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串联重复基因编码的多聚半乳糖醛酸酶抑制剂与豇豆(Vigna aconitifolia)对绿豆象(Callosobruchus chinensis)的抗性有关。

Tandemly duplicated genes encoding polygalacturonase inhibitors are associated with bruchid (Callosobruchus chinensis) resistance in moth bean (Vigna aconitifolia).

机构信息

Department of Agronomy, Faculty of Agriculture at Kamphaeng Saen, Kasetsart University, Kamphaeng Saen Campus, Kamphaeng Saen, Nakhon Pathom 73140, Thailand; Graduate School of Bioagricultural Sciences, Nagoya University, Furo-cho, Chikusa-ku, Nagoya 464-8601, Japan.

Department of Agronomy, Faculty of Agriculture at Kamphaeng Saen, Kasetsart University, Kamphaeng Saen Campus, Kamphaeng Saen, Nakhon Pathom 73140, Thailand.

出版信息

Plant Sci. 2022 Oct;323:111402. doi: 10.1016/j.plantsci.2022.111402. Epub 2022 Jul 26.

DOI:10.1016/j.plantsci.2022.111402
PMID:35905896
Abstract

Bruchids are stored-grain insect pests responsible for serious seed loss in legume crops. A previous study using an F population (F2OA) derived from a cross between wild moth-bean (Vigna aconitifolia [Jacq.] Maréchal) accession TN67 (resistant) and cultivated moth-bean accession ICPMO056 (susceptible) revealed that resistance to the azuki bean weevil (Callosobruchus chinensis L.) in TN67 was regulated by a single gene located in the major quantitative trait locus-qVacBrc2.1. In this study, qVacBrc2.1 was finely mapped and candidate genes in this locus were identified using F2OA and another large F population (F2NB) derived from the cross mentioned previously. In contrast to the previous study, segregation analysis in the F2NB population revealed that resistance against this pest was controlled by two genes. Furthermore, the addition of novel markers to qVacBrc2.1 and reanalysis of the QTL in the F2OA population demonstrated that qVacBrc2.1 constituted two linked QTLs-qVacBrc2.1-A and qVacBrc2.1-B. The presence of qVacBrc2.1-B was verified using the population F2NB. Comparative genomics using three Vigna spp. strongly suggested the presence of two tandemly duplicated genes, VacPGIP1 and VacPGIP2, which encoded polygalacturonase inhibitors (polygalacturonase-inhibiting proteins) as the candidates for conferring resistance, but only VacPGIP1 could be successfully cloned and sequenced. The alignment of VacPGIP1 coding sequences of TN67 and ICPMO056 revealed eight single nucleotide polymorphisms, three of which altered the amino-acid sequence of the predicted domains of polygalacturonase inhibitors in ICPMO056. Overall, these findings indicate that VacPGIP1 and VacPGIP2 regulated C. chinensis resistance in TN67.

摘要

象甲是为害豆科作物的重要储粮害虫,会导致严重的种子损失。先前的研究使用来自野生木豆(Vigna aconitifolia [Jacq.] Maréchal)TN67(抗性)和栽培木豆 ICPMO056(敏感)杂交的 F 群体(F2OA)表明,TN67 对红小豆象甲(Callosobruchus chinensis L.)的抗性由位于主数量性状位点 qVacBrc2.1 中的单个基因调控。在这项研究中,使用 F2OA 和先前提到的另一个大型 F 群体(F2NB)精细地映射了 qVacBrc2.1,并鉴定了该基因座中的候选基因。与先前的研究不同,F2NB 群体的分离分析表明,该害虫的抗性由两个基因控制。此外,向 qVacBrc2.1 添加新标记并重新分析 F2OA 群体中的 QTL 表明,qVacBrc2.1 由两个连锁 QTL 组成-qVacBrc2.1-A 和 qVacBrc2.1-B。使用群体 F2NB 验证了 qVacBrc2.1-B 的存在。使用三个 Vigna spp. 的比较基因组学强烈表明存在两个串联重复基因 VacPGIP1 和 VacPGIP2,它们编码果胶酶抑制剂(果胶酶抑制蛋白)作为赋予抗性的候选基因,但只有 VacPGIP1 可以成功克隆和测序。TN67 和 ICPMO056 的 VacPGIP1 编码序列的比对显示了 8 个单核苷酸多态性,其中 3 个改变了 ICPMO056 中预测的果胶酶抑制剂结构域的氨基酸序列。总的来说,这些发现表明 VacPGIP1 和 VacPGIP2 调节了 TN67 对红小豆象甲的抗性。

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