Open access peer-reviewed chapter

Molecular Breeding of Sweetpotato Carotenoids

Written By

Muhammad Zubair Khan, Miho Takemura, Takahashi Maoka, Jun-ichiro Hattan, Motoyasu Otani and Norihiko Misawa

Submitted: 01 July 2021 Reviewed: 01 December 2021 Published: 20 April 2022

DOI: 10.5772/intechopen.101849

From the Edited Volume

Natural Food Additives

Edited by Miguel A. Prieto and Paz Otero

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Abstract

Sweetpotato [sweet potato; Ipomoea batatas (L.) Lam.] is the seventh most valued food crop of the world. It has an inherent ability to grow under diverse agro-ecological and microclimatic zones ranging from tropical and subtropical zones to temperate areas with its tuberous roots enriched with the secondary metabolites of immense nutritional value. Among these, carotenoids are the most conspicuous one for having their use in nutritional, pharmaceutical, food, feed, aquaculture, and cosmetic industries. In food industries, carotenoids are used as food additives being antioxidants with attractive colors. Despite the immense economic importance, sweetpotato has received lesser attention in terms of its breeding with improved varieties. The conventional method of breeding by crossing has not been much successful due to the complexity of genome sterility and cross-incompatibility. Hence, the modern molecular breeding approaches, e.g. genetic, genomic, and metabolic (pathway) engineering, have been applied to this crop by some of researchers in Japan, Korea, and China to generate various cultivars with improved quantities and qualities of carotenoids. This has also opened a new gate for molecular breeders to engineer new sweetpotato cultivars enriched with carotenoids under current global scenario of dramatically rising climatic changes where novel food resources are bitterly needed, especially under alarmingly growing world population, the majority of which suffers from malnutrition.

Keywords

  • sweetpotato
  • carotenoids
  • molecular breeding
  • metabolic engineering
  • pathway engineering

1. Introduction

Sweetpotato [Ipomoea batatas (L.) Lam.], also described as “sweet potato,” belongs to the family Convolvulaceae and occupies the seventh position among the food crops of the world after wheat, rice, maize, potato, barley, and cassava [1, 2]. The largest genus in the family Convolvulaceae is Ipomoea, consisting of 600–700 species, among which, only I. batatas is cultivated widely as a food crop around the world [3, 4]. In comparison with other tuber crops, sweetpotato comprises higher contents of carbohydrates, many minerals, and more protein estimates than other vegetables [5, 6]. It also contains much higher levels of provitamin A, vitamin C, and minerals than those of rice or wheat [7]. Hundred grams of raw sweetpotato contain 1.57 g of protein, 20.12 g of carbohydrates, 3 g of total dietary fiber, 41.8 g of total sugars, 30 mg of calcium, 0.61 mg of iron, 25 mg of magnesium, 47 mg of phosphorous, 337 mg of potassium, 55 mg of sodium, 0.3 mg of zinc, 2.4 mg of vitamin C, 0.5 mg of niacin, 0.2 mg of vitamin B6, 14,187 IU of vitamin A (VA), 0.2 mg of vitamin E, 11 μg of vitamin B-9, and 8509 μg of β-carotene (β,β-carotene) [8]. The starch in sweetpotato is easy to digest. Therefore, it is a valuable constituent in the preparation of excellent weaning meals [9]. It is a source of food supply to combat malnutrition in the developing nations, since the tuberous roots (tubers) are enriched with starch and dietary fiber, along with carotenoids, anthocyanin, ascorbic acid, potassium, calcium, iron, and other bioactive ingredients [10, 11, 12, 13]. For people of South East Asia and Africa, this crop is the main source of β-carotene [10, 14]. The tubers of the Japanese cultivars are diverse concerning carotenoids accumulation [15]. Sweetpotato may exert diverse health positive effects, since it contains high amounts of numerous phytochemicals in roots or leaves [6, 16]. I. batatas cultivars with color-fleshed tubers have been reported for their excellent bioactivities, such as antimutagenic [17], free radical scavenging [18], hepatoprotactive, reduction of liver injury [19, 20], anticancer [21, 22, 23], antioxidative activities [23, 24, 25], antimicrobial activity, antihypertension, anti-inflammatory, antidiabetic, anticaries effect, ultraviolet protection [23], and chemopreventive activities [26]. Previous reports also suggest that its tubers may be useful for treating peptic ulcers [27]. The genome of I. batatas is structurally complex and has a size of 4.8–5.3 pg/2C nucleus [28]. Due to the existence of polyploidy, sweetpotato is a hexaploid species (2n = 6x = 90) that has a basic chromosome number of 15, [3] with a huge genome size of 2200–3000 Mbp [29]. The genetic studies on this species are exhausting, since it is difficult to generate seeds and to evaluate the effects of polyploidy on the genome [30, 31]. Complex structure of its genome also manifests self and cross-incompatibility, causing barrier for genetic studies on important agronomical characters [3, 32]. Its tubers exhibit various colors, such as white, yellow, orange and purple orange, and yellow and orange-fleshed lines, were shown to contain β-carotene as the predominant carotenoid [11, 12, 13, 33, 34]. Annual yield of sweetpotato is currently exceeding the value of 105 million metric tons, 95% of which is shared by the developing countries. China is the world’s leader among all in sweetpotato consumption that counts about 66% of the total global consumption. China is followed by Nigeria and Tanzania, though, each of these last two countries shares only 4% of the total global consumption [35]. By applying the conventional breeding, biofortification of sweetpotato involved the selection of orange-fleshed varieties, to combat vitamin A deficiency among the developing nations [36]. In Japan, high β-carotene-accumulating varieties, such as “Benihayato, “J-Red, and “Sunny-Red,” were initially developed by Japanese breeders at the Kyushu-Okinawa Agricultural Research Center (formerly the Kyushu National Agricultural Experiment Station), Miyakonojo, Miyazaki, Japan [37, 38, 39]. The enhancement of sweetpotato with provitamin A carotenoids (PVACs) has also been the area of research focus for the HarvestPlus (a company headquartered in Washington, DC, USA, involved in the development of nutritious food crops through biofortification and promotion of such crops) since the launch of its projects on biofortification [40]. Genetic modification of sweetpotato by using the transgenic tools and in order to improve the nutritional quality offers huge scope, and numerous research reports have already been published on genetic modification of sweetpotato using molecular gene engineering technologies [41]; however, it is the immense need to overcome hidden hunger, specially the one related with the insufficiency of provitamin A carotenoids among the poorly fed but rapidly growing populations in the developing countries by molecular breeding of sweetpotato varieties on sustainable basis.

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2. Carotenoids and their distribution

Carotenoids, the visible colors of life, are the 40-carbon isoprenoids synthesized naturally by fungi, bacteria, algae, and cyanobacteria [42, 43, 44] and conspicuously by green plants including bryophytes [45] and higher plants [44, 46, 47]. Being intracellular, carotenoids are commonly located in the membranes of chloroplasts, mitochondria, or endoplasmic reticulum [48]. Approximately 750 carotenoids have been reported so far [49, 50].

Maoka et al. (unpublished) analyzed carotenoids that were extracted from the orange tubers of the cultivar W71. It was consequently found that there were β-carotene-5,8,5′,8′-diepoxide (13.8% of the total carotenoids), β-carotene-5,6,5′,8′-diepoxide (9.2%), β-carotene-5,8-epoxide (4.6%), β-cryptoxanthin (3.2%), β-cryptoxanthin-5′,6′-epoxide (2.2%), lutein (2%), and zeaxanthin (trace amounts), in addition to β-carotene (59.3%). The biosynthetic pathway of these carotenoids is proposed in Figure 1. The carotenoids with 5,6-epoxy-β-ring or with 5,8-epoxy-β-ring are unique to sweetpotato. The tubers of the Japanese cultivar “Benimasari” were also found to accumulate not only the unique carotenoids, such as β-carotene-5,8,5′,8′-diepoxide (40.5% of the total carotenoids), β-carotene-5,8-epoxide (6.5%), β-cryptoxanthin-5′,8′-epoxide (10.5%), and β-carotene (10.5%), but also typical carotenoids that included 5,6-dihydroxy-β-ring (named ipomoeaxanthins) [15].

Figure 1.

Proposed carotenoid biosynthetic pathway in sweetpotato orange tubers [10].

2.1 Role of carotenoids in animals

Animals, with very few exceptions [51, 52] are unable to synthesize them [53, 54]; however, carotenoids are accumulated by crustaceans, crabs, fish, crayfish, prawns, mammals, and in insects such as butterflies. The animal and human diet must include carotenoids as essential nutrients [44].

In marine animals, astaxanthin (3,3′-dihydroxy-β,β-carotene-4,4′-dione) has been reported as the most commonly stored carotenoid pigment [55]. It is responsible for the red/pink coloration of crustaceans [56, 57] and the flesh of salmonoids [58]. Astaxanthin has received much attraction for its likely role in preventing cardiovascular diseases and aging caused by UV light in human body [59]. Chemical structures of some major dietary carotenoids are shown in Figure 2.

Figure 2.

Structures of some major dietary carotenoids.

Both α-carotene and β-carotene have provitamin A activity and are converted to retinol in the human body [60, 61, 62, 63, 64]. Carotenes such as the lycopene and β-carotene play a potential role in human nutrition and act as protectants against diseases, such as lycopene protects against cardiovascular [65], aging-related diseases, macular degradation of eye [66, 67], and certain types of cancers including gastrointestinal, cervix, breast, and prostate cancer [47, 61, 68, 69, 70, 71, 72, 73].

Beneficial effects of dietary carotenes, α-carotene, and β-carotene on human health related to enhancement of immune system and minimizing the risk of cancer are due to their antioxidant potential [69, 74]. β-Carotene, α-carotene, and β-cryptoxanthin are provitamin A carotenoids (PVACs) and hence they are the main precursors of vitamin A (VA) in the human body [75].

2.2 Carotenoids use in disease prevention

Carotenoids, especially astaxanthin, have been reported to enhance both the nonspecific and specific immune system and protect cell membranes and cellular DNA from mutation [44, 76]. Intake of fruits and vegetables rich in carotenoids mainly lycopene, α-carotene, β-carotene, β-cryptoxanthin, zeaxanthin, and lutein lowers the risk of morbidity and mortality by cardiovascular diseases and atherosclerosis [69]. Epidemiological studies have reported that lycopene can lower the risk of prostate cancer [77] and in its ability to quench singlet oxygen; it is 2- to 10-fold stronger than β-carotene and α-tocopherol, respectively [78]. Clinical studies have reported that the lycopene-enriched foods are protective against oxidative DNA damage in leukocytes in vitro [79] and prostate tissue in vivo [80]. β-Carotene is useful in reducing the risk of ischemic heart disease and myocardial infarction [81]. In the macular region of human eye including eye lens, two xanthophylls, lutein and zeaxanthin, exist in high concentrations and are regarded very important carotenoids for eye health. Reports suggest that these two carotenoids protect eye from high energy UV light and are excellent reactive oxygen species scavengers [82]. The role of lutein and zeaxanthin as macular pigments and their function in eye health has been reported in previous studies [83]. It has been anticipated that phytoene and phytofluene which are colorless precursors of other carotenoids possess light absorption in UV-A and UV-B range and protect skin by their photo-protective characteristics [84, 85]. Astaxanthin is also known as the super antioxidant. Since, it contains particular molecular configuration, making it extremely powerful antioxidant consequently, protecting cells against oxidation by quenching singlet oxygen and dissipating the energy as heat. It has the strong potential for scavenging free radicals and effectively breaks peroxide chain reactions [86, 87]. Studies have showed that the low-density lipoprotein (LDL) high cholesterol levels in mice decreased when supplemented with astaxanthin. Neither β-carotene nor canthaxanthin produced the same effect. Astaxanthin or other carotenoids can decrease the oxidation of the lipid carriers and thereby reduce the risk of atherosclerosis [88]. It also has positive effects in case of antitumor activity [89].

2.3 Industrial uses of carotenoids

All carotenoids show antioxidants activities appearing in a variety of colors in red, yellow, and orange; therefore, carotenoids are used as natural pigments in food, food supplements, nutraceuticals, pharmaceuticals, and cosmetic industry and various biotechnological purposes [90, 91]. Global carotenoids market touched $1.5 billion ($1500 million) in 2017 with a projection of $2.0 billion by 2022 [92]. In a previous report, the global market for carotenoids was $766 million in 2007. The expected projection for the year 2015 was $919 million with a compound annual growth rate (CAGR) of 2.3%. In 2007, β-carotene alone shared the market value at $247 million; this segment was predicted to be worth $285 million by 2015 with CAGR of 1.8% [91, 93]. In horticultural crops, they appear as a trait of attractiveness, adding value to the marketing potential of fruits and vegetables [94, 95]. Green algae Haematococcus pluvialis, which is the natural source of astaxanthin, has been reported for huge amounts ranging from 10,000 to 40,000 ppm (mg/kg) of astaxanthin in addition to other important carotenoids such as β -carotene, lutein, and canthaxanthin [58, 96]. Industrially, astaxanthin has been utilized as a feed supplement for cultured fish and shellfish [97, 98]. Other diverse biological functions of astaxanthin include an involvement in cancer prevention [99], enhancer of immune responses [100], and a free radical quencher [58, 101]. It is evident, therefore, that astaxanthin is a biomolecule with huge biofunction potential both to the pharmaceutical and food industries [58].

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3. Sweetpotato carotenoids

The carotenoids present in the sweetpotato leaves can scavenge free radical agents as singlet-oxygen quenchers [102, 103, 104, 105]. In a recent analytical report [105], the total phenol, carotenoid, anthocyanin, and flavonoids contents of the sweetpotato leaves ranged from 2.0 to 22.5 (g/100 g DW), 0.9 to 23.4 (β-carotene equivalents/100 g; BET/100 g), 2.2 to 24.5 (color value/g DW), and 62.8–272.2 (catechin equivalents; μg/g), respectively [105]. Consumption of sweetpotato in Asia ranges from its use as additional food of minute status to a very vital supplementary food to rice and/or other root and tuber crops [106]. It is cooked or used to make cakes, chapatis, mandazia, bread, buns, and cookies [107]. In the United States and some other developed countries, sweetpotato is strictly used as a luxury food. In Japan, it is used in novel plant products and/or nutraceuticals [108]. By using absorption spectroscopy, Ishiguro et al. [109] analyzed carotenoids from eight cultivars of yellow-fleshed sweetpotato and compared them in terms of their carotenoids. By HPLC analyses, they revealed some 17 different carotenoids from yellow- and orange-fleshed sweetpotato. In yellow-fleshed sweetpotato, the major carotenoids included β-carotene-5,8, 5′,8′-diepoxide (32–51%) and β-cryptoxanthin 5,8-epxide (11–30%), whereas β-carotene with amounts ranging from 80 to 92% were dominant in the orange-fleshed cultivars. For other orange cultivars, e.g. W71 and “Benimasari,” carotenoid composition in the tubers has already been described along with a comprehensive metabolic pathway [10, 15]. Kammona et al. [110] analyzed and compared the carotenoid composition in some Malaysian orange, yellow, purple, and white sweetpotato tubers. They reported the highest total carotenoid contents from orange sweetpotato followed by yellow, purple, and white sweetpotato. Among the individual carotenoids analyzed, β-carotene existed in all types ranging from 91.95 ± 2.05 μg/g DW in white sweetpotato to 376.03 ± 11.05 μg/g DW in orange sweetpotato tubers. Traces of zeaxanthin were reported with values 5.44 ± 3.23 μg/g DW and 20.47 ± 2.03 μg/g DW in yellow and white sweetpotato, respectively. Lutein was available only in orange sweetpotato at trace amount of 0.91 ± 1.03 μg/g DW. Purple sweetpotato contained only β-carotene (113.86 ± 14.17 μg/g DW) with absence of other carotenoids [110].

Islam et al. [111] performed HPLC analyzes of trans- and cis-β-carotene from raw and boiled sweetpotato which included three orange-fleshed, three yellowish-cream-fleshed, and one white-fleshed varieties of sweetpotato. The deep-orange-fleshed variety Kamalasundari (BARI SP-2) showed the highest amounts of β-carotene among all the varieties followed by yellow varieties. On the other hand, from one of the two white-fleshed varieties, only trace amounts of β-carotene were obtained with no amounts at all from the other one. Their results proposed that the orange-fleshed varieties of sweetpotato contain the highest amounts of β-carotene in raw as compared to those which were boiled.

Despite huge economic value, sweetpotato has not received due importance as compared with common staple crops such as wheat, maize, and rice. World increasing hidden hunger, especially in developing countries, needs new foods and nutrition sources on sustainable bases. In this regard, sweetpotato not only offers immense nutritional, medicinal, industrial, and potential benefits but is also a new horizon in modern industrial biotechnological uses for biofunction development through the latest molecular tools and technologies of molecular plant breeding.

3.1 Isolation and functional identification of carotenoids biosynthesis genes

The heterologous complementation expression system in Escherichia coli offers unique tool for functional analysis of isolated new carotenoids biosynthesis genes from different organisms [112]. Carotenoid biosynthetic pathway in microorganisms, such as Erwinia uredovora and Erwinia herbicola (reclassified as Pantoea ananatis and Pantoea agglomerans, respectively), is specified by a gene cluster, encoding biosynthetic enzymes that function in a pathway starting with the synthesis of geranylgeranyl pyrophosphate (GGPP) and ending in the synthesis of zeaxanthin glucosides [113, 114]. Complete carotenoid gene clusters or part of it from E. uredovora or E. herbicola have been introduced into E. coli, which is otherwise a nonpigmented bacterium, and such transformed E. coli engineered in a way that they accumulate a range of colorful carotenoids [114, 115]. Since carotenoids are derived from isoprenoid precursors, E. coli can accumulate carotenoids by coupling an endogenous isoprenoid biosynthetic pathway with enzymes encoded by transformed genes of carotenogenic organisms such as E. uredovora. Hence, the biosynthetic pathway can be reconstructed in vivo even if the enzymes are of such diverse origin as those encoded by bacteria and plants [116, 117, 118]. The expression of carotenoid genes in E. coli has been useful for identifying function of gene products [118, 119, 120], the manipulation of the pathway [121, 122], investigating transcriptional regulators of carotenoids biosynthesis genes [123], and the isolation of new genes encoding enzymes of the carotenoid biosynthetic pathway [124] or enzymes catalyzing the synthesis of carotenoid precursors [125].

Misawa et al. [55] isolated and functionally identified the carotenoids biosynthesis genes cluster that included crtB (phytoene synthase), crtI (phytoene desaturase), crtW (β-carotene ketolase), and crtZ (β-carotene hydroxylase) from Agrobacterium aurantiacum (reclassified as Paracoccus sp. strain N81106). The functional identification of the isolated gene cluster led them to propose astaxanthin biosynthetic pathway for the first time.

Misawa et al. [114] isolated and functionally identified the carotenoid biosynthesis genes, such as crtE (GGPP synthase), crtX (Zeaxanthin glucosyltransferase), crtY (lycopene β-cyclase), crtI (phytoene desaturase), crtB (phytoene synthase), and crtZ (β-carotene hydroxylase), form E. uredovora by analyzing carotenoids accumulated in E. coli transformants in which these genes were expressed. By analysis of accumulated carotenoids in the transformed E. coli by these individual genes, they found that carotenoids in this pathway appeared to be close to those in higher plants rather than to those in bacteria. Although HPLC is a routine analytical tool to analyze various metabolic products from plants, highly developed and comprehensive metabolome analytical techniques with respect to particular tissues now offer precise analytical approaches such as nuclear magnetic resonance (NMR; COSY and NOESY) and accurate mass spectrometry (MS) techniques [47, 126]. A foreign crtW gene was expressed in the W71 cultivar of sweetpotato, and carotenoids generated there have been successfully analyzed by UV-vis, ESI-MS, 1H-NMR, and CD spectral data [127]. As a result, novel carotenoids, shown in Figure 3, i.e. echinenone 5′,8′-epoxide, echinenone 5′,6′-epoxide, and 3′-hydroxyechinenone 5′,6′-epoxide, were identified besides ketocarotenoids including astaxanthin.

Figure 3.

Novel carotenoids produced in the tuber of the transgenic sweetpotato engineered with the crtW gene of bacterial origin.

3.2 Sweetpotato carotenoids biosynthesis genes, cloning, and genetic engineering

Although, sweetpotato is highly important as a valuable source of carotenoids especially β-carotene, very little research has been done on molecular biological aspects of its carotenoid biosynthesis [10, 14, 31, 128]. The development of an efficient and reproducible transformation system is needed for genetic manipulation of sweet potato to either improve the crop or establish it as a novel “transgenic plant bioreactor” [129]. Otani et al. [130] developed and reported the first successful transformation protocol for the production of transformed (transgenic) sweetpotato plants that was based on the formation of hairy roots using leaf disks as explants for Agrobacterium rhizogenes. However, the regenerated transgenic plants showed some morphological abnormalities such as short storage root and internodes. Later on, to overcome such anomalies, a modified and successful Agrobacterium tumefaciens-mediated transformation protocol was developed via somatic cell embryogenesis [131, 132, 133]. Liao et al. [14] isolated and functionally characterized an isopentenyl diphosphate isomerase (idi) gene from sweetpotato cultivar YUSU 303 from Southeast China. They isolated a full-length cDNA of idi gene by SMART™ RACE cDNA Amplification Kit (Clontech, USA). Isolated idi was 1155 bp with an open reading frame of 892 bp encoding a polypeptide of 296 amino acids (GenBank accession No. DQ150100). Isolated idi gene was cloned in pTrc expression vector and was fed to E. coli which contained pAC-BETA plasmid for β-carotene accumulation. E. coli were cultured and carotenoids were analyzed by color complementation. Cultures of E. coli which were transformed with idi gene turned orange indicative for β-carotene and suggested its potential activity in promoting β-carotene biosynthesis. Kim et al. [134] isolated a partial sequence of phytoene synthase (PSY) which contained 354 bp from a cultivar Shinhwangmi (accession No. HQ828092). It showed 94% sequence identity with a PSY isolated from Ipomoea species Kenyan (GenBank accession No. AB499050.1). However, no gene function of isolated PSY from sweetpotato could be reported. Ling et al. [135] isolated a lycopene ε-cyclase (LCYe) gene from sweetpotato cultivar Nongdafu 14 from China. However, they did not functionally characterize it. They isolated a full-length cDNA of idi gene by GeneRacer TM Kit (Invitrogen Carlsbad, CA, USA). Isolated LCYe was 1805 bp with an open reading frame of 1236 bp encoding a polypeptide of 411 amino acids. Quantitative real-time PCR analysis showed that IbLCYe expression levels were desirably higher in roots as compared to those in leaves. Isolated LCYe gene was expressed in tobacco cultivar Winconsin 38. Carotenoids from transgenic tobacco plants were extracted and analyzed by HPLC which revealed transgenes accumulating more β-carotene as compared to control plants. Kim et al. [128] isolated a partial lycopene β-cyclase (IbLCYb) from a cultivar Yulmi of sweetpotato. They synthesized primers by using a partial sequence of IbLCYb from database with accession number JX393306 and amplified a partial cDNA of IbLCYb by RT-PCR. By using isolated IbLCYb, an IbLCYb-RNAi vector was constructed and then used to transform white-fleshed sweetpotato. Transformed sweetpotatoes were cultured and analyzed for accumulated carotenoids. Their results showed a total increase in the carotenoids contents along with increase in resistance against salt stress in transgenic sweetpotato as compared to the control. Significant levels of carotenoids genes expression were observed in all plant parts with highest expression in leaves to lowest in the fibrous roots. But in case of transgenic calli, expressions of IbLCYb were dramatically reduced and found high in non-transgenic calli. Lycopene was not produced both by transgenic and non-transgenic sweetpotato. In an another experiment, Kim et al. [134] cloned a partial cDNA encoding β-carotene hydroxylase (BHY) from storage roots of sweetpotato cultivar Shinhwangmi and constructed an RNA-i-IbCHY-β vector for transformation of white-fleshed cultivar Yulmi and evaluation of inhibition effects of β-carotene hydroxylase (BHY) in transgenic lines. Downregulation of IbBHY gene expression altered the content and degree of carotenoids between transgenic and non-transgenic cells with an increase in the β-carotene and total carotenoids in transgenic sweetpotato cells along with an increase in their antioxidation potential.

3.3 Metabolic engineering of the carotenoid biosynthetic pathway to enhance carotenoid contents in higher plants

The pathway engineering approach using a variety of carotenoid biosynthesis genes is becoming a potential approach as one of the most effective methods to generate large quantities of structurally diverse carotenoids [59, 136, 137]. Astaxanthin (3,30-dihydroxy-4,40-diketo-β-carotene) is a high-value ketocarotenoid that is biosynthesized only by a few organisms typically at low levels. This red pigment (produced through chemical synthesis) has been used in large amounts in aquaculture. Currently, natural astaxanthin is employed as a health boosting food and is investigated for the treatment of a number of human diseases including cancers [138]. The limited renewable sources and growing demand for natural astaxanthin have attracted tremendous interest in its engineering into heterologous hosts, especially plants with the ability of sequestering 10- to 50-fold higher carotenoids than microorganisms, to produce the high-value pigment, during the past decade [139, 140]. The most promising approach reaching high astaxanthin yields was by chloroplast transformation using a bacterial ketolase gene [141]. Plastid genome transformation of lettuce (Lactuca sativa) has similarly been site-specifically modified with the addition of three transgenes, which encoded β,β-carotenoid 3,3′-hydroxylase (crtZ) and β,β-carotenoid 4,4′-ketolase (4,4′-oxygenase; crtW) from a marine bacterium Brevundimonas sp. strain SD212, and isopentenyl-diphosphate-isomerase (idi) from a marine bacterium Paracoccus sp. strain N81106. The resultant transplastomic lettuce leaves generated 49.2% astaxanthin fatty acid diester, 18.2% astaxanthin monoester, and 10.0% astaxanthin in its free forms along with the 17.5% of other ketocarotenoids. The ketocarotenoids produced in transplastomic lettuce were 94.9% of total carotenoids. The wild-type native carotenoids analyzed were 3.8% lactucaxanthin and 1.3% lutein in the transplastomic lettuce [142]. Likewise, by the introduction and heterologous expression of crtW gene, astaxanthin and other intermediates have been produced and reported in carrot (Daucus carota) roots [143], canola (Brassica napus) seeds [144], and maize (Zea mays) endosperms [145]. A comprehensive carotenoid biosynthetic pathway in these higher plants is shown in Figure 4 with a summarized illustration for the metabolic pathway engineering with heterologous crtW and crtZ genes expression.

Figure 4.

Carotenoid biosynthetic pathway in higher plants. A summarized illustration for the introduction and function of heterologous crtW and crtZ genes expressed in tobacco [141] and lettuce [142] leaves. The carotenoids shown in black represent native carotenoids accumulated by both tobacco and lettuce, and black and underlined are those reported from both of the transgenic tobacco and lettuce. Carotenoids underlined red are reported from lettuce only, where GGPS, is geranylgeranyl pyrophosphate synthase, PSY is phytoene synthase, PDS is phytoene-desaturase, ZDS is ζ-carotene desaturase, CRTISO is carotenoid isomerase, LCYb is lycopene β-cyclase, LCYe is lycopene ε-cyclase, LsLCYe is lettuce LCYe, LsCYP97C is lettuce heme-containing cytochrome P450-type carotene ε-ring hydroxylase, BHY is non-heme di-iron-type carotene β-ring hydroxylase, EHY is carotene ε-ring hydroxylase, ZEP is zeaxanthin-epoxidase, VDE is violaxanthin de-epoxidase, and NSY is neoxanthin synthase.

Through pathway engineering that utilizes the marine bacterial carotenoid 4,4′-ketolase (4,4′-oxygenase) gene named crtW, unique keto-carotenoids such as astaxanthindiglucoside, 2,2′-dihydroxyastaxanthin, and 2,2′-dihydroxycanthaxanthin have been produced in Escherichia coli [146, 147] and 4-ketoantheraxanthin in tobacco (Nicotiana tabacum) plants [148]. Breitenbach et al. [149] also synthesized α-echinenone (4-keto-α-carotene) in rice callus using crtW. Recently, 4-keto-zeinoxanthin was produced in E. coli cells by introducing the bacterial crtW gene and carotenogenic genes from liverwort [150].

3.4 Metabolic engineering of the carotenoids biosynthetic pathway in sweetpotato

Metabolic engineering of carotenoid biosynthetic pathway using a combinatorial approach has led to the efficient production of interesting carotenoids of high commercial value and pharmaceutical potential [44, 59, 151].

Starting with transgenic approach, prerequisite is to have a sound knowledge on the metabolic pathways regulating the carotenoid biosynthesis and their accumulation. Due to efforts of many scientists, the carotenoid metabolic pathway and the function of the biosynthetic enzymes involved in carotenoids biosynthesis have been elaborated well [152]. It was reported that sweetpotato contained not only β-carotene but also several epoxy carotenoids unique to the sweetpotato tubers, e.g. β-carotene-5, 8-epoxside and β-carotene-5, 8, 5′8′-diepoxside [15]. Therefore, it was assumed that the new structural carotenoids with epoxy and keto groups can be produced by expressing the ketolase crtW gene in sweetpotato tubers. Recently, marine bacterial genes that include the crtW gene encoding carotenoid 4,4′-ketolase [148] was introduced into sweetpotato cultivar W71 under the control of the CaMV promoter. Consequently, novel carotenoids with epoxy and keto groups 1, 2, and 3 were obtained along with a series of ketocarotenoids. The structural elucidation of these novel epoxy-keto carotenoids along with biosynthetic pathway in sweetpotato was also proposed [127]. A tabulated summary of recent developments in molecular breeding of sweet potato by genetic, metabolic, and pathway engineering approaches is presented in Table 1.

Gene engineeredPromoter usedCarotenoids enhancementReferences
ZDSCauliflower mosaic virus (CaMV) 35S3.96–2.37 increase in β-carotene and lutein and, 2.23-fold increase in total carotenoids accompanied with enhanced salt tolerance[153]
PSYTuber-specific primer6.3-fold increase in carotenoid, 19-fold increase in β-carotene[154]
LCYbCauliflower mosaic virus (CaMV) 35S1.4–1.8 times higher in β-carotene, increased tolerance to drought stress[128]
LCYe5.44-fold to 6.59-fold
Increase in β-carotene and 1.77–2.75 times increase in total carotenoids
[155]
BHYCauliflower mosaic virus (CaMV) 35STwofold increase in total carotenoids and 16-fold increase in β-carotene[152]
CrtWCauliflower mosaic virus (CaMV) 35SNovel carotenoids with epoxy and keto groups were produced including a series of ketocarotenoids[127]
CrtOCauliflower mosaic virus (CaMV) 35S10–12% increase in total carotenoid[156]
BHYSilencing of BHY117 μg/g (dry weight) increase in total carotenoids and 34.43 lg/g (dryweight) in β- carotene[134]
IbOr-R96Hcauliflower mosaic virus (CaMV) 35S promoter19.6- and 186.2-fold higher total carotenoid and β-carotene contents, respectively[157]

Table 1.

Role of metabolic engineering in carotenoids enhancement in sweetpotato*.

“White Star” (WS) and W71, which produce white- and orange-fleshed tubers, respectively, are important sweetpotato cultivars, since they are amenable to Agrobacterium-mediated transformation [10, 127, 158, 159]. Chemical analysis of the carotenoids and isolation and functional characterization of the carotenoids biosynthesis genes of these two cultivars was reported in more details by Khan et al. [10] for the first time. One of the initial works that led to the sweetpotato genetic improvement for enhancing provitamin A amounts was done by Kim et al. [160] which involved isolation and functional analysis of the orange (Or) gene, from orange-fleshed sweetpotato controlling the carotenoids accumulation in the transgenic calli of sweetpotato. White-fleshed sweetpotatoes were transformed by the orange (Or) gene, which resulted in the 10-fold increased accumulation of β-carotene and total carotenoids. Later, identical results were presented by Park et al. [161] who observed that the overexpression of IbOr gene boosted the carotenoid composition in purple-flesh sweetpotato cultivar. In higher plants, the biosynthesis of carotenoids from lycopene involves the enzymatic activity of lycopene ϵ-cyclase (LCYe) gene, via β-branch-specific biosynthetic pathway yielding β-carotene. By downregulating the expression of IbLCYe through RNA interference (RNAi) technology, higher amounts of β-carotene were recorded [162]. To increase the β-carotene contents in sweetpotato, researchers have also made use of the molecular markers along with the evaluation and screening of available germplasm.

This combined approach is thought very useful in selecting the desirable parents for breeding new sweetpotato varieties with the higher levels of β-carotenes [163]. To analyze the gene diversity and evolutionary relationships among various cultivars of sweetpotato, Hwang et al. [164] have applied the use of Simple Sequence Repeats (SSRs). Their results showed that polycross-derived cultivars have higher levels of genetic diversity suggesting the application of polycross breeding that overcomes the challenges of cross-incompatibility. For breeding high β-carotene sweetpotato varieties, Quantitative Trait Loci (QTLs) for β-carotene content in a cross sweetpotato were reported for the first time by Cervantes-Flores et al. [165] which led to the understanding of the inheritance pattern and is considered the foundation of the development of marker-assisted breeding techniques for breeding high β-carotene (provitamin A) accumulating sweetpotato cultivars.

Orange-fleshed sweetpotato, which is a genetically modified crop, is now well accepted by consumers [166, 167] and has appeared as a sound supply of provitamin A. To achieve the daily provitamin A needs, mere 125 g of fresh orange-fleshed sweetpotato roots from most varieties are enough [35].

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4. Conclusion

The rapidly increasing world population demands sustainable supply of ample quantities of quality food, especially under the changing climatic conditions. Food insecurity accompanied with already existing malnutrition among the developing countries is a grand challenge of the day. Foods rich in phytonutrients not only contribute toward enhancing the health but also reduce the risk of many diseases including early aging. In this regard, genetic improvement of the major staple crops such as sweetpotato needs additional strategies of the molecular plant breeding to overcome the genetic complexity. The application of metabolic engineering supplemented with the omics and the recently developed gene editing tools and technologies are the potential strategies to be adopted which promise scope for improving the quantity of phytonutrients, especially the carotenoids in sweet potato. It will contribute to prevent the malnutrition and the diseases linked with foods deficit in quality nutrients. There is a dire need to apply multiple gene engineering approaches for multi-phytonutrients improvement to meet the need.

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5. Recent development and future scope

Recent developments in carotenoids gene manipulations have helped to make insight that engineering sweetpotato with IbOr gene manipulations would be a potential strategy to improve the total carotenoids and specially the β-carotene through enhancing sink strength in storage roots of sweet potato. Moreover, site-directed mutagenesis supplanted with the genome editing tools such as CRISPR-Cas9 such as CRISPR-Cas9 and its different modifications will further lead to a fruitful biofortification of sweet potato for nutritional enhancement through carotenoids improvement.

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Acknowledgments

Principal and the corresponding author Dr. Muhammad Zubair Khan is highly thankful to the MEXT, Japan, for fully funding the research and studies conducted for the completion of doctoral degree. The author is also very much thankful to the laboratory technical staff members, Ms. Chisako Fuchimoto, Miyuki Murakami, Ayaka Atsumi, and Megumi Hashida for technical supports in the laboratory experiments. Author is highly thankful to the president of Ishikawa Prefectural University, Director, and office staff of the Research Institute for Bioresources and Biotechnology and the administrative staff of the Ishikawa Prefectural University, Ishikawa, Japan.

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Conflict of interest

The authors declare that they have no conflict of interest.

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Notes/thanks/other declarations

Corresponding author is highly thankful to the Prefectural government offices of Kanazawa city hall, Nonoichi city hall and Nagoya Regional Immigration Bureau Kanazawa Branch Office for facilitating stay pertaining to the whole term of the doctoral research and studies conducted.

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Written By

Muhammad Zubair Khan, Miho Takemura, Takahashi Maoka, Jun-ichiro Hattan, Motoyasu Otani and Norihiko Misawa

Submitted: 01 July 2021 Reviewed: 01 December 2021 Published: 20 April 2022