Nghiên cứu biểu hiện và thử nghiệm hoạt tính kháng khuẩn của lysin tái tổ hợp từ phage Staphylococus aureus

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Tác giả: Thị Thùy Dương Bùi, Duy Kháng Đinh, Văn Quyền Đồng, Đình Duy Nguyễn, Huy Thuần Nguyễn, Minh Hường Nguyễn

Ngôn ngữ: vie

Ký hiệu phân loại: 570.78 Life sciences Biology

Thông tin xuất bản: Công nghệ Sinh học, 2018

Mô tả vật lý: 345-351

Bộ sưu tập: Metadata

ID: 492092

Thêm vào giỏ

Tách dòng và biểu hiện lysin K (LysK) được phân lập từ phage vi khuẩn tụ cầu vàng (Staphylococus aureus) trong vi khuẩn E. coli đồng thời đánh giá hoạt tính diệt Staphylococus aureus của lysin tái tổ hợp trên chủng vi khuẩn chị thị S. aureus 816. LysK được thiết kế trong vector biểu hiện pET32a(+) và cảm ứng biểu hiện ở nồng độ 0,5 mM IPTG, nhiệt độ 25oC, thu mẫu sau 6 giờ cảm ứng. LysK tái tổ được tinh sạch bằng cột sắc ký ái lực ProBond Nickel-Chelating Resin theo phương pháp tự nhiên. Kết quả thử nghiệm bằng phương pháp khuếch tán trên đĩa thạch cho thấy LysK tái tổ hợp có hoạt tính diệt S. aureus cao.The discovery of antibiotics is considered to be one of the greatest medical achievements in the early part of 20th. Over the past six decades, these 'wonder drugs' have played a critical role in reducing the global burden of communicable diseases. As a country in the tropical zone, Vietnam faces numerous infectious disease outbreaks every year. In addition, the overuse of antibiotics in healthcare and the misuse of antibiotics as growth promoter in agriculture these past decades have led to serious antibiotic-resistance in bacterial pathogens of human, crops and livestock in Vietnam. This poses an urgent need for alternative strategies to fight against these pathogens. Lysins are phage-encoded peptidoglycan hydrolases which were recently demonstrated the strong potential in human and veterinary medicine to control and treat pathogens on mucosal surfaces and in systemic infections. These enzymes when applied exogenously to Gram-positive bacteria, bring about rapid lysis and death of the bacterial cell and therefore promise an effective alternative therapy against antibiotic-resistant bacterial pathogens. In this study, we applied the DNA technology to produce a recombinant S. aureus lysin (LysK). LysK was PCR amplified from phage S. aureus and cloned into a pET32a(+) expression vector. The recombinant fusion protein (LysK-Trx) was successfully expressed in E. coli, purified through nickel column chromatography, and further digested with Thrombin protease. The cleaved protein (intact LysK) was purified by nickel column again. The recombinant LysK was tested for its ability to kill S. aureus by a spot inoculation assay. The results showed that recombinant LysK induced the lysis of host bacteria, indicating that the protein was expressed and functionally active. Data from the current study can be used to develop therapeutic tools for treating diseases caused by drug-resistant S. aureus strains in Vietnam

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