The binding affinity-dependent inhibition of cell growth and viability by DNA sulfur-binding domains.

IF 2.6 2区 生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY
Molecular Microbiology Pub Date : 2024-05-01 Epub Date: 2024-03-13 DOI:10.1111/mmi.15249
Yuli Wang, Fulin Ge, Jinling Liu, Wenyue Hu, Guang Liu, Zixin Deng, Xinyi He
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引用次数: 0

Abstract

Increasing evidence suggests that DNA phosphorothioate (PT) modification serves several purposes in the bacterial host, and some restriction enzymes specifically target PT-DNA. PT-dependent restriction enzymes (PDREs) bind PT-DNA through their DNA sulfur binding domain (SBD) with dissociation constants (KD) of 5 nM~1 μM. Here, we report that SprMcrA, a PDRE, failed to dissociate from PT-DNA after cleavage due to high binding affinity, resulting in low DNA cleavage efficiency. Expression of SBDs in Escherichia coli cells with PT modification induced a drastic loss of cell viability at 25°C when both DNA strands of a PT site were bound, with one SBD on each DNA strand. However, at this temperature, SBD binding to only one PT DNA strand elicited a severe growth lag rather than lethality. This cell growth inhibition phenotype was alleviated by raising the growth temperature. An in vitro assay mimicking DNA replication and RNA transcription demonstrated that the bound SBD hindered the synthesis of new DNA and RNA when using PT-DNA as the template. Our findings suggest that DNA modification-targeting proteins might regulate cellular processes involved in DNA metabolism in addition to being components of restriction-modification systems and epigenetic readers.

Abstract Image

DNA 硫结合结构域对细胞生长和活力的抑制作用与结合亲和力有关。
越来越多的证据表明,DNA硫代磷酸酯(PT)修饰在细菌宿主中有多种作用,一些限制酶专门针对PT-DNA。PT 依赖性限制酶(PDREs)通过其 DNA 硫结合域(SBD)与 PT-DNA 结合,其解离常数(KD )为 5 nM~1 μM。在此,我们报告了一种 PDRE--SprMcrA,由于其结合亲和力较高,在裂解后未能与 PT-DNA 分离,导致 DNA 裂解效率较低。在具有 PT 修饰的大肠杆菌细胞中表达 SBD,在 25°C 时,当 PT 位点的两条 DNA 链都结合时,每条 DNA 链上都有一个 SBD,这会导致细胞活力急剧下降。然而,在这一温度下,SBD 只与一条 PT DNA 链结合会引起严重的生长迟缓,而不是致死。这种细胞生长抑制表型可通过提高生长温度得到缓解。模拟 DNA 复制和 RNA 转录的体外试验表明,当使用 PT-DNA 作为模板时,结合的 SBD 会阻碍新 DNA 和 RNA 的合成。我们的研究结果表明,DNA修饰靶向蛋白除了是限制修饰系统和表观遗传阅读器的组成部分外,还可能调控涉及DNA代谢的细胞过程。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Molecular Microbiology
Molecular Microbiology 生物-生化与分子生物学
CiteScore
7.20
自引率
5.60%
发文量
132
审稿时长
1.7 months
期刊介绍: Molecular Microbiology, the leading primary journal in the microbial sciences, publishes molecular studies of Bacteria, Archaea, eukaryotic microorganisms, and their viruses. Research papers should lead to a deeper understanding of the molecular principles underlying basic physiological processes or mechanisms. Appropriate topics include gene expression and regulation, pathogenicity and virulence, physiology and metabolism, synthesis of macromolecules (proteins, nucleic acids, lipids, polysaccharides, etc), cell biology and subcellular organization, membrane biogenesis and function, traffic and transport, cell-cell communication and signalling pathways, evolution and gene transfer. Articles focused on host responses (cellular or immunological) to pathogens or on microbial ecology should be directed to our sister journals Cellular Microbiology and Environmental Microbiology, respectively.
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