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园艺学报 ›› 2013, Vol. 40 ›› Issue (12): 2429-2440.

• 蔬菜 • 上一篇    下一篇

甘蓝花粉管钙感应蛋白CaM 与SRK 相互作用研究

 许俊强, 孙梓健, 宋 明, 汤青林, 王志敏, 王小佳   

  1. (西南大学园艺园林学院,南方山地园艺学教育部重点实验室,重庆市蔬菜学重点实验室,重庆 400715)
  • 出版日期:2013-12-25 发布日期:2013-12-25

Studies on the Interactions Between the Pollen Tube Calmodulin(CaM)and SRK from Brassica oleracea var. capitata

 XU  Jun-Qiang, SUN  Zi-Jian, SONG   Ming, TANG  Qing-Lin, WANG  Zhi-Min, WANG  Xiao-Jia   

  1. (Key Laboratory of Horticulture Science for Southern Mountainous Regions,Ministry of Education;Chongqing Key
    Laboratory of Olericulture,College of Horticulture and Landscape Architecture,Southwest University,Chongqing 400715,
    China)
  • Online:2013-12-25 Published:2013-12-25

摘要: 为研究甘蓝花粉管钙感应蛋白CaM 与SRK 相互作用的分子机理及其可能相互作用的区域,
从自交不亲和甘蓝材料‘E1’中分别克隆得到CaM12 基因450 bp 及S 位点受体激酶(SRK7)基因全长
序列2 118 bp,并亚克隆得到SRK 胞外域(eSRK)和胞内激酶域(iSRK),构建原核表达载体pGEX-CaM12、
pCold-eSRK 和pCold-iSRK,转化E. coli BL21(DE3)进行原核表达,表达产物纯化后进行体外相互作用,
结果表明CaM12 能够与SRK7 进行相互作用,但作用区域是iSRK7 而不是eSRK7。为进一步验证其相互
作用,本研究利用酵母双杂交系统,构建pGBKT7-CaM12、pGADT7-eSRK7、pGADT7-iSRK7 和
pGADT7-SRK7 酵母表达载体,转化相应酵母Y2HGold 和Y187 感受态细胞后未出现自激活和毒性现象,
相互作用结果与原核表达检测一致。同时将CaM12 的3 个EF-hands 结构域突变体CaM12-2-、CaM12-23-
和CaM12-234-与iSRK7 分别构建酵母表达载体pGADT7-CAM12-2-、pGADT7-CAM12-23-、pGADT7-
CAM12-234-,检测其相互作用。结果表明CaM12 EF-hands 突变体CaM12-2-、CaM12-23-和CaM12-234-
在酵母双杂交系统中均不能与iSRK7 片段发生相互作用,说明CaM12 的EF-hands 结构域突变后失去结
合Ca2+能力而不能与iSRK7 相互作用。该研究可为自交不亲和机理提供新的参考依据。
关键

关键词: 结球甘蓝, CaM12, S 位点受体激酶(SRK7)基因, 原核表达, 酵母双杂交

Abstract: In order to study the molecular mechanism and possible interaction domains between
pollen tube calmodulin(CaM) protein and S locus receptor kinase(SRK)from Brassica oleracea L. var.
capitata L. We got the full length sequence of CaM12 with 450 bp and SRK7 gene with 2 118 bp from
self-incompatibility of Brassica oleracea var. capitata E1,respectively,and got extracellular domain of
SRK(eSRK7) and intracellular kinase domain(iSRK7),then constructed prokaryotic expression vectors of pGEX-CaM12,pCold-eSRK7 and pCold-iSRK7,transformed into E. coli BL21(DE3)and checked the
interactions with purified expression products in vitro. The results showed that CaM12 protein and SRK7
could do interaction,and interactive domain is iSRK7 rather than eSRK7. In order to verify their
interaction furtherly,yeast two-hybrid system was used in this study,we constructed yeast expression
vectors pGBKT7-CaM12 , pGADT7-eSRK7 , pGADT7-iSRK7 and pGADT7-SRK7 , transformed
into corresponding Y2HGold and Y187 yeast cells,and made sure that they did not appear the
self-activation and toxicity. The results was consistent with prokaryotic expression. Simultaneously,we
constructed yeast expression vectors pGADT7-CAM12-2-,pGADT7-CAM12-23-,pGADT7-CAM12-234-
and pGBKT7-iSRK7 with CaM12-2-,CaM12-23-,CaM12-234- mutants from three EF-hands of CaM12
and iSRK7,and tested their interactions. The results showed that all CaM EF-hands mutants CaM12-2-,
CaM12-23- and CaM12-234- cannot interact with iSRK7 in yeast two-hybrid system. CaM12 protein lost
the ability to combine Ca2+ and cannot interact with iSRK7 after EF-hands structure domains were
mutated.This study could provide a new reference for the mechanism of self-incompatibility in Brassica
oleracea.

Key words: Brassica oleracea, CaM12, SRK7, prokaryotic expression, yeast two-hybrid

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