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组蛋白样蛋白 Hlp 是酿脓链球菌生长所必需的:研究必需基因的遗传方法比较。

The histone-like protein Hlp is essential for growth of Streptococcus pyogenes: comparison of genetic approaches to study essential genes.

机构信息

Department of Microbiology and Immunology, Emory University School of Medicine, 1510 Clifton Road, Atlanta, GA 30322, USA.

出版信息

Appl Environ Microbiol. 2011 Jul;77(13):4422-8. doi: 10.1128/AEM.00554-11. Epub 2011 Apr 29.

DOI:10.1128/AEM.00554-11
PMID:21531823
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3127713/
Abstract

Selection of possible targets for vaccine and drug development requires an understanding of the physiology of bacterial pathogens, for which the ability to manipulate expression of essential genes is critical. For Streptococcus pyogenes (the group A streptococcus [GAS]), an important human pathogen, the lack of genetic tools for such studies has seriously hampered research. To address this problem, we characterized variants of the inducible Ptet cassette, in both sense and antisense contexts, as tools to regulate transcription from GAS genes. We found that although the three-operator Ptet construct [Ptet(O)3] had low uninduced expression, its induction level was low, while the two-operator construct [Ptet(O)2] was inducible to a high level but showed significant constitutive expression. Use of Ptet(O)3 in the chromosome allowed us to demonstrate previously that RNases J1 and J2 are required for growth of GAS. Here we report that the uninduced level from the chromosomally inserted Ptet(O)2 construct was too high for us to observe differential growth. For the highly expressed histone-like protein (Hlp) of GAS, neither chromosomal insertion of Ptet(O)2 or Ptet(O)3 nor their use on a high-copy-number plasmid to produce antisense RNA specific to hlp resulted in adequate differential expression. However, by replacing the ribosome binding site of hlp with an engineered riboswitch to control translation of Hlp, we demonstrated for the first time that this protein is essential for GAS growth.

摘要

疫苗和药物开发的可能靶点的选择需要了解细菌病原体的生理学,对于这些病原体,操纵必需基因表达的能力至关重要。对于化脓性链球菌(A 组链球菌[GAS])这种重要的人类病原体,缺乏用于此类研究的遗传工具严重阻碍了研究。为了解决这个问题,我们对诱导型 Ptet 盒的变体进行了特征分析,包括正反义两种情况,将其作为调节 GAS 基因转录的工具。我们发现,尽管三操作子 Ptet 构建体[Ptet(O)3]的非诱导表达水平较低,但诱导水平较低,而两操作子构建体[Ptet(O)2]的诱导水平较高,但表现出明显的组成型表达。在染色体上使用 Ptet(O)3 使我们能够证明先前 RNase J1 和 J2 对于 GAS 的生长是必需的。在这里,我们报告说,插入染色体的 Ptet(O)2 构建体的非诱导水平太高,以至于我们无法观察到差异生长。对于 GAS 的高度表达组蛋白样蛋白(Hlp),无论是在染色体上插入 Ptet(O)2 还是 Ptet(O)3,还是使用高拷贝数质粒产生针对 hlp 的反义 RNA,都没有导致足够的差异表达。然而,通过用工程化的核糖体开关替换 hlp 的核糖体结合位点来控制 Hlp 的翻译,我们首次证明该蛋白对于 GAS 的生长是必需的。

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