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Impact of actin on adhesion and translocation of Enterococcus faecalis
Authors:Zhen Peng  Viktoria Krey  Hua Wei  Qianglai Tan  Roger Vogelmann  Matthias A Ehrmann  Rudi F Vogel
Institution:1. Lehrstuhl für Technische Mikrobiologie, Technische Universit?t München, Weihenstephaner Steig 16, 85350, Freising, Germany
2. Lehrstuhl für Mikrobielle ?kologie, Technische Universit?t München, Freising, Germany
3. Nanchang University, Nanchang, China
4. Second Department of Internal Medicine, Universit?tsmedizin Mannheim, University Heidelberg, 68167, Mannheim, Germany
Abstract:This study focuses on the impact of actin on adhesion and translocation of Enterococcus (E.) faecalis OG1RF, E. faecalis Symbioflor®, and E. faecalis V583. Insight into the role of actin aggregation in the mediation of bacterial adhesion and translocation was provided by a two-chamber translocation assay, which employed Ptk6 cells. Determination of translocation rates, cytochalasin D treatment, and laser scanning confocal microscopic observation revealed actin as a predominant brace for enterococci to pass through the epithelial cell layer. As the three enterococci had moderate adhesion ability to actin, actin-binding proteins were isolated and characterized by LC–MS/MS. The isolated proteins were identified as pyruvate formate lyase, enolase, glyceraldehyde-3-phosphate dehydrogenase, and GroEL. All these proteins belong to two major groups of moonlighting proteins, i.e., proteins, which display additional functions other than their described major biochemical catalysis. Both groups of moonlight proteins were determined to be associated with epithelial cell binding.
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