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与球形红杆菌2.4.1中光合作用基因表达相关的组氨酸激酶PrrB的复杂调控活动。

Complex regulatory activities associated with the histidine kinase PrrB in expression of photosynthesis genes in Rhodobacter sphaeroides 2.4.1.

作者信息

Eraso J M, Kaplan S

机构信息

Department of Microbiology and Molecular Genetics, The University of Texas Medical School, Houston 77030, USA.

出版信息

J Bacteriol. 1996 Dec;178(24):7037-46. doi: 10.1128/jb.178.24.7037-7046.1996.

DOI:10.1128/jb.178.24.7037-7046.1996
PMID:8955382
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC178613/
Abstract

Rhodobacter sphaeroides 2.4.1 synthesizes a specialized photosynthetic membrane upon reduction of the O2 tension below threshold levels. The genes prrB and prrA encode a sensor kinase and a response regulator, respectively, of a two-component regulatory system that presumably is involved in transduction of the signal(s) that monitors alterations in oxygen levels. A third gene, prrC, is also involved in this cascade of events. Previously, we described a mutant form of PrrB, namely, PrrB78 (J. M. Eraso and S. Kaplan, J. Bacteriol. 177:2695-2706, 1995), which results in aerobic expression of the photosynthetic apparatus. Here we examine three mutated forms of the prrB gene that have the potential to encode truncated polypeptides containing the N-terminal 6, 63, or 163 amino acids, respectively. The resulting mutant strains showed residual levels of the light-harvesting spectral complexes and had diminished photosynthetic growth rates at high light intensities with no discernible growth under intermediate or low light conditions. When either lacZ transcriptional fusions or direct mRNA determinations were used to monitor specific photosynthesis gene expression, all the mutant strains showed unexpectedly high levels of gene expression when compared to mutant strains affected in prrA. Conversely, when translational fusions were used to monitor photosynthesis gene expression in these mutant strains, expression of both puc and puf operons was reduced, especially puf expression. In light of these studies and those of the PrrB78 mutant, the data suggest that PrrA can be activated in situ by something other than PrrB, and it also appears that PrrB can function as a negative regulator acting through PrrA. Finally, we consider the role of the Prr regulatory system in the posttranscriptional control of photosynthesis gene expression.

摘要

球形红杆菌2.4.1在将氧气张力降低到阈值水平以下时会合成一种特殊的光合膜。基因prrB和prrA分别编码一个双组分调节系统的传感激酶和响应调节因子,该系统可能参与监测氧气水平变化的信号转导。第三个基因prrC也参与了这一系列事件。此前,我们描述了一种PrrB的突变形式,即PrrB78(J. M. 埃拉索和S. 卡普兰,《细菌学杂志》177:2695 - 2706,1995),它导致光合装置的有氧表达。在这里,我们研究了prrB基因的三种突变形式,它们有可能分别编码包含N端6个、63个或163个氨基酸的截短多肽。所得突变菌株显示出捕光光谱复合体的残留水平,并且在高光强度下光合生长速率降低,在中等或低光条件下没有明显生长。当使用lacZ转录融合或直接mRNA测定来监测特定光合作用基因表达时,与prrA受影响的突变菌株相比,所有突变菌株都显示出意外高的基因表达水平。相反,当使用翻译融合来监测这些突变菌株中的光合作用基因表达时,puc和puf操纵子的表达都降低了,尤其是puf表达。根据这些研究以及PrrB78突变体的研究,数据表明PrrA可以被PrrB以外的其他物质原位激活,并且似乎PrrB可以作为一种通过PrrA起作用的负调节因子。最后,我们考虑Prr调节系统在光合作用基因表达的转录后控制中的作用。

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