonal antibodies [109].
Molecular indexing: Different nucleic acid based indexing methods have been developed for the quick detection of CTV. The adaptability of these methods depends upon the reliability, time duration and sensitivity. Alteration in protein patterns in rootstock bark from CTV infected tree were analyzed through PAGE [110]. There was a clear modification in protein pattern but not in CTV free trees. Similarly, Northern blot technique was used to compare dsDNAs extracted from CTV infected and CTV free plants. Two out of the three CTV isolates were detected by this method [111]. CTV was also detected in the three aphid species through RT-PCR. IC-RT-PCR was used to amplify the coat protein gene [112]. Sensitivity of cDNA probe was slightly better than hybridization with 32P-labeled probe. Similarly, hybridization with tissue print with DIG-probe could differentiate CTV isolates grown under green house or field conditions [113]. In Taiwan, RT-PCR was found to be a rapid and sensitive assay than other serological methods but one step RT-PCR, which is the combination of reverse transcriptase and polymerase chain reaction in one tube. It is more sensitive and detects the CTV when virus concentration is very low. Comparison between ELISA and RT-PCR revealed that ELISA was better than RT-PCR at detecting mild CTV strains as the virus was detected in all parishes, while RT-PCR detected CTV in only 8 parishes. It would appear that the primers used for RT-PCR are more specific for severe CTV isolates [114]. Some modifications were introduced in PCR-ELISA to increase its sensitivity and reduced the costs of detection. PCR-ELISA is the immune-detection of PCR products and effective for detection and differentiation of plant viral nucleic acids. PCR-ELISA being a laborious and expensive method was modified and simplified by using asymmetric PCR. It made PCR-ELISA more sensitive than TaqMAN™, a fluorescence-based detection method.
Three microscopy procedures for detecting CTV were compared which provided additional alternatives for very rapid CTV indexing, including the use of EM, SSEM and light microscopy. In light microscopy, inclusions were found in young phloem tissues of all CTV-infected hosts examined. Similarly, in SSEM virus particles were found on grids prepared with antiserum and extracts from infected tissue. CTV particles could be detected in pooled samples representing one in 100. Similarly, virus particle fragments were observed infrequently in samples representing one infected plant in 1,000 samples [32].
6. Conclusion
Citrus is an important fruit crop of the world and has a great potential for local consumption, export purposes and industrial uses. Unfortunately, citrus orchards are facing the problem of low productivity due to citrus decline. This is mainly attributed, among other factors to the prevalence of graft-transmissible virus and virus-like diseases, unhygienic nursery operations and poor orchard management. However, most of the problems arise from nurseries. It is the time that the nurseries should operate on highly technical and scientific lines and should work on providing disease-free and certified plants to the citrus growers. To establish the disease free nurseries, indexing of virus and virus-like diseases are the major area that needs to be focused. Implication of traditional and modern high-throughput biological, serological and molecular indexing techniques, such as ELISA, RT-PCR, PAGE, should be put in practice for the detection and indexing of virus and virus-like diseases of citrus plants. Moreover, citrus nurseries should be registered and indiscriminate multiplication and sale of uncertified citrus plants should be prohibited.
\n',keywords:"citrus, detection, diseases indexing, viruses and virus-like pathogens, graft-transmissible diseases, viroids, RT-PCR, ELISA",chapterPDFUrl:"https://cdn.intechopen.com/pdfs/75243.pdf",chapterXML:"https://mts.intechopen.com/source/xml/75243.xml",downloadPdfUrl:"/chapter/pdf-download/75243",previewPdfUrl:"/chapter/pdf-preview/75243",totalDownloads:263,totalViews:0,totalCrossrefCites:1,dateSubmitted:"October 1st 2020",dateReviewed:"January 8th 2021",datePrePublished:"April 26th 2021",datePublished:"November 3rd 2021",dateFinished:"February 13th 2021",readingETA:"0",abstract:"Citrus is a highly nutritive and prized fruit crop around the world. It contributes a substantial share in local consumption and exports of a nation to earn a handsome foreign exchange. The production of citrus is under the threat of citrus decline. Different factors are responsible for the citrus decline but virus and virus-like diseases have the major role in this decline. Virus and virus-like diseases alone or in association with other biotic and abiotic factors exist in the citrus orchards. Therefore, indexing of diseases caused by virus and virus-like pathogens is the key factor to manage these citrus diseases. Proper facilities and skilled personnel are the pre-requisite for the diseases indexing procedures. Biological, serological and molecular indexing is sensitive, reliable and durable strategy for managing different citrus virus and virus-like diseases under different conditions. Moreover, indexing of viruses and virus-like pathogens are very important for the production of disease free citrus nurseries. This chapter gives a brief review for the commonly used biological, serological and molecular assays for the detection of citrus virus and virus-like pathogens.",reviewType:"peer-reviewed",bibtexUrl:"/chapter/bibtex/75243",risUrl:"/chapter/ris/75243",signatures:"Yasir Iftikhar, Muhammad Zeeshan Majeed, Ganesan Vadamalai and Ashara Sajid",book:{id:"8108",type:"book",title:"Citrus",subtitle:"Research, Development and Biotechnology",fullTitle:"Citrus - Research, Development and Biotechnology",slug:"citrus-research-development-and-biotechnology",publishedDate:"November 3rd 2021",bookSignature:"Muhammad Sarwar Khan and Iqrar Ahmad Khan",coverURL:"https://cdn.intechopen.com/books/images_new/8108.jpg",licenceType:"CC BY 3.0",editedByType:"Edited by",isbn:"978-1-83968-724-2",printIsbn:"978-1-83968-723-5",pdfIsbn:"978-1-83968-725-9",isAvailableForWebshopOrdering:!0,editors:[{id:"212511",title:"Prof.",name:"Muhammad Sarwar",middleName:null,surname:"Khan",slug:"muhammad-sarwar-khan",fullName:"Muhammad Sarwar Khan"}],productType:{id:"1",title:"Edited Volume",chapterContentType:"chapter",authoredCaption:"Edited by"}},authors:[{id:"260766",title:"Dr.",name:"Muhammad Zeeshan",middleName:null,surname:"Majeed",fullName:"Muhammad Zeeshan Majeed",slug:"muhammad-zeeshan-majeed",email:"zeeshan.majeed@uos.edu.pk",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/260766/images/15456_n.jpg",institution:{name:"University of Sargodha",institutionURL:null,country:{name:"Pakistan"}}},{id:"333703",title:"Assistant Prof.",name:"Yasir",middleName:null,surname:"Iftikhar",fullName:"Yasir Iftikhar",slug:"yasir-iftikhar",email:"yasiriftikharpp@gmail.com",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",institution:{name:"University of Sargodha",institutionURL:null,country:{name:"Pakistan"}}},{id:"345159",title:"Dr.",name:"Ganesan",middleName:null,surname:"Vadamalai",fullName:"Ganesan Vadamalai",slug:"ganesan-vadamalai",email:"ganesanv@upm.edu.my",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",institution:{name:"Universiti Putra Malaysia",institutionURL:null,country:{name:"Malaysia"}}},{id:"345160",title:"Mrs.",name:"Ashara",middleName:null,surname:"Sajid",fullName:"Ashara Sajid",slug:"ashara-sajid",email:"phytodoctor123@gmail.com",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",institution:{name:"University of Sargodha",institutionURL:null,country:{name:"Pakistan"}}}],sections:[{id:"sec_1",title:"1. Introduction",level:"1"},{id:"sec_1_2",title:"1.1 Citrus pathology",level:"2"},{id:"sec_3",title:"2. Virus and virus-like diseases of citrus",level:"1"},{id:"sec_4",title:"3. Insects as vectors of virus and virus-like pathogens",level:"1"},{id:"sec_5",title:"4. Indexing strategies",level:"1"},{id:"sec_5_2",title:"4.1 Biological indexing",level:"2"},{id:"sec_6_2",title:"4.2 Serological assays",level:"2"},{id:"sec_7_2",title:"4.3 Molecular assays",level:"2"},{id:"sec_9",title:"5. Detection of citrus viroids",level:"1"},{id:"sec_9_2",title:"5.1 Pathogen description and characterization",level:"2"},{id:"sec_10_2",title:"5.2 Diagnostic methods for citrus viroids",level:"2"},{id:"sec_10_3",title:"Table 7.",level:"3"},{id:"sec_10_4",title:"5.2.1.1 Samples collection",level:"4"},{id:"sec_11_4",title:"5.2.1.2 Nucleic acid extraction",level:"4"},{id:"sec_12_4",title:"5.2.1.3 Synthesis of cDNA",level:"4"},{id:"sec_13_4",title:"Table 7.",level:"4"},{id:"sec_14_4",title:"5.2.1.5 Agarose gel electrophoresis",level:"4"},{id:"sec_15_4",title:"5.2.1.6 PCR product purification",level:"4"},{id:"sec_16_4",title:"5.2.1.7 Molecular Cloning (TOPO TA cloning kit, Invitrogen)",level:"4"},{id:"sec_17_4",title:"5.2.1.8 Two Dimensional poly acrylamide gel electrophoresis (2D PAGE)",level:"4"},{id:"sec_20_2",title:"5.3 Citrus tristeza virus (Ctv): a case study",level:"2"},{id:"sec_20_3",title:"Table 8.",level:"3"},{id:"sec_21_3",title:"5.3.2 Indexing",level:"3"},{id:"sec_24",title:"6. 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Detection of different strains of Potato virus Y and their mixed infections using competitive fluorescent RT–PCR. Journal of Virological Methods, 2001; 91: 167–173'},{id:"B42",body:'López, MM, Bertolini, E, Marco-Noales, E, Llop, P, Cambra, M. Update on molecular tools for detection of plant pathogenic bacteria and viruses. In Molecular diagnostics: current technology and applications, J.R. Rao, C.C. Fleming, and J.E. Moore, eds. Horizon Bioscience, Wymondham, UK, 2006: 1–46'},{id:"B43",body:'Rocha-Pena, MA, Lee, RF, Lastra, R, Niblett, CL, Ochoa-Corona, FM, Garnsey, SM, Yokomi, RK. Citrus tristeza virus and its aphid vector Toxoptera citricida: threats to citrus production in the carribean and central and North America. Plant Disease, 1995; 79(5): 437–445'},{id:"B44",body:'Ahlawat, YS. Viruses, greening bacterium and viroids associated with citrus (Citrus species) decline in India. Indian Journal of Agricultural Science, 1997; 67:51–57'},{id:"B45",body:'Bar-Joseph M, Marcus R, Lee RF. The continous challenges of citrus tristeza virus control. Annual Review of Phytopathology, 1989;27: 291–316'},{id:"B46",body:'Biswas, KK. Molecular diagnosis of Citrus tristeza virus in mandarin (Citrus reticulata) orchards of Darjeeling hills of West Bengal. Indian Journal of Virology, 2008; 19: 26–31'},{id:"B47",body:'López, MM, Llop, P, Olmos, A, Marco-Noales, E, Cambra, M, Bertolini, E. Are molecular tools solving the challenges posed by detection of plant pathogenic bacteria and viruses?. Current issues in molecular biology, 2009; 11(1): 13'},{id:"B48",body:'Lukhtanov, EA, Lokhov, SG, Gorn, VV, Podyminogin, MA, Mahoney, W. Novel DNA probes with low background and high hybridization-triggered fluorescence. Nucleic Acids Research, 2007; 35: 5 e30. doi:10.1093/nar/gkl1136'},{id:"B49",body:'Gasparic, MB, Cankar, K, Zel, J, and Gruden, K. Comparison of different real-time PCR chemistries and their suitability for detection and quantification of genetically modified organisms. BMC Biotechnology, 2008; doi:10.1186/1472-6750-8-26'},{id:"B50",body:'Korimbocus, J, Coates, D, Barker, I, and Boonham, N. Improved detection of Sugarcane yellow leaf virus using a real-time fluorescent (TaqMan) RT-PCR assay. Journal of Virological Methods, 2002; 103: 109–120'},{id:"B51",body:'Beuret, C. Simultaneous detection of enteric viruses by multiplex real-time RT-PCR. Journal of Virological Methods, 2004; 115: 1–8'},{id:"B52",body:'Munford, RA, Skelton, A, Metcalfe, E, Walsh, K, and Boonham, N. The reliable detection of Barley yellow and mild mosaic viruses using realtime PCR (TaqMan). Journal of Virological Methods, 2004; 117: 153–159'},{id:"B53",body:'Varga, A, and James, D. Use of reverse transcription loop-mediated isothermal amplification for the detection of Plum pox virus. Journal of Virological Methods, 2006; 138: 184–190'},{id:"B54",body:'Agindotan, BO, Shiel, PJ, and Berger, PH. Simultaneou detection of potato virus, PLRV, PVA, PVX and PVY from dormant potato tubers by TaqMan(®) real-time RT-PCR. Journal of Virological Methods, 2007; 142: 1–9'},{id:"B55",body:'Kogovsek, P, Gow, ., Pompe-Novak, M, Gruden, K, Foster, GD, Boonham, N, and Ravnikar, M. Single-step RT real-time PCR for sensitive detection and discrimination of Potato virus Y isolates. Journal of Virological Methods, 2008; 149: 1–11'},{id:"B56",body:'Agrios, G.N. (2005). Plant Pathology 5th Edition. Department of Plant Pathology, University of Florida.'},{id:"B57",body:'Hadidi, A., Flores, R., Randles, J.W., and Semancik, J.S. (2003). Viroids. Science Publisher, Inc.'},{id:"B58",body:'Bostan H, Nie X, Singh RP (2004). An RT-PCR primer pair for the detection of Pospiviroid and its application in surveying ornamental plants for viroids. J. Virol. Methods, 116: 189–193'},{id:"B59",body:'Bar-Joseph, M. (1996) A contribution to the natural history of viroids.Proc. 13th IOCV Conf. (Riverside, CA, USA), pp. 226–229'},{id:"B60",body:'Pagliano, G., Umaña, R., Pritsch, C., Rivas, F. and Duran-Vila, N. (2013). Occurrence, prevalence and distribution of citrus viroids in Uruguay. Journal of Plant Pathology. pp. 631-635'},{id:"B61",body:'Bani Hashemian, S.M., Taheri, H., Duran-Vila, N. and Serra, P. (2010). First Report of Citrus viroid V in Moro Blood Sweet Orange in Iran. Plant Disease: An International Journal of Applied Plant Pathology. pp. 129-129'},{id:"B62",body:'Semancik, J.S., Morris, T.J., Weathers, L.G., Rordorf, G.F., and Kearns, D.R. (1975). Physical properties of a minimal infectious RNA (viroid) associated with the exocortis disease. Virology 63: 160-167'},{id:"B63",body:'Duran-Vila, N., Pina, J.A., Ballester, J.F., Juarez, J., Roistacher, C.N., Rivera-Bustamante, R., and Semancik, J.S. (1988). The Citrus Exocortis Disease: A complex of viroid-RNAs. Tenth IOCV.'},{id:"B64",body:'Ashulin, L., Lachman, O., Hadas, R., and Bar-Joseph, M. (1991). Nucleotide sequence of a new viroid species, Citrus bent leaf viroid (CBLVd) isolated from grapefruit in Israel. Nucleic Acids Res'},{id:"B65",body:'Cao, M. J., Atta, S., Liu, Y. Q., Wang, X. F., Zhou, C. Y., Mustafa, A. and Iftikhar, Y. (2009). First report of Citrus bent leaf viroid and Citrus dwarfing viroid from citrus in Punjab, Pakistan. Plant Disease 2009 Vol. 93 No. 8 pp. 840'},{id:"B66",body:'Rakowski, A.G., Szychowski, J.A., Avena, Z.S. and Semancik, J.S. (1994). Nucleotide sequence and structural features of the group III citrus viroids. J Gen Virol 75:3581-3584'},{id:"B67",body:'Putcha, H., Ramm, K., Luckinger, R., Haddas, R., Bar-Joseph, M. and Sanger, H.L. (1991). Primary and secondary structure of citrus viroid IV, a new chimeric viroid present in dwarfed grapefruit in Israel. Nucleic Acids Res 19:6640'},{id:"B68",body:'Serra, P., Eiras, M., Bani-Hashemian, S. M., Murcia, N., Kitajima, E. W., Daròs, J. A., Flores, R., and Duran-Vila, N. (2008). Citrus viroid V: Occurrence, host range, diagnosis, and identification of new variants. Phytopathology 98:1199-1204'},{id:"B69",body:'Ito, T., Ieki, H. and Ozaki, K. (2002). Simultaneous detection of six citrus viroids and Apple stem grooving virus from citrus plants by multiplex reverse transcription polymerase chain reaction. Journal of Virological Methods 106, 235–239'},{id:"B70",body:'Srivastava, S., & Prasad, V. (2020). Viroids: small entities with a mean punch. In Applied Plant Virology (pp. 209–226). Academic Press'},{id:"B71",body:'Garnsey, S.M, Zies, D.L., Irey, M., Sieburth, J.S., Semancik, J.S., Levy, L. and Hilf, M.E. (2002). Practical field detection of citrus viroids in Florida by RT-PCR. Fifteenth IOCV Conference.'},{id:"B72",body:'Eiras, M., Silva, S.R., Stuchi, E.S., Carvalho, S.A., and Garcez, R.M. (2013). Identification and characterization of viroids in ‘Naveline ISA 315’ sweet orange. Tropical Plant Pathology, 38: 058–062'},{id:"B73",body:'Abubaker, M. Y. A., & Elhassan, S. M. (2010). Survey and molecular detection of two citrus viroids affecting commercial citrus orchards in the Northern part of Sudan. Agric. Biol. JN Am, 1(5), 930–937'},{id:"B74",body:'Pagliano, G., Peyrou, M., Campo, R.D., Orlando, L., Gravina, A., Wettstein, R., and Francis, M. (2000). Detection and characterization of citrus viroids in Uruguay. Fourteenth IOCV Conference.'},{id:"B75",body:'Nakahara, K., Hataya, T., Uyeda, I., and Ieki, H. (1998). An Improved Procedure for Extracting Nucleic Acids from Citrus Tissues for Diagnosis of Citrus Viroids. Ann. Phytopathol. Soc. Jpn. 64: 532–538'},{id:"B76",body:'Murcia, N., Serra, P., Olmos, A., and Duran-Vila, N. (2009). A novel hybridization approach for detection of citrus viroids. Molecular and Cellular Probes 23'},{id:"B77",body:'Schumacher, J., Randles, J.W., and Riesner, D. (1983). A two dimensional electrophoretic technique for detection of circular viroids and virusoids. Anal. Biochem. 135:288'},{id:"B78",body:'Nakaune, R. and Nakano, M. (2006). Efficient methods for sample processing and cDNA synthesis by RT-PCR for the detection of grapevine viruses and viroids. Journal of Virological Methods 134: 244–249'},{id:"B79",body:'Jiang, D., Hou, W., Kang, N., Qin, L., Wu, Z., Li, S., and Xie, L. (2012). Rapid detection and identification of viroids in the genus Coleviroid using a universal probe. Journal of Virological Methods.'},{id:"B80",body:'Kunta, M., Gracxa, J.V.D., and Skaria, M. (2007). Molecular Detection and Prevalence of Citrus Viroids in Texas. Hortscience 42(3):600–604'},{id:"B81",body:'Papayiannis, L.C. (2013). Diagnostic real-time RT-PCR for the simultaneous detection of Citrus exocortis viroid and Hop stunt viroid. Virological Methods 196: 93–99'},{id:"B82",body:'Targon, M.L.P.N., Carvalho, S.A.D., Stuchi, E.S., Souza, J.M., Muller, G.D. and Machado, K.M.B.M.A. (2005). Hybridization techniques for indexing of citrus viroids in Sao Paulo State, Brazil. LARANJA, Cordeiropolis: Volume 26, p25–38'},{id:"B83",body:'Narayanasamy, P. (2010). Microbial Plant Pathogens-Detection and Disease Diagnosis: Viral and Viroid Pathogens.Vol 3. Springer Science & Business Media.'},{id:"B84",body:'Ito, T., Ieki, H. and Ozaki, K. (2000). A population of variants of a viroid closely related to citrus viroid-I in citrus plants. Archives of Virology 145: 2105–2114'},{id:"B85",body:'Bernard, L., and Duran-Vila, N. (2006). A novel RT-PCR approach for detection and characterization of citrus viroids. Mollecular and Cellular Probes 20: 105–113'},{id:"B86",body:'Mehta P, Brlansky RH, Gowda S. Reverse Transcription Polymerase Chain Reaction Detection of Citrus Tristiza Virus in Aphids. Plant Disease, 1997; 81:1066–1069'},{id:"B87",body:'Mathews DM, Riley KR, Dodds JA. Comparison of detection methods for citrus tristeza virus in field trees during months of non-optimal titer. Plant Disease, 1997; 81: 525–529'},{id:"B88",body:'Niblett CL, Genc H, Cevik B, Halbert S, Brown I, Nolasco G, Bonacalza B, Manjunath KL, Febres VJ, Pappu HR, Lee RF. Progress on strain differentiation of citrus tristeza virus and its application to the epidemiology of citrus tristeza disease. Virus Research, 2000; 71:97–106'},{id:"B89",body:'Suastika G, Natsuaki T, Terui H, Kano T, Leki H, Okuda S. Nucleotide sequence of citrus tristeza virus seedlig yellows isolates. Journal of General Plant Pathology, 2001; 67: 73–77'},{id:"B90",body:'Bar-Joseph M, Lee RF. 1989. Citrus tristeza virus. AAB Descriptions of Plant Viruses no. 353. AAB, Wellesbourne (GB). http://www.ncbi.nlm.nih.gov/ICTVdb/ICTVdB/'},{id:"B91",body:'Anonymous. 2004. Citrus Tristeza Closterovirus. Data sheets on Quarantine pests. EPPO A2 list, No.93. www.eppo.org/QUARANTINE/virus/Citrus_tristeza/'},{id:"B92",body:'Bar-Joseph M, Marcus R, Lee RF. The continous challenges of citrus tristeza virus control. Annual Review of Phytopathology, 1989;27: 291–316'},{id:"B93",body:'Kallsen C. 2002. Controlling citrus tristeza virus in the San Joaquin valley of California. Citrus subtropical Horticulture/Pistachios. http://cekern.ucdavis.edu/Custom_Program143/Controlling_Citrus_Tristeza_Virus_in_the_SJ_Valley_of_California.htm'},{id:"B94",body:'Mooney P, Harty A. 1992. Citrus tristeza virus. The Orchardist. http://www.hortnet.co.nz/publications/science/kk0992.htm'},{id:"B95",body:'Futch SH, Brlansky RH. 2005. Field diagnosis of citrus tristeza virus. HS996, one of a series of the Horticultural services department, Florida cooperative extension service. IFAS, University of Florida, U.S.A. http://edis.ifas.ufl.edu'},{id:"B96",body:'Bar-Joseph M, Roistacher CN, Garnsey SM, Gumpf DJ. A review of tristeza, an ongoing threat to citriculture. In: Proceeding of International Society of Citriculture, Tokyo, Japan, 1981; 419–423'},{id:"B97",body:'Mooney P, Dawson T, Harty A. 1994. Citrus tristeza virus preimmunization strategies. The Orchadist. http://www.hortnet.co.nz/publications/science/kk0894.htm'},{id:"B98",body:'Chung KR, Brlansky RH. Citrus diseases exotic to Florida: Citrus Tristeza Virus-Stem Pitting (CTV-SP). Fact Sheet. pp 227. Plant Pathology Department, Florida Cooperative Extension Service, Institute of Food and Agricultural Sciences, University of Florida, 2006, Florida. http://edis.ifas.ufl.edu'},{id:"B99",body:'Brlansky RH, Damsteegt VD, Howd DS, Roy A. Molecular analysis of citrus tristeza virus subisolates separated by aphid transmission. Plant Disease, 2003;87:397–401'},{id:"B100",body:'EPPO Bulletin. Protocol for the diagnosis of quarantine organism, citrus tristeza closterovirus. 2004; 34: 239–246'},{id:"B101",body:'Lbida B, Bennani A, Serrhini MN, Zemzami M. Biological, serological and molecular characterization of three isolates of citrus tristeza closterovirus introduced into Morocco. OEPP/EPPO Bulletin 2005; 35:511–517'},{id:"B102",body:'Brown LG, Denmark HA, Yakomi RK. Citrus Tristeza Virus and its vectors. In; Florida. Plant Pathology circular no.311. Florida Department of Agriculture and Consumer Service. Division of Plant Industry. 1988'},{id:"B103",body:'Komazaki S. Biology and virus transmission of citrus aphid. Akitsu Branch, Fruit and Tree Research Station, Ministry of Agriculture, Forestry and Fisheries, Hiroshima, Japan, 1993. http://www.fftc.agnet.org/library/tb/136/'},{id:"B104",body:'Ballester OJF, Pina JA, Carbonell EA, Moreno P, Hermoso de Mandoza A, Cambra M, Navarro L. Biological diversity of citrus tristeza virus (CTV) isolates in Spain. Plant Pathology, 1993;42:219–229'},{id:"B105",body:'Zemzami M, Garnsey SM, Nadori EB, Hill JH. Biological and serological characterization of citrus tristeza virus (CTV) isolates from Morocco. Phytopathologia-Mediterranea, 1999; 38: 95–100'},{id:"B106",body:'Malla S, Sah DN. Severity and prevalence of citrus tristeza virus (CTV) in the western and Mid-Western regions of Nepal. Working paper lumle Agricultral Research Centre, 2001; 14'},{id:"B107",body:'Besoain XA, Valenzuela M, Castro M, Ballester Olmos JF. Current status of some virus and virus like diseases of citrus in Chile. Fitopatologia. 2000;35: 98–104'},{id:"B108",body:'Polek M, Gumpf DJ, C. M. Wallen CM, Riley KM. Biological Characterization of Naturally Occurring Citrus tristeza virus Strains in California Citrus. In: In: M.E. Hilf, N. Duran-Vila and M.A. Rocha-Pena (Eds.), Proceeding of the 16th International Organization of Citrus Virologist Conference, California, Riverside, 2005, USA:68–74'},{id:"B109",body:'Cambra M, Serra J, Bonet JC, Moreno P. Present status of the citrus tristeza virus in the valencian community. In: L. W. Timmer, S. M. Garnsey and L. Navarro. (Eds), Proceeding of 10th International Organization of Citrus Virologists, California Riverside, 1998; 1–7'},{id:"B110",body:'Moreno, P., J. Guerri and J. Ortiz. Alteration of bark proteins associated with citrus tristeza virus (CTV) infection on susceptible citrus species and scion-rootstock combinations. Phytopathology, 1989; 125:55–66'},{id:"B111",body:'Acikgoz S. Detection of citrus tristeza virus (CTV) isolates with northern blot hybridization. Doga Turk Tarim-ve-Ormancilik Dergisi, 1991;15:836–840'},{id:"B112",body:'Anfoka GH, Abhary MK, Fattash I, Nakhla MK. Occurrence and distribution of citrus tristeza virus in the Jordan valley. Phytopathologia Mediterranea, 2007;44:17–23'},{id:"B113",body:'Narvaez G, Skander BS, Ayllon MA, Rubio L, Guerri J, Moreno P. A new procedure to differentiate citrus tristeza virus isolates by hybridization with digoxigenin-labelled cDNA probes. Journal of Virological Methods, 2000; 85: 83–92'},{id:"B114",body:'Fisher L, Tennant P, Molaughlin W. 2005. Detection and differentiation of Citrus Tristiza Virus (CTV) in Jamaica using ELISA, RT-PCR, DNA hybridization and RFLP. Ministry of Agriculture’s citrus replanting project-research services. Conference, The Environment: Biodiversity, O-23, Faculty of Pure and Applied Sciences, University of West Indies. www.mona.uwi.edu/fpas/conference/fpas7'}],footnotes:[],contributors:[{corresp:"yes",contributorFullName:"Yasir Iftikhar",address:"yasir.iftikhar@uos.edu.pk",affiliation:'
Department of Plant Pathology, College of Agriculture, University of Sargodha, Pakistan
Department of Plant Pathology, College of Agriculture, University of Sargodha, Pakistan
'}],corrections:null},book:{id:"8108",type:"book",title:"Citrus",subtitle:"Research, Development and Biotechnology",fullTitle:"Citrus - Research, Development and Biotechnology",slug:"citrus-research-development-and-biotechnology",publishedDate:"November 3rd 2021",bookSignature:"Muhammad Sarwar Khan and Iqrar Ahmad Khan",coverURL:"https://cdn.intechopen.com/books/images_new/8108.jpg",licenceType:"CC BY 3.0",editedByType:"Edited by",isbn:"978-1-83968-724-2",printIsbn:"978-1-83968-723-5",pdfIsbn:"978-1-83968-725-9",isAvailableForWebshopOrdering:!0,editors:[{id:"212511",title:"Prof.",name:"Muhammad Sarwar",middleName:null,surname:"Khan",slug:"muhammad-sarwar-khan",fullName:"Muhammad Sarwar Khan"}],productType:{id:"1",title:"Edited Volume",chapterContentType:"chapter",authoredCaption:"Edited by"}}},profile:{item:{id:"159998",title:"Dr.",name:"Arnis",middleName:null,surname:"Abolins",email:"Arnis.Abolins@rsu.lv",fullName:"Arnis Abolins",slug:"arnis-abolins",position:null,biography:null,institutionString:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",totalCites:0,totalChapterViews:"0",outsideEditionCount:0,totalAuthoredChapters:"5",totalEditedBooks:"0",personalWebsiteURL:null,twitterURL:null,linkedinURL:null,institution:null},booksEdited:[],chaptersAuthored:[{id:"40425",title:"Primary and Metastatic Tumours of the Liver: Expanding Scope of Morphological and Immunohistochemical Details in the Biopsy",slug:"primary-and-metastatic-tumours-of-the-liver-expanding-scope-of-morphological-and-immunohistochemical",abstract:null,signatures:"Ilze Strumfa, Janis Vilmanis, Andrejs Vanags, Ervins Vasko, Dzeina Sulte, Zane Simtniece, Arnis Abolins and Janis Gardovskis",authors:[{id:"54021",title:"Prof.",name:"Ilze",surname:"Strumfa",fullName:"Ilze Strumfa",slug:"ilze-strumfa",email:"ilze.strumfa@rsu.lv"},{id:"159993",title:"Dr.",name:"Janis",surname:"Vilmanis",fullName:"Janis Vilmanis",slug:"janis-vilmanis",email:"Janis.Vilmanis@rsu.lv"},{id:"159994",title:"Dr.",name:"Andrejs",surname:"Vanags",fullName:"Andrejs Vanags",slug:"andrejs-vanags",email:"vanags314@inbox.lv"},{id:"159996",title:"Dr.",name:"Zane",surname:"Simtniece",fullName:"Zane Simtniece",slug:"zane-simtniece",email:"Zane.Simtniece@rsu.lv"},{id:"159997",title:"Dr.",name:"Dzeina",surname:"Sulte",fullName:"Dzeina Sulte",slug:"dzeina-sulte",email:"ilzestrumfa@yahoo.co.uk"},{id:"159998",title:"Dr.",name:"Arnis",surname:"Abolins",fullName:"Arnis Abolins",slug:"arnis-abolins",email:"Arnis.Abolins@rsu.lv"},{id:"160000",title:"Prof.",name:"Janis",surname:"Gardovskis",fullName:"Janis Gardovskis",slug:"janis-gardovskis",email:"Janis.Gardovskis@rsu.lv"},{id:"165981",title:"Dr.",name:"Ervins",surname:"Vasko",fullName:"Ervins Vasko",slug:"ervins-vasko",email:"ervinsvasko@gmail.com"}],book:{id:"3329",title:"Liver Biopsy",slug:"liver-biopsy-indications-procedures-results",productType:{id:"1",title:"Edited Volume"}}},{id:"56232",title:"Systemic Inflammatory Reaction in Gastric Cancer: Biology and Practical Implications of Neutrophil to Lymphocyte Ratio, Glasgow Prognostic Score and Related Parameters",slug:"systemic-inflammatory-reaction-in-gastric-cancer-biology-and-practical-implications-of-neutrophil-to",abstract:"Gastric cancer induces systemic inflammatory reaction (SIR) manifesting with changes in counts of white blood cell fractions and concentrations of acute phase proteins, clotting factors and albumins. Thus, protein-based scores or blood cell ratios (neutrophil to lymphocyte ratio (NLR); platelet to lymphocyte ratio (PLR)) are used to evaluate SIR. SIR tests are biologically justified by multiple clinically important and fascinating events including bone marrow activation, development of immune-suppressing immature myeloid cells, generation of pre-metastatic niches and neutrophil extracellular trap formation from externalised DNA network in bidirectional association with platelet activation. Despite biological complexity, clinical SIR assessment is widely available, patient-friendly and economically feasible. Here we present concise review on NLR, PLR, Glasgow prognostic score and fibrinogen – parameters that have prognostic role regarding overall, cancer-free and cancer-specific survival in early and advanced cases. Tumour burden can be predicted helping in preoperative detection of serosal or lymph node involvement. Practical consequences abound, including selection of surgical approach in respect to tumour burden, adjustments in treatment intensity by prognosis or evaluation of chemotherapy response. The chapter also scrutinises main controversies including different cut-off levels. Future developments should include elaboration of complex scores as described here. SIR parameters should be wisely incorporated in patients’ treatment.",signatures:"Ilze Strumfa, Tatjana Bogdanova, Arturs Kalva, Boriss Strumfs,\nRoberts Rumba, Andrejs Vanags, Inese Drike, Dzeina Mezale, Arnis\nAbolins, Arvids Jakovlevs, Dainis Balodis and Janis Gardovskis",authors:[{id:"54021",title:"Prof.",name:"Ilze",surname:"Strumfa",fullName:"Ilze Strumfa",slug:"ilze-strumfa",email:"ilze.strumfa@rsu.lv"},{id:"159998",title:"Dr.",name:"Arnis",surname:"Abolins",fullName:"Arnis Abolins",slug:"arnis-abolins",email:"Arnis.Abolins@rsu.lv"},{id:"174929",title:"Dr.",name:"Andrejs",surname:"Vanags",fullName:"Andrejs Vanags",slug:"andrejs-vanags",email:"Andrejs.Vanags@rsu.lv"},{id:"202249",title:"Dr.",name:"Tatjana",surname:"Bogdanova",fullName:"Tatjana Bogdanova",slug:"tatjana-bogdanova",email:"Tatjana.Bogdanova@rsu.lv"},{id:"202250",title:"Dr.",name:"Roberts",surname:"Rumba",fullName:"Roberts Rumba",slug:"roberts-rumba",email:"Roberts.Rumba@rsu.lv"},{id:"202251",title:"Dr.",name:"Inese",surname:"Drike",fullName:"Inese Drike",slug:"inese-drike",email:"Inese.Drike@rsu.lv"},{id:"202252",title:"Dr.",name:"Arvids",surname:"Jakovlevs",fullName:"Arvids Jakovlevs",slug:"arvids-jakovlevs",email:"Arvids.Jakovlevs@rsu.lv"},{id:"202253",title:"Dr.",name:"Dainis",surname:"Balodis",fullName:"Dainis Balodis",slug:"dainis-balodis",email:"Dainis.Balodis@rsu.lv"},{id:"202548",title:"Dr.",name:"Dzeina",surname:"Mezale",fullName:"Dzeina Mezale",slug:"dzeina-mezale",email:"Dzeina.Mezale@rsu.lv"},{id:"205692",title:"MSc.",name:"Boriss",surname:"Strumfs",fullName:"Boriss Strumfs",slug:"boriss-strumfs",email:"boriss@osi.lv"}],book:{id:"5881",title:"Gastric Cancer",slug:"gastric-cancer",productType:{id:"1",title:"Edited Volume"}}},{id:"61254",title:"Diagnostic Algorithm of Hepatocellular Carcinoma: Classics and Innovations in Radiology and Pathology",slug:"diagnostic-algorithm-of-hepatocellular-carcinoma-classics-and-innovations-in-radiology-and-pathology",abstract:"In the global cancer statistics, hepatocellular carcinoma (HCC) ranges sixth by incidence and second by oncological mortality. The risk factors comprise hepatitis B and C virus infection, non-alcoholic steatohepatitis, as well as long-lasting peroral exposure to alcohol or aflatoxins. Liver cirrhosis is the most important single predisposing factor. Ultrasonography once per 6 months is recommended for surveillance in cirrhotic patients. Computed tomography (CT) and magnetic resonance imaging (MRI) represent the gold standard of non-invasive diagnostics while core biopsy and/or immunohistochemistry (IHC) are indicated for controversial and non-cirrhotic HCC cases. Molecular classification is under development. At present, classics of HCC diagnostics is based on evaluation of risk factors, surveillance in cirrhotic patients, preference for CT or MRI-confirmed non-invasive diagnosis and biopsy proof in equivocal cases. Diffusion-weighted imaging and hepatobiliary phase contrasting represent significant recent developments in MRI. Contrast-enhanced ultrasonography is recommended by some but not all guidelines. Positron emission tomography is advocated before liver transplantation to detect extrahepatic metastases but has limited role in the initial diagnostic evaluation of liver nodule. Innovations are expected in the field of molecular diagnostics, including IHC panels and novel antigens, e.g. clathrin and bile salt export pump protein, and development of molecular classification.",signatures:"Dzeina Mezale, Ilze Strumfa, Andrejs Vanags, Arturs Kalva, Dainis\nBalodis, Boriss Strumfs, Ilze Fridrihsone, Arnis Abolins and Janis\nGardovskis",authors:[{id:"54021",title:"Prof.",name:"Ilze",surname:"Strumfa",fullName:"Ilze Strumfa",slug:"ilze-strumfa",email:"ilze.strumfa@rsu.lv"},{id:"159998",title:"Dr.",name:"Arnis",surname:"Abolins",fullName:"Arnis Abolins",slug:"arnis-abolins",email:"Arnis.Abolins@rsu.lv"},{id:"160000",title:"Prof.",name:"Janis",surname:"Gardovskis",fullName:"Janis Gardovskis",slug:"janis-gardovskis",email:"Janis.Gardovskis@rsu.lv"},{id:"174929",title:"Dr.",name:"Andrejs",surname:"Vanags",fullName:"Andrejs Vanags",slug:"andrejs-vanags",email:"Andrejs.Vanags@rsu.lv"},{id:"202253",title:"Dr.",name:"Dainis",surname:"Balodis",fullName:"Dainis Balodis",slug:"dainis-balodis",email:"Dainis.Balodis@rsu.lv"},{id:"202548",title:"Dr.",name:"Dzeina",surname:"Mezale",fullName:"Dzeina Mezale",slug:"dzeina-mezale",email:"Dzeina.Mezale@rsu.lv"},{id:"205692",title:"MSc.",name:"Boriss",surname:"Strumfs",fullName:"Boriss Strumfs",slug:"boriss-strumfs",email:"boriss@osi.lv"},{id:"203012",title:"Dr.",name:"Ilze",surname:"Fridrihsone",fullName:"Ilze Fridrihsone",slug:"ilze-fridrihsone",email:"Ilze.Fridrihsone@rsu.lv"},{id:"215127",title:"Dr.",name:"Arturs",surname:"Kalva",fullName:"Arturs Kalva",slug:"arturs-kalva",email:"Arturs.Kalva@rsu.lv"}],book:{id:"6341",title:"Hepatocellular Carcinoma",slug:"hepatocellular-carcinoma-advances-in-diagnosis-and-treatment",productType:{id:"1",title:"Edited Volume"}}},{id:"62764",title:"Thyroid Nodules in Diagnostic Pathology: From Classic Concepts to Innovations",slug:"thyroid-nodules-in-diagnostic-pathology-from-classic-concepts-to-innovations",abstract:"Thyroid nodules are frequent in general population, found in 3.7–7% of people by palpation and 42–67% by ultrasonography (US). The differential diagnosis ranges from papillary (PC), follicular (FC) and medullary (MC) carcinomas to follicular adenoma (FA) and colloid goitre. Cancer risk in thyroid nodules varies: 5% in masses found by palpation, 1.6–15% by US, 3.9–11.3% by computed tomography (CT), 5–6% by magnetic resonance imaging (MRI) and 30–50% by positron emission tomography (PET). The final diagnosis depends on fine needle aspiration (FNA) findings and histopathology. The recent WHO classification (2017) is based on classic morphology, including assessment of invasion and nuclei. New entities are defined to designate tumours with doubtful invasion or controversial nuclear features. By immunohistochemistry, PC expresses HBME-1, TROP-2, CITED1 and CK19. Notably, PC can stain for CD20. MC is recognised by neuroendocrine differentiation. To distinguish FA vs. FC, evaluation of HBME-1, p27 and galectin has been suggested. Regarding miRNAs, miR-146b, miR-222, miR-221 and miR-181b are upregulated, while miR-145, miR-451, miR-613 and miR-137 are downregulated in PC. FC features downregulated miR-199a-5p and upregulated miR-197 and miR-346. In MC, miR-21 and miR-129-5p are downregulated. In addition, increased systemic inflammatory reaction can be poor prognostic factor in thyroid cancer. The aim of this chapter is to review classic and innovative histopathology of thyroid nodules for diagnostic pathology practice and research in multidisciplinary thyroid teams.",signatures:"Ilze Fridrihsone, Ilze Strumfa, Boriss Strumfs, Andrejs Vanags, Dainis\nBalodis, Arvids Jakovlevs, Arnis Abolins and Janis Gardovskis",authors:[{id:"54021",title:"Prof.",name:"Ilze",surname:"Strumfa",fullName:"Ilze Strumfa",slug:"ilze-strumfa",email:"ilze.strumfa@rsu.lv"},{id:"159998",title:"Dr.",name:"Arnis",surname:"Abolins",fullName:"Arnis Abolins",slug:"arnis-abolins",email:"Arnis.Abolins@rsu.lv"},{id:"160000",title:"Prof.",name:"Janis",surname:"Gardovskis",fullName:"Janis Gardovskis",slug:"janis-gardovskis",email:"Janis.Gardovskis@rsu.lv"},{id:"174929",title:"Dr.",name:"Andrejs",surname:"Vanags",fullName:"Andrejs Vanags",slug:"andrejs-vanags",email:"Andrejs.Vanags@rsu.lv"},{id:"202252",title:"Dr.",name:"Arvids",surname:"Jakovlevs",fullName:"Arvids Jakovlevs",slug:"arvids-jakovlevs",email:"Arvids.Jakovlevs@rsu.lv"},{id:"202253",title:"Dr.",name:"Dainis",surname:"Balodis",fullName:"Dainis Balodis",slug:"dainis-balodis",email:"Dainis.Balodis@rsu.lv"},{id:"205692",title:"MSc.",name:"Boriss",surname:"Strumfs",fullName:"Boriss Strumfs",slug:"boriss-strumfs",email:"boriss@osi.lv"},{id:"203012",title:"Dr.",name:"Ilze",surname:"Fridrihsone",fullName:"Ilze Fridrihsone",slug:"ilze-fridrihsone",email:"Ilze.Fridrihsone@rsu.lv"}],book:{id:"6297",title:"Histopathology",slug:"histopathology-an-update",productType:{id:"1",title:"Edited Volume"}}},{id:"62790",title:"Innovative Blood Tests for Hepatocellular Carcinoma: Liquid Biopsy and Evaluation of Systemic Inflammatory Reaction",slug:"innovative-blood-tests-for-hepatocellular-carcinoma-liquid-biopsy-and-evaluation-of-systemic-inflamm",abstract:"Hepatocellular carcinoma (HCC) is an aggressive tumour associated with dismal prognosis. To improve the outcome, early diagnostics is important. At present, classical HCC diagnostics is based on evaluation of risk factors, surveillance in cirrhotic patients, preference for non-invasive diagnosis by computed tomography or magnetic resonance imaging and biopsy confirmation in controversial cases. However, ambiguous radiological presentation, biopsy-related complications or insufficient representation of the pathology in the tissue core are well-known problems. Panel assessment of microRNAs has diagnostic and prognostic value; thus, in future, microRNA-based liquid biopsy could partially reduce the need for core biopsies. Systemic inflammatory reaction (SIR), characterised mainly by neutrophil-to-lymphocyte ratio, platelet-to-lymphocyte ratio and Glasgow prognostic score, may have prognostic value and can be incorporated in criteria for certain treatment approaches, e.g., becoming an adjunct to Milan criteria. Thus, innovations in HCC diagnostics are expected in the field of miRNA-based liquid biopsy for diagnosis/prognosis and SIR for prognosis/selection of treatment.",signatures:"Ilze Strumfa, Dzeina Mezale, Boriss Strumfs, Andrejs Vanags, Arturs\nKalva, Dainis Balodis, Ilze Fridrihsone, Arnis Abolins and Janis\nGardovskis",authors:[{id:"54021",title:"Prof.",name:"Ilze",surname:"Strumfa",fullName:"Ilze Strumfa",slug:"ilze-strumfa",email:"ilze.strumfa@rsu.lv"},{id:"159998",title:"Dr.",name:"Arnis",surname:"Abolins",fullName:"Arnis Abolins",slug:"arnis-abolins",email:"Arnis.Abolins@rsu.lv"},{id:"160000",title:"Prof.",name:"Janis",surname:"Gardovskis",fullName:"Janis Gardovskis",slug:"janis-gardovskis",email:"Janis.Gardovskis@rsu.lv"},{id:"174929",title:"Dr.",name:"Andrejs",surname:"Vanags",fullName:"Andrejs Vanags",slug:"andrejs-vanags",email:"Andrejs.Vanags@rsu.lv"},{id:"202253",title:"Dr.",name:"Dainis",surname:"Balodis",fullName:"Dainis Balodis",slug:"dainis-balodis",email:"Dainis.Balodis@rsu.lv"},{id:"202548",title:"Dr.",name:"Dzeina",surname:"Mezale",fullName:"Dzeina Mezale",slug:"dzeina-mezale",email:"Dzeina.Mezale@rsu.lv"},{id:"205692",title:"MSc.",name:"Boriss",surname:"Strumfs",fullName:"Boriss Strumfs",slug:"boriss-strumfs",email:"boriss@osi.lv"},{id:"203012",title:"Dr.",name:"Ilze",surname:"Fridrihsone",fullName:"Ilze Fridrihsone",slug:"ilze-fridrihsone",email:"Ilze.Fridrihsone@rsu.lv"},{id:"215127",title:"Dr.",name:"Arturs",surname:"Kalva",fullName:"Arturs Kalva",slug:"arturs-kalva",email:"Arturs.Kalva@rsu.lv"}],book:{id:"6341",title:"Hepatocellular Carcinoma",slug:"hepatocellular-carcinoma-advances-in-diagnosis-and-treatment",productType:{id:"1",title:"Edited Volume"}}}],collaborators:[{id:"37764",title:"Dr",name:"Teresa",surname:"Casanovas",slug:"teresa-casanovas",fullName:"Teresa Casanovas",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"53975",title:"Prof.",name:"Ludmila",surname:"Viksna",slug:"ludmila-viksna",fullName:"Ludmila Viksna",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"54021",title:"Prof.",name:"Ilze",surname:"Strumfa",slug:"ilze-strumfa",fullName:"Ilze Strumfa",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/54021/images/system/54021.jpg",biography:'Professor Ilze Strumfa, MD, Ph.D., is an outstanding medical lecturer, actively involved in the research in pathology. She graduated from the Medical Academy of Latvia with distinction in 1998, underwent board certification in pathology in 2001, and received a Ph.D. in 2005. Currently, she is a professor and head of the Department of Pathology, Riga Stradins University (RSU), Latvia. Her twelve years of teaching experience have culminated with the RSU \\"Lecturer of the Year\\" Annual Award (2018), given to the most distinguished teachers. As the head of the Department of Pathology, she is leading a skilled, motivated team of teachers and scientists that have won awards such as Best Academic Unit (2011), Best Ph.D. Student (2012), and Best Digital Junior Teacher (2016). Prof. Strumfa is an author/co-author of more than 100 peer-reviewed journal articles and 16 chapters in scientific monographs and medical textbooks. She has been acting as the leading expert in several European and national research projects devoted to the development of diagnostic technologies, neuroendocrine and endocrine tumors, breast cancer, laboratory training in research, and tumor microenvironment. Her main research interests include morphological and molecular diagnostics and prognostic assessment of tumors as well as digital pathology and other innovations in pathology and cytology.',institutionString:"Riga Stradiņš University",institution:{name:"Riga Stradiņš University",institutionURL:null,country:{name:"Latvia"}}},{id:"57834",title:"Dr.",name:"Ivan",surname:"Tokin",slug:"ivan-tokin",fullName:"Ivan Tokin",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"159993",title:"Dr.",name:"Janis",surname:"Vilmanis",slug:"janis-vilmanis",fullName:"Janis Vilmanis",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"159994",title:"Dr.",name:"Andrejs",surname:"Vanags",slug:"andrejs-vanags",fullName:"Andrejs Vanags",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"159996",title:"Dr.",name:"Zane",surname:"Simtniece",slug:"zane-simtniece",fullName:"Zane Simtniece",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"159997",title:"Dr.",name:"Dzeina",surname:"Sulte",slug:"dzeina-sulte",fullName:"Dzeina Sulte",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"160000",title:"Prof.",name:"Janis",surname:"Gardovskis",slug:"janis-gardovskis",fullName:"Janis Gardovskis",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/160000/images/7691_n.png",biography:"Professor habilitated medical doctor Janis Gardovskis integrates outstanding academic and research activity with the tasks of practicing surgeon. He assumes the positions of the Head of the Department of Surgery at Riga Stradiņš University and Head of the Surgical Clinics in Pauls Stradins Clinical University Hospital. Professor Janis Gardovskis is an Actual Member of the Latvian Academy of Sciences and member of the Latvian Association of Surgeons. He has received fellowships in surgery in Denmark, Lithuania, Finland, Sweden, and Germany. The scientific preferences of professor Janis Gardovskis include videosurgery, pancreatic surgery, oncologic surgery, transplantation, hereditary cancers and life quality in surgical patients. J.Gardovskis has participated in many international and local scientific projects and clinical trials. He has authored/ co-authored 5 monographs, 12 book chapters, and 44 scientific publications in international citation databases (Scopus, PubMed) as well as numerous other papers. In addition, 18 doctoral dissertations have been defended under his supervision. As an eminent specialist in surgery with a strong focus on future development, Professor Janis Gardovskis has a genuine interest and expert skills in the evaluation of next-generation diagnostic methods to meet the clinical needs.",institutionString:null,institution:null},{id:"165981",title:"Dr.",name:"Ervins",surname:"Vasko",slug:"ervins-vasko",fullName:"Ervins Vasko",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null}]},generic:{page:{slug:"our-story",title:"Our story",intro:"
The company was founded in Vienna in 2004 by Alex Lazinica and Vedran Kordic, two PhD students researching robotics. While completing our PhDs, we found it difficult to access the research we needed. So, we decided to create a new Open Access publisher. A better one, where researchers like us could find the information they needed easily. The result is IntechOpen, an Open Access publisher that puts the academic needs of the researchers before the business interests of publishers.
",metaTitle:"Our story",metaDescription:"The company was founded in Vienna in 2004 by Alex Lazinica and Vedran Kordic, two PhD students researching robotics. While completing our PhDs, we found it difficult to access the research we needed. So, we decided to create a new Open Access publisher. A better one, where researchers like us could find the information they needed easily. The result is IntechOpen, an Open Access publisher that puts the academic needs of the researchers before the business interests of publishers.",metaKeywords:null,canonicalURL:"/page/our-story",contentRaw:'[{"type":"htmlEditorComponent","content":"
We started by publishing journals and books from the fields of science we were most familiar with - AI, robotics, manufacturing and operations research. Through our growing network of institutions and authors, we soon expanded into related fields like environmental engineering, nanotechnology, computer science, renewable energy and electrical engineering, Today, we are the world’s largest Open Access publisher of scientific research, with over 4,200 books and 54,000 scientific works including peer-reviewed content from more than 116,000 scientists spanning 161 countries. Our authors range from globally-renowned Nobel Prize winners to up-and-coming researchers at the cutting edge of scientific discovery.
\\n\\n
In the same year that IntechOpen was founded, we launched what was at the time the first ever Open Access, peer-reviewed journal in its field: the International Journal of Advanced Robotic Systems (IJARS).
\\n\\n
The IntechOpen timeline
\\n\\n
2004
\\n\\n
\\n\\t
Intech Open is founded in Vienna, Austria, by Alex Lazinica and Vedran Kordic, two PhD students, and their first Open Access journals and books are published.
\\n\\t
Alex and Vedran launch the first Open Access, peer-reviewed robotics journal and IntechOpen’s flagship publication, the International Journal of Advanced Robotic Systems (IJARS).
\\n
\\n\\n
2005
\\n\\n
\\n\\t
IntechOpen publishes its first Open Access book: Cutting Edge Robotics.
\\n
\\n\\n
2006
\\n\\n
\\n\\t
IntechOpen publishes a special issue of IJARS, featuring contributions from NASA scientists regarding the Mars Exploration Rover missions.
\\n
\\n\\n
2008
\\n\\n
\\n\\t
Downloads milestone: 200,000 downloads reached
\\n
\\n\\n
2009
\\n\\n
\\n\\t
Publishing milestone: the first 100 Open Access STM books are published
\\n
\\n\\n
2010
\\n\\n
\\n\\t
Downloads milestone: one million downloads reached
\\n\\t
IntechOpen expands its book publishing into a new field: medicine.
\\n
\\n\\n
2011
\\n\\n
\\n\\t
Publishing milestone: More than five million downloads reached
\\n\\t
IntechOpen publishes 1996 Nobel Prize in Chemistry winner Harold W. Kroto’s “Strategies to Successfully Cross-Link Carbon Nanotubes”. Find it here.
\\n\\t
IntechOpen and TBI collaborate on a project to explore the changing needs of researchers and the evolving ways that they discover, publish and exchange information. The result is the survey “Author Attitudes Towards Open Access Publishing: A Market Research Program”.
\\n\\t
IntechOpen hosts SHOW - Share Open Access Worldwide; a series of lectures, debates, round-tables and events to bring people together in discussion of open source principles, intellectual property, content licensing innovations, remixed and shared culture and free knowledge.
\\n
\\n\\n
2012
\\n\\n
\\n\\t
Publishing milestone: 10 million downloads reached
\\n\\t
IntechOpen holds Interact2012, a free series of workshops held by figureheads of the scientific community including Professor Hiroshi Ishiguro, director of the Intelligent Robotics Laboratory, who took the audience through some of the most impressive human-robot interactions observed in his lab.
\\n
\\n\\n
2013
\\n\\n
\\n\\t
IntechOpen joins the Committee on Publication Ethics (COPE) as part of a commitment to guaranteeing the highest standards of publishing.
\\n
\\n\\n
2014
\\n\\n
\\n\\t
IntechOpen turns 10, with more than 30 million downloads to date.
\\n\\t
IntechOpen appoints its first Regional Representatives - members of the team situated around the world dedicated to increasing the visibility of our authors’ published work within their local scientific communities.
\\n
\\n\\n
2015
\\n\\n
\\n\\t
Downloads milestone: More than 70 million downloads reached, more than doubling since the previous year.
\\n\\t
Publishing milestone: IntechOpen publishes its 2,500th book and 40,000th Open Access chapter, reaching 20,000 citations in Thomson Reuters ISI Web of Science.
\\n\\t
40 IntechOpen authors are included in the top one per cent of the world’s most-cited researchers.
\\n\\t
Thomson Reuters’ ISI Web of Science Book Citation Index begins indexing IntechOpen’s books in its database.
\\n
\\n\\n
2016
\\n\\n
\\n\\t
IntechOpen is identified as a world leader in Simba Information’s Open Access Book Publishing 2016-2020 report and forecast. IntechOpen came in as the world’s largest Open Access book publisher by title count.
\\n
\\n\\n
2017
\\n\\n
\\n\\t
Downloads milestone: IntechOpen reaches more than 100 million downloads
\\n\\t
Publishing milestone: IntechOpen publishes its 3,000th Open Access book, making it the largest Open Access book collection in the world
We started by publishing journals and books from the fields of science we were most familiar with - AI, robotics, manufacturing and operations research. Through our growing network of institutions and authors, we soon expanded into related fields like environmental engineering, nanotechnology, computer science, renewable energy and electrical engineering, Today, we are the world’s largest Open Access publisher of scientific research, with over 4,200 books and 54,000 scientific works including peer-reviewed content from more than 116,000 scientists spanning 161 countries. Our authors range from globally-renowned Nobel Prize winners to up-and-coming researchers at the cutting edge of scientific discovery.
\n\n
In the same year that IntechOpen was founded, we launched what was at the time the first ever Open Access, peer-reviewed journal in its field: the International Journal of Advanced Robotic Systems (IJARS).
\n\n
The IntechOpen timeline
\n\n
2004
\n\n
\n\t
Intech Open is founded in Vienna, Austria, by Alex Lazinica and Vedran Kordic, two PhD students, and their first Open Access journals and books are published.
\n\t
Alex and Vedran launch the first Open Access, peer-reviewed robotics journal and IntechOpen’s flagship publication, the International Journal of Advanced Robotic Systems (IJARS).
\n
\n\n
2005
\n\n
\n\t
IntechOpen publishes its first Open Access book: Cutting Edge Robotics.
\n
\n\n
2006
\n\n
\n\t
IntechOpen publishes a special issue of IJARS, featuring contributions from NASA scientists regarding the Mars Exploration Rover missions.
\n
\n\n
2008
\n\n
\n\t
Downloads milestone: 200,000 downloads reached
\n
\n\n
2009
\n\n
\n\t
Publishing milestone: the first 100 Open Access STM books are published
\n
\n\n
2010
\n\n
\n\t
Downloads milestone: one million downloads reached
\n\t
IntechOpen expands its book publishing into a new field: medicine.
\n
\n\n
2011
\n\n
\n\t
Publishing milestone: More than five million downloads reached
\n\t
IntechOpen publishes 1996 Nobel Prize in Chemistry winner Harold W. Kroto’s “Strategies to Successfully Cross-Link Carbon Nanotubes”. Find it here.
\n\t
IntechOpen and TBI collaborate on a project to explore the changing needs of researchers and the evolving ways that they discover, publish and exchange information. The result is the survey “Author Attitudes Towards Open Access Publishing: A Market Research Program”.
\n\t
IntechOpen hosts SHOW - Share Open Access Worldwide; a series of lectures, debates, round-tables and events to bring people together in discussion of open source principles, intellectual property, content licensing innovations, remixed and shared culture and free knowledge.
\n
\n\n
2012
\n\n
\n\t
Publishing milestone: 10 million downloads reached
\n\t
IntechOpen holds Interact2012, a free series of workshops held by figureheads of the scientific community including Professor Hiroshi Ishiguro, director of the Intelligent Robotics Laboratory, who took the audience through some of the most impressive human-robot interactions observed in his lab.
\n
\n\n
2013
\n\n
\n\t
IntechOpen joins the Committee on Publication Ethics (COPE) as part of a commitment to guaranteeing the highest standards of publishing.
\n
\n\n
2014
\n\n
\n\t
IntechOpen turns 10, with more than 30 million downloads to date.
\n\t
IntechOpen appoints its first Regional Representatives - members of the team situated around the world dedicated to increasing the visibility of our authors’ published work within their local scientific communities.
\n
\n\n
2015
\n\n
\n\t
Downloads milestone: More than 70 million downloads reached, more than doubling since the previous year.
\n\t
Publishing milestone: IntechOpen publishes its 2,500th book and 40,000th Open Access chapter, reaching 20,000 citations in Thomson Reuters ISI Web of Science.
\n\t
40 IntechOpen authors are included in the top one per cent of the world’s most-cited researchers.
\n\t
Thomson Reuters’ ISI Web of Science Book Citation Index begins indexing IntechOpen’s books in its database.
\n
\n\n
2016
\n\n
\n\t
IntechOpen is identified as a world leader in Simba Information’s Open Access Book Publishing 2016-2020 report and forecast. IntechOpen came in as the world’s largest Open Access book publisher by title count.
\n
\n\n
2017
\n\n
\n\t
Downloads milestone: IntechOpen reaches more than 100 million downloads
\n\t
Publishing milestone: IntechOpen publishes its 3,000th Open Access book, making it the largest Open Access book collection in the world
\n
\n"}]},successStories:{items:[]},authorsAndEditors:{filterParams:{},profiles:[{id:"396",title:"Dr.",name:"Vedran",middleName:null,surname:"Kordic",slug:"vedran-kordic",fullName:"Vedran Kordic",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/396/images/7281_n.png",biography:"After obtaining his Master's degree in Mechanical Engineering he continued his education at the Vienna University of Technology where he obtained his PhD degree in 2004. He worked as a researcher at the Automation and Control Institute, Faculty of Electrical Engineering, Vienna University of Technology until 2008. His studies in robotics lead him not only to a PhD degree but also inspired him to co-found and build the International Journal of Advanced Robotic Systems - world's first Open Access journal in the field of robotics.",institutionString:null,institution:{name:"TU Wien",country:{name:"Austria"}}},{id:"441",title:"Ph.D.",name:"Jaekyu",middleName:null,surname:"Park",slug:"jaekyu-park",fullName:"Jaekyu Park",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/441/images/1881_n.jpg",biography:null,institutionString:null,institution:{name:"LG Corporation (South Korea)",country:{name:"Korea, South"}}},{id:"465",title:"Dr",name:"Christian",middleName:null,surname:"Martens",slug:"christian-martens",fullName:"Christian Martens",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:null},{id:"479",title:"Dr.",name:"Valentina",middleName:null,surname:"Colla",slug:"valentina-colla",fullName:"Valentina Colla",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/479/images/358_n.jpg",biography:null,institutionString:null,institution:{name:"Sant'Anna School of Advanced Studies",country:{name:"Italy"}}},{id:"494",title:"PhD",name:"Loris",middleName:null,surname:"Nanni",slug:"loris-nanni",fullName:"Loris Nanni",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/494/images/system/494.jpg",biography:"Loris Nanni received his Master Degree cum laude on June-2002 from the University of Bologna, and the April 26th 2006 he received his Ph.D. in Computer Engineering at DEIS, University of Bologna. On September, 29th 2006 he has won a post PhD fellowship from the university of Bologna (from October 2006 to October 2008), at the competitive examination he was ranked first in the industrial engineering area. He extensively served as referee for several international journals. He is author/coauthor of more than 100 research papers. He has been involved in some projects supported by MURST and European Community. His research interests include pattern recognition, bioinformatics, and biometric systems (fingerprint classification and recognition, signature verification, face recognition).",institutionString:null,institution:null},{id:"496",title:"Dr.",name:"Carlos",middleName:null,surname:"Leon",slug:"carlos-leon",fullName:"Carlos Leon",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"University of Seville",country:{name:"Spain"}}},{id:"512",title:"Dr.",name:"Dayang",middleName:null,surname:"Jawawi",slug:"dayang-jawawi",fullName:"Dayang Jawawi",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"University of Technology Malaysia",country:{name:"Malaysia"}}},{id:"528",title:"Dr.",name:"Kresimir",middleName:null,surname:"Delac",slug:"kresimir-delac",fullName:"Kresimir Delac",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/528/images/system/528.jpg",biography:"K. 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He received his Ph.D. in Molecular Biology with his thesis “Genetic variability of the tick-borne encephalitis virus in natural foci of Novosibirsk city and its suburbs.” His primary field is molecular virology with research emphasis on vector-borne viruses, especially tick-borne encephalitis virus, Kemerovo virus and Omsk hemorrhagic fever virus, rabies virus, molecular genetics, biology, and epidemiology of virus pathogens.",institutionString:"Russian Academy of Sciences",institution:{name:"Russian Academy of Sciences",country:{name:"Russia"}}},{id:"310962",title:"Dr.",name:"Amlan",middleName:"Kumar",surname:"Patra",slug:"amlan-patra",fullName:"Amlan Patra",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/310962/images/system/310962.jpg",biography:"Amlan K. Patra, FRSB, obtained a Ph.D. in Animal Nutrition from Indian Veterinary Research Institute, India, in 2002. He is currently an associate professor at West Bengal University of Animal and Fishery Sciences. He has more than twenty years of research and teaching experience. He held previous positions at the American Institute for Goat Research, The Ohio State University, Columbus, USA, and Free University of Berlin, Germany. His research focuses on animal nutrition, particularly ruminants and poultry nutrition, gastrointestinal electrophysiology, meta-analysis and modeling in nutrition, and livestock–environment interaction. He has authored around 175 articles in journals, book chapters, and proceedings. Dr. Patra serves on the editorial boards of several reputed journals.",institutionString:null,institution:{name:"West Bengal University of Animal and Fishery Sciences",country:{name:"India"}}},{id:"53998",title:"Prof.",name:"László",middleName:null,surname:"Babinszky",slug:"laszlo-babinszky",fullName:"László Babinszky",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/53998/images/system/53998.png",biography:"László Babinszky is Professor Emeritus, Department of Animal Nutrition Physiology, University of Debrecen, Hungary. He has also worked in the Department of Animal Nutrition, University of Wageningen, Netherlands; the Institute for Livestock Feeding and Nutrition (IVVO), Lelystad, Netherlands; the Agricultural University of Vienna (BOKU); the Institute for Animal Breeding and Nutrition, Austria; and the Oscar Kellner Research Institute for Animal Nutrition, Rostock, Germany. In 1992, Dr. Babinszky obtained a Ph.D. in Animal Nutrition from the University of Wageningen. His main research areas are swine and poultry nutrition. He has authored more than 300 publications (papers, book chapters) and edited four books and fourteen international conference proceedings.",institutionString:"University of Debrecen",institution:{name:"University of Debrecen",country:{name:"Hungary"}}},{id:"201830",title:"Dr.",name:"Fernando",middleName:"Sanchez",surname:"Davila",slug:"fernando-davila",fullName:"Fernando Davila",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/201830/images/5017_n.jpg",biography:"I am a professor at UANL since 1988. My research lines are the development of reproductive techniques in small ruminants. We also conducted research on sexual and social behavior in males.\nI am Mexican and study my professional career as an engineer in agriculture and animal science at UANL. Then take a masters degree in science in Germany (Animal breeding). Take a doctorate in animal science at the UANL.",institutionString:null,institution:{name:"Universidad Autónoma de Nuevo León",country:{name:"Mexico"}}},{id:"309250",title:"Dr.",name:"Miguel",middleName:null,surname:"Quaresma",slug:"miguel-quaresma",fullName:"Miguel Quaresma",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/309250/images/9059_n.jpg",biography:"Miguel Nuno Pinheiro Quaresma was born on May 26, 1974 in Dili, Timor Island. He is married with two children: a boy and a girl, and he is a resident in Vila Real, Portugal. He graduated in Veterinary Medicine in August 1998 and obtained his Ph.D. degree in Veterinary Sciences -Clinical Area in February 2015, both from the University of Trás-os-Montes e Alto Douro. He is currently enrolled in the Alternative Residency of the European College of Animal Reproduction. He works as a Senior Clinician at the Veterinary Teaching Hospital of UTAD (HVUTAD) with a role in clinical activity in the area of livestock and equine species as well as to support teaching and research in related areas. He teaches as an Invited Professor in Reproduction Medicine I and II of the Master\\'s in Veterinary Medicine degree at UTAD. Currently, he holds the position of Chairman of the Portuguese Buiatrics Association. He is a member of the Consultive Group on Production Animals of the OMV. He has 19 publications in indexed international journals (ISIS), as well as over 60 publications and oral presentations in both Portuguese and international journals and congresses.",institutionString:"University of Trás-os-Montes and Alto Douro",institution:{name:"University of Trás-os-Montes and Alto Douro",country:{name:"Portugal"}}},{id:"38652",title:"Prof.",name:"Rita",middleName:null,surname:"Payan-Carreira",slug:"rita-payan-carreira",fullName:"Rita Payan-Carreira",position:null,profilePictureURL:"https://s3.us-east-1.amazonaws.com/intech-files/0030O00002bRiFPQA0/Profile_Picture_1614601496313",biography:"Rita Payan Carreira earned her Veterinary Degree from the Faculty of Veterinary Medicine in Lisbon, Portugal, in 1985. She obtained her Ph.D. in Veterinary Sciences from the University of Trás-os-Montes e Alto Douro, Portugal. After almost 32 years of teaching at the University of Trás-os-Montes and Alto Douro, she recently moved to the University of Évora, Department of Veterinary Medicine, where she teaches in the field of Animal Reproduction and Clinics. Her primary research areas include the molecular markers of the endometrial cycle and the embryo–maternal interaction, including oxidative stress and the reproductive physiology and disorders of sexual development, besides the molecular determinants of male and female fertility. She often supervises students preparing their master's or doctoral theses. She is also a frequent referee for various journals.",institutionString:null,institution:{name:"University of Évora",country:{name:"Portugal"}}},{id:"283019",title:"Dr.",name:"Oudessa",middleName:null,surname:"Kerro Dego",slug:"oudessa-kerro-dego",fullName:"Oudessa Kerro Dego",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/283019/images/system/283019.png",biography:"Dr. Kerro Dego is a veterinary microbiologist with training in veterinary medicine, microbiology, and anatomic pathology. Dr. Kerro Dego is an assistant professor of dairy health in the department of animal science, the University of Tennessee, Institute of Agriculture, Knoxville, Tennessee. He received his D.V.M. (1997), M.S. (2002), and Ph.D. (2008) degrees in Veterinary Medicine, Animal Pathology and Veterinary Microbiology from College of Veterinary Medicine, Addis Ababa University, Ethiopia; College of Veterinary Medicine, Utrecht University, the Netherlands and Western College of Veterinary Medicine, University of Saskatchewan, Canada respectively. He did his Postdoctoral training in microbial pathogenesis (2009 - 2015) in the Department of Animal Science, the University of Tennessee, Institute of Agriculture, Knoxville, Tennessee. Dr. Kerro Dego’s research focuses on the prevention and control of infectious diseases of farm animals, particularly mastitis, improving dairy food safety, and mitigation of antimicrobial resistance. Dr. Kerro Dego has extensive experience in studying the pathogenesis of bacterial infections, identification of virulence factors, and vaccine development and efficacy testing against major bacterial mastitis pathogens. Dr. Kerro Dego conducted numerous controlled experimental and field vaccine efficacy studies, vaccination, and evaluation of immunological responses in several species of animals, including rodents (mice) and large animals (bovine and ovine).",institutionString:"University of Tennessee at Knoxville",institution:{name:"University of Tennessee at Knoxville",country:{name:"United States of America"}}},{id:"251314",title:"Dr.",name:"Juan Carlos",middleName:null,surname:"Gardón",slug:"juan-carlos-gardon",fullName:"Juan Carlos Gardón",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/251314/images/system/251314.jpeg",biography:"Juan Carlos Gardón Poggi received University degree from the Faculty of Agrarian Science in Argentina, in 1983. Also he received Masters Degree and PhD from Córdoba University, Spain. He is currently a Professor at the Catholic University of Valencia San Vicente Mártir, at the Department of Medicine and Animal Surgery. He teaches diverse courses in the field of Animal Reproduction and he is the Director of the Veterinary Farm. He also participates in academic postgraduate activities at the Veterinary Faculty of Murcia University, Spain. His research areas include animal physiology, physiology and biotechnology of reproduction either in males or females, the study of gametes under in vitro conditions and the use of ultrasound as a complement to physiological studies and development of applied biotechnologies. Routinely, he supervises students preparing their doctoral, master thesis or final degree projects.",institutionString:"Catholic University of Valencia San Vicente Mártir, Spain",institution:null},{id:"125292",title:"Dr.",name:"Katy",middleName:null,surname:"Satué Ambrojo",slug:"katy-satue-ambrojo",fullName:"Katy Satué Ambrojo",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/125292/images/system/125292.jpeg",biography:"Katy Satué Ambrojo received her Veterinary Medicine degree, Master degree in Equine Technology and doctorate in Veterinary Medicine from the Faculty of Veterinary, CEU-Cardenal Herrera University in Valencia, Spain. She is a Full Professor at the Department of Medicine and Animal Surgery at the same University. She developed her research activity in the field of Endocrinology, Hematology, Biochemistry and Immunology of horses. She is a scientific reviewer of several international journals : American Journal of Obstetrics and Gynecology, Comparative Clinical Pathology, Veterinary Clinical Pathology, Journal of Equine Veterinary Science, Reproduction in Domestic Animals, Research Veterinary Science, Brazilian Journal of Medical and Biological Research, Livestock Production Science and Theriogenology. Since 2014, she has been the Head of the Clinical Analysis Laboratory of the Hospital Clínico Veterinario from the Faculty of Veterinary, CEU-Cardenal Herrera University.",institutionString:"CEU-Cardenal Herrera University",institution:{name:"CEU Cardinal Herrera University",country:{name:"Spain"}}},{id:"309529",title:"Dr.",name:"Albert",middleName:null,surname:"Rizvanov",slug:"albert-rizvanov",fullName:"Albert Rizvanov",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/309529/images/9189_n.jpg",biography:'Albert A. Rizvanov is a Professor and Director of the Center for Precision and Regenerative Medicine at the Institute of Fundamental Medicine and Biology, Kazan Federal University (KFU), Russia. He is the Head of the Center of Excellence “Regenerative Medicine” and Vice-Director of Strategic Academic Unit \\"Translational 7P Medicine\\". Albert completed his Ph.D. at the University of Nevada, Reno, USA and Dr.Sci. at KFU. He is a corresponding member of the Tatarstan Academy of Sciences, Russian Federation. Albert is an author of more than 300 peer-reviewed journal articles and 22 patents. He has supervised 11 Ph.D. and 2 Dr.Sci. dissertations. Albert is the Head of the Dissertation Committee on Biochemistry, Microbiology, and Genetics at KFU.\nORCID https://orcid.org/0000-0002-9427-5739\nWebsite https://kpfu.ru/Albert.Rizvanov?p_lang=2',institutionString:"Kazan Federal University",institution:{name:"Kazan Federal University",country:{name:"Russia"}}},{id:"210551",title:"Dr.",name:"Arbab",middleName:null,surname:"Sikandar",slug:"arbab-sikandar",fullName:"Arbab Sikandar",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/210551/images/system/210551.jpg",biography:"Dr. Arbab Sikandar, PhD, M. Phil, DVM was born on April 05, 1981. He is currently working at the College of Veterinary & Animal Sciences as an Assistant Professor. He previously worked as a lecturer at the same University. \nHe is a Member/Secretory of Ethics committee (No. CVAS-9377 dated 18-04-18), Member of the QEC committee CVAS, Jhang (Regr/Gen/69/873, dated 26-10-2017), Member, Board of studies of Department of Basic Sciences (No. CVAS. 2851 Dated. 12-04-13, and No. CVAS, 9024 dated 20/11/17), Member of Academic Committee, CVAS, Jhang (No. CVAS/2004, Dated, 25-08-12), Member of the technical committee (No. CVAS/ 4085, dated 20,03, 2010 till 2016).\n\nDr. Arbab Sikandar contributed in five days hands-on-training on Histopathology at the Department of Pathology, UVAS from 12-16 June 2017. He received a Certificate of appreciation for contributions for Popularization of Science and Technology in the Society on 17-11-15. He was the resource person in the lecture series- ‘scientific writing’ at the Department of Anatomy and Histology, UVAS, Lahore on 29th October 2015. He won a full fellowship as a principal candidate for the year 2015 in the field of Agriculture, EICA, Egypt with ref. to the Notification No. 12(11) ACS/Egypt/2014 from 10 July 2015 to 25th September 2015.; he received a grant of Rs. 55000/- as research incentives from Director, Advanced Studies and Research, UVAS, Lahore upon publications of research papers in IF Journals (DR/215, dated 19-5-2014.. He obtained his PhD by winning a HEC Pakistan indigenous Scholarship, ‘Ph.D. fellowship for 5000 scholars – Phase II’ (2av1-147), 17-6/HEC/HRD/IS-II/12, November 15, 2012. \n\nDr. Sikandar is a member of numerous societies: Registered Veterinary Medical Practitioner (life member) and Registered Veterinary Medical Faculty of Pakistan Veterinary Medical Council. The Registration code of PVMC is RVMP/4298 and RVMF/ 0102.; Life member of the University of Veterinary and Animal Sciences, Lahore, Alumni Association with S# 664, dated: 6-4-12. ; Member 'Vets Care Organization Pakistan” with Reference No. VCO-605-149, dated 05-04-06. :Member 'Vet Crescent” (Society of Animal Health and Production), UVAS, Lahore.",institutionString:"University of Veterinary & Animal Science",institution:{name:"University of Veterinary and Animal Sciences",country:{name:"Pakistan"}}},{id:"311663",title:"Dr.",name:"Prasanna",middleName:null,surname:"Pal",slug:"prasanna-pal",fullName:"Prasanna Pal",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/311663/images/13261_n.jpg",biography:null,institutionString:null,institution:{name:"National Dairy Research Institute",country:{name:"India"}}},{id:"202192",title:"Dr.",name:"Catrin",middleName:null,surname:"Rutland",slug:"catrin-rutland",fullName:"Catrin Rutland",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/202192/images/system/202192.png",biography:"Catrin Rutland is an Associate Professor of Anatomy and Developmental Genetics at the University of Nottingham, UK. 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She continued as a post-doctoral fellow at the University of Copenhagen with a Lundbeck foundation fellowship. She is the editor of three books and author/coauthor of 23 articles in peer-reviewed scientific journals, 16 book chapters, and 68 communications at scientific congresses. Since 2008 she has been the Editor Assistant for the Slovenian Veterinary Research journal. She is a member of Slovenian Biochemical Society, The Endocrine Society, European Association of Veterinary Anatomists and Society for Laboratory Animals, where she is board member.",institutionString:"University of Ljubljana",institution:{name:"University of Ljubljana",country:{name:"Slovenia"}}},{id:"258334",title:"Dr.",name:"Carlos Eduardo",middleName:null,surname:"Fonseca-Alves",slug:"carlos-eduardo-fonseca-alves",fullName:"Carlos Eduardo Fonseca-Alves",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/258334/images/system/258334.jpg",biography:"Dr. Fonseca-Alves earned his DVM from Federal University of Goias – UFG in 2008. He completed an internship in small animal internal medicine at UPIS university in 2011, earned his MSc in 2013 and PhD in 2015 both in Veterinary Medicine at Sao Paulo State University – UNESP. Dr. Fonseca-Alves currently serves as an Assistant Professor at Paulista University – UNIP teaching small animal internal medicine.",institutionString:null,institution:{name:"Universidade Paulista",country:{name:"Brazil"}}},{id:"245306",title:"Dr.",name:"María Luz",middleName:null,surname:"Garcia Pardo",slug:"maria-luz-garcia-pardo",fullName:"María Luz Garcia Pardo",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/245306/images/system/245306.png",biography:"María de la Luz García Pardo is an agricultural engineer from Universitat Politècnica de València, Spain. She has a Ph.D. in Animal Genetics. Currently, she is a lecturer at the Agrofood Technology Department of Miguel Hernández University, Spain. Her research is focused on genetics and reproduction in rabbits. The major goal of her research is the genetics of litter size through novel methods such as selection by the environmental sensibility of litter size, with forays into the field of animal welfare by analysing the impact on the susceptibility to diseases and stress of the does. 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After a general CertAVP (2015) I gained the designated Certificate in Veterinary Dermatology (2017) after taking the synoptic examination and then applied for the RCVS ADvanced Practitioner status. After that, I completed the Postgraduate Diploma in Veterinary Professional Studies at the University of Liverpool (2018). My main area of work is cross-species veterinary dermatology.",institutionString:null,institution:null},{id:"291226",title:"Dr.",name:"Monica",middleName:null,surname:"Cassel",slug:"monica-cassel",fullName:"Monica Cassel",position:null,profilePictureURL:"https://mts.intechopen.com/storage/users/291226/images/8232_n.jpg",biography:'Degree in Biological Sciences at the Federal University of Mato Grosso with scholarship for Scientific Initiation by FAPEMAT (2008/1) and CNPq (2008/2-2009/2): Project \\"Histological evidence of reproductive activity in lizards of the Manso region, Chapada dos Guimarães, Mato Grosso, Brazil\\". Master\\\'s degree in Ecology and Biodiversity Conservation at Federal University of Mato Grosso with a scholarship by CAPES/REUNI program: Project \\"Reproductive biology of Melanorivulus punctatus\\". PhD\\\'s degree in Science (Cell and Tissue Biology Area) \n at University of Sao Paulo with scholarship granted by FAPESP; Project \\"Development of morphofunctional changes in ovary of Astyanax altiparanae Garutti & Britski, 2000 (Teleostei, Characidae)\\". She has experience in Reproduction of vertebrates and Morphology, with emphasis in Cellular Biology and Histology. She is currently a teacher in the medium / technical level courses at IFMT-Alta Floresta, as well as in the Bachelor\\\'s degree in Animal Science and in the Bachelor\\\'s degree in Business.',institutionString:null,institution:null},{id:"442807",title:"Dr.",name:"Busani",middleName:null,surname:"Moyo",slug:"busani-moyo",fullName:"Busani Moyo",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Gwanda State University",country:{name:"Zimbabwe"}}},{id:"423023",title:"Dr.",name:"Yosra",middleName:null,surname:"Soltan",slug:"yosra-soltan",fullName:"Yosra Soltan",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Alexandria University",country:{name:"Egypt"}}},{id:"349788",title:"Dr.",name:"Florencia Nery",middleName:null,surname:"Sompie",slug:"florencia-nery-sompie",fullName:"Florencia Nery Sompie",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Sam Ratulangi University",country:{name:"Indonesia"}}},{id:"345713",title:"Dr.",name:"Csaba",middleName:null,surname:"Szabó",slug:"csaba-szabo",fullName:"Csaba Szabó",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"University of Debrecen",country:{name:"Hungary"}}},{id:"345719",title:"Mrs.",name:"Márta",middleName:null,surname:"Horváth",slug:"marta-horvath",fullName:"Márta Horváth",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"University of Debrecen",country:{name:"Hungary"}}},{id:"420151",title:"Prof.",name:"Novirman",middleName:null,surname:"Jamarun",slug:"novirman-jamarun",fullName:"Novirman Jamarun",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Andalas University",country:{name:"Indonesia"}}},{id:"420149",title:"Dr.",name:"Rusmana",middleName:"Wijaya Setia",surname:"Wijaya Setia Ningrat",slug:"rusmana-wijaya-setia-ningrat",fullName:"Rusmana Wijaya Setia Ningrat",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Andalas University",country:{name:"Indonesia"}}},{id:"339759",title:"Mr.",name:"Abu",middleName:null,surname:"Macavoray",slug:"abu-macavoray",fullName:"Abu Macavoray",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Njala University",country:{name:"Sierra Leone"}}},{id:"339758",title:"Prof.",name:"Benjamin",middleName:null,surname:"Emikpe",slug:"benjamin-emikpe",fullName:"Benjamin Emikpe",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"University of Ibadan",country:{name:"Nigeria"}}},{id:"339760",title:"Mr.",name:"Moinina Nelphson",middleName:null,surname:"Kallon",slug:"moinina-nelphson-kallon",fullName:"Moinina Nelphson Kallon",position:null,profilePictureURL:"//cdnintech.com/web/frontend/www/assets/author.svg",biography:null,institutionString:null,institution:{name:"Njala University",country:{name:"Sierra Leone"}}}]}},subseries:{item:{id:"5",type:"subseries",title:"Parasitic Infectious Diseases",keywords:"Blood Borne Parasites, Intestinal Parasites, Protozoa, Helminths, Arthropods, Water Born Parasites, Epidemiology, Molecular Biology, Systematics, Genomics, Proteomics, Ecology",scope:"Parasitic diseases have evolved alongside their human hosts. In many cases, these diseases have adapted so well that they have developed efficient resilience methods in the human host and can live in the host for years. Others, particularly some blood parasites, can cause very acute diseases and are responsible for millions of deaths yearly. Many parasitic diseases are classified as neglected tropical diseases because they have received minimal funding over recent years and, in many cases, are under-reported despite the critical role they play in morbidity and mortality among human and animal hosts. The current topic, Parasitic Infectious Diseases, in the Infectious Diseases Series aims to publish studies on the systematics, epidemiology, molecular biology, genomics, pathogenesis, genetics, and clinical significance of parasitic diseases from blood borne to intestinal parasites as well as zoonotic parasites. We hope to cover all aspects of parasitic diseases to provide current and relevant research data on these very important diseases. In the current atmosphere of the Coronavirus pandemic, communities around the world, particularly those in different underdeveloped areas, are faced with the growing challenges of the high burden of parasitic diseases. At the same time, they are faced with the Covid-19 pandemic leading to what some authors have called potential syndemics that might worsen the outcome of such infections. Therefore, it is important to conduct studies that examine parasitic infections in the context of the coronavirus pandemic for the benefit of all communities to help foster more informed decisions for the betterment of human and animal health.",coverUrl:"https://cdn.intechopen.com/series_topics/covers/5.jpg",hasOnlineFirst:!0,hasPublishedBooks:!0,annualVolume:11401,editor:{id:"67907",title:"Dr.",name:"Amidou",middleName:null,surname:"Samie",slug:"amidou-samie",fullName:"Amidou Samie",profilePictureURL:"https://mts.intechopen.com/storage/users/67907/images/system/67907.jpg",biography:"Dr. Amidou Samie is an Associate Professor of Microbiology at the University of Venda, in South Africa, where he graduated for his PhD in May 2008. He joined the Department of Microbiology the same year and has been giving lectures on topics covering parasitology, immunology, molecular biology and industrial microbiology. He is currently a rated researcher by the National Research Foundation of South Africa at category C2. He has published widely in the field of infectious diseases and has overseen several MSc’s and PhDs. His research activities mostly cover topics on infectious diseases from epidemiology to control. His particular interest lies in the study of intestinal protozoan parasites and opportunistic infections among HIV patients as well as the potential impact of childhood diarrhoea on growth and child development. He also conducts research on water-borne diseases and water quality and is involved in the evaluation of point-of-use water treatment technologies using silver and copper nanoparticles in collaboration with the University of Virginia, USA. He also studies the use of medicinal plants for the control of infectious diseases as well as antimicrobial drug resistance.",institutionString:null,institution:{name:"University of Venda",institutionURL:null,country:{name:"South Africa"}}},editorTwo:null,editorThree:null,series:{id:"6",title:"Infectious Diseases",doi:"10.5772/intechopen.71852",issn:"2631-6188"},editorialBoard:[{id:"188881",title:"Dr.",name:"Fernando José",middleName:null,surname:"Andrade-Narváez",slug:"fernando-jose-andrade-narvaez",fullName:"Fernando José Andrade-Narváez",profilePictureURL:"https://s3.us-east-1.amazonaws.com/intech-files/0030O00002bRIV7QAO/Profile_Picture_1628834308121",institutionString:null,institution:{name:"Autonomous University of Yucatán",institutionURL:null,country:{name:"Mexico"}}},{id:"269120",title:"Dr.",name:"Rajeev",middleName:"K.",surname:"Tyagi",slug:"rajeev-tyagi",fullName:"Rajeev Tyagi",profilePictureURL:"https://s3.us-east-1.amazonaws.com/intech-files/0030O00002bRaBqQAK/Profile_Picture_1644331884726",institutionString:"CSIR - Institute of Microbial Technology, India",institution:null},{id:"336849",title:"Prof.",name:"Ricardo",middleName:null,surname:"Izurieta",slug:"ricardo-izurieta",fullName:"Ricardo Izurieta",profilePictureURL:"https://mts.intechopen.com/storage/users/293169/images/system/293169.png",institutionString:null,institution:{name:"University of South Florida",institutionURL:null,country:{name:"United States of America"}}}]},onlineFirstChapters:{paginationCount:0,paginationItems:[]},publishedBooks:{paginationCount:4,paginationItems:[{type:"book",id:"9528",title:"Current Topics and Emerging Issues in Malaria Elimination",subtitle:null,coverURL:"https://cdn.intechopen.com/books/images_new/9528.jpg",slug:"current-topics-and-emerging-issues-in-malaria-elimination",publishedDate:"July 21st 2021",editedByType:"Edited by",bookSignature:"Alfonso J. 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