\\n\\n
More than half of the publishers listed alongside IntechOpen (18 out of 30) are Social Science and Humanities publishers. IntechOpen is an exception to this as a leader in not only Open Access content but Open Access content across all scientific disciplines, including Physical Sciences, Engineering and Technology, Health Sciences, Life Science, and Social Sciences and Humanities.
\\n\\nOur breakdown of titles published demonstrates this with 47% PET, 31% HS, 18% LS, and 4% SSH books published.
\\n\\n“Even though ItechOpen has shown the potential of sci-tech books using an OA approach,” other publishers “have shown little interest in OA books.”
\\n\\nAdditionally, each book published by IntechOpen contains original content and research findings.
\\n\\nWe are honored to be among such prestigious publishers and we hope to continue to spearhead that growth in our quest to promote Open Access as a true pioneer in OA book publishing.
\\n\\n\\n\\n
\\n"}]',published:!0,mainMedia:{caption:"IntechOpen Maintains",originalUrl:"/media/original/113"}},components:[{type:"htmlEditorComponent",content:'
Simba Information has released its Open Access Book Publishing 2020 - 2024 report and has again identified IntechOpen as the world’s largest Open Access book publisher by title count.
\n\nSimba Information is a leading provider for market intelligence and forecasts in the media and publishing industry. The report, published every year, provides an overview and financial outlook for the global professional e-book publishing market.
\n\nIntechOpen, De Gruyter, and Frontiers are the largest OA book publishers by title count, with IntechOpen coming in at first place with 5,101 OA books published, a good 1,782 titles ahead of the nearest competitor.
\n\nSince the first Open Access Book Publishing report published in 2016, IntechOpen has held the top stop each year.
\n\n\n\nMore than half of the publishers listed alongside IntechOpen (18 out of 30) are Social Science and Humanities publishers. IntechOpen is an exception to this as a leader in not only Open Access content but Open Access content across all scientific disciplines, including Physical Sciences, Engineering and Technology, Health Sciences, Life Science, and Social Sciences and Humanities.
\n\nOur breakdown of titles published demonstrates this with 47% PET, 31% HS, 18% LS, and 4% SSH books published.
\n\n“Even though ItechOpen has shown the potential of sci-tech books using an OA approach,” other publishers “have shown little interest in OA books.”
\n\nAdditionally, each book published by IntechOpen contains original content and research findings.
\n\nWe are honored to be among such prestigious publishers and we hope to continue to spearhead that growth in our quest to promote Open Access as a true pioneer in OA book publishing.
\n\n\n\n
\n'}],latestNews:[{slug:"webinar-introduction-to-open-science-wednesday-18-may-1-pm-cest-20220518",title:"Webinar: Introduction to Open Science | Wednesday 18 May, 1 PM CEST"},{slug:"step-in-the-right-direction-intechopen-launches-a-portfolio-of-open-science-journals-20220414",title:"Step in the Right Direction: IntechOpen Launches a Portfolio of Open Science Journals"},{slug:"let-s-meet-at-london-book-fair-5-7-april-2022-olympia-london-20220321",title:"Let’s meet at London Book Fair, 5-7 April 2022, Olympia London"},{slug:"50-books-published-as-part-of-intechopen-and-knowledge-unlatched-ku-collaboration-20220316",title:"50 Books published as part of IntechOpen and Knowledge Unlatched (KU) Collaboration"},{slug:"intechopen-joins-the-united-nations-sustainable-development-goals-publishers-compact-20221702",title:"IntechOpen joins the United Nations Sustainable Development Goals Publishers Compact"},{slug:"intechopen-signs-exclusive-representation-agreement-with-lsr-libros-servicios-y-representaciones-s-a-de-c-v-20211123",title:"IntechOpen Signs Exclusive Representation Agreement with LSR Libros Servicios y Representaciones S.A. de C.V"},{slug:"intechopen-expands-partnership-with-research4life-20211110",title:"IntechOpen Expands Partnership with Research4Life"},{slug:"introducing-intechopen-book-series-a-new-publishing-format-for-oa-books-20210915",title:"Introducing IntechOpen Book Series - A New Publishing Format for OA Books"}]},book:{item:{type:"book",id:"10543",leadTitle:null,fullTitle:"Psychology and Pathophysiological Outcomes of Eating",title:"Psychology and Pathophysiological Outcomes of Eating",subtitle:null,reviewType:"peer-reviewed",abstract:"The psychology of eating is regulated by neural mechanisms. When not well controlled, eating may result in disorders and health hazards such as obesity, type 2 diabetes mellitus, and vascular diseases. Lifestyles and cultures influence eating habits, thus there are differences in the prevalence of health problems depending upon living environments. This book examines the psychology and the pathophysiological outcomes of eating. Chapters address such topics as the influence of lifestyle, circadian rhythm, sleep, and fragrant odors on appetite and weight regulation; the impact of glucose, sucrose, lactate, and ketone bodies on the brain; the consequences of glycation stress on the skeletal muscle; and much more.",isbn:"978-1-83968-777-8",printIsbn:"978-1-83968-776-1",pdfIsbn:"978-1-83968-778-5",doi:"10.5772/intechopen.92917",price:119,priceEur:129,priceUsd:155,slug:"psychology-and-pathophysiological-outcomes-of-eating",numberOfPages:272,isOpenForSubmission:!1,isInWos:null,isInBkci:!1,hash:"2464b5fb6a39df380e935096743410a0",bookSignature:"Akikazu Takada and Hubertus Himmerich",publishedDate:"December 1st 2021",coverURL:"https://cdn.intechopen.com/books/images_new/10543.jpg",numberOfDownloads:2573,numberOfWosCitations:0,numberOfCrossrefCitations:1,numberOfCrossrefCitationsByBook:0,numberOfDimensionsCitations:8,numberOfDimensionsCitationsByBook:0,hasAltmetrics:0,numberOfTotalCitations:9,isAvailableForWebshopOrdering:!0,dateEndFirstStepPublish:"September 11th 2020",dateEndSecondStepPublish:"October 9th 2020",dateEndThirdStepPublish:"March 29th 2021",dateEndFourthStepPublish:"May 14th 2021",dateEndFifthStepPublish:"June 15th 2021",currentStepOfPublishingProcess:5,indexedIn:"1,2,3,4,5,6",editedByType:"Edited by",kuFlag:!1,featuredMarkup:null,editors:[{id:"248459",title:"Dr.",name:"Akikazu",middleName:null,surname:"Takada",slug:"akikazu-takada",fullName:"Akikazu Takada",profilePictureURL:"https://mts.intechopen.com/storage/users/248459/images/system/248459.png",biography:"Akikazu Takada was born in Japan, 1935. After graduation from\nKeio University School of Medicine and finishing his post-graduate studies, he worked at Roswell Park Memorial Institute NY,\nUSA. He then took a professorship at Hamamatsu University\nSchool of Medicine. In thrombosis studies, he found the SK\npotentiator that enhances plasminogen activation by streptokinase. He is very much interested in simultaneous measurements\nof fatty acids, amino acids, and tryptophan degradation products. By using fatty\nacid analyses, he indicated that plasma levels of trans-fatty acids of old men were\nfar higher in the US than Japanese men. . He also showed that eicosapentaenoic acid\n(EPA) and docosahexaenoic acid (DHA) levels are higher, and arachidonic acid\nlevels are lower in Japanese than US people. By using simultaneous LC/MS analyses\nof plasma levels of tryptophan metabolites, he recently found that plasma levels of\nserotonin, kynurenine, or 5-HIAA were higher in patients of mono- and bipolar\ndepression, which are significantly different from observations reported before. In\nview of recent reports that plasma tryptophan metabolites are mainly produced by\nmicrobiota. He is now working on the relationships between microbiota and depression or autism.",institutionString:"Hamamatsu University School of Medicine",position:null,outsideEditionCount:0,totalCites:0,totalAuthoredChapters:"7",totalChapterViews:"0",totalEditedBooks:"2",institution:{name:"Hamamatsu University School of Medicine",institutionURL:null,country:{name:"Japan"}}}],equalEditorOne:null,equalEditorTwo:null,equalEditorThree:null,coeditorOne:{id:"231568",title:"Dr.",name:"Hubertus",middleName:null,surname:"Himmerich",slug:"hubertus-himmerich",fullName:"Hubertus Himmerich",profilePictureURL:"https://mts.intechopen.com/storage/users/231568/images/system/231568.png",biography:"Dr. Hubertus Himmerich is a clinical senior lecturer for eating disorders at King’s College London and a consultant psychiatrist on an inpatient ward for patients with eating disorders at Bethlem Royal Hospital, London, UK. Following medical school, Dr. Himmerich received his scientific and clinical training at the Max Planck Institute of Psychiatry, Germany, and the Universities of Mainz and Marburg, Germany. Afterwards, he worked as a consultant psychiatrist at the RWTH Aachen University Hospital and Professor of Neurobiology of Affective Disorders at the University of Leipzig, Germany. He has led and performed national and international scientific projects with researchers from Europe, Australia, and North America, and he has published more than 160 articles in peer-reviewed scientific journals, books, and book chapters.",institutionString:"King’s College London",position:null,outsideEditionCount:0,totalCites:0,totalAuthoredChapters:"3",totalChapterViews:"0",totalEditedBooks:"2",institution:{name:"King's College London",institutionURL:null,country:{name:"United Kingdom"}}},coeditorTwo:null,coeditorThree:null,coeditorFour:null,coeditorFive:null,topics:[{id:"1061",title:"Psychiatry",slug:"mental-and-behavioural-disorders-and-diseases-of-the-nervous-system-psychiatry"}],chapters:[{id:"74852",title:"Attenuation of Food Intake by Fragrant Odors: Comparison between Osmanthus fragrans and Grapefruit Odors",doi:"10.5772/intechopen.95757",slug:"attenuation-of-food-intake-by-fragrant-odors-comparison-between-em-osmanthus-fragrans-em-and-grapefr",totalDownloads:207,totalCrossrefCites:0,totalDimensionsCites:1,hasAltmetrics:0,abstract:"Odors affect various physiological and mental activities. Previous studies in rats have shown that the odors of grapefruit and Osmanthus fragrans (OSM, fragrant tea olive) attenuate food intake, leading to a reduction in body weight gain, but it is not yet clear whether the causative mechanisms underlying these effects are the same for both odors. The first part of the present study revealed that grapefruit odor had no effect on the expression of feeding-related neuropeptides, in contrast to the previous finding that OSM odor suppresses orexigenic and activates anorexigenic neuropeptides in the hypothalamus of the rat. The second part revealed that OSM odor activated the parasympathetic nerve, in contrast to the previous finding demonstrating that grapefruit odor activates sympathetic nerve activity. The third part was performed to confirm the previous findings about the effects of OSM odor on appetitive reactions in humans. In human subjects, we found that continuous exposure to OSM odor attenuated appetite and consumption of snacks (cookies) and improved mood, when evaluated using the POMS (Profile of Mood States) data from university students. In conclusion, OSM odor attenuated appetite and decreased food intake in humans, and the underlying causative mechanisms differed from those mediating the effects of grapefruit odor, specifically in terms of the expression of hypothalamic feeding-related neuropeptides and autonomic nerve activity.",signatures:"Takashi Yamamoto, Kayoko Ueji, Tadashi Inui and Haruno Mizuta",downloadPdfUrl:"/chapter/pdf-download/74852",previewPdfUrl:"/chapter/pdf-preview/74852",authors:[{id:"332858",title:"Prof.",name:"Takashi",surname:"Yamamoto",slug:"takashi-yamamoto",fullName:"Takashi Yamamoto"},{id:"344751",title:"Dr.",name:"Kayoko",surname:"Ueji",slug:"kayoko-ueji",fullName:"Kayoko Ueji"},{id:"344752",title:"Dr.",name:"Tadashi",surname:"Inui",slug:"tadashi-inui",fullName:"Tadashi Inui"},{id:"344753",title:"Ms.",name:"Haruno",surname:"Mizuta",slug:"haruno-mizuta",fullName:"Haruno Mizuta"}],corrections:null},{id:"75814",title:"Lactate and Ketone Bodies Act as Energy Substrates as Well as Signal Molecules in the Brain",doi:"10.5772/intechopen.97035",slug:"lactate-and-ketone-bodies-act-as-energy-substrates-as-well-as-signal-molecules-in-the-brain",totalDownloads:332,totalCrossrefCites:1,totalDimensionsCites:5,hasAltmetrics:0,abstract:"Astroglia or astrocytes, the most abundant cells in the brain, are interposed between neuronal synapses and the microvasculature in the brain’s gray matter. This unique anatomical location allows astroglia to play pivotal roles in brain metabolism as well as in the regulation of cerebral blood flow. In particular, astroglial cellular metabolic compartmentation exerts supportive roles in dedicating neurons to the generation of action potentials and protects neurons against the oxidative stress associated with their high energy consumption. Key products of astroglia include lactate and ketone bodies (beta-hydroxybutyrate and acetoacetate), which can also be produced avidly by muscle and liver, respectively. Therefore, brain cells, skeletal muscles, and hepatocytes constitute a metabolic compartmentation in the whole body. In this chapter, I will focus on brain cells, especially astroglia, since the impairment of normal astroglial function can lead to numerous neurological disorders including stroke, neurodegenerative diseases, and neuro-immunological diseases. I will also discuss the metabolic responses of brain cells in terms of food consumption and exercise. A better understanding of the astroglial metabolic response is expected to lead to the development of novel therapeutic strategies for diverse neurological diseases.",signatures:"Shinichi Takahashi",downloadPdfUrl:"/chapter/pdf-download/75814",previewPdfUrl:"/chapter/pdf-preview/75814",authors:[{id:"334122",title:"Dr.",name:"Shinichi",surname:"Takahashi",slug:"shinichi-takahashi",fullName:"Shinichi Takahashi"}],corrections:null},{id:"77738",title:"Roles of Glucose and Sucrose Intakes on the Brain Functions Measured by the Working Ability and Morris Maze",doi:"10.5772/intechopen.99203",slug:"roles-of-glucose-and-sucrose-intakes-on-the-brain-functions-measured-by-the-working-ability-and-morr",totalDownloads:142,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"Sugars such as glucose or sucrose are considered hazardous foods because their intakes lead to obesity, further causing diabetes mellitus (DM), or cardiovascular diseases. However, glucose is needed for many brain functions such as memory and emotion among others. Glucose induces the secretion of insulin, which is needed for transportation of tryptophan from the blood to the brain. Serotonin, which is converted from tryptophan, is important for mood stability, control of emotion, and feeding is inhibited by serotonin in the hypothalamus. We discuss transportation of glucose from the blood to the glia cells. After glycolysis of glucose in the glia lactic acid is transported to cells such as glutaminergic neurons. After the release from neurons glutamic acid is taken up into glia cells and further to neurons again. Sucrose is degraded into glucose and fructose in the intestine thus intake of sucrose increases plasma levels of glucose. We show that intake of sucrose enhanced memory measured by Morris maze in rats and improved the working ability in humans. Roles of glucose and sucrose intakes are discussed together with the function of serotonin in feeding.",signatures:"Akikazu Takada, Fumiko Shimizu, Yukie Ishii, M. Ogawa and Tetsuya Takao",downloadPdfUrl:"/chapter/pdf-download/77738",previewPdfUrl:"/chapter/pdf-preview/77738",authors:[{id:"248459",title:"Dr.",name:"Akikazu",surname:"Takada",slug:"akikazu-takada",fullName:"Akikazu Takada"}],corrections:null},{id:"78899",title:"Circadian Clock, Sleep, and Diet",doi:"10.5772/intechopen.100421",slug:"circadian-clock-sleep-and-diet",totalDownloads:120,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"Circadian rhythm is a fundamental process of sustaining metabolic homeostasis by predicting changes in the environment. This is driven by biological clocks, which operate within a 24-h period to orchestrate daily variation of metabolism and sleep. The central clock in the hypothalamus is the master keeper of the circadian rhythm and is primarily reset by light, while the feeding-fasting rhythm, that is, nutritional stimulus, entrains peripheral clocks in peripheral organs such as the intestine and liver. Nutritional stimuli are important modulators of peripheral circadian rhythms and may affect the central clock and sleep homeostasis through metabolic alterations. In this chapter, I will summarize the significance of circadian rhythm and sleep in metabolic regulation as well as discuss the impact that diet has on circadian rhythm and sleep.",signatures:"Junichiro Irie",downloadPdfUrl:"/chapter/pdf-download/78899",previewPdfUrl:"/chapter/pdf-preview/78899",authors:[{id:"335497",title:"Assistant Prof.",name:"Junichiro",surname:"Irie",slug:"junichiro-irie",fullName:"Junichiro Irie"}],corrections:null},{id:"78567",title:"ER Stress Response Failure and Steatohepatitis Comorbid with Diabetes",doi:"10.5772/intechopen.100054",slug:"er-stress-response-failure-and-steatohepatitis-comorbid-with-diabetes",totalDownloads:144,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"Dynamic metabolic changes occur in the liver during the transition between fasting and eating, which is mainly mediated by insulin, a hormone to promote anabolism and suppress catabolism. In obesity and diabetes, insulin resistance is induced via various mechanisms, and among them is endoplasmic reticulum (ER) stress. We recently reported that eating induces transient ER stress and consequent ER stress response in the liver. During eating, expression of Sdf2l1, an ER-resident molecule involved in ER stress-associated degradation, is induced as a part of ER stress response. XBP-1s regulates expression of Sdf2l1 at the transcription level, and Sdf2l1 terminates eating-induced ER stress in the liver, consequently regulating glucose and lipid metabolism. In obesity and diabetes, however, ER stress response is impaired, partly because insulin-mediated translocation of XBP-1s to the nucleus is suppressed, which results in further excessive ER stress. Induction of Sdf2l1 by XBP-1s is highly down-regulated, but restoration of Sdf2l1 ameliorates glucose intolerance and fatty liver. In diabetic patients, hepatic insulin resistance induces enhanced ER stress and ER stress response failure in the liver, which in turn promote hepatic fibrosis and contribute to the development of steatohepatitis comorbid with diabetes.",signatures:"Takayoshi Sasako and Kohjiro Ueki",downloadPdfUrl:"/chapter/pdf-download/78567",previewPdfUrl:"/chapter/pdf-preview/78567",authors:[{id:"344302",title:"Assistant Prof.",name:"Takayoshi",surname:"Sasako",slug:"takayoshi-sasako",fullName:"Takayoshi Sasako"},{id:"429058",title:"Prof.",name:"Kohjiro",surname:"Ueki",slug:"kohjiro-ueki",fullName:"Kohjiro Ueki"}],corrections:null},{id:"76602",title:"The Effect of Glycation Stress on Skeletal Muscle",doi:"10.5772/intechopen.97769",slug:"the-effect-of-glycation-stress-on-skeletal-muscle",totalDownloads:242,totalCrossrefCites:0,totalDimensionsCites:1,hasAltmetrics:0,abstract:"Glycation stress (glycative stress) is a general concept of biological stress caused by a series of non-enzymatic glycation reactions, including advanced glycation end products (AGEs) formation, AGEs accumulation, glycation-associated dysfunction of proteins and cellular signaling, inflammation, oxidation, and/or tissue damage. There has been increasing evidence supporting a profound effect of AGEs on human diseases such as type 2 diabetes, cardiovascular disease, cancer, Alzheimer’s disease, osteoporosis, and dementia, as well as aging process itself. In addition, dietary AGEs intake has also been suggested to contribute to tissue dysfunction and development of the diseases. Skeletal muscle is the largest organ in the human body and important responsibility for maintaining our health as not only locomotor system but also metabolic and endocrine systems. Especially in past decades, numerous studies have suggested the contribution of glycation stress to skeletal muscle dysfunctions (e.g. muscle atrophy, reducing contractile property, and insulin resistance). In this chapter, we provide current evidence on the potential role of glycation stress in the impairment of skeletal muscle functions.",signatures:"Tatsuro Egawa, Kohei Kido, Takumi Yokokawa, Mami Fujibayashi, Katsumasa Goto and Tatsuya Hayashi",downloadPdfUrl:"/chapter/pdf-download/76602",previewPdfUrl:"/chapter/pdf-preview/76602",authors:[{id:"193127",title:"Prof.",name:"Katsumasa",surname:"Goto",slug:"katsumasa-goto",fullName:"Katsumasa Goto"},{id:"193128",title:"Prof.",name:"Tatsuya",surname:"Hayashi",slug:"tatsuya-hayashi",fullName:"Tatsuya Hayashi"},{id:"342798",title:"Dr.",name:"Tatsuro",surname:"Egawa",slug:"tatsuro-egawa",fullName:"Tatsuro Egawa"},{id:"355790",title:"Dr.",name:"Kohei",surname:"Kido",slug:"kohei-kido",fullName:"Kohei Kido"},{id:"355791",title:"Dr.",name:"Takumi",surname:"Yokokawa",slug:"takumi-yokokawa",fullName:"Takumi Yokokawa"},{id:"355792",title:"Prof.",name:"Mami",surname:"Fujibayashi",slug:"mami-fujibayashi",fullName:"Mami Fujibayashi"}],corrections:null},{id:"78900",title:"Metabolic Responses to Energy-Depleted Conditions",doi:"10.5772/intechopen.100391",slug:"metabolic-responses-to-energy-depleted-conditions",totalDownloads:180,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:1,abstract:"Dietary intervention is one of the most important approaches for the treatment of metabolic diseases such as diabetes mellitus. Fasting and caloric restriction have profound effects on systemic metabolism. The energy source-producing organs, such as the liver, and peripheral tissues rewire their metabolism to meet the energy demands of the whole body. Glycogenolysis, fatty acid oxidation, and ketone body production are characteristic metabolic changes that occur during fasting and caloric restriction. These metabolic changes are regulated by various signaling cascades including PPARα and FGF21. Moderate fasting and caloric restriction have also been implicated in extending the lifespan in a variety of organisms from nematodes to vertebrates. Intensive research has unveiled several regulatory mechanisms of longevity including metabolic regulators such as mTOR and sirtuins. The epigenome has been attracting attention as a mechanism underlying metabolic diseases and longevity. The epigenome is the concept that involves covalent modifications of DNA, histones, and RNA, which are mediated by the action of epigenetic enzymes. The activity of these enzymes is regulated by energy states, i.e. metabolites including ketone bodies and intermediates of various metabolic pathways. Thus, energy states are recorded in cells as an epigenetic memory, which may cause future onset of metabolic diseases and affect lifespan.",signatures:"Tomohiro Suzuki, Tetsuro Komatsu, Hiroshi Shibata and Takeshi Inagaki",downloadPdfUrl:"/chapter/pdf-download/78900",previewPdfUrl:"/chapter/pdf-preview/78900",authors:[{id:"344282",title:"Prof.",name:"Takeshi",surname:"Inagaki",slug:"takeshi-inagaki",fullName:"Takeshi Inagaki"},{id:"435038",title:"Dr.",name:"Tomohiro",surname:"Suzuki",slug:"tomohiro-suzuki",fullName:"Tomohiro Suzuki"},{id:"435300",title:"Dr.",name:"Tetsuro",surname:"Komatsu",slug:"tetsuro-komatsu",fullName:"Tetsuro Komatsu"},{id:"435301",title:"Dr.",name:"Hiroshi",surname:"Shibata",slug:"hiroshi-shibata",fullName:"Hiroshi Shibata"}],corrections:null},{id:"78805",title:"Role of Gut Microbiota in Bile-Acid Metabolism",doi:"10.5772/intechopen.100440",slug:"role-of-gut-microbiota-in-bile-acid-metabolism",totalDownloads:136,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"The role of the gut microbiota in modifying the pathophysiology of various diseases, including neurodegenerative diseases, is increasingly becoming clear. Bile acids have been shown to be endogenous factors that affect gut microbiota, and bile-acid metabolites directly or indirectly affect host physiology and pathophysiology. The development of metagenomic analysis for gut microbiota and systematic bile-acid measurement using LC–MS/MS has triggered a breakthrough for research in this field. Clinically, an inhibitor of the ileal bile-acid transporter (Elobixibat) was used as a therapeutic agent for chronic constipation, which also paved the way for progress in bile-acid signal research. Additionally, this review emphasizes the importance of gut microbiota-bile acid-receptor signals when considering nutritional approaches to promote healthy longevity.",signatures:"Yuji Naito, Tomohisa Takagi and Ryo Inoue",downloadPdfUrl:"/chapter/pdf-download/78805",previewPdfUrl:"/chapter/pdf-preview/78805",authors:[{id:"157629",title:"Dr.",name:"Yuji",surname:"Naito",slug:"yuji-naito",fullName:"Yuji Naito"}],corrections:null},{id:"77355",title:"Relations between Dietary Habits, Lifestyle and Leading Obesity",doi:"10.5772/intechopen.98307",slug:"relations-between-dietary-habits-lifestyle-and-leading-obesity",totalDownloads:131,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"Obesity, hypertension, depression currently in the rise are some of the many problems faced by a common person due to poor dietary and sleeping habits along with some genetic disorders. An extensive study has been done over two years with 205 subjects regarding their eating & sleeping habits and their mental & physical state on a day-to-day basis. The subjects include both males and females ranging from 15 years of age to 70 above. Altogether 12.68% of people suffer from obesity while just 51.21% of them have an appropriate weight. Women below the age of 25 have shown an overpowering presence of PCOS affecting their health and 38.53% of the population showcasing suffering from hypertension and 14.14% suffering from depression. Sleep has yet proven to be a defining factor in wellbeing. 17.07% of the population exhibit signs of sleep deprivation while just 63.9% of the population sleep over 7 hours daily. Like many other countries, in India, the shift from traditional healthy food to fast food & processed food is taking place, resulting in various health problems like obesity, heart problems, arthritis, weakness, diabetes, high blood pressure, difficulty in breathing, stroke & so on. The aim of this meta-analysis was to quantify the effects of nutrition, mental health and exercise on the various aspects of a person’s well-being.",signatures:"Shradha Mistri",downloadPdfUrl:"/chapter/pdf-download/77355",previewPdfUrl:"/chapter/pdf-preview/77355",authors:[{id:"339672",title:"M.Sc.",name:"Shradha",surname:"Mistri",slug:"shradha-mistri",fullName:"Shradha Mistri"}],corrections:null},{id:"77563",title:"Hypertension as Three Systematic Dysregulations of Na+ Homeostasis in Terrestrial Mammal, and Salt in Gut Might Cause Brain Inflammation",doi:"10.5772/intechopen.98904",slug:"hypertension-as-three-systematic-dysregulations-of-na-sup-sup-homeostasis-in-terrestrial-mammal-and-",totalDownloads:153,totalCrossrefCites:0,totalDimensionsCites:1,hasAltmetrics:0,abstract:"Although Na+ homeostasis in vivo is essential for mammals, it is known that excessive salt (NaCl) intake has played a major role in the development of hypertension. In vivo, there is a hormonal system, the renin-angiotensin-aldosterone system (RAAS), that specializes in regulating Na+ retention, especially the amount of Na+ in plasma. Na+ homeostasis in vivo has been achieved mainly by the RAAS, through regulation of vascular tonus (blood pressure) and Na+ handling in the kidney (Na+ diuresis). Recent studies have revealed a third mechanism of Na+ homeostasis in vivo: regulation of interstitial Na+ levels in tissues, such as subcutaneous tissues, by tissue macrophage immunity. In the pathogenesis of salt-sensitive hypertension, Recent research have been revealed that three molecular axes (Ang II - Rho/NOX-eNOS system, Aldosterone-rac1 -ENaC system, and tissue Na+ − TonEBP in macrophage -VEGF-c) are significantly involved in maintaining Na+ homeostasis in salt induced hypertension. Furthermore, the mechanism by which salt causes hypertension via the immune system (intestinal, local mucosal, and tissue immunity) has also been reported. In this article, we would like to propose that three molecular dysfunctions are involved in the development of salt-sensitive hypertension through three immunological mechanisms in the maintenance of Na+ homeostasis. Next, I would like to explain the importance of gut-RAAS and abnormality of intestinal microflora (dysbiosis) in salt-sensitive hypertension. It has been known that the metabolites (e.g., short-chain fatty acid neural amino) produced by microflora are deeply involved in central (CNS) and sympathetic nervous system (SNS) activity. In addition, we would like to explain of the importance of brain-RAAS and cerebral inflammation in salt-sensitive hypertension. Moreover, recent research have revealed that the detection-mechanism in the brain for Na+ concentration([Na+]) in vivo and in the tongue for [Na+] in diet. These finding suggests that excessive salt intake may cause brain dysfunction, most delicate organ, before the onset of salt sensitive hypertension, and may also destroy brain structure after the onset of salt sensitive hypertension. Thus, we would like to insist that excessive salt intake might not only induce hypertension, but also be toxic especially for brain. Finally, we would like to explain that The DASH diet (Dietary Approaches to Stop Hypertension) is one of the universal diets for adult human, not only by reducing salt, but also by reducing metabolic stress and improving of dysbiosis.",signatures:"Mizuo Mifune and Yoshihiko Kanno",downloadPdfUrl:"/chapter/pdf-download/77563",previewPdfUrl:"/chapter/pdf-preview/77563",authors:[{id:"332618",title:"Prof.",name:"Yoshihiko",surname:"Kanno",slug:"yoshihiko-kanno",fullName:"Yoshihiko Kanno"},{id:"419975",title:"Dr.",name:"Mizuo",surname:"Mifune",slug:"mizuo-mifune",fullName:"Mizuo Mifune"}],corrections:null},{id:"76800",title:"Effect of Lifestyle Modification on Glycemic Control of Type 2 Diabetic Patients at Suez Canal University Hospitals",doi:"10.5772/intechopen.97738",slug:"effect-of-lifestyle-modification-on-glycemic-control-of-type-2-diabetic-patients-at-suez-canal-unive",totalDownloads:217,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"Type 2 Diabetes mellitus, as one of the major universal public health disorders wide spread, requires patients’ lifestyle modulation which would be conducive in dominating blood glucose. The aim of the study was to evaluate the effect of lifestyle modification on glycemic control of type 2 diabetic patients at Suez Canal University Hospitals at Ismailia city. A quasi-experimental design made up of a control group and a study group with pre- and post-test administration was applied. This study was carried out at the Family Medicine Outpatient Clinic and the Diabetic Outpatient Clinic of Suez Canal University Hospitals at Ismailia city in Egypt. 92 type 2 diabetic patients were included in this study. The Diabetes Knowledge Questionnaire; Health promoting lifestyle profile II Scale; and Physical assessment sheet were used for data collection in the two groups. After implementing of the program, those patients who received lifestyle modification intervention achieved better total score of knowledge & knowledge related practice about DM, health promoting lifestyle domains values and glycated hemoglobin, compared with the control group. Factors related to lower glycated hemoglobin in the present study were lower fasting blood sugar level and increasing physical activity. Overall, lifestyle modification program has a positive influence on blood glucose control of patients with type 2 diabetes mellitus. Therefore, it is recommended to that lifestyle modification interventions should be integral part of the curative management of type 2 diabetic patients, and further study in other places to investigate the effect of lifestyle modification on glycemic control of those patients.",signatures:"Fatma Ibrahim Abdel-Latif Megahed, Salwa Abbas Ali Hassan, Hassan Ali Abdelwahid and Hanaa Kassem Farg",downloadPdfUrl:"/chapter/pdf-download/76800",previewPdfUrl:"/chapter/pdf-preview/76800",authors:[{id:"338636",title:"Dr.",name:"Fatma Ibrahim Abdel-Latif",surname:"Megahed",slug:"fatma-ibrahim-abdel-latif-megahed",fullName:"Fatma Ibrahim Abdel-Latif Megahed"},{id:"415846",title:"Dr.",name:"Salwa Abbas",surname:"Ali Hassan",slug:"salwa-abbas-ali-hassan",fullName:"Salwa Abbas Ali Hassan"},{id:"415847",title:"Dr.",name:"Hassan Ali",surname:"Abdelwahid",slug:"hassan-ali-abdelwahid",fullName:"Hassan Ali Abdelwahid"},{id:"415848",title:"Dr.",name:"Hanaa Kassem",surname:"Farg",slug:"hanaa-kassem-farg",fullName:"Hanaa Kassem Farg"}],corrections:null},{id:"77713",title:"Psychotherapeutic Interventions for Type 2 Diabetes Mellitus",doi:"10.5772/intechopen.97653",slug:"psychotherapeutic-interventions-for-type-2-diabetes-mellitus",totalDownloads:115,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"This chapter explores the efficacy of psychotherapeutic interventions for patients with type 2 diabetes mellitus (T2DM). This condition can lead to serious adverse health outcomes (e.g., cardiovascular disease, blindness, loss of limbs, etc.). Medical interventions alone are often not sufficient to manage the disease. Psychotherapy can promote behavioral change that improves medication adherence, dietary choices, exercise, stress, and other variables that affect blood sugar levels. The current chapter summarizes the trends in recent research for psychotherapeutic interventions for the management of T2DM. The results from 16 randomized controlled trials on cognitive-behavioral therapy, motivational interviewing, counseling, and mindfulness-based therapies are discussed. These interventions varied in length (3 to 18 months) and were conducted in many geographic regions (e.g., Australia, Netherlands, Saudi Arabia, Thailand, and more). Changes in biological health outcomes (i.e., HbA1c levels) were the primary focus of this chapter, but diabetes-related behavioral changes (e.g., diet and exercise) and psychological variables (e.g., stress, depression, and well-being) are also discussed. This chapter highlights that recent research has provided the most support for mindfulness-based therapies for improving blood sugar levels in patients with T2DM.",signatures:"Keisha C. Gobin, Jennifer S. Mills and Joel D. Katz",downloadPdfUrl:"/chapter/pdf-download/77713",previewPdfUrl:"/chapter/pdf-preview/77713",authors:[{id:"202110",title:"Dr.",name:"Jennifer S.",surname:"Mills",slug:"jennifer-s.-mills",fullName:"Jennifer S. Mills"},{id:"343000",title:"Ph.D. Student",name:"Keisha C.",surname:"Gobin",slug:"keisha-c.-gobin",fullName:"Keisha C. Gobin"},{id:"354578",title:"Dr.",name:"Joel D.",surname:"Katz",slug:"joel-d.-katz",fullName:"Joel D. Katz"}],corrections:null},{id:"77412",title:"Diet and Obesity",doi:"10.5772/intechopen.98326",slug:"diet-and-obesity",totalDownloads:128,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"Obesity is a complex disease that involves an excessive amount of body fat. It is a medical problem that increases the risk of other diseases, such as heart disease, diabetes, high blood pressure and certain cancers. Although there are genetic, behavioral, metabolic and hormonal influences on body weight, obesity occurs when you take in more calories than you burn through exercise and daily activities that is when energy intake exceeds energy expenditure. Diet plays an important role in the pathogenesis of obesity; fatty foods are energy dense and gives 9calories per gram compared to carbohydrate and protein that gives 4calories per gram. Also, if physical activity is inadequate, excess consumption of fat can results into weight gain. It does not take as much energy (about 3%), to convert and store dietary fat as it does to convert and store glucose. Fats are easily stored by the body. The aim of this chapter is to provide an understanding of physiological causes and effects of obesity as this will help to promote positive food choices. It is probable that an understanding of dietary patterns and how it relates to obesity will go a long way in the treatment of this complex problem.",signatures:"Olariike Oyindasola Kayode",downloadPdfUrl:"/chapter/pdf-download/77412",previewPdfUrl:"/chapter/pdf-preview/77412",authors:[{id:"334944",title:"Ph.D. Student",name:"Olariike",surname:"Oyindasola Kayode",slug:"olariike-oyindasola-kayode",fullName:"Olariike Oyindasola Kayode"}],corrections:null},{id:"74591",title:"The Outcome of Eating Disorders: Relapse, Childbirth, Postnatal Depression, Family Support",doi:"10.5772/intechopen.95452",slug:"the-outcome-of-eating-disorders-relapse-childbirth-postnatal-depression-family-support",totalDownloads:328,totalCrossrefCites:0,totalDimensionsCites:0,hasAltmetrics:0,abstract:"This study was aimed to identify eating disorder (ED) relapse, childbirth, postnatal depression,and the family support. Of the ED patients during treatment from 1994 to 2004,55 were pregnant and had ED recovery. Of them, 25 (21 Bulimia Nervosa (BN)and 4 Anorexia Nervosa (AN)) agreed to take part in this study. We interviewed them every 2 wk. both during the pregnancy and after childbirth. We also interviewed family members each month. The Eating Attitudes Test-26 (EAT-26) and Edinburgh Postnatal Depression Scale (EPDS) were helpful for diagnosing the EDs and postnatal depression. As the statistical analysis, We conducted t-test.67%relapsed ED while pregnant and 50%relapsed postnatal. In the non-relapse group, all the subjects had vaginal delivery and their infants were male. 50% of the subjects had postnatal depression. Non-Postnatal depression group had average body- weight infants. With regard to family support, there was no relationship between ED relapse and postnatal depression. We found that the rate of ED relapse and that of suffering from postnatal depression were remarkable in this group, suggesting the necessity for long-term follow-up for the EDs.",signatures:"Mariko Makino, Mitsuo Yasushi and Masahiro Hashizume",downloadPdfUrl:"/chapter/pdf-download/74591",previewPdfUrl:"/chapter/pdf-preview/74591",authors:[{id:"332255",title:"Ph.D.",name:"Mariko",surname:"Makino",slug:"mariko-makino",fullName:"Mariko Makino"},{id:"336867",title:"Dr.",name:"Masahiro",surname:"Hashizume",slug:"masahiro-hashizume",fullName:"Masahiro Hashizume"},{id:"345671",title:"Dr.",name:"Mitsuo",surname:"Yasushi",slug:"mitsuo-yasushi",fullName:"Mitsuo Yasushi"}],corrections:null}],productType:{id:"1",title:"Edited Volume",chapterContentType:"chapter",authoredCaption:"Edited by"},subseries:null,tags:null},relatedBooks:[{type:"book",id:"7841",title:"New Insights Into Metabolic Syndrome",subtitle:null,isOpenForSubmission:!1,hash:"ef5accfac9772b9e2c9eff884f085510",slug:"new-insights-into-metabolic-syndrome",bookSignature:"Akikazu Takada",coverURL:"https://cdn.intechopen.com/books/images_new/7841.jpg",editedByType:"Edited by",editors:[{id:"248459",title:"Dr.",name:"Akikazu",surname:"Takada",slug:"akikazu-takada",fullName:"Akikazu Takada"}],equalEditorOne:null,equalEditorTwo:null,equalEditorThree:null,productType:{id:"1",chapterContentType:"chapter",authoredCaption:"Edited by"}},{type:"book",id:"510",title:"Anxiety Disorders",subtitle:null,isOpenForSubmission:!1,hash:"183445801a9be3bfbce31fe9752ad3db",slug:"anxiety-disorders",bookSignature:"Vladimir Kalinin",coverURL:"https://cdn.intechopen.com/books/images_new/510.jpg",editedByType:"Edited by",editors:[{id:"31572",title:null,name:"Vladimir V.",surname:"Kalinin",slug:"vladimir-v.-kalinin",fullName:"Vladimir V. 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The history of lateral flow immunoassay (LFIA, immunochromatography) began in the 1980s. The first solved task was to transfer pregnancy tests from a specialized laboratory directly to the point of sample collection [1]. The test strip developed for this purpose fully complied with the requirements for nonlaboratory diagnostics, and its basic principles remain to this day.
\nThe overall design of the immunochromatographic test strip is shown in Figure 1. It is a composite of several membranes of different structures and porosities, fixed on a support. The bundling of the test strip can vary, so it makes sense to consider its design based on what analytical tasks are being performed on its different sites.
Typically, the lower portion of the test strip contains a
The following is a section with immunoreagents that are washed out during the analysis and move upward along with the components of the sample. As a rule, a
The next two sections are located on the main
First, there is a zone along which the movement of the absorbed components of the sample and the washed immunoreagents continues. During this movement, immune reactions occur, and specific intermolecular complexes are formed.
Next, a mixture of reacted and unreacted molecules enters the
The upper part of the test strip with the
Components of the immunochromatographic test strip and their functions.
Membrane components of the test strip are fixed on a
Depending on the tasks to be performed, additional reagents can be used in the test strip, and some of the membranes can be added, combined, or eliminated. However, at the same time, the general design and principle of conducting analytical interactions during the movement of reagents along membranes is preserved.
\nSimplification of the analysis is achieved by refraining from additional processing and incubation enhancing the signal as well as by visual (device-free) evaluation of the results. Because of this, traditional LFIA, meeting the needs of practice in simplicity and speed, is generally considered inferior to alternative immunoassays (such as ELISA) in sensitivity.
\nAt first, this restriction was not critical. Test systems made it possible to control target compounds in diagnostically demanded concentration ranges, which was enough for their mass application. The implementation of standard LFIA protocols for the detection of new compounds was viewed as an exclusively technological task for manufacturing companies, uninteresting in the scientific sense. In this regard, the number of publications on LFIA in the late 1990s to early 2000s was relatively small. It was believed that the all main methodological problems of LFIA had already been solved.
\nHowever, the application of LFIA did not stop at the control of the formed row of objects. This method actively developed (especially in the last decade) and covered an increasing number of analytes. What were the reasons for this?
As applied to medicine: the general trend toward the diagnosis at the site of the requirement (point-of-care (POC)): (i) the use of tests for quick decisions outside the clinic; (ii) the provision of mass screening tests by rapid and inexpensive diagnostic tools; and (iii) providing the doctor with information for decision-making during the time of communication with the patient without transporting samples to the laboratory.
With regard to other areas of application: interest in promptly obtaining information about mass consumption products, for example, about the quality of raw materials coming to food enterprises and the end products being sent to the trading network.
Biosafety control is extremely important in modern society. The conclusion about the presence of a toxin should be given promptly and directly at the testing site.
Taking into account this expansion of controlled analytes and types of tested samples, tasks were frequently encountered for which highly sensitive detection was required but not provided by traditional analytic formats.
\nDuring the last decade, the development of LFIA modifications has been intensified, allowing highly sensitive analysis, while maintaining the basic merits of the analysis—the rapidity, ease of implementation and interpretation of the results. These developments are systematized in a number of recent reviews that characterize the general trends in the development of LFIA, its application in different practical spheres, and the most successful methodological decisions [2, 3, 4, 5, 6, 7, 8].
\nOn the one hand, this progress is accompanied by the expansion of the assortment of commercial tests and the more active application of LFIA for solving a variety of practical problems. On the other hand, a significant part of new developments remains at the level of single publications and approbation using the example of a single analyte, without realistic assessment of their advantages and limitations. From such isolated examples, it remains unclear how much gain in sensitivity will be achieved if we apply the proposed approach to the new analytes and what conditions must be used for this. A simple demonstration of the minimum detectable concentrations in traditional and modified LFIA leaves open the question of how correctly all the conditions for the analyses were selected, including the concentration and composition of the immunoreagents. It is also unclear which of the approaches for reducing sensitivity can be combined and whether this combination leads to a multiplication of results improvements achieved for each of these approaches individually.
\nOf course, general theoretical arguments are not enough to answer these questions. Further studies of many research teams are needed. However, it is important to evaluate new developments with the use of a grounded concept to understand (i) what changes are introduced into the traditional LFIA protocol and for what purpose; (ii) by what criteria are the new LFIA protocols assessed and compared with existing ones. Such ordering is the subject of this review. We did not attempt to form a limited list of developments that are most widely represented in recent publications. Our goal was to create a general classification within which different existing and future developments can be characterized.
\nThe structure of the immunochromatographic test system considered (Figure 1) allows us to identify groups of problems that should be solved to ensure high-sensitivity, as well as other practically significant characteristics of the analysis (productivity, selectivity, etc.). We matched each element of the test system and the reagent or process used at this element. Therefore, the choice of the most appropriate (proper) actions during the analysis includes
Choice of the sample preparation method—
The choice of receptor molecules used to selectively bind the target analyte—
Choice of the conditions for interaction of reagents during the analysis—
Choice of the registered response of the test system—
Choice of the procedure for processing the measurement results—
These five groups of requirements (“big five demands”, Figure 2) make it possible to simply and uniquely classify the methodical solutions proposed for the improvement of the LFIA protocols.
\nCompounds of immunochromatographic test and “big five demands” associated with them.
This review will be based on our results (from the Laboratory of Immunobiochemistry in the A.N. Bach Institute of Biochemistry of the Federal Centre of Biotechnology of the Russian Academy of Sciences, Moscow, Russia) and on examples from the literature that will be ordered and characterized in accordance with this classification.
\nSome types of liquid samples, characterized by the LFIA method, do not require sample preparation: urine, blood serum, natural and drinking water, milk and juices. Their analysis can be initiated by contacting the test strip with the sample as is. To accelerate the movement of the fluid (blood serum and milk), the sample can be diluted immediately before analysis [9]. However, in most cases, the analysis should be preceded by sample preparation.
\nThe main difficulty of sample preparation is the need for a short period to destroy the matrix structures that interfere with the analyte molecules contained in it to interact with antibodies. Actions that separate matrix components that interfere with analysis, or to destroy these components, are also reasonable. Such complex types of matrices may be tested as tissues of organisms, food and agricultural products, soil, and so on. Sample preparation is extremely important to easily detect the target compounds in these matrices.
\nThe requirements for sample preparation were studied in detail with respect to other analytical methods—liquid and gas chromatography, enzyme immunoassay, and so on. However, the accumulated research results cannot be transferred to LFIA without further development. The main advantage of LFIA—rapidity—cannot be lost because of the long (lasting several hours) extractions recommended in many chromatographic techniques. Work with samples cannot begin from complex procedures that require expensive equipment.
\nAn additional feature of sample preparation for LFIA is that many analytes are extracted efficiently only with organic solvents and water-organic mixtures, but not with aqueous-salt solutions. (Such situations are usually associated with the hydrophobicity of the compounds and their surroundings in the samples.) However, these solvents inactivate antibodies; it means that the extract cannot be directly used as is as a sample for LFIA. As a result, the extracts are either significantly diluted (which is accompanied by a loss in sensitivity), or by means of additional steps, the analyte is transferred to another medium.
\nThe complexity described above determines the tasks that should be solved for effective sample preparation—see their summation in Figure 3. In Figure 3 and the following ones, we depict
Main research and development tasks to obtain proper samples for LFIA.
With respect to proper samples, the success of the developments offered directly by test system manufacturers should be noted. Alexeter Technologies (United States) uses special adhesives placed at the beginning of the test strip, which allow one to collect target molecules of the analyte from a large surface area by simple contact. In many cases, portable homogenizers and low-speed centrifuges are proposed for completing the analytical laboratory. In the case of the 4MycoSensor test systems (Unisensor, Belgium), mycotoxins are extracted from the ground grain in a special Mycobuffer on a shaker for 3 min (5 min for corn). Similar solutions are offered by other manufacturers. A special aqueous two-phase system for the concentration of protein analytes, containing polyethylene glycol, potassium phosphate, and phosphate-buffered saline, was used by Chiu et al. [10]. With its help, a 100-fold reduction in the detection limit was achieved. Concentration of samples combined with dialysis was used by Tang et al. [11] on the examples of myoglobin detection (fourfold signal growth) and nucleic acid of HIV (10-fold growth). Mosley et al. [12], using the examples of
Efficient approaches for sample preparation are pseudo-homogeneous analytical techniques, where a dispersed carrier with immobilized receptor molecules is added to a large volume of tested samples. This carrier quickly and efficiently, without diffusion restrictions, captures the analyte from the entire volume of the sample, and then the carrier is separated from the solution rapidly. Note that when the separated carrier is then redissolved in a small volume, the analyte is not only concentrated but also cleared from the organic solvent, thus excluding the influence of this solvent on LFIA. Antibodies, immobilized on a carrier, are often more stable to the denaturing influence of organic substances than free antibodies. According to the data of Urusov et al. [15], when working with magnetic immunosorbents, the content of methanol in the test sample can be increased from 10 to 30%.
\nThe use of particles of iron oxide and other carriers with magnetic properties is extremely promising for immunochromatography because of the simple and rapid separation of the carrier by contact with a permanent magnet. The principle of such an analysis is shown in Figure 4, and approaches to the production of magnetic immunosorbents are systematized in the review [16].
\nAdvantages of magnetic immunosorbents application in LFIA.
Liu et al. [17] showed that the combination of magnetic concentration and immunochromatography yields a 25–50-fold gain in the detection limit of aflatoxin M1 in milk compared to the variants in which magnetic or gold nanoparticles are used as conventional labels. A 40-fold gain in the detection limit was demonstrated by Lu et al. [18] upon the detection of
Concentration can also be achieved if LFIA is preceded by a stage with a transverse flow of large volumes of samples through a small volume of a membrane with antibodies or other binding reagents applied to it (immunofiltration). Such analyses usually complete the detection of binding results directly in the filtration zone [21, 22]. Note that the use of LFIA for control of toxicants in solid foods is associated with a certain restriction. To correctly determine the content of the unevenly distributed analyte, several samples of large volumes are selected from different parts of the tested object and combined for subsequent extraction [23, 24]. However, the small volume of liquid absorbed by the test strip allows only a small part of the analyte molecules present in the extract to be taken into account (even with magnetic concentration). Immunofiltration concentration will overcome this limitation and come close to obtaining the proper samples for highly sensitive analyses.
\nThe basic requirements for antibodies used in LFIA are related to their affinity and selectivity. However, the topic of which characteristics of antibodies provide the most sensitive analysis requires additional clarification. Immune reactions during immunochromatography are carried out in the kinetic regime. Therefore, it is unimportant whether the detectable complexes will dissociate for hours or days. Their number is determined primarily by the kinetic constants of the association, which for receptors that are the same in structure and antigens that are similar in size vary within a limited range. In the case of competitive LFIA, the dependence of the number of complexes formed on the analyte concentration in the sample is determined primarily by the affinity of antibodies to the free analyte. Effective binding to a competitor modified by the analyte will interfere with the highly sensitive detection of the free analyte in the sample. In other words, the binding of antibodies to the analyte-protein conjugate should be somewhat worse than with the native analyte. The influence of the characteristics of immunoreagents on the sensitivity of analysis is considered in detail in works devoted to the mathematical modeling of LFIA [25, 26, 27, 28, 29, 30].
\nGiven the above limitations, the affinity of antibodies is an important characteristic that affects their analytical use. However, the possibility of natural production of antibodies with more and higher binding to the analyte is limited. This is because an increase in the half-life of an antigen complex with B-cellular receptors greater than the endocytosis time of the complex is not supported by the selection of the corresponding B-cellular receptor lines [31]. The cases of “infinite affinity” of antibodies are rare exceptions for the analytes that form covalent bonds after the immune interaction [32]. An additional way to increase affinity is the genetic modification (directed design) of the active center of antibodies. The use of these methods in routine development is still very limited, despite confirmations of their effectiveness [33].
\nAs far as specificity is concerned, an important problem is which series of structurally close compounds should be detected using this antibody to solve practical problems. Two kinds of situations are possible: (i) it is necessary to recognize a single compound possessing biological activity, in contrast to its analogs and metabolites and (ii) information is required on the total content in the sample of a significant number of homologous compounds. For the second, class-specific assay, it is desirable that affinity of antibodies to homologous compounds correlate with their biological activities, but this is not always possible. In some cases, regulatory documents establish maximum residue levels (MRLs) on the basis of the sum of concentrations of structurally similar toxicants, without correction factors, taking into account their biological activity. Therefore, class-specific analysis usually requires the detection of the maximum number of compounds of this class with at least 10–15% cross-reactivity with respect to the maximum [8].
\nAdditional practically important characteristics of antibodies are the values of their stability under storage and in the course of the assay. The stability may be effectively enhanced by chemical modification of antibodies as well as by addition of protective agents that are common for drying of different immunoreactants.
\nThe strategic tasks for improving receptors for immunoassays are summarized in Figure 5. However, in the final development of test systems, commercially available antibodies are usually used, and there is no possibility of directed production of new, improved antibodies. This is the reason for the interest in the use of receptor compounds of a different nature as a substitute for traditional immunoglobulins.
\nMain research and development tasks to obtain proper receptors for LFIA.
Thus, the single-domain antibodies produced by
Requirements for proper receptors also include its effectiveness after immobilization on a membrane or on the surface of a marker nanoparticle label. Physical adsorption and random covalent coupling may be accompanied by significant loss of antibody reactivity. Therefore, systems are needed in which the oriented immobilization of antibodies is realized through the chemical conjugation of IgG in areas remote from the active center, or by their indirect binding with a preformed antibody-binding layer. In the role of this layer, staphylococcal protein A, streptococcal protein G, or (strept)avidin (reactive with biotinylated antibodies) can act. Approaches to the oriented immobilization of antibodies are systematized in a number of recent reviews [40, 41, 42, 43].
\nFilbrun et al. proposed a procedure for chemical modification of the lysine residues of antibodies before conjugation with gold nanoparticles and showed that it provided conjugates that were stable over a wide pH range [44]. Bauer et al. [45] developed a technique for the preparation and use of antibody conjugates modified with histidine-rich peptides (called “capture and release” antibody reagents). These preparations are affine to metal surfaces and magnetic particles and so may release immobilized antibodies when necessary. The benefits of oriented binding of antibodies to magnetic nanoparticles through modification of antibodies’ carbohydrate components were shown by Puertas et al. using the example of LFIA for choriogonadotropin [46]. A comparison of methods of immobilization for receptors in bacteriophage-based LFIA is given in the works of Kim et al. [47, 48]. In particular, article [48] discussed the use of in vivo-biotinylated peptide for oriented immobilization of receptor molecules on a test strip.
\nThe composition of conjugates of antibodies with nanoparticles also plays an important role. Although the increase in valencies for immune interaction is accompanied by an increase in conjugates’ affinity [49], structural changes of antibodies or steric restriction of their availability to interact with antigens may occur in parallel. With adsorption immobilization of antibodies (i.e. the widespread approach for LFIA purposes), their excessive loading causes the formation of additional layers, the molecules in which can dissociate during the analysis, and preventing the formation of a detectable labeled complex. Additional complications are associated with the use of antibody-nanoparticle conjugates having high surface density in competitive LFIA (Figure 6). Such conjugates can form high-affine polyvalent complexes in the analytical zone, which impede competitive interaction with the monovalent analyte from the sample. Further, the resulting complexes contain a significant number of unreacted antibodies and can bind analyte molecules without weakening the detected signal [50]. Therefore, the composition of the conjugate should be selected in relation to the features of each analytical system as well as other variable parameters—see the list of tactical tasks in Figure 5. Describing the development of LFIA for aflatoxin M1 [51], Anfossi et al. found that the lowering the ratio between antibodies and gold nanoparticles caused improvement in the assay sensitivity. The proposed change was to decrease amount of antibodies used for immobilization twice as compared with saturating conditions and by that way to lower the limit of detection, too, almost twice with a minimal weakening of the staining.
\nLimitations in the use of common antibody-nanoparticle conjugates in competitive LFIA.
Because LFIA is a fast analysis, all the processes that should be performed during the time of reagents’ movement along the test strip and proper conditions for the interaction of these reagents are necessary (Figure 7).
Main research and development tasks to obtain proper interaction for LFIA.
These general requirements remain little studied. Studies of the localization of reagents and immune complexes in a 3D membrane structure are limited [52, 53]. A significant variation in reaction media causes problems with mobility and nonspecific sorption of reagents on commercial membranes, the structure and coating of which are established by manufacturers. The developer can only compare several membranes and select reagents that affect the release of dried components and the speed of the flow. An example of such recommendations is provided by Lee et al. [54]. The contribution of fast nonspecific processes of formation of the so-called “protein corona” on the surface of gold nanoparticles to the effectiveness of immune interactions in LFIA is described in a recent paper by de Plug et al. [55]. Choi et al. [56] characterized the effects of temperature and humidity on the analytical characteristics of test systems and somewhat unexpectedly found that the transition to room temperature, conditioned by the requirements of point-of-care diagnostics, may be accompanied by a deterioration in sensitivity. In their work, the analysis at 37–40°C and relative humidity beyond 60% was three times more sensitive. Posthuma-Trumpie et al. [57] focused on the effects of the composition of solutions used in the manufacture of test systems on the analysis parameters. Interesting opportunities for further development are provided by the use of so-called nanomotors for enhanced reagent mixing, which has so far been described only for other types of immunoassays [58, 59].
\nMore accessible tools are the choice of concentrations of reagents applied to the test strip and their locations. By varying these parameters, it is possible to provide extremely sensitive detection or to select the threshold of discrimination between positive and negative samples (cut-off level) that meets the regulatory requirements for the maximum permissible level of contamination. A number of works have been published with analyses of the individual effects of these parameters on the analytical characteristics [60, 61] and with the application of multiparametric optimization procedures [62]. Hsieh et al. [52] described a general scheme for the consideration of various factors in the course of LFIA optimization.
\nIn Zvereva et al. [63], the possibility to change the cut-off level by varying the composition of the hapten-protein and the antibody-(gold nanoparticles) conjugates is considered. Using an example of competitive LFIA of chloramphenicol, it was shown that by reducing the load of immunoreagents on carriers, it was possible to shift the detection limit by two orders of magnitude. For sandwich analysis, Liu et al. [64] showed theoretically and experimentally the optimality of the antibody: the nanoparticle ratio was equal to 30:1, but the universality of these recommendations requires further study.
\nFu et al. proposed the use of a two-dimensional paper network to control the sequence of interactions in LFIA and, using the example of choriogonadotropin, showed the gain achieved in sensitivity [65]. Similar problems were solved in Rivas et al. [66] using wax-printed pillars as delay barriers (three-fold gain for human IgG detection) and Choi et al. [67] by incorporating agarose into the test strip to achieve flow control (10-fold gain for detecting dengue viral RNA). A sponge shunt was applied by Tang et al. [68] to reduce the fluid flow rate during LFIA (10-fold signal enhancement in nucleic acid testing of Hepatitis B virus). Liu et al. [69] considered the use of a pencil made from polyethylene glycols for the application of reagents to control the rate of their subsequent release. Shin et al. [70] developed a rotary device for this purpose, the rotation of which makes it possible to initiate a reaction and then sequentially introduce into the system the necessary reagents. The volume of reagents introduced into the system during analysis can be controlled by the vertical flow immunoassay method proposed by Oh et al. [71] and successfully implemented by them for the detection of C-reactive protein. For the same antigen, Rey et al. [72] described an approach to managing the kinetics of interactions that allowed exclusion of the so-called hook effect (falsely low results for very high concentrations of the analyte). The existing variety of approaches to controlling the order of interaction of reagents in test systems is summarized in Jeong et al. [73].
\nThe position of the binding zone influences the degree of equilibrium reached for the reactions occurring during the flow of reactants along the test strip. Moving these zones along the test strip, we can adjust the assay sensitivity. Theoretical aspects of this approach were considered by Ragavendar et al. [74]. However, despite successful overlapping of monotests in multi-tests with a sequential arrangement of binding zones [75, 76], general practical recommendations for ensuring a highly sensitive detection of all analytes have not yet been formulated.
\nBecause synchronous movement in the flow of antigen, antibody, and immune complex molecules is difficult to provide, an alternative is to start the analysis with a quick (several minutes) preincubation of the analyte molecules in the sample with the free or labeled antibodies that are specific to analyte. A number of commercial systems operate on this principle, such as tests for antibiotic control in food produced by Bioo Scientific, United States, and Nankai Biotech, China. Developing this idea, it is possible to implement universal test strips without compounds specific for a concrete analyte. The combination of such test strips with specific reagents added during the incubation stage with the sample allows adaptation of the consumption of test strips to the tasks being solved. Such strips are manufactured by D-r Fuke, Germany, for the detection of immunoglobulin E against various allergens: a complex of immobilized streptavidin, a biotinylated allergen from a preincubation mixture, specific immunoglobulins E, and colloidal gold-labeled anti-species antibodies is detected in the analytic zone of these tests.
\nThe problem of the polyvalence of antibody-nanoparticle conjugates in competitive LFIA noted in the previous section can be solved by replacing the conjugate of analyte-specific antibodies with gold nanoparticles by a combination of native specific antibodies and labels conjugated with anti-species antibodies. It gives possibility to vary the content of antigen-binding sites and the marker independently and therefore combine the high-sensitivity of competitive immunodetection (requiring a low content of specific antibodies) and the intensity of the detected signal (achieved with a high label content). This principle was implemented in our developments in the immunodetection of mycotoxins and demonstrated gains in sensitivity from one to three orders of magnitude [50, 77, 78].
\nNote that the implementation of competitive analysis in LFIA involves another problem. Visual out-of-laboratory diagnostics makes it possible to distinguish only assay results consisting of the presence or absence of a colored line in the analytical zone. For a visible disappearance of color, the sample must contain a sufficient number of analyte molecules to block all binding sites for labeled specific antibodies (Figure 8). In this respect, analysis formats with a direct dependence of the detected signal on the analyte content are preferred. For these formats already small concentrations of the analyte ensure the coloration of the analytical zone in contrast to the absence of color in the absence of the analyte (see Figure 8).
\nLimitations of competitive immunoassay and one of the ways to overcome them.
However, the implementation of such an analysis for low molecular monovalent antigens is not an easy task. Its solutions for various types of immunoassay are summarized in the reviews of Fan and He [79] and Liu et al. [80]. Unfortunately, many of these approaches, such as idiometric assay [81] and immunoassay using anti-metatype antibodies [82] require the production of antibodies not simply against the target analyte but against more complex antigenic structures, which limits their widespread use. A more universal idea is to use quenching of fluorescence caused approaching between donor and acceptor in the binding zone of the test strip. Such pairs can be two kinds of nanoparticles attached to different immunoreagents. Thus, Shi et al. [83] successfully used for this purpose quantum dots and gold nanoparticles in the analysis of ractopamine, Anfossi et al. [84]—quantum dots and gold or silver nanoparticles in the analysis of fumonisin, and Jiang et al. [85]—ruthenium-doped silicon nanoparticles and silver nanoparticles in the analysis of ochratoxin A. Another perspective approach is open sandwich immunoassay (OSI). The given assay is based on the association of the separated VH and VL chains of the antibody and reinforcement of this association after addition of the target antigen [86]. This approach with the use of so named Quenchbodies is implemented in different versions, mainly with fluorescent detection [87, 88], and it seems promising for LFIA.
\nIn our works, two types of immunoassay for low molecular compounds with direct analyte-signal dependence are described. They do not require special reagents. In Urusov et al. [89], an assay was described in which labeled antibodies in the absence of the antigen in the sample completely bind in the first zone to the immobilized analyte. The appearance of the analyte in the sample blocks some of the antigen-binding sites of the antibodies and allows them to reach the second binding zone on the test strip, ensuring the appearance of staining (see Figure 9). For the case of deoxynivalenol detection, the proposed approach is 60 times more sensitive than the traditional LFIA. In Berlina et al. [90], an analysis of the food colorant Sudan was described based on the use of two conjugates of gold nanoparticles with (i) antibodies specific to Sudan and (ii) Sudan-ovalbumin conjugates. In the absence of Sudan, the conjugated Sudan-ovalbumin was coated with antibodies on the surface of the gold nanoparticle. So the interaction with the anti-mouse IgG in the test area is prevented. The added Sudan displaced the Sudan-ovalbumin causing the binding of labeled anti-Sudan antibodies in the test area and the appearance of coloration.
\nCharacteristics of labels that determine their applicability and competitive potential in LFIA.
The response of the immunochromatographic system is the recorded signal of the label (its color or other parameters), which reflects the formation of a specific immune complex and allows for highly sensitive detection of the target analyte. Therefore, the question of proper response for LFIA is first and foremost a question of choosing a label.
\nThe variety of molecular or colloidal labels that can be used in LFIA is extremely large [91, 92]. According to Goryacheva et al. [92], compounds such as gold nanoparticles of various shapes and sizes, carbon nanoparticles, selenium nanoparticles, iron oxide nanoparticles, fluorescent dyes, fluorescent dye-doped nanoparticles, quantum dots, infrared emitters, up-converting emitters, nanoparticles with long-lived emission, liposomes, and enzymes may be used for this purpose. There are many articles that demonstrate the advantages of a new marker on the example of the detection of one randomly chosen analyte. However, the question of correct comparison of different labels remains open. Indeed, the differences between test systems depend not only on the label but also on the affinity of the antibodies, the regimen of intermolecular interaction, and the correctness of the choice of reactant content. Therefore, the gain achieved for one analyte does not necessarily persist after the transition to another analyte.
\nIn this situation, it is justified to have “passports” of analytical labels, which are determined by their own properties and can be taken into account when implementing various analytical systems. The proposed list of such parameters is summarized in Figure 9.
\nNote that along with single-valued quantitative parameters reflecting the physical properties of a label, a number of qualitative parameters must be taken into account. Unfortunately, to date, researchers do not have universally recognized quantitative characteristics of existing labels and rules for a priori evaluation of proposed labels. Therefore, when deciding on responses (Figure 10), we are forced to follow the data of disparate comparisons of labels in different experimental developments.
\nMain research and development tasks to obtain proper responses for LFIA.
Even within the framework of the use of gold nanoparticles, the developer has the opportunity to choose preparations of different sizes and shapes. The well-known recommendation [93] on the preferable use of spherical gold nanoparticles with an average diameter of 30–40 nm is confirmed by published experimental comparisons [49]. Serebrennikova et al. [94] showed the advantages of high-branched gold nanoparticles (“nanoflowers”) as optical markers—a fivefold decrease in the detection limit of procalcitonin. These patterns were confirmed by Xu et al. [95], and the preferable use of long-tip (13–15 nm) nanoflowers was stated. Ji et al. [96], using gold nanoflowers, reached the detection limit of aflatoxin B1, equal to 0.32 pg./ml.
\nOptical markers for immunochromatography of different chemical natures are compared in a number of works. The possibilities of using carbon nanoparticles described in Van Amerongen et al. [97, 98] and Liu et al. [99], using the example of salbutamol detection, also showed the advantages of colloidal carbon compared to colloidal gold and nanogold-polyaniline-nanogold microspheres. For ractopamine detection, Hu et al. [100] showed the advantages of time-resolved fluorescent nanobeads compared with fluorescent submicrospheres, quantum dots, and colloidal gold. Effective integration of palladium nanoparticles and horseradish peroxidase with a 10-fold gain in sensitivity as compared to colloidal gold in the detection of
Of great interest are fluorescent markers. In many respects, this is due to the fact that with the correct choice of the wavelengths of excitation and emission, it is possible, by increasing the intensity of the exciting light, to proportionally increase the response in the practical absence (in contrast to the colorimetry) of the nonspecific signal. The gain in sensitivity achieved in this case is one or two orders of magnitude [103, 104]. The use of fluorescent markers in LFIA is summarized in the reviews of Pyo and Yoo [105] and Gong et al. [106]. A comparison of the analytical capabilities of quantum dot nanobeads, large-sized (50–600 nm) particles with impregnated quantum dots was given in Duan et al. [107].
\nAdditional capabilities of high-sensitivity analysis are achieved by the registration of energy transfer with the spatial convergence of two labels—fluorescence resonance energy transfer (FRET). Systems using fluorescein isothiocyanate and gold nanoparticles were developed by Wang et al. for the detection of cancer embryonic antigens [108]. Other variants of fluorescent LFIA were also described, for example, registration of background fluorescence quenching in Chen et al. [109], silver nanoparticle-based fluorescence quenching in Jiang et al. [85], and quenching of the fluorescence of quantum dots by gold and silver nanoparticles in Anfossi et al. [84]. (See also Section 5 with their consideration as examples of competitive immunoassays with a direct dependence of the detected signal on the analyte content.)
\nExtremely promising is the use of surface-enhanced Raman spectroscopy (SERS) for detection of optical labels. SERS signals are based on the increase of optical absorption for reporter molecules by orders of magnitude after their immobilization on the surface of nanoparticles. The possibility of such highly sensitive analyses is demonstrated in the works of Sanchez-Purra et al. [110], Fu et al. [111], and Marks et al. [112]. Clarke et al. [113] described the combination of SERS registration with rapid vertical flow technology as an additional means of increasing sensitivity. In Maneeprakorn et al. [114], SERS detection with 4-aminothiophenol as a signal reporter lowered the detection limit by 300 times compared to traditional LFIA. In Cho et al. [115], the transition to SERS based on silver-intensifying gold nanoparticles led to a 1000-fold decrease in the detection limit. Blanco-Covian et al. [116] proposed the use of a combination of Au @ Ag core-shell nanoparticles and rhodamine B isothiocyanate in LFIA, which allowed them to perform highly sensitive detection of pneumolysin with a detection limit of 1 pg/ml, recording the surface-enhanced resonance Raman scattering (SERRS).
\nNote that optical recording methods allow us to evaluate only labels that are in the upper layers of the test strip and are not shielded by membrane fibers. The loss of the optical signal depends on the properties of the material but is usually estimated [93] as about one order of magnitude. In this regard, the work of Jacinto et al. [117] is extremely interesting. They offer an electromagnetic relocation of reporter particles for amplifying an optical signal and describing the fourfold reduction in the detection limit of human chorionic gonadotropin.
\nThis restriction is excluded for analytical methods in which registration of a label is based on other physical principles. Thus, Wang et al. [118] developed the Thermal Contrast Amplification Reader for the registration of gold nanoparticles, which, for systems of influenza and malaria diagnostics and detection of
The capabilities of high-sensitivity detection in LFIA are not limited to the choice of a label. Additional reserves provide
treatment of the test strip with additional reagents that enhance the coloration or other detectable parameters;
aggregation of label particles, thereby increasing their number, attached to a single immune complex;
or initiation by the label of additional reactions, leading to the generation of the detected signal.
The existing variety of developments in this area is summarized in a review of Shan et al. [125]. The systems that implement the aggregation of several types of functionalized nanoparticles cause particular interest. Such approaches are described, for example, by Choi et al. [126] with a 100-fold gain in sensitivity for the detection of troponin I using two kinds of gold nanoparticles; by Razo et al. [20] with the generation of an optical signal by complexes of iron oxide nanoparticles (also used as a concentrating agent) and gold nanoparticles with a 32-fold decrease in the detection limit of potato virus X; by Taranova et al. [127] with a 30-fold gain in the analysis of procalcitonin due to biotin-streptavidin aggregation of gold nanoparticles; by Shi et al. [128] with complexation of gold nanoparticles of two sizes in the analysis of imidaclothiz; by Zhong et al. [129] with the formation of two layers of antibody conjugates with gold nanoparticles in the detection of melamine; and by Shen et al. [130] with aggregation of gold nanoparticles using polyamidoamine dendrimer, which lowered the detection limit of rabbit immunoglobulin G 20 times.
\nThe growth of the size of gold nanoparticles with the help of the catalyzed reaction of their surface between HAuCl4 and NH2OH was examined by Bu et al. [131] as a means of amplification for LFIA. The layered build-up of gold nanoparticles was described by Li et al. [132]. Anfossi et al. [133] and Panferov et al. [134, 135] considered the possibilities of silver enhancement (restoration of the silver salt on the surface of a gold nanoparticle with an increase in its size) in LFIA. In a study by Rodriguez et al. [136], the optimal regimes of silver and gold enhancements were determined to enhance the signal from the gold nanoparticles. Enzymatic amplification using alkaline phosphatase was studied by Panferov et al. [137] for LFIA of potato virus X and by Kim et al. [138] for LFIA of C-reactive protein. A feature of the latest development was the use of a water-swellable polymer for the accumulation of a colored product. An original polymerization-based amplification approach for enhancing staining was described by Lathwal and Sikes [139].
\nThe basic requirement for amplification approaches is the maintenance of low laboriousness of analysis. Variants using additional reagents, although considered in development, should be finally transformed into devices of dry chemistry, in which all components of the test strip are applied to its membranes.
\nThe generation of a signal reflecting the formation of immune complexes during LFIA is not the final stage of the analysis. The analysis is only completed when a diagnostically meaningful conclusion is made on the basis of this signal.
\nEffective use of LFIA is possible only when it is combined with modern means for documenting, storing, and processing information. In the absence of these tools, the advantages of rapid and high-performance nonlaboratory diagnostics are lost because of time-consuming processing and description of test results. Of fundamental importance is the transition from a subjective yes-no evaluation of results to automatic quantitative registration and the formation of databases that integrate the results of mass screenings or information on the dynamics of the state of patients (objects). Such systems will allow rapid collection of various indicators “at the time of request,” contributing to an accurate diagnosis. Taking into account the foregoing, Figure 11 summarizes the requirements for proper output in LFIA.
\nMain research and development tasks to obtain proper output for LFIA.
In some cases, the developer does not need to achieve maximum sensitivity but to fix the threshold that separates the positive and negative results in accordance with the regulatory requirements for MRLs. This allows the composition of conjugates used in the analysis discussed above to be varied [63]. A qualitative “yes-no” analysis can be transformed into a semiquantitative one with a change in the number of colored bands corresponding to several threshold levels. To do this, depletion of the conjugate can be used when interacting with several consecutive identical binding zones. Additional opportunities arise when using antibodies with different affinities, varying the surface density of the reagents applied in the binding zones and the distance between these zones and the beginning of the test strip. An example of an appropriate development with three thresholds of potato X virus concentrations corresponding to the degree of plant infection was described by Panferov et al. [140].
\nInitially, attempts were made to create detectors for membrane tests that recorded the total intensity of the staining (brightness of the reflected light) in certain sections of the test strip using a row of light-emitting diodes and individual systems of signal transformation for each diode. However, such detectors were extremely cumbersome. Blatt et al. [141] proposed a device made from 28 photosensitive sensors located along the test strip. Nowadays, the dominant means of detecting the results of LFIA, allowing a full-color image of the test strip to be received, are digital cameras. This technology is based on the use of inexpensive portable detectors or household recording devices—such as a mobile phone camera [142]. Serially produced cameras record images with a resolution of up to 2400 dpi, which corresponds to the size of an individually characterized section of less than 1 μm2. Figure 12 summarizes the advantages of digital photometry in LFIA.
\nComparison of traditional and digital photometry as a means for registration and processing of immunochromatographic data.
Trends in the transformation of LFIA from the visual to the instrumental method are summarized by Cheung et al. [5]. Reviews by Quesada-Gonzalez and Merkoci [143] and Zarei [144] present the current state of analytical technologies based on the use of mobile phones/smartphones. At the same time, a significant number of manufacturers of test systems offer portable detectors that are adapted to work with their own products [8]. Of the original solutions, mention should be made of Feng et al. [145], in which the registration tool for LFIA was Google Glasses. In recent years, a number of companies have introduced cloud technologies into practice, where external servers receive data about testing results via standard communication devices and store and process this information. Thus, since 2017, Abbott has proposed a set of tools named i-STAT Alinity for distant diagnostics. Special cartridges allow 14 parameters of blood composition by bio- and immuno-chemical techniques to be controlled.
\nAn extremely important means of increasing informativeness, although not related to an increase in sensitivity, is to conduct a multiplex analysis—that is, detection of the presence and level of several analytes using a single test strip. Data on the control of several analytes can be discriminated in space (by the position of binding zones) or by signals (by using different labels). Quantum dots are an effective tool for multi-analysis with different signals. The use of conjugated quantum dots with different spectral characteristics allows one to perform highly sensitive diagnostics with simultaneous detection of, for example, three antibiotics (“traffic light” in Taranova et al. [146]) or four mycotoxins (“rainbow” in Foubert et al. [147]).
\nBecause the number of binding zones that can be sequentially located on one test strip while preserving the rapidity of the analysis and the reliability of the information obtained for each analyte is limited (usually no more than five zones), the transition to “two-dimensional immunochromatography” is promising—see Figure 13. This approach, combining the advantages of immunochromatographic tests and immunochips, is based on the formation of an ordered two-dimensional array of points with immunoreagents of different specificity on the membrane of a test strip. In such systems, interaction occurs in several dozens of binding zones. Due to this, the 2D immunochromatography increases the information content of LFIA results and reduces the consumption of reagents and materials for one analysis.
\nConcept of 2-D immunochromatography.
Examples of test systems based on the principle of “two-dimensional immunochromatography” are presented in the works of Taranova et al. [104] on the detection of drugs and Safenkova et al. [148] on the detection of phytopathogens. General approaches to multizonal LFIA were discussed in Hu et al. [149], and the current state of the development of multiplex immunoassays was discussed in Li et al. [150].
\nIt would be reasonable to summarize the presented review of LFIA developments using two outcomes—strategic (research) and tactical (development) outcomes.
\nWe may identify the following main tasks, the solutions of which are extremely important regardless of the specific analyte and type of tested samples that are of interest to the developer: To create an effective test, the developer must
Obtain the most concentrated sample
Select the membranes that ensure rapid movement of reagents and high intensity of staining when working with this matrix
Select the optimal label
Use conjugates of immunoreagents having optimal composition
Choose the optimal location of the reagents applied to the test strip
Find the optimal ratio of immunoreagents, combining a sufficient level of label binding and a low detection limit for the analyte.
Considering the strategic situation of the development of LFIA, we should expect test systems of the future to implement high-performance and informative analyses integrated with the tools for collection, storage, and processing of information. With the development of molecular biological methods for the production of modified and new receptors, bioanalytical systems will be able to effectively discriminate various structurally close compounds and, on the basis of their levels in the sample, make more informative diagnostic conclusions.
\nThis work was supported by the Russian Science Foundation (grant 14-16-00149).
\nPhotovoltaic (PV) technology is the most emerging way of harnessing huge amount of energy from sun light as compared to solar thermal and photo electrochemical cells [1]. PV devices convert incident photons from sunlight to electricity upon exposed to light. PVs are popular because of its compactness and can be used anywhere for different application [2]. Additionally, involvement of nanostructures further boost the performance of solar cell. Over the past decade, nanostructured solar cell has become hot topics within research community due to its potential to enhance the spectral response of cell. Although, first generation silicon wafer based solar cell leads the current global PV market, however this conventional technology do not have any further scope to improve efficiency and reduce cost [3]. Additionally, it is also not recommended to use Silicon based solar cell for space application due to its low radiation tolerance. Second generation thin film technology such as hydrogenated amorphous silicon (a-Si: H), CIGS, and CdTe could not line-up with wafer-based silicon due to use of rare earth elements and low stability [4, 5]. Furthermore, highly efficient compound semiconductors based third generation solar cell have a demerit of high cost which limits its use in terrestrial applications. Hence, the hunt for low cost high performance solar cell are still unachievable. In the meantime, involvement of nanotechnology could bring a ray of hope for future generation solar cell. Nanowire (NW) geometry has remarkable advantages over planner geometry due to optical, electrical, and mechanical effects. New charge separation mechanisms, low defects and low cost also add more mileage to this journey. Looking towards the current scenario, existing PV technologies aren’t the solid foundation for the future projection of the renewable energy generation. None of the existing technology can satisfy global energy demand in future [2, 5]. Moreover, if the material or technological limitations restrict the future roadmap of PV technology, then the incorporation of new efficient materials and transpose of technology will be an assurance against high cost and low efficiency solar cells. Newly explored InxGa1-xN material brings an bunch of opportunities for future PV technology, having capability to absorb full solar spectrum using a single absorber material. One of the major properties of InGaN material is its tunable bandgap from 0.6 to 3.4 eV by changing ‘In’ content [6, 7, 8, 9, 10]. It also has easy growth of nanowire and nanorod structures with proven technology [11, 12, 13, 14]. It is a direct bandgap material where photon absorption and direct interband transition can be occurred without interference of phonons to conserve momentum. Additionally, high absorption coefficient of 105 is an additional benefit for good absorption with thin layer. Hence the cost can be minimized as well as recombination rate can also be minimized. InGaN also possess a high saturation velocity and a low effective mass of charge carriers, which ensures the more carrier separation along the junction. High radiation tolerance of InGaN are always appreciated for harsh environments. Moreover, InGaN solar cell do not contain any toxic elements such as arsenic, cadmium or phosphorous as used in MJ solar cell. Thus, it is evident that In
In the present context mainly different geometry of III-Nitride GaN/InGaN material based solar cell are considered, such as planar, nanodisk and nanowire types. Theoretically, it is anticipated that power conversion efficiency more than 40% could be achievable with GaN/InGaN junctions [19, 20]. However, practically achievable efficiency is quite low [21, 22]. One of the major challenges is the association of in-house defects with InGaN layer at higher ‘In’ content. Which in turn leads to stuck of immobile charges (known as polarization charges) along interfaces and reduces minority lifetime. Recently III-Nitride nanowires (NWs) are proposed as stand-alone PV devices due to enhanced light trapping, defect and stress-free growth [23, 24]. In general, two widely used structure for nanowire solar cell are (i) axial junction and (ii) radial junction. Axial junction is also known as nanodisk (ND) whereas radial junction is known as core-shell-shell (CSS) solar cell. Vapor–liquid–solid (VLS) technique is one of the popular methods to grow the GaN/InGaN nnaowires [23]. The fabricated NWs have hexagonal cross-section with {0001} orientation of top facet and {1–100}/ {10–10} orientation alongside walls of NWs [23]. Literature shows the comparative analysis of planar and circular NWs reported by Y. Zeng
Schematics of
Where
All the material parameters for GaN and InGaN with different compostion can be found from [30]. The interpolation method is used to calculate all parameters for InxGa1-xN composite alloys. Defect density in the order of 1017, 1014 and 1012 are incorporated for planar, ND and CSS-NW SCs respectively [31].
The model developed by Romanov
Where
Vertical illumination of light source on the front surface of the device is consider during all analysis as shown in Figure 1. Transport of carriers and separation mechanisms in the device depends solely on its geometrical structure. Here, carrier transport in planar, ND and NW type solar cell are explored with the help of energy band diagram. Figure 2(a) shows that tilt of energy band along
Energy band diagram of (a) planar (b) ND and (c) CSS-NW solar cell at 100 nm, 150 nm, and 180 nm
Thus, with increase in bias voltage, photogenerated carriers accumulate inside the potential valley rather than traveling in
Figure 3 shows dependency of short-circuit current density (
Short circuit current density (
Where volume of the absorption region is,
Thus
Where, active absorption layer is,
Figure 4 shows the current density-voltage-power density (J-V-P) curve of n-GaN/i-In0.1Ga0.9N/p-GaN planar, ND and NW type solar cell. The optimized thickness of 100 nm, 150 nm and 180 nm i-InGaN is considered for all performance analysis. It shows a higher Jsc in CSS-NW as compared to ND and planar structure. It is anticipated that higher current in CSS-NW solar cell is mainly due to higher active absorption region and efficient carrier separation. It is important to highlight that planar and ND type solar cells shows a stair-case type
Open circuit voltage,
Current density (black line) – Voltage – Power density (red line) of (a) planar (b) ND and (c) CSS-NW solar cell at 100 nm, 150 nm, and 180 nm i-InGaN thickness respectively.
It is also observed that due to high degree of strain relation, low defects density and more active area of absorption, CSS-NW structure can accommodate higher thickness of active InGaN layer (W) region. Moreover, higher thickness of absorber enhances the probability of more absorption of photons from sunlight. In other hand, active region of planar and ND type solar cells cannot be increased due to are limitation of surface recombination arte, polarization induced electric field, low degree of strain relaxation and defect density. Voc of ND type solar cell is seen to be higher than CSS-NW type solar cell which is may be due to the recombination rate along the junction. However, the rate of increase in Jsc of CSS-NW structure is comparatively higher than ND and planar solar cell. Similarly, planar solar cell possesses a low as compared to ND and NW solar cell. It is mainly due to appearance of staircase type
W (nm) | Jsc (mA/cm2) | Voc (V) | FF (%) | Efficiency η (%) | |
---|---|---|---|---|---|
Planar | 100 | 0.90 | 2.41 | 82.7 | 1.8 |
Nanodisk (ND) | 150 | 1.93 | 2.52 | 87.6 | 4.28 |
CSS-Nanowire (NW) | 180 | 2.84 | 2.47 | 91.6 | 6.46 |
In this chapter, the importance of nanowire solar cell with III-Nitride material is explored in a detailed manner. A comparative analysis is carried out with planar, nanodisk and nanowire type solar cell and concluded that nanowire type structure shows a better performance as compared to others. Additionally, it is found that nanowires in InGaN materials are grown either in triangular or hexagonal orientation. The strain relaxation is more in CSS-nanowires which in turns leads to low in-house defect density along the interfaces. CSS-NWs are also able to accommodate higher thickness of intrinsic material due to high carrier diffusion length. Radial separation of carriers also provides more surface area and better control on carrier separation mechanisms. Hence, it is concluded that radial growth of nanowire provides a broad range of opportunity for performance enhancement of solar cell. The similar type of observation are also applicable to LASER and light emitting diodes, where III-Nitride materials are used.
The authors acknowledge Dept. of Science and Technology, Govt. of India for financial support for providing the instrumental facility under DST-FIST in Dept. of ECE, SRM Institute of Science and Technology, Chennai, India.
The authors also acknowledge Visvesvaraya PhD Fellowship of MeitY, Govt. of India and TEQIP-II for procurement of Silvaco TCAD tool in Department of ECE, NIT Silchar for carrying out the research work.
The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this chapter.
indium gallium nitride gallium nitride copper indium gallium selenide cadmium telluride
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Although POP can occur in younger women, it is commonly seen in aging population with a prevalence of 45–50%. Older terms describing pelvic organ prolapse (e.g., cystocele, urethrocele, rectocele) have been replaced because they do not provide complete information regarding the structures on the other side of the vaginal bulge, especially in women who have had previous pelvic organ prolapse surgery. Therefore, a thorough history and performing a careful physical examination with dignity and care, using some basic tools that aid in the accurate evaluation of anatomical and functional defects, should be conducted. 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