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替考拉宁相关位点调节因子(TcaR)和细胞间黏附素位点调节因子(IcaR)是金黄色葡萄球菌ica位点的转录抑制剂。

The teicoplanin-associated locus regulator (TcaR) and the intercellular adhesin locus regulator (IcaR) are transcriptional inhibitors of the ica locus in Staphylococcus aureus.

作者信息

Jefferson Kimberly K, Pier Danielle B, Goldmann Donald A, Pier Gerald B

机构信息

Channing Laboratory, Brigham and Women's Hospital, Harvard Medical School, Boston, Massachusetts 02115, USA.

出版信息

J Bacteriol. 2004 Apr;186(8):2449-56. doi: 10.1128/JB.186.8.2449-2456.2004.

Abstract

Infections involving Staphylococcus aureus are often more severe and difficult to treat when the organism assumes a biofilm mode of growth. The polysaccharide poly-N-acetylglucosamine (PNAG), also known as polysaccharide intercellular adhesin, is synthesized by the products of the intercellular adhesin (ica) locus and plays a key role in biofilm formation. Numerous conditions and exogenous factors influence ica transcription and PNAG synthesis, but the regulatory factors and pathways through which these environmental stimuli act have been only partially characterized. We developed a DNA affinity chromatography system to purify potential regulatory proteins that bind to the ica promoter region. Using this technique, we isolated four proteins, including the staphylococcal gene regulator SarA, a MarR family transcriptional regulator of the teicoplanin-associated locus TcaR, DNA-binding protein II, and topoisomerase IV, that bound to the ica promoter. Site-directed deletion mutagenesis of tcaR indicated that TcaR was a negative regulator of ica transcription, but deletion of tcaR alone did not induce any changes in PNAG production or in adherence to polystyrene. We also investigated the role of IcaR, encoded within the ica locus but divergently transcribed from the biosynthetic genes. As has been shown previously in Staphylococcus epidermidis, we found that IcaR was also a negative regulator of ica transcription in S. aureus. We also demonstrate that mutation of icaR augmented PNAG production and adherence to polystyrene. Transcription of the ica locus, PNAG production, and adherence to polystyrene were further increased in a tcaR icaR double mutant. In summary, TcaR appeared to be a weak negative regulator of transcription of the ica locus, whereas IcaR was a strong negative regulator, and in their absence PNAG production and biofilm formation were enhanced.

摘要

当金黄色葡萄球菌呈现生物膜生长模式时,其所引发的感染通常更为严重且难以治疗。多糖聚 - N - 乙酰葡糖胺(PNAG),也被称为胞间黏附多糖,由胞间黏附素(ica)基因座的产物合成,在生物膜形成中起关键作用。众多条件和外源性因素会影响ica转录和PNAG合成,但这些环境刺激发挥作用的调控因子和途径仅得到了部分表征。我们开发了一种DNA亲和层析系统,以纯化与ica启动子区域结合的潜在调控蛋白。利用该技术,我们分离出了四种蛋白,包括葡萄球菌基因调节蛋白SarA、替考拉宁相关基因座TcaR的MarR家族转录调节蛋白、DNA结合蛋白II和拓扑异构酶IV,它们均与ica启动子结合。对tcaR进行定点缺失诱变表明,TcaR是ica转录的负调节因子,但单独缺失tcaR并未引起PNAG产生或对聚苯乙烯黏附的任何变化。我们还研究了ica基因座内编码但与生物合成基因反向转录的IcaR的作用。正如先前在表皮葡萄球菌中所显示的那样,我们发现IcaR在金黄色葡萄球菌中也是ica转录的负调节因子。我们还证明,icaR突变会增加PNAG产生和对聚苯乙烯的黏附。在tcaR icaR双突变体中,ica基因座的转录、PNAG产生和对聚苯乙烯的黏附进一步增加。总之,TcaR似乎是ica基因座转录的弱负调节因子,而IcaR是强负调节因子,在它们缺失时,PNAG产生和生物膜形成会增强。

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