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miRNA164e 抑制鹰嘴豆中 NAC100 转录因子介导的种子贮藏蛋白的合成。

MicroRNA164e suppresses NAC100 transcription factor-mediated synthesis of seed storage proteins in chickpea.

机构信息

National Institute of Plant Genome Research, Aruna Asaf Ali Marg, PO Box No. 10531, New Delhi, 110067, India.

出版信息

New Phytol. 2024 Jun;242(6):2652-2668. doi: 10.1111/nph.19770. Epub 2024 Apr 22.

DOI:10.1111/nph.19770
PMID:38649769
Abstract

Development of protein-enriched chickpea varieties necessitates an understanding of specific genes and key regulatory circuits that govern the synthesis of seed storage proteins (SSPs). Here, we demonstrated the novel involvement of Ca-miR164e-CaNAC100 in regulating SSP synthesis in chickpea. Ca-miRNA164e was significantly decreased during seed maturation, especially in high-protein accessions. The miRNA was found to directly target the transactivation conferring C-terminal region of a nuclear-localized transcription factor, CaNAC100 as revealed using RNA ligase-mediated-rapid amplification of cDNA ends and target mimic assays. The functional role of CaNAC100 was demonstrated through seed-specific overexpression (NACOE) resulting in significantly augmented seed protein content (SPC) consequential to increased SSP transcription. Further, NACOE lines displayed conspicuously enhanced seed weight but reduced numbers and yield. Conversely, a downregulation of CaNAC100 and SSP transcripts was evident in seed-specific overexpression lines of Ca-miR164e that culminated in significantly lowered SPC. CaNAC100 was additionally demonstrated to transactivate the SSP-encoding genes by directly binding to their promoters as demonstrated using electrophoretic mobility shift and dual-luciferase reporter assays. Taken together, our study for the first time established a distinct role of CaNAC100 in positively influencing SSP synthesis and its critical regulation by CamiR164e, thereby serving as an understanding that can be utilized for developing SPC-rich chickpea varieties.

摘要

开发富含蛋白质的鹰嘴豆品种需要了解特定的基因和关键调控回路,这些基因和回路控制着种子贮藏蛋白(SSP)的合成。在这里,我们证明了 Ca-miR164e-CaNAC100 参与调控鹰嘴豆 SSP 合成的新功能。在种子成熟过程中,Ca-miRNA164e 显著下调,尤其是在高蛋白品系中。通过 RNA 连接酶介导的快速 cDNA 末端扩增和靶标模拟试验,发现该 miRNA 直接靶向核定位转录因子的 C 端激活区。通过种子特异性过表达(NACOE)证明了 CaNAC100 的功能作用,导致种子蛋白含量(SPC)显著增加,这是由于 SSP 转录增加所致。此外,NACOE 系的种子重量明显增加,但种子数量和产量减少。相反,Ca-miR164e 的种子特异性过表达系中 CaNAC100 和 SSP 转录物的下调明显,导致 SPC 显著降低。通过电泳迁移率变动和双荧光素酶报告基因试验,进一步证明 CaNAC100 通过直接结合其启动子来转录激活 SSP 编码基因。综上所述,我们的研究首次确立了 CaNAC100 在正向影响 SSP 合成及其对 CamiR164e 的关键调控中的独特作用,从而为开发富含 SPC 的鹰嘴豆品种提供了一定的理解。

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