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在原核生物中基因内 FliA 启动子的进化影响。

The evolutionary impact of intragenic FliA promoters in proteobacteria.

机构信息

Department of Biomedical Sciences, School of Public Health, University at Albany, Albany, New York, USA.

Wadsworth Center, New York State Department of Health, Albany, New York, USA.

出版信息

Mol Microbiol. 2018 May;108(4):361-378. doi: 10.1111/mmi.13941. Epub 2018 Mar 23.

Abstract

In Escherichia coli, one sigma factor recognizes the majority of promoters, and six 'alternative' sigma factors recognize specific subsets of promoters. The alternative sigma factor FliA (σ ) recognizes promoters upstream of many flagellar genes. We previously showed that most E. coli FliA binding sites are located inside genes. However, it was unclear whether these intragenic binding sites represent active promoters. Here, we construct and assay transcriptional promoter-lacZ fusions for all 52 putative FliA promoters previously identified by ChIP-seq. These experiments, coupled with integrative analysis of published genome-scale transcriptional datasets, strongly suggest that most intragenic FliA binding sites are active promoters that transcribe highly unstable RNAs. Additionally, we show that widespread intragenic FliA-dependent transcription may be a conserved phenomenon, but that specific promoters are not themselves conserved. We conclude that intragenic FliA-dependent promoters and the resulting RNAs are unlikely to have important regulatory functions. Nonetheless, one intragenic FliA promoter is broadly conserved and constrains evolution of the overlapping protein-coding gene. Thus, our data indicate that intragenic regulatory elements can influence bacterial protein evolution and suggest that the impact of intragenic regulatory sequences on genome evolution should be considered more broadly.

摘要

在大肠杆菌中,一个西格玛因子识别大多数启动子,而六个“替代”西格玛因子识别特定的启动子子集。替代西格玛因子 FliA(σ)识别许多鞭毛基因上游的启动子。我们之前表明,大多数大肠杆菌 FliA 结合位点位于基因内部。然而,这些基因内结合位点是否代表活性启动子尚不清楚。在这里,我们构建并检测了之前通过 ChIP-seq 鉴定的 52 个推定 FliA 启动子的所有转录启动子-lacZ 融合。这些实验,结合对已发表的全基因组转录数据集的综合分析,强烈表明大多数基因内 FliA 结合位点是活性启动子,转录高度不稳定的 RNA。此外,我们表明广泛的基因内 FliA 依赖性转录可能是一种保守现象,但特定的启动子本身并不保守。我们得出的结论是,基因内 FliA 依赖性启动子和由此产生的 RNA 不太可能具有重要的调节功能。尽管如此,一个基因内的 FliA 启动子广泛保守,并限制了重叠的编码蛋白基因的进化。因此,我们的数据表明,基因内的调节元件可以影响细菌蛋白质的进化,并表明应该更广泛地考虑基因内调节序列对基因组进化的影响。

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