Exome-based new allele-specific PCR markers and transferability for sodicity tolerance in bread wheat (Triticum aestivum L.).

IF 2.3 3区 生物学 Q2 PLANT SCIENCES
Plant Direct Pub Date : 2023-08-18 eCollection Date: 2023-08-01 DOI:10.1002/pld3.520
Roopali Bhoite, Rosemary Smith, Urmil Bansal, Mirza Dowla, Harbans Bariana, Darshan Sharma
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引用次数: 0

Abstract

Targeted exome-based genotype by sequencing (t-GBS), a sequencing technology that tags SNPs and haplotypes in gene-rich regions was used in previous genome-wide association studies (GWAS) for sodicity tolerance in bread wheat. Thirty-nine novel SNPs including 18 haplotypes for yield and yield-components were identified. The present study aimed at developing SNP-derived markers by precisely locating new SNPs on ~180 bp allelic sequence of t-GBS, marker validation, and SNP functional characterization based on its exonic location. We identified unknown locations of significant SNPs/haplotypes by aligning allelic sequences on to IWGSC RefSeqv1.0 on respective chromosomes. Eighteen out of the target 39 SNP locations fulfilled the criteria for producing PCR markers, among which only eight produced polymorphic signals. These eight markers associated with yield, plants m-2, heads m-2, and harvest index, including a pleiotropic marker for yield, harvest index, and grains/head were validated for its amplification efficiency and phenotypic effects in focused identification germplasm strategy (FIGS) wheat set and a doubled haploid (DH) population (Scepter/IG107116). The phenotypic variation explained by these markers are in the range of 4.1-37.6 in the FIGS population. High throughput PCR-based genotyping using new markers and association with phenotypes in FIGS wheat set and DH population validated the effect of functional SNP on closely associated genes-calcineurin B-like- and dirigent protein, basic helix-loop-helix (BHLH-), plant homeodomain (PHD-) and helix-turn-helix myeloblastosis (HTH myb) type -transcription factor. Further, genome-wide SNP annotation using SnpEff tool confirmed that these SNPs are in gene regulatory regions (upstream, 3'-UTR, and intron) modifying gene expression and protein-coding. This integrated approach of marker design for t-GBS alleles, SNP functional annotation, and high-throughput genotyping of functional SNP offers translation solutions across crops and complex traits in crop improvement programs.

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基于外显子组的新等位基因特异性 PCR 标记和面包小麦(Triticum aestivum L. )耐碱性的可转移性。
基于外显子组的靶向基因型测序(t-GBS)是一种在基因丰富区域标记 SNPs 和单倍型的测序技术,曾用于面包小麦耐钠性的全基因组关联研究(GWAS)。结果发现了 39 个新的 SNPs,包括 18 个与产量和产量成分有关的单倍型。本研究旨在通过精确定位 t-GBS 约 180 bp 等位基因序列上的新 SNP、标记验证和基于其外显子位置的 SNP 功能表征来开发 SNP 衍生标记。通过将等位基因序列与相应染色体上的 IWGSC RefSeqv1.0 进行比对,我们确定了重要 SNPs/haplotypes 的未知位置。在目标的 39 个 SNP 位点中,有 18 个符合产生 PCR 标记的标准,其中只有 8 个产生了多态性信号。在重点鉴定种质策略(FIGS)小麦组和一个加倍单倍体(DH)群体(Scepter/IG107116)中验证了这八个与产量、株数 m-2、头数 m-2 和收获指数相关的标记(包括一个与产量、收获指数和粒/头相关的多效标记)的扩增效率和表型效应。在 FIGS 群体中,这些标记解释的表型变异范围为 4.1-37.6。在 FIGS 小麦群体和 DH 群体中,使用新标记物进行基于高通量 PCR 的基因分型以及与表型的关联验证了功能性 SNP 对密切相关基因--类钙调蛋白 B 和 dirigent 蛋白、碱性螺旋-环-螺旋(BHLH-)、植物同源染色体(PHD-)和螺旋-转-螺旋骨髓母细胞病(HTH myb)型转录因子--的影响。此外,利用 SnpEff 工具进行的全基因组 SNP 注释证实,这些 SNP 位于基因调控区(上游、3'-UTR 和内含子),可改变基因表达和蛋白质编码。这种针对 t-GBS 等位基因的标记设计、SNP 功能注释和功能 SNP 的高通量基因分型的综合方法为作物改良计划中跨作物和复杂性状的转化提供了解决方案。
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来源期刊
Plant Direct
Plant Direct Environmental Science-Ecology
CiteScore
5.00
自引率
3.30%
发文量
101
审稿时长
14 weeks
期刊介绍: Plant Direct is a monthly, sound science journal for the plant sciences that gives prompt and equal consideration to papers reporting work dealing with a variety of subjects. Topics include but are not limited to genetics, biochemistry, development, cell biology, biotic stress, abiotic stress, genomics, phenomics, bioinformatics, physiology, molecular biology, and evolution. A collaborative journal launched by the American Society of Plant Biologists, the Society for Experimental Biology and Wiley, Plant Direct publishes papers submitted directly to the journal as well as those referred from a select group of the societies’ journals.
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