首页> 外文期刊>Journal of Molecular Biology >Defining the Bacillus subtilis sigma(W) regulon: a comparative analysis of promoter consensus search, run-off transcription/macroarray analysis (ROMA), and transcriptional profiling approaches.
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Defining the Bacillus subtilis sigma(W) regulon: a comparative analysis of promoter consensus search, run-off transcription/macroarray analysis (ROMA), and transcriptional profiling approaches.

机译:定义枯草芽孢杆菌σ(W)调节剂:启动子共有搜索,径流转录/宏阵列分析(ROMA)和转录谱分析方法的比较分析。

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The Bacillus subtilis extracytoplasmic function (ECF) sigma factor sigma(W) controls a large regulon that is strongly induced by alkali shock. To define the physiological role of sigma(W) we have sought to identify the complete set of genes under sigma(W) control. Previously, we described a promoter consensus search procedure to identify sigma(W) controlled genes. Herein, we introduce a novel method to identify additional target promoters: run-off transcription followed by macroarray analysis (ROMA). We compare the resulting list of targets with those identified in conventional transcriptional profiling studies and using the consensus search approach. While transcriptional profiling identifies genes that are strongly dependent on sigma(W) for in vivo expression, some sigma(W)-dependent promoters are not detected due to the masking effects of other promoter elements, overlapping recognition with other ECF sigma factors, or both. Taken together, the consensus search, ROMA, and transcriptional profiling approaches establish a minimum of 30 promoter sites (controlling approximately 60 genes) as direct targets for activation by sigma(W). Significantly, no single approach identifies more than approximately 80% of the regulon so defined. We therefore suggest that a combination of two or more complementary approaches be employed in studies seeking to achieve maximal coverage when defining bacterial regulons. Our results indicate that sigma(W) controls genes that protect the cell against agents that impair cell wall biosynthesis but fail to reveal any connection to operons likely to function in adaptation to alkaline growth conditions. This is consistent with the observation that a sigW mutant is unaffected in its ability to survive alkali shock. We conclude that in B. subtilis sudden imposition of alkali stress activates the sigma(W) stress response, perhaps by impairing the ability of the cell wall biosynthetic machinery to function.
机译:枯草芽孢杆菌胞外功能(ECF)sigma因子sigma(W)控制着被碱性休克强烈诱导的大调节子。为了定义sigma(W)的生理作用,我们寻求确定在sigma(W)控制下的完整基因集。以前,我们描述了启动子共有搜索程序,以识别sigma(W)控制的基因。在这里,我们介绍了一种新的方法来识别其他目标启动子:径流转录,然后进行宏阵列分析(ROMA)。我们将目标结果列表与常规转录谱研究中确定的目标列表进行比较,并使用共识搜索方法进行比较。尽管转录谱分析鉴定出在体内表达中高度依赖sigma(W)的基因,但由于其他启动子元件的掩盖作用,与其他ECF sigma因子的重叠识别或两者均未检测到某些sigma(W)依赖性启动子。 。总而言之,共识搜索,ROMA和转录谱分析方法建立了至少30个启动子位点(控制大约60个基因)作为sigma(W)激活的直接目标。值得注意的是,没有任何一种方法能识别出如此定义的规则量的大约80%以上。因此,我们建议在研究中定义细菌调节子时实现最大覆盖率的研究中应采用两种或多种互补方法的组合。我们的结果表明,sigma(W)控制着保护细胞免受损害细胞壁生物合成作用的因子的基因,但未能揭示与操纵子的任何联系,操纵子可能在适应碱性生长条件下起作用。这与sigW突变体在碱冲击下存活的能力不受影响的观察结果一致。我们得出的结论是,在枯草芽孢杆菌中,突然施加碱胁迫会激活sigma(W)胁迫响应,这可能是通过削弱细胞壁生物合成机制发挥作用的能力来实现的。

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