GFP fusions of Sec-routed extracellular proteins in Staphylococcus aureus reveal surface-associated coagulase in biofilms.

IF 4.1 3区 生物学 Q2 CELL BIOLOGY
Dominique C S Evans, Amanda B Khamas, Lisbeth Marcussen, Kristian S Rasmussen, Janne K Klitgaard, Birgitte H Kallipolitis, Janni Nielsen, Daniel E Otzen, Mark C Leake, Rikke L Meyer
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Abstract

Staphylococcus aureus is a major human pathogen that utilises many surface-associated and secreted proteins to form biofilms and cause disease. However, our understanding of these processes is limited by challenges of using fluorescent protein reporters in their native environment, because they must be exported and fold correctly to become fluorescent. Here, we demonstrate the feasibility of using the monomeric superfolder GFP (msfGFP) exported from S. aureus. By fusing msfGFP to signal peptides for the Secretory (Sec) and Twin Arginine Translocation (Tat) pathways, the two major secretion pathways in S. aureus, we quantified msfGFP fluorescence in bacterial cultures and cell-free supernatant from the cultures. When fused to a Tat signal peptide, we detected msfGFP fluorescence inside but not outside bacterial cells, indicating a failure to export msfGFP. However, when fused to a Sec signal peptide, msfGFP fluorescence was present outside cells, indicating successful export of the msfGFP in the unfolded state, followed by extracellular folding and maturation to the photoactive state. We applied this strategy to study coagulase (Coa), a secreted protein and a major contributor to the formation of a fibrin network in S. aureus biofilms that protects bacteria from the host immune system and increases attachment to host surfaces. We confirmed that a genomically integrated C-terminal fusion of Coa to msfGFP does not impair the activity of Coa or its localisation within the biofilm matrix. Our findings demonstrate that msfGFP is a good candidate fluorescent reporter to consider when studying proteins secreted by the Sec pathway in S. aureus.

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金黄色葡萄球菌细胞外蛋白的GFP融合显示生物膜中的表面相关凝固酶。
金黄色葡萄球菌是一种主要的人类病原体,它利用许多表面相关和分泌的蛋白质形成生物膜并引起疾病。然而,我们对这些过程的理解受到在其原生环境中使用荧光蛋白报告蛋白的挑战的限制,因为它们必须导出并正确折叠才能成为荧光蛋白。在这里,我们证明了使用从金黄色葡萄球菌导出的单体超级文件夹GFP (msfGFP)的可行性。通过将msfGFP融合到金黄色葡萄球菌分泌(Sec)和双精氨酸易位(Tat)途径的信号肽中,我们定量了细菌培养物和培养物无细胞上清中的msfGFP荧光。当与Tat信号肽融合时,我们在细菌细胞内检测到msfGFP荧光,而不是在细菌细胞外,表明msfGFP无法输出。然而,当与Sec信号肽融合时,msfGFP荧光出现在细胞外,表明未折叠状态的msfGFP成功输出,随后进行细胞外折叠并成熟到光活性状态。我们应用这一策略来研究凝固酶(Coa),这是一种分泌蛋白,是金黄色葡萄球菌生物膜中纤维蛋白网络形成的主要贡献者,该网络保护细菌免受宿主免疫系统的侵害,并增加对宿主表面的附着。我们证实,Coa与msfGFP的基因组整合c端融合不会损害Coa的活性或其在生物膜基质中的定位。我们的研究结果表明,msfGFP是研究金黄色葡萄球菌中Sec途径分泌的蛋白质时考虑的一个很好的候选荧光报告者。
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
Microbial Cell
Microbial Cell Multiple-
CiteScore
6.40
自引率
0.00%
发文量
32
审稿时长
12 weeks
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