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枯草芽孢杆菌芽孢特有的新型小酸溶性蛋白:编码基因的鉴定以及其中两个基因的调控与功能

New small, acid-soluble proteins unique to spores of Bacillus subtilis: identification of the coding genes and regulation and function of two of these genes.

作者信息

Bagyan I, Setlow B, Setlow P

机构信息

Department of Biochemistry, University of Connecticut Health Center, Farmington, Connecticut 06032, USA.

出版信息

J Bacteriol. 1998 Dec;180(24):6704-12. doi: 10.1128/JB.180.24.6704-6712.1998.

Abstract

Eleven small, acid-soluble proteins (SASP) which are present in spores but not in growing cells of Bacillus subtilis were identified by sequence analysis of proteins separated by acrylamide gel electrophoresis of acid extracts from spores which lack the three major SASP (alpha, beta, and gamma). Six of these proteins are encoded by open reading frames identified previously or by analysis of the complete sequence of the B. subtilis genome, including two minor alpha/beta-type SASP (SspC and SspD) and a putative spore coat protein (CotK). Five proteins are encoded by short open reading frames that were not identified as coding regions in the analysis of the complete B. subtilis genomic sequence. Studies of the regulation of two of the latter genes, termed sspG and sspJ, showed that both are expressed only in sporulation. The sspG gene is transcribed in the mother cell compartment by RNA polymerase with the mother cell-specific sigma factor for RNA polymerase, sigmaK, and is cotranscribed with a downstream gene, yurS; sspG transcription also requires the DNA binding protein GerE. In contrast, sspJ is transcribed in the forespore compartment by RNA polymerase with the forespore-specific sigmaG and appears to give a monocistronic transcript. A mutation eliminating SspG had no effect on sporulation or spore properties, while loss of SspJ caused a slight decrease in the rate of spore outgrowth in an otherwise wild-type background.

摘要

通过对缺乏三种主要小酸溶性蛋白(SASP,即α、β和γ)的芽孢酸提取物进行丙烯酰胺凝胶电泳分离的蛋白质进行序列分析,鉴定出了11种存在于枯草芽孢杆菌芽孢中但不存在于生长细胞中的小酸溶性蛋白。其中六种蛋白由先前鉴定的开放阅读框或通过枯草芽孢杆菌基因组完整序列分析编码,包括两种次要的α/β型SASP(SspC和SspD)和一种假定的芽孢衣蛋白(CotK)。另外五种蛋白由短开放阅读框编码,这些短开放阅读框在枯草芽孢杆菌基因组完整序列分析中未被鉴定为编码区。对后两个基因(称为sspG和sspJ)的调控研究表明,二者均仅在芽孢形成过程中表达。sspG基因在母细胞区室中由RNA聚合酶与母细胞特异性的RNA聚合酶σ因子σK转录,并与下游基因yurS共转录;sspG转录还需要DNA结合蛋白GerE。相比之下,sspJ在芽孢前体区室中由RNA聚合酶与芽孢前体特异性的σG转录,并且似乎产生单顺反子转录本。消除SspG的突变对芽孢形成或芽孢特性没有影响,而在其他方面为野生型背景下,SspJ的缺失导致芽孢萌发速率略有下降。

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