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两种非编码 RNA 对溶壁酶编码基因的调控。

Regulation of a muralytic enzyme-encoding gene by two non-coding RNAs.

机构信息

a Department of Biology and Michael G. DeGroote Institute for Infectious Disease Research , McMaster University , Hamilton , Ontario , Canada.

出版信息

RNA Biol. 2017 Nov 2;14(11):1592-1605. doi: 10.1080/15476286.2017.1338241. Epub 2017 Nov 3.

Abstract

Non-coding regulatory RNAs fine-tune gene expression post-transcriptionally. In the streptomycetes, rpfA - encoding a muralytic enzyme required for establishing and exiting dormancy - is flanked by non-coding regulatory RNA elements both upstream (riboswitch) and downstream [antisense small RNA (sRNA)]. In Streptomyces coelicolor, the upstream riboswitch decreases rpfA transcript abundance in response to the second messenger cyclic di-AMP, itself involved in cell wall metabolism and dormancy. There is, however, no obvious expression platform associated with this riboswitch and consequently, its mechanism of action is entirely unknown. Using in vitro transcription assays, we discovered that the rpfA riboswitch promoted premature transcription termination in response to cyclic di-AMP. Through an extensive mutational analysis, we determined that attenuation required ligand binding and involved an unusual extended stem-loop region unique to a subset of rpfA riboswitches in the actinobacteria. At the other end of the rpfA gene, an antisense sRNA, termed Scr3097, is expressed opposite the predicted rpfA terminator. Using northern blotting, we found that Scr3097 accumulation mirrored that of the rpfA mRNA. In liquid culture, we detected Scr3097 exclusively in exponential-phase cells, and in plate-grown culture, we observed the sRNA primarily in differentiating cultures. Using mutational analyses, we found that the sRNA increased rpfA mRNA abundance in cells. Taken together, our work revealed multiple regulatory RNAs controlling rpfA expression in the streptomycetes.

摘要

非编码调控 RNA 在后转录水平上精细调节基因表达。在链霉菌中,rpfA 编码一种需要建立和退出休眠的溶壁酶,其上下游都有非编码调控 RNA 元件(核糖体开关和反义小 RNA [sRNA])。在天蓝色链霉菌中,上游核糖体开关会根据第二信使环二腺苷酸(cyclic di-AMP)的变化来减少 rpfA 转录本的丰度,而环二腺苷酸本身也参与细胞壁代谢和休眠。然而,这个核糖体开关并没有明显的表达平台,因此其作用机制尚不清楚。通过体外转录实验,我们发现 rpfA 核糖体开关可以响应环二腺苷酸促进转录过早终止。通过广泛的突变分析,我们确定了衰减需要配体结合,并涉及到一个不寻常的扩展茎环区域,该区域仅存在于放线菌中 rpfA 核糖体开关的一个亚群中。在 rpfA 基因的另一端,一个反义 sRNA,称为 Scr3097,在预测的 rpfA 终止子的对面表达。通过 northern blot 分析,我们发现 Scr3097 的积累与 rpfA mRNA 的积累一致。在液体培养中,我们仅在指数生长期的细胞中检测到 Scr3097,而在平板培养中,我们主要观察到该 sRNA 在分化培养中表达。通过突变分析,我们发现该 sRNA 增加了细胞中 rpfA mRNA 的丰度。综上所述,我们的工作揭示了多个调控 RNA 控制链霉菌中 rpfA 的表达。

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Regulation of a muralytic enzyme-encoding gene by two non-coding RNAs.两种非编码 RNA 对溶壁酶编码基因的调控。
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