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首页> 外文期刊>Brazilian Journal of Microbiology >Cloning and characterization of the gene encoding the PepF endopeptidase from the aquatic bacterium Caulobacter crescentus
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Cloning and characterization of the gene encoding the PepF endopeptidase from the aquatic bacterium Caulobacter crescentus

机译:水生细菌Caulobacter crescentus PepF内肽酶编码基因的克隆与鉴定

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摘要

The metallopeptidases have a very important role in bacteria, being involved in several processes that rely on protein turnover, such as nutrition, degradation of signal peptides, protein localization and virulence. We have cloned and characterized the gene of the metalloendopeptidase PepF from the aquatic bacterium Caulobacter crescentus. The gene upstream of pepF (orf1) encodes a conserved hypothetical protein found in Mycobacterium and Streptomyces. pepF is co-transcribed with the gene downstream (orf3), which encodes a protein that belongs to the ABC1 protein kinase family, suggesting that these two proteins may share a common function in the cell. The C. crescentus PepF protein possesses the conserved HEXGH motif present in zinc binding domains of PepF homologs. Disruption of the pepF gene by insertion of a vector sequence did not produced any growth defect, but the mutant strain possesses only 30% of the specific activity of endopeptidases present in the wild type strain. Deletions and point mutations in the regulatory region showed that there are two putative promoter regions, and the operon expression is independent of the transcription regulator CtrA. The results indicate that PepF is not essential for either growth or development of this bacterium using peptides as the sole carbon source, suggesting that other peptidases can be sharing this function.
机译:金属肽酶在细菌中具有非常重要的作用,涉及依赖蛋白质更新的多个过程,例如营养,信号肽的降解,蛋白质定位和毒力。我们已经从水生细菌Caulobacter crescentus克隆并鉴定了金属内肽酶PepF的基因。 pepF(orf1)上游的基因编码在分枝杆菌和链霉菌中发现的保守的假设蛋白质。 pepF与下游基因(orf3)共转录,该基因编码一种属于ABC1蛋白激酶家族的蛋白,表明这两种蛋白可能在细胞中具有共同的功能。 C.crescentus PepF蛋白具有在PepF同源物的锌结合域中存在的保守的HEXGH基序。通过插入载体序列破坏pepF基因没有产生任何生长缺陷,但是突变株仅具有野生型株中存在的内肽酶的比活性的30%。调控区域中的缺失和点突变表明存在两个推定的启动子区域,操纵子的表达独立于转录调控子CtrA。结果表明,使用肽作为唯一碳源,PepF对这种细菌的生长或发育不是必不可少的,这表明其他肽酶可以共享这一功能。

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