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病程相关蛋白PRB-1b的暗诱导及亚细胞定位

Dark induction and subcellular localization of the pathogenesis-related PRB-1b protein.

作者信息

Sessa G, Yang X Q, Raz V, Eyal Y, Fluhr R

机构信息

Department of Plant Genetics, Weizmann Institute of Science, Rehovot, Israel.

出版信息

Plant Mol Biol. 1995 Jun;28(3):537-47. doi: 10.1007/BF00020400.

DOI:10.1007/BF00020400
PMID:7632922
Abstract

The PRB-1b gene codes for a basic-type pathogenesis-related protein of the PR-1 family of tobacco. PRB-1b mRNA accumulation is induced in response to biotic and abiotic elicitors, such as TMV, ethylene, salicylic acid, alpha-amino butyric acid and darkness. In order to determine the location of elements that control dark-regulated PRB-1b gene expression, we tested promoter, transcribed regions and 3'-downstream regions of the gene for their ability to respond to dark induction in transgenic tobacco plants. An ethylene-inducible promoter region of 863 bp was not able to confer dark induction to a beta-glucuronidase reporter gene, while a construct containing the transcribed region of the gene and 3'-downstream sequences, driven by the cauliflower mosaic virus 35S promoter, was correctly dark-regulated. The results indicate that dark-induction of the PRB-1b gene can be controlled by 3'-downstream elements at the transcriptional level or by transcribed sequences at the post-transcriptional level. A circadian clock regulation of the PRB-1b gene was excluded, as fluctuations of PRB-1b transcript levels were not observed in plants placed in constant light or darkness. Subcellular localization of the PRB-1b protein was also determined, in tobacco protoplasts preparations and in cell cultures. The PRB-1b polypeptide was predominantly detected in protoplast vacuoles and was not secreted to the media in cell cultures. These results support an intracellular localization for the PRB-1b protein, as reported for other basic-type components of the pathogenesis-related proteins family.

摘要

PRB - 1b基因编码烟草PR - 1家族的一种碱性病程相关蛋白。PRB - 1b mRNA的积累可被生物和非生物激发子诱导,如烟草花叶病毒、乙烯、水杨酸、α - 氨基丁酸和黑暗。为了确定控制PRB - 1b基因黑暗调控表达的元件位置,我们检测了该基因的启动子、转录区和3'下游区在转基因烟草植株中对黑暗诱导的响应能力。一个863 bp的乙烯诱导型启动子区域不能赋予β - 葡萄糖醛酸酶报告基因黑暗诱导能力,而一个由花椰菜花叶病毒35S启动子驱动、包含该基因转录区和3'下游序列的构建体则能被正确地进行黑暗调控。结果表明,PRB - 1b基因的黑暗诱导可在转录水平上由3'下游元件控制,或在转录后水平上由转录序列控制。由于在持续光照或黑暗条件下的植株中未观察到PRB - 1b转录水平的波动,因此排除了PRB - 1b基因的昼夜节律调控。还在烟草原生质体制备物和细胞培养物中确定了PRB - 1b蛋白的亚细胞定位。PRB - 1b多肽主要在原生质体液泡中被检测到,在细胞培养中不分泌到培养基中。这些结果支持了PRB - 1b蛋白定位于细胞内,这与病程相关蛋白家族其他碱性类型成分的报道一致。

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