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在集胞藻 PCC 6803 中,抑制组 2σ 因子会上调转录和翻译机器的产生。

Inactivation of group 2 σ factors upregulates production of transcription and translation machineries in the cyanobacterium Synechocystis sp. PCC 6803.

机构信息

Department of Biochemistry, University of Turku, FI-20014, Turku, Finland.

出版信息

Sci Rep. 2018 Jul 9;8(1):10305. doi: 10.1038/s41598-018-28736-9.

Abstract

We show that the formation of the RNAP holoenzyme with the primary σ factor SigA increases in the ΔsigBCDE strain of the cyanobacterium Synechocystis sp. PCC 6803 lacking all group 2 σ factors. The high RNAP-SigA holoenzyme content directly induces transcription of a particular set of housekeeping genes, including ones encoding transcription and translation machineries. In accordance with upregulated transcripts, ΔsigBCDE contain more RNAPs and ribosomal subunits than the control strain. Extra RNAPs are fully active, and the RNA content of ΔsigBCDE cells is almost tripled compared to that in the control strain. Although ΔsigBCDE cells produce extra rRNAs and ribosomal proteins, functional extra ribosomes are not formed, and translation activity and protein content remained similar in ΔsigBCDE as in the control strain. The arrangement of the RNA polymerase core genes together with the ribosomal protein genes might play a role in the co-regulation of transcription and translation machineries. Sequence logos were constructed to compare promoters of those housekeeping genes that directly react to the RNAP-SigA holoenzyme content and those ones that do not. Cyanobacterial strains with engineered transcription and translation machineries might provide solutions for construction of highly efficient production platforms for biotechnical applications in the future.

摘要

我们发现,在缺乏所有组 2 σ 因子的蓝藻集胞藻 PCC 6803 的ΔsigBCDE 菌株中,与主要 σ 因子 SigA 形成的 RNA 聚合酶全酶的形成增加。高 RNA 聚合酶-SigA 全酶含量直接诱导一组特定的看家基因的转录,包括编码转录和翻译机制的基因。与上调的转录物一致,ΔsigBCDE 比对照菌株含有更多的 RNA 聚合酶和核糖体亚基。额外的 RNA 聚合酶具有完全的活性,与对照菌株相比,ΔsigBCDE 细胞的 RNA 含量几乎增加了三倍。尽管ΔsigBCDE 细胞产生额外的 rRNA 和核糖体蛋白,但没有形成功能性的额外核糖体,并且ΔsigBCDE 中的翻译活性和蛋白质含量与对照菌株相似。RNA 聚合酶核心基因与核糖体蛋白基因的排列可能在转录和翻译机制的共同调控中发挥作用。构建了序列 logo 来比较直接对 RNA 聚合酶-SigA 全酶含量做出反应的那些看家基因和那些不做出反应的看家基因的启动子。未来,具有工程化转录和翻译机制的蓝藻菌株可能为生物技术应用的高效生产平台的构建提供解决方案。

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