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(pp)pGpp 合酶在金黄色葡萄球菌中的诱导表达与应激反应基因的激活有关。

Inducible expression of (pp)pGpp synthetases in Staphylococcus aureus is associated with activation of stress response genes.

机构信息

Interfaculty Institute of Microbiology and Infection Medicine, University of Tuebingen, Germany.

Quantitative Proteomics & Proteome Center Tuebingen, University of Tuebingen, Germany.

出版信息

PLoS Genet. 2020 Dec 30;16(12):e1009282. doi: 10.1371/journal.pgen.1009282. eCollection 2020 Dec.

DOI:10.1371/journal.pgen.1009282
PMID:33378356
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7802963/
Abstract

The stringent response is characterized by the synthesis of the messenger molecules pppGpp, ppGpp or pGpp (here collectively designated (pp)pGpp). The phenotypic consequences resulting from (pp)pGpp accumulation vary among species and can be mediated by different underlying mechanisms. Most genome-wide analyses have been performed under stress conditions, which often mask the immediate effects of (pp)pGpp-mediated regulatory circuits. In Staphylococcus aureus, (pp)pGpp can be synthesized via the RelA-SpoT-homolog, RelSau upon amino acid limitation or via one of the two small (pp)pGpp synthetases RelP or RelQ upon cell wall stress. We used RNA-Seq to compare the global effects in response to induction of the synthetase of rel-Syn (coding for the enzymatic region of RelSau) or relQ without the need to apply additional stress conditions. Induction of rel-Syn resulted in changes in the nucleotide pool similar to induction of the stringent response via the tRNA synthetase inhibitor mupirocin: a reduction in the GTP pool, an increase in the ATP pool and synthesis of pppGpp, ppGpp and pGpp. Induction of all three enzymes resulted in similar changes in the transcriptome. However, RelQ was less active than Rel-Syn and RelP, indicating strong restriction of its (pp)pGpp-synthesis activity in vivo. (pp)pGpp induction resulted in the downregulation of many genes involved in protein and RNA/DNA metabolism. Many of the (pp)pGpp upregulated genes are part of the GTP sensitive CodY regulon and thus likely regulated through lowering of the GTP pool. New CodY independent transcriptional changes were detected including genes involved in the SOS response, iron storage (e.g. ftnA, dps), oxidative stress response (e.g., perR, katA, sodA) and the psmα1-4 and psmß1-2 operons coding for cytotoxic, phenol soluble modulins (PSMs). Analyses of the ftnA, dps and psm genes in different regulatory mutants revealed that their (pp)pGpp-dependent regulation can occur independent of the regulators PerR, Fur, SarA or CodY. Moreover, psm expression is uncoupled from expression of the quorum sensing system Agr, the main known psm activator. The expression of central genes of the oxidative stress response protects the bacteria from anticipated ROS stress derived from PSMs or exogenous sources. Thus, we identified a new link between the stringent response and oxidative stress in S. aureus that is likely crucial for survival upon phagocytosis.

摘要

严谨反应的特征是信使分子 pppGpp、ppGpp 或 pGpp(此处统称为 (pp)pGpp)的合成。(pp)pGpp 积累所导致的表型后果因物种而异,并可通过不同的潜在机制进行介导。大多数全基因组分析都是在应激条件下进行的,这往往掩盖了 (pp)pGpp 介导的调节回路的即时效应。在金黄色葡萄球菌中,(pp)pGpp 可以通过 RelA-SpoT-同源物 RelSau 在氨基酸限制时合成,或者通过细胞壁应激时的两种小分子 (pp)pGpp 合成酶 RelP 或 RelQ 之一合成。我们使用 RNA-Seq 来比较在诱导合成酶 rel-Syn(编码 RelSau 的酶区域)或 relQ 而无需施加额外应激条件时的全局效应。诱导 rel-Syn 导致核苷酸池的变化类似于通过 tRNA 合成酶抑制剂 mupirocin 诱导严谨反应:GTP 池减少,ATP 池增加,pppGpp、ppGpp 和 pGpp 的合成。三种酶的诱导都导致转录组的相似变化。然而,RelQ 的活性低于 Rel-Syn 和 RelP,表明其体内 (pp)pGpp 合成活性受到强烈限制。(pp)pGpp 的诱导导致许多参与蛋白质和 RNA/DNA 代谢的基因下调。许多 (pp)pGpp 上调的基因是 GTP 敏感 CodY 调控子的一部分,因此可能通过降低 GTP 池来调节。检测到新的 CodY 独立转录变化,包括参与 SOS 反应、铁储存(如 ftnA、dps)、氧化应激反应(如 perR、katA、sodA)和编码细胞毒性、酚溶性调节素(PSMs)的 psmα1-4 和 psmβ1-2 操纵子的基因。在不同调节突变体中分析 ftnA、dps 和 psm 基因表明,它们的 (pp)pGpp 依赖性调节可以独立于调节剂 PerR、Fur、SarA 或 CodY 发生。此外,psm 的表达与群体感应系统 Agr 的表达解耦,Agr 是主要已知的 psm 激活剂。氧化应激反应的中心基因的表达保护细菌免受源自 PSMs 或外源性来源的预期 ROS 应激。因此,我们在金黄色葡萄球菌中鉴定到严谨反应和氧化应激之间的新联系,这对于吞噬作用后存活可能至关重要。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/f12634b3a933/pgen.1009282.g007.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/f12634b3a933/pgen.1009282.g007.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/2ca9ee69b62c/pgen.1009282.g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/3acafff039d2/pgen.1009282.g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/a897d2f82417/pgen.1009282.g003.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/44576d190de0/pgen.1009282.g006.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ecf/7802963/f12634b3a933/pgen.1009282.g007.jpg

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