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2
Proteomic response in DL1 biofilm cells during attachment to salivary MUC5B.DL1生物膜细胞附着于唾液MUC5B过程中的蛋白质组学反应。
J Oral Microbiol. 2021 Aug 23;13(1):1967636. doi: 10.1080/20002297.2021.1967636. eCollection 2021.
3
Periscope Proteins are variable-length regulators of bacterial cell surface interactions.潜望镜蛋白是细菌细胞表面相互作用的可变长度调节剂。
Proc Natl Acad Sci U S A. 2021 Jun 8;118(23). doi: 10.1073/pnas.2101349118.
4
The Multifaceted Nature of Streptococcal Antigen I/II Proteins in Colonization and Disease Pathogenesis.链球菌抗原I/II蛋白在定植和疾病发病机制中的多面性
Front Microbiol. 2020 Nov 25;11:602305. doi: 10.3389/fmicb.2020.602305. eCollection 2020.
5
Deciphering Streptococcal Biofilms.解读链球菌生物膜
Microorganisms. 2020 Nov 21;8(11):1835. doi: 10.3390/microorganisms8111835.
6
Uncovering Roles of Streptococcus gordonii SrtA-Processed Proteins in the Biofilm Lifestyle.揭示戈登链球菌 SrtA 加工蛋白在生物膜生活方式中的作用。
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7
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8
Mechanomicrobiology: how bacteria sense and respond to forces.力学生物学:细菌如何感知和响应力。
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The structural basis of T-cell receptor (TCR) activation: An enduring enigma.T 细胞受体 (TCR) 激活的结构基础:一个持久的谜。
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10
Streptococcus gordonii Type I Lipoteichoic Acid Contributes to Surface Protein Biogenesis.戈登链球菌 I 型脂磷壁酸有助于表面蛋白生物发生。
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戈登链球菌通过 MUC5B 区分、脂磷壁酸介导的外向信号通路准备进行聚糖摄取。

Streptococcus gordonii Poised for Glycan Feeding through a MUC5B-Discriminating, Lipoteichoic Acid-Mediated Outside-In Signaling Circuit.

机构信息

Department of Diagnostic and Biological Sciences, School of Dentistry, University of Minnesotagrid.17635.36, Minneapolis, Minnesota, USA.

Section for Oral Biology and Pathology, Faculty of Odontology, Malmö Universitygrid.32995.34, Malmö, Sweden.

出版信息

J Bacteriol. 2022 Jun 21;204(6):e0011822. doi: 10.1128/jb.00118-22. Epub 2022 Jun 2.

DOI:10.1128/jb.00118-22
PMID:35652671
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9210975/
Abstract

Many oral bacteria employ cell wall-anchored adhesins to bind to the salivary films coating the teeth and mucosal surfaces. Surface binding prevents clearance and facilitates catabolism of salivary film glycoproteins. We asked whether Streptococcus gordonii adhesin expression changes in response to surface salivary cues using a eukaryote-like, outside-in recognition and signaling circuit. To determine whether the cues were discriminated, S. gordonii was tested during cell adhesion and biofilm formation on a MUC5B-rich or lower-molecular-mass salivary fraction or an uncoated abiotic surface. Cells were recovered and analyzed for differences in gene expression and proteins in cell wall fractions. In salivary-free conditions, planktonic S. gordonii presented three prominent cell wall LPXTG-motif proteins, SGO_1487, SGO_0890, and MbpA (mucin-binding protein A; SGO_0707). During biofilm formation on MUC5B-coated surfaces, MbpA, a MUC5B-binding protein, and key genes in the tagatose and quorum-sensing pathways were strongly promoted. The response to MUC5B required the two-component system (TCS), streptococcal regulator of adhesins sensor and regulator (SraSR, SGO_1180/81), lipoteichoic acid (LTA), and the homologous paired adhesins, SspA and SspB (SspAB). LTA appears to link the outside signal (MUC5B) to intramembrane SraSR. Tagatose pathway gene expression may poise cells to metabolize MUC5B glycans and, with a quorum-sensing gene (), may direct formation of a consortium to facilitate glycan cross-feeding by S. gordonii. We now show that a Gram-positive bacterium discriminates specific surface environmental cues using an outside-in signaling mechanism to apparently optimize colonization of saliva-coated surfaces. All organisms throughout the tree of life sense and respond to their surface environments. To discriminate among mucosal surface environmental cues, we report that Streptococcus gordonii recognizes a high-molecular-weight mucin glycoprotein, MUC5B, using the paired adhesins SspAB and lipoteichoic acid; the latter bridges the outside signal to an intramembrane two-component system to transcriptionally regulate a MUC5B-specific adhesin and genes that may facilitate glycan catabolism.

摘要

许多口腔细菌利用细胞壁锚定的黏附素与覆盖牙齿和黏膜表面的唾液膜结合。表面结合可防止清除并促进唾液膜糖蛋白的分解代谢。我们使用真核生物样的外向识别和信号转导电路来询问唾液表面线索是否会影响链球菌 gordonii 黏附素的表达。为了确定是否可以区分这些线索,在富含 MUC5B 的唾液部分或低分子量唾液部分或非涂层的无生命表面上,对 S. gordonii 的细胞黏附和生物膜形成过程进行了测试。回收细胞并分析细胞壁部分的基因表达和蛋白质差异。在无唾液的条件下,浮游 S. gordonii 呈现三种突出的细胞壁 LPXTG 基序蛋白,SGO_1487、SGO_0890 和 MbpA(粘蛋白结合蛋白 A;SGO_0707)。在 MUC5B 涂层表面形成生物膜时,MbpA 是一种 MUC5B 结合蛋白,以及标签果糖和群体感应途径中的关键基因得到了强烈的促进。对 MUC5B 的反应需要双组分系统(TCS)、链球菌黏附素传感器和调节剂(SraSR,SGO_1180/81)、脂磷壁酸(LTA)和同源配对黏附素 SspA 和 SspB(SspAB)。LTA 似乎将外部信号(MUC5B)与膜内 SraSR 联系起来。标签果糖途径基因表达可能使细胞准备好代谢 MUC5B 聚糖,并且与一个群体感应基因()一起,可能指导 S. gordonii 形成 consortium 以促进聚糖交叉喂养。我们现在表明,革兰氏阳性细菌使用外向信号机制来区分特定的表面环境线索,从而优化对唾液覆盖表面的定植。生命之树中的所有生物都能感知并响应其表面环境。为了在粘膜表面环境线索中进行区分,我们报告称,链球菌 gordonii 使用配对的黏附素 SspAB 和脂磷壁酸识别高分子量粘蛋白糖蛋白 MUC5B;后者将外部信号桥接到膜内双组分系统,以转录调控 MUC5B 特异性黏附素和可能促进聚糖分解代谢的基因。