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Analysis of Bacillus subtilis tag gene expression using transcriptional fusions

机译:用转录融合分析枯草芽孢杆菌标签基因表达

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Five of the genes known to encode the synthesis of poly(glycerol phosphate), the major teichoic acid of Bacillus subtilis 168, are organized in two divergently transcribed operons (a divergon), denoted tagAB and tagDEF. To monitor their expression, the 399 bp intergenic region separating the first structural genes of these operons was fused, in both orientations, to a lacZ reporter gene, allowing measurement of promoter activity under specific physiological conditions. Under all experimental conditions, tagA and tagD appeared coordinately expressed, the level of tagD being always higher than that of tagA. No influence of the chromosomal context was observed. Phosphate limitation was accompanied by reduced tag gene expression. Following the onset of sporulation, expression of tag genes diminished rapidly and was essentially abolished by stage II. During germination, the activity of tag genes was detectable before the rise in culture turbidity associated with spore outgrowth. In contrast to tagC (dinC), the expression of which is DNA-damage-inducible, the induction of SOS functions had no effect on tagA and tagD gene expression. The biological significance of these results is discussed.
机译:已知用于编码聚(甘油磷酸盐)合成的五种基因,枯草芽孢杆菌168的主要沸石酸,在两种发散转录的操纵子(分发)中组织,表示Tagab和Tagdef。为了监测它们的表达,将这些操纵子的第一个结构基因分离的399bp族代族区域在方向上融合到LacZ报告基因,允许在特定的生理条件下测量启动子活性。在所有实验条件下,Taga和Tagd出现协调,TAGD的水平总是高于TAGA的水平。没有观察到染色体背景的影响。磷酸盐限制伴随着减少标签基因表达。在孢子术开始之后,标签基因的表达迅速减少,基本上被阶段废除。在萌发期间,在与孢子过剩相关的培养浊度升高之前,标签基因的活性可检测。与TAGC(DINC)相反,其表达是DNA损伤诱导,SOS功能的诱导对TAGA和TAGD基因表达没有影响。讨论了这些结果的生物学意义。

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