生物技术通报 ›› 2022, Vol. 38 ›› Issue (10): 73-79.doi: 10.13560/j.cnki.biotech.bull.1985.2021-1597

• 技术与方法 • 上一篇    下一篇

烟草NtCBT基因启动子酵母单杂诱饵载体构建及互作蛋白筛选

余婧1(), 杨慧1, 余世洲1, 赵会纳1, 郑庆霞2, 王兵1, 雷波1()   

  1. 1.贵州省烟草科学研究院 烟草行业烟草分子遗传重点实验室,贵阳 550081
    2.中国烟草总公司郑州烟草研究院,郑州 450001
  • 收稿日期:2021-12-25 出版日期:2022-10-26 发布日期:2022-11-11
  • 作者简介:余婧,女,硕士,高级农艺师,研究方向:烟草分子生物学;E-mail:yujingbio@126.com
  • 基金资助:
    中国烟草总公司贵州省公司科技项目(2021XM02);中国烟草总公司科技项目(110202101005(JY-05));中国烟草总公司科技项目(110202001021(JY-04))

Construction of Yeast One-hybrid Bait Vector of Tobacco NtCBT Gene Promoter and Screening of Interacted Proteins

YU Jing1(), YANG Hui1, YU Shi-zhou1, ZHAO Hui-na1, ZHENG Qing-xia2, WANG Bing1, LEI Bo1()   

  1. 1. Guizhou Academy of Tobacco Science,Molecular Genetics Key Laboratory of China Tobacco,Guiyang 550081
    2. Zhengzhou Tobacco Research Institute of CNTC,Zhengzhou 450001
  • Received:2021-12-25 Published:2022-10-26 Online:2022-11-11

摘要:

为了筛选烟草类西柏烷生物合成途径中西柏三烯一醇合酶基因(NtCBT)的上游调控转录因子,将NtCBT基因启动子截为6段(P1-P6区域),分别构建酵母单杂诱饵载体pAbAi-Px,将pAbAi-Px 转化Y1H酵母感受态细胞构建诱饵菌株并进行自激活检测,从烟草腺毛酵母cDNA文库中筛选与P5区域(-279 - -119 bp)互作的转录因子。结果表明,P1-P5区域所构建的诱饵菌株,在AbA浓度为200 ng/mL时转录自激活得到有效抑制;在以P5区域为诱饵菌株的筛库实验中,共获得49个阳性克隆,去除冗余序列后35个克隆为非重复序列,其中3个克隆注释为ANL2、ML1及NF-Y转录因子。以上结果为进一步研究NtCBT基因的表达调控机制奠定了基础。

关键词: 酵母单杂交, 转录因子, 栽培烟草, 启动子, NtCBT基因, 类西柏烷

Abstract:

To screen the upstream regulatory transcription factors of cembratrienol synthase(NtCBT)in the cembranoids synthesis pathway of tobacco(Nicotiana tabacum L.),the promoter of NtCBT gene was cut into P1 to P6 regions,six yeast one-hybrid bait vectors pAbAi-Px were constructed and transformed into Y1H competent yeast cells,bait strains were constructed,and a self-activation experiment was completed. Furthermore,a screening was finished from yeast cDNA library of tobacco trichomes in order to obtain the transcription factors that interacted with P5 regions(-279 - -119 bp). The results showed that,the growths of the strains containing P1 to P5 regions bait strain were inhibited on the medium added with 200 ng/mL AbA. A total of 49 positive colonies were obtained through Y1H screening when P5 regions as bait strain,among them,35 colonies were non-repeating sequences,and 3 of colonies were annotated as transcription factors of ANL2,ML1 and NF-Y. Above results lay a foundation for further study of gene expression and regulation mechanism of NtCBT.

Key words: yeast one-hybrid, transcription factors, Nicotiana tabacum L., promoter, NtCBT gene, cembranoids