在 sp. 株 PCC 7120 中,烯醇酶和 DEAD 框 RNA 解旋酶 CrhB 均可与 RNase E 形成复合物。
Both Enolase and the DEAD-Box RNA Helicase CrhB Can Form Complexes with RNase E in sp. Strain PCC 7120.
机构信息
State Key Laboratory of Agricultural Microbiology, College of Life Science and Technology, Huazhong Agricultural University, Wuhan, China.
State Key Laboratory of Agricultural Microbiology, College of Life Science and Technology, Huazhong Agricultural University, Wuhan, China
出版信息
Appl Environ Microbiol. 2020 Jun 17;86(13). doi: 10.1128/AEM.00425-20.
At present, little is known about the RNA metabolism driven by the RNA degradosome in cyanobacteria. RNA helicase and enolase are the common components of the RNA degradosome in many bacteria. Here, we provide evidence that both enolase and the DEAD-box RNA helicase CrhB can interact with RNase E in () sp. strain PCC 7120 (referred to here as PCC 7120). Furthermore, we found that the C-terminal domains of CrhB and AnaEno (enolase of PCC 7120) are required for the interaction, respectively. Moreover, their recognition motifs for AnaRne (RNase E of PCC 7120) turned out to be located in the N-terminal catalytic domain, which is obviously different from those identified previously in We also demonstrated in enzyme activity assays that CrhB can induce AnaRne to degrade double-stranded RNA with a 5' tail. Furthermore, we investigated the localization of CrhB and AnaRne by green fluorescent protein (GFP) translation fusion and found that they both localized in the center of the PCC 7120 cytoplasm. This localization pattern is also different from the membrane binding of RNase E and RhlB in Together with the previous identification of polynucleotide phosphorylase (PNPase) in PCC 7120, our results show that there is an RNA degradosome-like complex with a different assembly mechanism in cyanobacteria. In all domains of life, RNA turnover is important for gene regulation and quality control. The process of RNA metabolism is regulated by many RNA-processing enzymes and assistant proteins, where these proteins usually exist as complexes. However, there is little known about the RNA metabolism, as well as about the RNA degradation complex. In the present study, we described an RNA degradosome-like complex in cyanobacteria and revealed an assembly mechanism different from that of Moreover, CrhB could help RNase E in sp. strain PCC 7120 degrade double-stranded RNA with a 5' tail. In addition, CrhB and AnaRne have similar cytoplasm localizations, in contrast to the membrane localization in .
目前,人们对蓝藻中由 RNA 降解体驱动的 RNA 代谢知之甚少。RNA 解旋酶和烯醇酶是许多细菌中 RNA 降解体的常见组成部分。在这里,我们提供的证据表明,烯醇酶和 DEAD 盒 RNA 解旋酶 CrhB 都可以与 () sp. strain PCC 7120(这里称为 PCC 7120)中的 RNase E 相互作用。此外,我们发现 CrhB 和 AnaEno(PCC 7120 的烯醇酶)的 C 端结构域分别是相互作用所必需的。此外,它们识别 AnaRne(PCC 7120 的 RNase E)的模体位于 N 端催化结构域,这与之前在 中鉴定的明显不同。我们还在酶活性测定中证明,CrhB 可以诱导 AnaRne 降解带有 5' 尾巴的双链 RNA。此外,我们通过绿色荧光蛋白 (GFP) 翻译融合来研究 CrhB 和 AnaRne 的定位,并发现它们都定位于 PCC 7120 细胞质的中心。这种定位模式也与 RNase E 和 RhlB 在 中的膜结合不同。结合之前在 PCC 7120 中鉴定的多核苷酸磷酸化酶 (PNPase),我们的结果表明,在蓝藻中存在一种具有不同组装机制的 RNA 降解体样复合物。在所有生命领域中,RNA 周转对于基因调控和质量控制都很重要。RNA 代谢过程受许多 RNA 加工酶和辅助蛋白的调节,这些蛋白通常以复合物的形式存在。然而,人们对 RNA 代谢以及 RNA 降解复合物知之甚少。在本研究中,我们描述了蓝藻中的一种 RNA 降解体样复合物,并揭示了一种与 不同的组装机制。此外,CrhB 可以帮助 sp. strain PCC 7120 中的 RNase E 降解带有 5' 尾巴的双链 RNA。此外,CrhB 和 AnaRne 具有相似的细胞质定位,与 中的膜定位相反。
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