Next Article in Journal
Differential Responses of LINE-1 in the Dentate Gyrus, Striatum and Prefrontal Cortex to Chronic Neurotoxic Methamphetamine: A Study in Rat Brain
Next Article in Special Issue
Identification of Regulatory SNPs Associated with Vicine and Convicine Content of Vicia faba Based on Genotyping by Sequencing Data Using Deep Learning
Previous Article in Journal
Genome-Wide Identification and Analysis of P-Type Plasma Membrane H+-ATPase Sub-Gene Family in Sunflower and the Role of HHA4 and HHA11 in the Development of Salt Stress Resistance
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Genes
Volume 11
Issue 4
10.3390/genes11040363
genes-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles thumb_up
...
Endorse textsms
...
Comment
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Article

Narrowing Down a Major QTL Region Conferring Pod Fiber Contents in Yardlong Bean (Vigna unguiculata), a Vegetable Cowpea

by
Phurisorn Watcharatpong
1,
Akito Kaga
2,
Xin Chen
3 and
Prakit Somta
1,4,*
1
Department of Agronomy, Faculty of Agriculture at Kamphaeng Saen, Kasetsart University, Kamphaeng Saen Campus, Nakhon Pathom 73140, Thailand
2
Soybean and Field Crop Applied Genomics Research Unit, Institute of Crop Science, National Agriculture and Food Research Organization, 2-1-2, Kannondai, Tsukuba, Ibaraki 305-8602, Japan
3
Institute of Industrial Crops, Jiangsu Academy of Agricultural Sciences, 50 Zhongling Street, Nanjing, Jiangsu 210014, China
4
Center of Excellence on Agricultural Biotechnology: (AG-BIO/PERDO-CHE), Bangkok 10900, Thailand
*
Author to whom correspondence should be addressed.
Genes 2020, 11(4), 363; https://doi.org/10.3390/genes11040363
Submission received: 25 February 2020 / Revised: 18 March 2020 / Accepted: 24 March 2020 / Published: 27 March 2020
(This article belongs to the Special Issue Food Legume Genomics)
Browse Figures
Versions Notes

Abstract

:
Yardlong bean (Vigna unguiculata (L.) Walp. ssp. sesquipedalis), a subgroup of cowpea, is an important vegetable legume crop of Asia where its young pods are consumed in both fresh and cooked forms. Pod fiber contents (cellulose, hemicellulose and lignin) correlates with pod tenderness (softness/hardness) and pod shattering. In a previous study using populations derived from crosses between yardlong bean and wild cowpea (V. unguiculata ssp. unguiculata var. spontanea), three major quantitative trait loci (QTLs), qCel7.1, qHem7.1 and qLig7.1, controlling these fibers were identified on linkage group 7 (cowpea chromosome 5) and are co-located with QTLs for pod tenderness and pod shattering. The objective of this study was to identify candidate gene(s) controlling the pod fiber contents. Fine mapping for qCel7.1, qHem7.1 and qLig7.1 was conducted using F2 and F2:3 populations of 309 and 334 individuals, respectively, from the same cross combination. New DNA markers were developed from cowpea reference genome sequence and used for fine mapping. A QTL analysis showed that in most cases, each pod fiber content was controlled by one major and one minor QTLs on the LG7. The major QTLs for cellulose, hemicellulose and lignin in pod were always mapped to the same regions or close to each other. In addition, a major QTL for pod shattering was also located in the region. Although there were several annotated genes relating to pod fiber contents in the region, two genes including Vigun05g266600 (VuBGLU12) encoding a beta glucosidase and Vigun05g273500 (VuMYB26b) encoding a transcription factor MYB26 were identified as candidate genes for the pod fiber contents and pod shattering. Function(s) of these genes in relation to pod wall fiber biosynthesis and pod shattering was discussed.

1. Introduction

The cowpea (Vigna unguiculata L. Walp.) is an economically important crop legume in Africa, America and Asia [1,2,3]. This crop has five cultivar groups/subspecies including unguiculata (grain cowpea (also known as black-eye pea)), biflora, texilis, melanopthamus and sesquipedalis (yardlong bean (also known as asparagus bean)) [2,4]. Of these five groups, the grain cowpea and yardlong bean are the most popular. The grain cowpea is commonly grown for dry seeds, although sometimes, young pods and young leaves are harvested and consumed as vegetable [5]. The grain cowpea is popularly cultivated in Africa, America and Asia. The yardlong bean is chiefly grown for immature long and tender pods. This crop is popularly cultivated in Asia, especially Southeast Asia and China [5]. Immature pods of yardlong bean are consumed as vegetable in both cooked and fresh forms. It is a source of vitamin, mineral and dietary fibers for human [6,7]. The grain cowpea has been domesticated in Africa [8], whereas the yardlong bean has been domesticated in Asia [9,10,11,12].
There are morphological differences between the grain cowpea and the yardlong bean in pod characteristics, including pod length, pod tenderness, pod shattering and pod fibers [5,7,13,14]. The pod length of the yardlong bean is about 30–100 cm, while that of the grain cowpea is about 15–30 cm. The pods of yardlong beans are much softer than those of the grain cowpea. The yardlong bean shows complete loss of pod shattering under any environmental conditions, while the grain cowpea shows some degree of pod shattering in some environmental conditions such as high temperature. The pods of the yardlong bean are less fibrous than those of the grain cowpea. These pod-related traits are genetically correlated. Kongjaimun et al. [14] located quantitative trait loci (QTL) controlling several domestication-related traits using F2 and backcross (BC1F1) populations derived from crosses between yardlong bean accession “JP81610” and wild cowpea (V. unguiculata ssp. unguiculata var. spontanea) accession “TVnu-457”. They found that the largest-effect QTLs for pod length and pod shattering are co-located on linkage group (LG) 7 (corresponding to chromosome 5 of cowpea reference genome) [7]. Later, by using the same F2 and BC1F1 populations, Kongjaimun et al. [7] identified QTLs for pod tenderness and found that the major QTL for this trait is located on the LG7 near to the QTLs for pod length and pod shattering. The difference in pod tenderness and shattering between the yardlong bean and the cowpea is believed to be due to the pod fiber contents [5].
By using the F2 and BC1F1 population used by Kongjaimun et al. [7,14], Suanum et al. [5] showed that the contents of pod cellulose, hemicellulose and lignin showed statistically positive and moderate correlation with degree of pod shattering. The authors mapped QTLs for pod fiber content and pod shattering and demonstrated that major QTLs for pod fiber content, qCel7.1, qHem7.1 and qLig7.1, are co-localized with major QTL for pod length, pod shattering and pod tenderness on LG7. These QTLs are clustered in the marker interval cp06388 and VR294. In addition, by comparing the linkage maps they used for QTL mapping with a reference whole genome sequence of azuki bean (Vigna angularis (Ohwi) Ohwi and Ohashi) [15], they suggested that the gene encoding transcription factor MYB46 is a candidate gene for pod fiber contents and pod shattering. Recently, Lo et al. [16] identified QTLs for the domestication of cowpea using a recombinant inbred line population developed from a cross between grain cowpea breeding line “IT99K-573-1-1” and wild cowpea accession “TVNu-1158”. They detected two significant QTLs, CPshat3 on chromosome 3 and CPshat5 on chromosome 5, for pod shattering. These QTLs explained 37.69% and 30.27% of the phenotypic variation, respectively. Interestingly, no QTL for pod length detected on the chromosome 5 where QTL for shattering located onto. This result is contrast to the results reported by Kongjaimun et al. [7] and Suanum et al. [5], who showed localization of QTLs for pod length and pod shattering on the cowpea chromosome 5. Very recently, by employing fine mapping in combination with whole-genome sequencing, Takahashi et al. [17] identified Vigun05g27350 (MYB26b) as the gene responsible for pod shattering (shattering vs. none shattering) in cowpea and azuki bean.
We are interested in the role(s) of pod fiber content in pod shattering and pod tenderness. In this paper, we report narrowing down the QTL region controlling pod fiber content in the yardlong bean. The objective of this study is to identify candidate gene(s) controlling the pod fiber contents in yardlong bean.

2. Materials and Methods

2.1. Mapping Population

Three mapping populations were used in this study; F2A, F2B and F2C. They were all developed from hybridization between JP81610 (female parent) and TVnu-457 (male parent). JP81610 is a yardlong bean (V. unguiculata ssp. sesquipedalis) from Sri Lanka, whereas TVnu-457 is a wild cowpea (V. unguiculata ssp. unguiculata var. spontanea) from Mali. A diagram of population development is shown in Supplementary Figure S1. Population F2A was an F2 population of 177 previously used to locate QTLs for pod shattering [5,7], pod fiber contents [5] and pod tenderness [14]. Population F2B was an F2 population of 309 individuals developed in this study. The F2B population and their parents were grown under field conditions during December 2016 to February 2017 in an experimental field of Kasetsart University, Kamphaeng Saen Campus, Nakhon Patom, Thailand. Spacing between plants was 0.70 m. Population F2C was an F2:3 generation of 334 plants derived from a self-pollination of 28 F2 plants (10–32 F3 plants per F2 plant) of the F2B population. These 28 F2 plants were selected based on heterozygosity of marker at least one genotype between cp08202 to Van07-SSR12 resulting from QTL mapping of the pod fiber contents. The genotypes of these plants are shown in Supplementary Table S1. The F2C population and the parents were planted during October to December in 2017 in the same field as in the F2B population. The total genomic DNA of each plants of the F2B and F2C populations was extracted from young leaves as per Lodhi et al. [18]. The quality and quantity of the DNA was determined by 1% agarose gel electrophoresis and Nanodrop spectrophotometer (Thermo Fisher Scientific™, USA), respectively. At maturity, dry pods of each plant were harvested for a fiber analysis.

2.2. Determination of Pod Fiber Contents

Since the pod fiber content data, including cellulose, hemicellulose and lignin in the F2A were available from previous study [5], the traits were determined only in the F2B and F2C populations. In the F2A population, F2:3 lines were sown in randomized complete block design with two replicates under field condition. In each replicate, pods of five plants of each line were harvested and used for fiber analysis. In the F2B population, the dry pods harvested from each F2 plants and the parental plants were determined for fiber contents including cellulose, hemicellulose and lignin. Initially, the pods were dried at 80 °C for 48 h. Then, the pods were ground into the powder and sieved through 1 µm sieve. Two samples/replicates of the sieved powder of 0.5 g of each plant were used for a fiber analysis. Before conducting the fiber analysis, the samples were subjected to near infrared (NIR) spectroscopy using BUCHI NIRFlex N-500 Solids (Switzerland). Each sample was measured for NIR spectrum three times. Subsequently, the samples were determined for neutral detergent fiber (NDF), acid detergent fiber (ADF), and acid detergent lignin (ADL) by fiber bag technology using an ANKOM-200 Fiber Analyzer in combination with a Daisy Incubator (ANKOM Technology, Macedon, NY) following the procedures described by Vogel et al. [19]. After that, ADL and ash were determined as per Suanum et al. [5]. Briefly, the ANKOM bags containing the residual of the ADF procedure were placed in a 3-L Daisy incubator and submerged under 72% H2SO4. The samples were altered in the incubator for 3 h, washed using hot water for 15 min and in acetone for 10 min, dried in a 105 °C oven for 4 h, and then weighed. Subsequently, the sample bag containing the remaining residual fiber was burnt at 550 °C for 4 h. Then, the resultant ash was weighed. Finally, the amount of NDF, ADF, ADL and ash were used to calculate cellulose, hemicellulose and lignin contents following Suanum et al. [5].
In the F2C population, dry pods harvested from each F3 plants were determined for the fiber contents using NIR spectroscopy. The preparation of the samples and the NIR spectroscopy were the same as described above. NIR equations for cellulose, hemicellulose and lignin were obtained using 206 samples of the F2B populations. The samples were separated into calibration sets (51 samples) and validation sets (152 samples). The formulae were modified using functions “Smooth Savitzky-Golay 9 points”, “Second Derivative”, “Smoothing and SNV (Standard Normal Variate)” for precision adjustment. NIR equation for cellulose was f(x) = 0.8764x + 4.1513; R2 = 0.7992; BIAS = 0.0119. NIR equation for hemicellulose was f(x) = 0.8250x + 1.8343; R2 = 0.7785; BIAS = 0.2663. NIR equation for was lignin was f(x) = 0.6781x + 5.8806; R2 = 0.7440; BIAS = 0.1327.

2.3. Fine Mapping for the Pod Fiber Contents

Since the major QTLs controlling cellulose, hemicellulose and lignin were mapped between SSR markers cp06388 and VR294 on LG7 [5], 80 SSR markers from cowpea (24 markers) and azuki bean (56 markers) residing around this genome region were developed to finely map the QTLs for the traits (Supplementary Table S2). In brief, primer sequences of the markers cp06388 and VR294 were BLASTed to reference whole genome sequence of cowpea (Vigna unguiculata v.1.1; https://phytozome.jgi.doe.gov/pz/portal.html#!info?alias=Org_Vunguiculata_er) [20] and azuki bean (https://viggs.dna.affrc.go.jp) [15] and searched for SSRs using SSRIT [21]. Primers for the 82 SSRs were then designed using Primer3 [22]. In addition, two insertion/deletion (InDel) markers were developed from our in-house transcript sequence data of cowpea. These markers were screened for polymorphism between the parents and those showing polymorphism were used to analyze DNA of all the three population. The marker analysis (polymerase chain reaction (PCR) and gel electrophoresis and DNA band visualization) were the same as described by Somta et al. [13] and Kongjaimun et al. [23].

2.4. Fine Mapping of Pod Shattering

Since a previous study using population F2A by Suanum et al. [5] revealed co-localization between major QTLs for pod fiber contents and pod shattering on LG7, fine mapping of the QTLs for pod fiber contents as well as pod shattering of the F2A population was conducted using additional genetic markers in the present study. Briefly, the pod shattering was evaluated in the F2:3 lines grown under field conditions by Suanum et al. [5]. Pod shattering of each F2:3 plant was evaluated by visual scoring using a scale of 1 to 5; 1 = no shattering, 2 = pod valves slightly opened, 3 = pod valves opened all along the pod length with minor or without twist, 4 = pod valves opened all along the pod length with moderate twist, and 5 = pod valves opened and twisted all along the pod length. Pod shattering data of the population F2A is shown in Supplementary Figure S2.

2.5. Linkage Map and QTL Analyses

A linkage map for each population was constructed from the polymorphic SSRs using QTL IciMapping 4.2 software [24]. Grouping of the markers was done with a minimum logarithm of the odds (LOD) of 3.0. Markers were ordered based on their position on the cowpea reference genome [20]. Recombination frequencies were converted into genetic map distance (centimorgan; cM) using Kosambi’s mapping function [25].
Location of the QTL conditioning cellulose, hemicelluloses and lignin content in pod was determined by inclusive composite interval mapping (ICIM) [26] using the same software as for the linkage analysis [24,27]. The significant LOD score threshold for the QTLs of each trait was determined by running a 10,000 permutations test at P = 0.001. ICIM was carried out at every 1.0 cM.

3. Results

3.1. Segreation of Pod Fiber Content in F2B and F2C Population

In the F2B population, pod cellulose contents varied between 19.04% and 40.22% with a mean of 32.78%. Pod hemicellulose contents ranged from 8.82% to 25.96% with a mean of 18.50%. Pod lignin contents were between 3.76% and 14.02% with a mean of 8.78%. The frequency distribution of all the three fibers showed a continuous segregation but skewed towards the wild cowpea (Figure 1). Transgressive segregation to both directions was observed for all the fiber traits (Figure 2).
In the F2C population, pod fiber contents were measured using NIR microscopy. Pod cellulose contents varied between 21.19% and 46.48% with a mean of 38.25%. Pod hemicellulose contents varied from 9.54% to 19.94% with a mean of 15.42%. Pod lignin contents ranged from 2.57% to 9.54% with a mean of 7.12%. Similarly to the F2B population, all the fibers showed continuous segregation (Figure 2).

3.2. Fine Mapping of QTL for Pod Fiber Content and Pod Shattering

New SSR and InDel markers were developed to fine map major QTLs for cellulose, hemicelulose and lignin. Among the 82 markers developed, only nine of them (three from azuki bean and six markers from cowpea) including Van07-SSR12, Van07-SSR48, Van07-SSR54, cp05951, cp08202, Vu-SSR01-2, VU05-GHIndel, Vu-SSR04, Vu-SSR11 showed clear polymorphism between parents. These markers were used for fine mapping QTLs for pod fiber contents.
In the population F2A, the newly six polymorphic markers together with four markers, previously localized with QTLs for pod fiber contents and pod shattering on LG7 by Suanum et al. [5]) were used to construct a new LG7 for fine mapping. The linkage analysis showed that all the markers were clustered in the same LG7. The new LG7 was 62.0 cM in length (Figure 3A). QTL analysis using this new LG by ICIM detected five QTLs in total; four major QTLs for cellulose, hemicellulose, lignin and pod shattering, and one minor QTL for hemicellulose (Table 1 and Figure 3A). The major QTLs for hemicellulose, lignin and pod shattering were mapped to the same position, which was 44.09 cM between markers cp05951 and VR294. In contrast, the major QTL for cellulose was located far apart from other major QTLs, mapped at 34.30 cM. The major QTLs for cellulose, hemicellulose, lignin and pod shattering accounted for 14.51%, 51.32%, 47.28% and 32.12% of the trait variation, respectively. The minor QTL for hemicellulose was mapped near to the major QTL for cellulose, about 1.2 cM apart. The QTL accounted for about 6% of the total trait variation. This QTL expressed nearly to zero additive effect, but a high dominant effect.
In the popultion F2B, the linkage analysis showed that the eight polymorphic markers grouped together. This linkage group was 58.7 cM in length. ICIM detected three QTLs for pod fiber contents; one each for cellulose, hemicellulose and lignin (Table 2 and Figure 3B). Although the QTLs of these traits were mapped to different marker intervals, they were clustered in a region of about 5.0 cM between markers Van07-SSR54 and cp05951. These QTL accounted for 11.31%, 33.31%, and 58.14% of the trait variation, respectively.
In the population F2C, the linkage analysis showed that the eight polymorphic markers clustered in the same linkage group with a length of 76.6 cM (Figure 3C). ICIM identified six QTLs for pod fiber contents; two each for cellulose, hemicellulose and lignin (Table 3 and Figure 3C). The major QTLs for these traits were mapped near to one another in a 3-cM region, covering by markers VU05-GHIndel, VR294, cp05951 and Vu-SSR11. The major QTLs for these fibers accounted for 33.14%, 39.10%, and 57.18% of the total trait variation, respectively. The minor QTLs for these traits were mapped to the same marker interval, cp08202 and VUSSR01-2. They explained 10.77%, 5.23%, and 6.57% of the trait variation, respectively.

4. Discussion

In legume crops, non-shattering of pods is one of the most important traits that has been selected during domestication by humans. The selection for non-shattering of pods is beneficial for reduced yield loss and ease of harvest. In cowpea/yardlong beans, selection for non-shattering is accompanied by edibility (pod softness/tenderness) of immature pods [5,14,17] and increased seed size [17], although it is unknown whether these traits are controlled by the same gene or tightly linked genes. In this study, we finely mapped major QTLs for pod fiber content in yardlong bean on LG7 using three segregating populations derived from the same parents. In most cases, each type of fiber was controlled by one major and one minor QTL on the LG7. In the same population, the major QTLs for cellulose, hemicellulose and lignin in pod were always mapped to the same regions or close to each other (Table 1, Table 2 and Table 3 and Figure 3A–C). In different populations, the major QTLs for different fibers were always detected in the region of markers Van07-SSR54, Vu05-GHIndel, VR294, cp05951, and Vu-SSR011 (Table 1, Table 2 and Table 3 and Figure 3A–C), while the minor QTLs were in general mapped to different regions (Table 1, Table 2 and Table 3 and Figure 3A–C).
Based on the current cowpea reference genome sequences [20], physical distance between Van07-SSR54 and Vu-SSR011 is 0.545 Mbp (Figure 3D). There were 91 annotated genes in this region. Among those genes, genes encoding for beta-glucosidases and MYB26 (Figure 3D) are found to be related to cell wall biosynthesis. Surprisingly, fifteen genes encoding for beta glucosidases existed in the region, 14 of which are in tandem. Beta-glucosidase is a glycoside hydrolase enzyme and is involved in the phenylpropanoid pathway that leads to lignin biosynthesis. Moreover, beta-glucosidase is a cellulase enzyme playing a part in metabolism of cell wall polysaccharides in both prokaryotes and eukaryotes. It is involved in plant cell wall development from cell wall degradation pathway [28]. In barley (Hordeum vulgare L.), a seed-specific beta-glucosidase is accumulated to high levels during late seed development and participates in endosperm cell wall degradation during germination [29]. Recently, a study in cotton (Gossypium hirsutum L.) revealed that a gene, GhBG1A, encoding beta-glucosidase plays role in cotton fiber elongation and secondary cell wall cellulose deposition [30]. The overexpression of the GhBG1A at the fiber elongation stage repressed fiber length but promoted cellulose biosynthesis resulting in thicker fiber cell wall [26]. Based on gene expression analysis in two near-isogenic lines (NILs) showing contrast pod tenderness (soft vs. hard) derived from the cross between JP81610 and TVnu-457 revealed that Vigun266600 (VuBGLU12) encoding for beta-glucosidase shows markedly differential expression between the two NILs during stage of pod growth and development (A. Kaga, unpublished data). Interestingly, VuBGLU12 resides in the 0.545-Mb region controlling pod fiber content and pod shattering (Figure 3). In fact, the indel marker VU05-GHIndel is developed from the transcript sequence of VuBGLU12. Thus, the indel polymorphism detected between JP81610 and TVnu-457 by the marker VU05-GHIndel suggests that the VuBGLU12 in these accessions is different. Therefore, VuBGLU12 is considered as a candidate gene for pod fiber contents in yardlong bean and pod shattering. Additional study is necessary to clarify the association between VuBGLU12 and fiber contents and shattering of pod in cowpea.
MYB26 is a transcription factor related to cell wall biosynthesis. In poplar (Populus trichocarpa), PtMYB26 activates lignin biosynthesis genes [31]. In Arabidopsis, AtMYB26 functions as master switches, activating secondary wall biosynthesis in anther endothecium affecting anther dehiscence [32,33] and regulates NAC domain transcription factors NST1 and NST2 that act as master regulator in cell wall biosynthesis [34]. Recently, fine mapping in backcross inbred lines ((JP81610 × TVnu-457) × JP81610) together with whole genome sequencing and gene expression analysis revealed Vigun05g273500 (VuMYB26b) as the gene responsible for pod shattering [17]. The authors showed that a SNP disrupting the junction site of the 1st intron and the 2nd exon of the gene and resulting in premature stop codon in JP81610. VuMYB26b was expressed only in pods. The function of VuMYB26b is believed to be lignification of pod sclerenchyma tissue (increase pod lignin content and thus pod shattering) [17]. It is worth noting that in these two studies, pod shattering was evaluated by binarizing pod characteristics, visual scoring of pod shattering (shattering vs. non-shattering) and feeling tenderness of pods (hard vs. soft), respectively [16,17]. However, in our study, the SSR marker Vu-SSR11 developed from VuMYB26b was always not the best marker showing association with major QTLs for fiber contents and pod shattering (Table 1, Table 2 and Table 3 and Figure 2 and Figure 3). It is worth mentioning that Suanum et al. [5] showed that pod shattering determined by scoring degrees of pod shattering in cowpea/yardlong bean shows the highest correlation with pod hemicellulose content, not pod lignin content [5]. A similar result was reported in the common bean (Phaseolus vulgaris (L.)), a legume closely related to cowpea, where PvMYB26 is one of the genes identified in the major QTL region on chromosome 5 controlling pod shattering but the gene was not the best candidate gene showing association with the trait [35,36]. Parker et al. [35] noted that the most significant marker at this QTL located very near to PvMYB46, being only about 22 Kb from the gene. Based on reference genome of azuki bean [15], Suanum et al. [5] suggested that VuMYB46 (Vigun05g262100) is a candidate gene at the major QTLs on LG7 for pod fiber contents and pod shattering in cowpea. MYB46 function as master switches activating secondary cell wall biosynthesis [37]. Although, in the present study, VuMYB46 was not in the core QTL region controlling cellulose and pod shattering, in the F2A population, a major QTL for cellulose was mapped near to VuMYB46 (Figure 3D). In Arabidopsis, AtMYB46 directly regulates expression of secondary wall-associated cellulose synthase genes (CESA4, CESA7 and CESA8) [38]. This suggests VuMYB46 as another candidate gene involved in the pod fiber contents. In fact, MYB26 is an upstream regulator of MYB46 [34]. Additional study is necessary to determine whether VuBGLU12, VuMYB26 and VuMYB46 are involved in the pod fiber contents in yardlong bean. Large-effect QTLs controlling pod fiber contents on chromosome 5 of yardlong bean may be synergetic effect of more than one genes that are tightly linked and function in network fashion.

Supplementary Materials

The following are available online at https://www.mdpi.com/2073-4425/11/4/363/s1. Figure S1: A diagram depicting development of mapping populations (F2A, F2B and F2C) used in this study. Figure S2: Frequency distribution of pod fiber content (hemicellulose (A), cellulose (B) and lignin (C)) and pod shattering (D) in F2A population (F2:3 generation) of the JP81610 × TVnu-457. Figures are drawn using data from the study of Suanum et al. [5] with permission from Springer Nature. Table S1: Marker genotypes of 28 F2 plants of F2B population (JP81610 x TVnu-457) selected for generating F2C population (F2:3 generation). A, B, H and—represent JP81610 genotype, TVnu-457 genotype, heterozygous and missing data, respectively. Table S2: Characteristics of DNA markers used in this study.

Author Contributions

Conceptualization, P.S.; methodology, P.S. and A.K.; formal analysis, P.W. and A.K.; investigation, P.W.; resources, P.S., X.C. and A.K.; data curation, P.S.; writing—original draft preparation, P.W.; writing—review and editing, P.S. and A.K.; supervision, P.S. and A.K.; funding acquisition, P.S. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by the Graduated School, Kasetsart University, Thailand.

Acknowledgments

We are thankful to Anochar Kaewwongwal for her assistance in marker genotyping. This research was funded by the Graduated School, Kasetsart University, Thailand.

Conflicts of Interest

The authors declare no conflict of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript, or in the decision to publish the results.

References

  1. Gondwe, T.M.; Alamu, E.O.; Mdziniso, P.; Maziya-Dixon, B. Cowpea (Vigna unguiculata (L.) Walp) for food security: An evaluation of end-user traits of improved varieties in Swaziland. Sci. Rep. 2019, 9, 15991. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  2. Pasquet, R. Wild cowpea (Vigna unguiculata) evolution. In Advances in Legume Systematics 8: Legumes of Economic Importance; Pickersgill, B., Lock, J.M., Eds.; Royal Botanic Gardens: Kew, UK, 1996; pp. 95–100. [Google Scholar]
  3. Timko, M.P.; Ehlers, J.D.; Roberts, P.A. Cowpea. In Pulses, Sugar and Tuber Crops; Kole, C., Ed.; Springer: Berlin/Heidelberg, Germany, 2007; pp. 49–67. [Google Scholar] [CrossRef]
  4. Fang, J.; Chao, C.-C.T.; Roberts, P.A.; Ehlers, J.D. Genetic diversity of cowpea [Vigna unguiculata (L.) Walp.] in four West African and USA breeding programs as determined by AFLP analysis. Genet. Resour. Crop Evol. 2007, 54, 1197–1209. [Google Scholar] [CrossRef]
  5. Suanum, W.; Somta, P.; Kongjaimun, A.; Yimram, T.; Kaga, A.; Tomooka, N.; Takahashi, Y.; Srinives, P. Co-localization of QTLs for pod fiber content and pod shattering in F2 and backcross populations between yardlong bean and wild cowpea. Mol. Breed. 2016, 36, 80. [Google Scholar] [CrossRef]
  6. Xu, P.; Wu, X.; Wang, B.; Liu, Y.; Qin, D.; Ehlers, J.D.; Close, T.J.; Hu, T.; Lu, Z.; Li, G. Development and polymorphism of Vigna unguiculata ssp. unguiculata microsatellite markers used for phylogenetic analysis in asparagus bean (Vigna unguiculata ssp. sesquipedialis (L.) Verdc.). Mol. Breed. 2010, 25, 675–684. [Google Scholar] [CrossRef]
  7. Kongjaimun, A.; Kaga, A.; Tomooka, N.; Somta, P.; Vaughan, D.A.; Srinives, P. The genetics of domestication of yardlong bean, Vigna unguiculata (L.) Walp. ssp. unguiculata cv.-gr. sesquipedalis. Ann. Bot. 2012, 109, 1185–1200. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  8. Ba, F.S.; Pasquet, R.S.; Gepts, P. Genetic diversity in cowpea [Vigna unguiculata (L.) Walp.] as revealed by RAPD markers. Genet. Resour. Crop Evol. 2004, 51, 539–550. [Google Scholar] [CrossRef]
  9. Xu, P.; Wu, X.; Wang, B.; Liu, Y.; Ehlers, J.D.; Close, T.J.; Roberts, P.A.; Diop, N.-N.; Qin, D.; Hu, T.; et al. A SNP and SSR based genetic map of asparagus Bean (Vigna. unguiculata ssp. sesquipedialis) and comparison with the broader species. PLoS ONE 2011, 6, e15952. [Google Scholar] [CrossRef] [Green Version]
  10. Liu, S.; Ding, F.; Chen, W.; Xu, G.; Cheng, J. Effects of organic fertilizers on soil nutrients and enzyme activities of continuous cropping soil of asparagus bean. Acta Agric. Zhejiangensis 2014, 26, 770–774. [Google Scholar]
  11. Xu, P.; Wu, X.; Wang, B.; Luo, J.; Liu, Y.; Ehlers, J.D.; Close, T.J.; Roberts, P.A.; Lu, Z.; Wang, S.; et al. Genome wide linkage disequilibrium in Chinese asparagus bean (Vigna unguiculata ssp. sesquipedialis) germplasm: Implications for domestication history and genome wide association studies. Heredity 2012, 109, 34–40. [Google Scholar] [CrossRef] [Green Version]
  12. Hegde, V.S.; Mishra, S.K. Landraces of cowpea, Vigna unguiculata (L.) Walp., as potential sources of genes for unique characters in breeding. Genet. Resour. Crop Evol. 2009, 56, 615–627. [Google Scholar] [CrossRef]
  13. Kongjaimun, A.; Kaga, A.; Tomooka, N.; Somta, P.; Shimizu, T.; Shu, Y.; Isemura, T.; Vaughan, D.A.; Srinives, P. An SSR-based linkage map of yardlong bean (Vigna unguiculata (L.) Walp. subsp. unguiculata Sesquipedalis Group) and QTL analysis of pod length. Genome 2012, 55, 81–92. [Google Scholar] [CrossRef] [PubMed]
  14. Kongjaimun, A.; Somta, P.; Tomooka, N.; Kaga, A.; Vaughan, D.A.; Srinives, P. QTL mapping of pod tenderness and total soluble solid in yardlong bean [Vigna unguiculata (L.) Walp. subsp.unguiculata cv.-gr. sesquipedalis]. Euphytica 2013, 189, 217–223. [Google Scholar] [CrossRef]
  15. Sakai, H.; Naito, K.; Takahashi, Y.; Sato, T.; Yamamoto, T.; Muto, I.; Itoh, T.; Tomooka, N. The Vigna Genome Server, ‘VigGS’: A Genomic Knowledge Base of the Genus Vigna Based on High-Quality, Annotated Genome Sequence of the Azuki Bean, Vigna angularis (Willd.) Ohwi & Ohashi. Plant Cell Physiol. 2015, 57. [Google Scholar] [CrossRef] [Green Version]
  16. Lo, S.; Muñoz-Amatriaín, M.; Boukar, O.; Herniter, I.; Cisse, N.; Guo, Y.-N.; Roberts, P.A.; Xu, S.; Fatokun, C.; Close, T.J. Identification of QTL controlling domestication-related traits in cowpea (Vigna unguiculata L. Walp). Sci. Rep. 2018, 8, 6261. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  17. Takahashi, Y.; Kongjaimun, A.; Muto, C.; Kobayashi, Y.; Kumagai, M.; Sakai, H.; Satou, K.; Teruya, K.; Shiroma, A.; Shimoji, M.; et al. Genetic factor for twisting legume pods identified by fine-mapping of shattering-related traits in azuki bean and yard-long bean. bioRxiv 2019, 774844. [Google Scholar] [CrossRef]
  18. Lodhi, M.A.; Ye, G.-N.; Weeden, N.F.; Reisch, B.I. A simple and efficient method for DNA extraction from grapevine cultivars andVitis species. Plant Mol. Biol. Rep. 1994, 12, 6–13. [Google Scholar] [CrossRef]
  19. Vogel, K.P.; Pedersen, J.F.; Masterson, S.D.; Toy, J.J. Evaluation of a filter bag system for NDF, ADF, and IVDMD forage analysis. Crop Sci. 1999, 39, 276–279. [Google Scholar] [CrossRef]
  20. Lonardi, S.; Muñoz-Amatriaín, M.; Liang, Q.; Shu, S.; Wanamaker, S.I.; Lo, S.; Tanskanen, J.; Schulman, A.H.; Zhu, T.; Luo, M.-C.; et al. The genome of cowpea (Vigna unguiculata [L.] Walp.). Plant J. 2019, 98, 767–782. [Google Scholar] [CrossRef] [Green Version]
  21. Temnykh, S.; DeClerck, G.; Lukashova, A.; Lipovich, L.; Cartinhour, S.; McCouch, S. Computational and experimental analysis of microsatellites in rice (Oryza sativa L.): Frequency, length variation, transposon associations, and genetic marker potential. Genome Res. 2001, 11, 1441–1452. [Google Scholar] [CrossRef] [Green Version]
  22. Untergasser, A.; Cutcutache, I.; Koressaar, T.; Ye, J.; Faircloth, B.C.; Remm, M.; Rozen, S.G. Primer3—New capabilities and interfaces. Nucleic Acids Res. 2012, 40, e115. [Google Scholar] [CrossRef] [Green Version]
  23. Seehalak, W.; Somta, P.; Sommanas, W.; Srinives, P. Microsatellite markers for mungbean developed from sequence database. Mol. Ecol. Resour. 2009, 9, 862–864. [Google Scholar] [CrossRef]
  24. Meng, L.; Li, H.; Zhang, L.; Wang, J. QTL IciMapping: Integrated software for genetic linkage map construction and quantitative trait locus mapping in biparental populations. Crop J. 2015, 3, 269–283. [Google Scholar] [CrossRef] [Green Version]
  25. Kosambi, D.D. The Estimation of Map Distances from Recombination Values. In D.D. Kosambi: Selected Works in Mathematics and Statistics; Ramaswamy, R., Ed.; Springer: New Delhi, India, 2016. [Google Scholar]
  26. Li, H.; Ribaut, J.-M.; Li, Z.; Wang, J. Inclusive composite interval mapping (ICIM) for digenic epistasis of quantitative traits in biparental populations. Theor. Appl. Genet. 2008, 116, 243–260. [Google Scholar] [CrossRef] [PubMed]
  27. Li, S.; Wang, J.; Zhang, L. Inclusive composite interval mapping of qtl by environment interactions in biparental populations. PLoS ONE 2015, 10, e0132414. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  28. Minic, Z.; Jouanin, L. Plant glycoside hydrolases involved in cell wall polysaccharide degradation. Plant Physiol. Biochem. 2006, 44, 435–449. [Google Scholar] [CrossRef] [PubMed]
  29. Leah, R.; Kigel, J.; Svendsen, I.; Mundy, J. Biochemical and molecular characterization of a barley seed beta-glucosidase. J. Biol. Chem. 1995, 270, 15789–15797. [Google Scholar] [CrossRef] [Green Version]
  30. Shang, X.H.; Wang, H.; Zhu, L.; Chai, Q.; Yu, Y.; Li, S.; Guo, W. Cotton Beta-Glucosidase Gene GhBG1A Coordinates Fiber Transition from Elongation to Secondary Cell Wall Deposition. In Proceedings of the 2018 International Cotton Genome Initiative (ICGI) Research Conference. Available online: https://www.cottongen.org/node/8287825 (accessed on 18 February 2020).
  31. Zhong, R.; McCarthy, R.L.; Lee, C.; Ye, Z.-H. Dissection of the transcriptional program regulating secondary wall biosynthesis during wood formation in poplar. Plant Physiol. 2011, 157, 1452. [Google Scholar] [CrossRef] [Green Version]
  32. Steiner-Lange, S.; Unte, U.S.; Eckstein, L.; Yang, C.; Wilson, Z.A.; Schmelzer, E.; Dekker, K.; Saedler, H. Disruption of Arabidopsis thaliana MYB26 results in male sterility due to non-dehiscent anthers. Plant J. 2003, 34, 519–528. [Google Scholar] [CrossRef]
  33. Yang, X.Y.; Li, J.G.; Pei, M.; Gu, H.; Chen, Z.L.; Qu, L.J. Over-expression of a flower-specific transcription factor gene AtMYB24 causes aberrant anther development. Plant Cell Rep. 2007, 26, 219–228. [Google Scholar] [CrossRef]
  34. Yang, J.H.; Wang, H. Molecular mechanisms for vascular development and secondary cell wall formation. Front. Plant Sci. 2016, 7, 356. [Google Scholar] [CrossRef] [Green Version]
  35. Parker, T.A.; Mier y Teran, J.C.B.; Palkovic, A.; Jernstedt, J.; Gepts, P. Genetic control of pod dehiscence in domesticated common bean: Associations with range expansion and local aridity conditions. bioRxiv 2019, 517516. [Google Scholar] [CrossRef]
  36. Rau, D.; Murgia, M.L.; Rodriguez, M.; Bitocchi, E.; Bellucci, E.; Fois, D.; Albani, D.; Nanni, L.; Gioia, T.; Santo, D.; et al. Genomic dissection of pod shattering in common bean: Mutations at non-orthologous loci at the basis of convergent phenotypic evolution under domestication of leguminous species. Plant J. 2019, 97, 693–714. [Google Scholar] [CrossRef] [PubMed]
  37. Zhong, R.; Ye, Z.-H. Complexity of the transcriptional network controlling secondary wall biosynthesis. Plant Sci. 2014, 229, 193–207. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  38. Kim, W.-C.; Ko, J.-H.; Kim, J.-Y.; Kim, J.; Bae, H.-J.; Han, K.-H. MYB46 directly regulates the gene expression of secondary wall-associated cellulose synthases in Arabidopsis. Plant J. 2013, 73, 26–36. [Google Scholar] [CrossRef] [PubMed]
Genes 11 00363 g001 550
Figure 1. Frequency distribution of cellulose (A), hemicellulose (B) and lignin (C) content of dry pod in F2 population F2B of the cross JP81610 × TVnu-457. The fibers were determined by the fiber bag technology method.
Figure 1. Frequency distribution of cellulose (A), hemicellulose (B) and lignin (C) content of dry pod in F2 population F2B of the cross JP81610 × TVnu-457. The fibers were determined by the fiber bag technology method.
Genes 11 00363 g001
Genes 11 00363 g002 550
Figure 2. Frequency distribution of cellulose (A), hemicellulose (B) and lignin (C) content of dry pod in F2:3 population F2C of the cross JP81610 × TVnu-457. The fibers were determined by the NIR microscopy method.
Figure 2. Frequency distribution of cellulose (A), hemicellulose (B) and lignin (C) content of dry pod in F2:3 population F2C of the cross JP81610 × TVnu-457. The fibers were determined by the NIR microscopy method.
Genes 11 00363 g002
Genes 11 00363 g003 550
Figure 3. Location of QTLs for cellulose, hemicellulose, and lignin contents in pod and pod shattering identified on linkage group 7 of populations F2A (A), F2B (B) and F2C (C) derived from a cross between JP81610 (yardlong bean) and TVnu-457 (wild cowpea) (see Materials and Methods Section for details). The QTLs were identified by inclusive composite interval mapping. The relationship between the QTLs on linkage maps (A, B and C) and candidate genes on the physical map is also shown (D).
Figure 3. Location of QTLs for cellulose, hemicellulose, and lignin contents in pod and pod shattering identified on linkage group 7 of populations F2A (A), F2B (B) and F2C (C) derived from a cross between JP81610 (yardlong bean) and TVnu-457 (wild cowpea) (see Materials and Methods Section for details). The QTLs were identified by inclusive composite interval mapping. The relationship between the QTLs on linkage maps (A, B and C) and candidate genes on the physical map is also shown (D).
Genes 11 00363 g003
Table
Table 1. Locations and effects of QTLs identified for pod fiber contents and pod shattering in F2:3 population F2A of the cross JP81610 × TVnu-457 by inclusive composite interval mapping.
Table 1. Locations and effects of QTLs identified for pod fiber contents and pod shattering in F2:3 population F2A of the cross JP81610 × TVnu-457 by inclusive composite interval mapping.
QTL NameTraitPositionFlanking MarkerLODPVE (%)AddDom
Hem7.1.1Hemicellulose35.30Vu-SSR01-2–Van07-SSR543.755.790.031.68
Hem7.1.2Hemicellulose44.09Vu05-GHIndel–VR29425.3051.32−3.500.33
Cel7.1.1Cellulose34.30Vu-SSR01-2–Van07-SSR545.4414.51−2.370.86
Lig7.1.1Lignin44.09Vu05-GHIndel–VR29422.8547.28−1.870.39
Shat7.1.1Shattering44.09Vu05-GHIndel–VR29413.2032.12−0.680.23
Table
Table 2. Locations and effects of QTLs identified for pod fiber contents in F2 population F2B of the cross JP81610 × TVnu-457 by inclusive composite interval mapping.
Table 2. Locations and effects of QTLs identified for pod fiber contents in F2 population F2B of the cross JP81610 × TVnu-457 by inclusive composite interval mapping.
QTL NameTraitPositionFlanking MarkerLODPVE (%)AddDom
Hem7.1.2Hemicellulose40.10VR294–cp0595151.4833.31−3.232.17
Cel7.1.1Cellulose35.70Van07-SSR54–Vu05-GHIndel9.6411.31−2.031.44
Lig7.1.1Lignin38.60Vu05-GHIndel–VR29457.0958.14−2.171.53
Table
Table 3. Locations and effects of QTLs identified for pod fiber contents in F2:3 population of the cross JP81610 × TVnu-457 by inclusive composite interval mapping.
Table 3. Locations and effects of QTLs identified for pod fiber contents in F2:3 population of the cross JP81610 × TVnu-457 by inclusive composite interval mapping.
QTL NameTraitPositionFlanking MarkerLODPVE (%)AddDom
Hem7.1.3Hemicellulose11.40cp08202–Vu-SSR01-24.465.23−0.651.08
Hem7.1.2Hemicellulose57.19Vu05-GHIndel–VR29444.4439.10−2.170.14
Cel7.1.3Cellulose7.80cp08202–Vu-SSR01-211.2510.77−1.721.09
Cel7.1.2Cellulose58.09VR294–cp0595141.0033.14−2.930.38
Lig7.1.2Lignin9.30cp08202–Vu-SSR01-26.515.47−0.790.72
Lig7.1.1Lignin60.19cp05951–Vu-SSR1172.9557.68−2.272.31

Share and Cite

MDPI and ACS Style

Watcharatpong, P.; Kaga, A.; Chen, X.; Somta, P. Narrowing Down a Major QTL Region Conferring Pod Fiber Contents in Yardlong Bean (Vigna unguiculata), a Vegetable Cowpea. Genes 2020, 11, 363. https://doi.org/10.3390/genes11040363

AMA Style

Watcharatpong P, Kaga A, Chen X, Somta P. Narrowing Down a Major QTL Region Conferring Pod Fiber Contents in Yardlong Bean (Vigna unguiculata), a Vegetable Cowpea. Genes. 2020; 11(4):363. https://doi.org/10.3390/genes11040363

Chicago/Turabian Style

Watcharatpong, Phurisorn, Akito Kaga, Xin Chen, and Prakit Somta. 2020. "Narrowing Down a Major QTL Region Conferring Pod Fiber Contents in Yardlong Bean (Vigna unguiculata), a Vegetable Cowpea" Genes 11, no. 4: 363. https://doi.org/10.3390/genes11040363

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop