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植物研究 ›› 2026, Vol. 46 ›› Issue (2): 246-258.doi: 10.7525/j.issn.1673-5102.2026.02.005

• 研究论文column:Original Paper • 上一篇    下一篇

大花红景天盐胁迫调控基因RcNAC22克隆及功能分析

张力鹏1(), 武美2, 王宏鹏2, 李天宇2   

  1. 1.天津商业大学生物技术与食品科学学院,食品生物技术重点实验室,天津 300134
    2.南开大学生命科学学院,天津 300071
  • 收稿日期:2025-08-27 出版日期:2026-03-20 发布日期:2026-04-02
  • 通讯作者: 张力鹏 E-mail:zhanglp@tjcu.edu.cn
  • 作者简介:张力鹏(1989—),男,博士,实验师,主要从事药用植物基因分子生物学研究。

Salt Stress-related RcNAC22 Gene Cloning and Function Analysis in Rhodiolacrenulata

Lipeng ZHANG1(), Mei WU2, Hongpeng WANG2, Tianyu LI2   

  1. 1.Key Laboratory of Food Biotechnology,School of Biotechnology and Food Science,Tianjin University of Commerce,Tianjin 300134
    2.College of Life Sciences,Nankai University,Tianjin 300071
  • Received:2025-08-27 Online:2026-03-20 Published:2026-04-02
  • Contact: Lipeng ZHANG E-mail:zhanglp@tjcu.edu.cn

摘要:

本研究克隆大花红景天(Rhodiola crenulata)转录因子NAC家族成员之一RcNAC22基因,并对其进行生物信息学分析和功能验证。结果表明:RcNAC22基因全长为1 049 bp,含2个内含子、3个外显子,编码293个氨基酸。其蛋白质相对分子质量为33 625.02,属亲水蛋白,性质较稳定,不具有跨膜结构域和信号肽且亚细胞定位于细胞核,含有32个可磷酸化位点。RcNAC22基因包含1个NAM结构域(no apical meristem),第4结构域为转录抑制结构域NARD区,与狭叶红景天(R. kirilowii)亲缘关系最近。RcNAC22基因在6个器官(根、成熟茎、幼茎、叶、顶芽和花)中均有表达但主要存在于绿色器官(茎、叶、顶芽)中,同时受多种非生物胁迫和植物激素脱落酸(ABA)、水杨酸(SA)的诱导表达。RcNAC22蛋白对酵母细胞没有毒性,其全长基因和截短C端均具有自激活活性。此外,以丹参(Salviamiltiorrhiza)为转基因受体研究RcNAC22基因过表达对植物生长的影响,结果显示:提高RcNAC22基因表达量不会影响丹参的生长发育过程,但降低其对盐胁迫的耐受性。本研究揭示了RcNAC22基因的生物学功能,为进一步开展大花红景天分子生物学研究提供理论基础。

关键词: 大花红景天, 转录因子, 基因克隆, 盐胁迫

Abstract:

This study cloned the RcNAC22 gene of R. crenulata and conducted bioinformatics analysis and functional verification. The results showed that the full length of RcNAC22 gene was 1 049 bp, containing two introns and three exons, and encoding 293 amino acids. Its protein relative molecular weight was 33 625.02, belonging to a hydrophilic protein, with relatively stable properties, no transmembrane domain or signal peptide, and subcellular localization in the nucleus, containing 32 phosphorylation sites. RcNAC22 contains one NAM domain (no apical meristem), and the fourth domain is the transcriptional repression domain NARD region, and it was most closely related to that of R.kirilowii. RcNAC22 gene was expressed in all six tested organs (root, mature stem, young stem, leaf, apical bud, flower) but mainly in green organs (stem, leaf, apical bud), and its expression could be induced by various abiotic stresses and plant hormones ABA and SA. RcNAC22 gene had no cytotoxicity to yeast cells, and both the full-length gene and truncated C-terminal had self-activation activity. In addition, using Salvia miltiorrhiza as the transgenic receptor to study the RcNAC22 gene effect on plant growth, the results showed that overexpression of RcNAC22 gene did not affect the growth and development of Salviamiltiorrhiza, but reduced the tolerance to salt stress. This study revealed the biological function of the RcNAC gene, providing a theoretical basis for further molecular biological research on R. crenulata.

Key words: Rhodiolacrenulata, transcription factor, gene cloning, salt stress

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