1. Mycobacterium leprae Phenolglycolipid-1 Expressed by Engineered M. bovis BCG Modulates Early Interaction with Human Phagocytes
- Author
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Nadine Honoré, Patricia Constant, Caroline Demangel, Wladimir Malaga, Catherine Astarie-Dequeker, Mamadou Daffé, Christophe Guilhot, Esther Perez, Nana Fatimath Bello, Guillaume Tabouret, Aurélie Ray, Institut de pharmacologie et de biologie structurale (IPBS), Université Toulouse III - Paul Sabatier (UT3), Université de Toulouse (UT)-Université de Toulouse (UT)-Centre National de la Recherche Scientifique (CNRS), Pathogénomique mycobactérienne intégrée, Institut Pasteur [Paris] (IP), This work was funded by the Centre National de la Recherche Scientifique (CNRS), and the Agence Nationale de la Recherche grant 06-MIME-032-02. The NMR spectrometers were financed by the CNRS, the University Paul Sabatier, the Région Midi-Pyrénées and the European Structural Funds (FEDER)., ANR-06-MIME-0032,PGLEP,Le rôle du phénol-glycolipide 1 du bacille lépreux dans l'invasion cellulaire, la neuropathie et l'immunosuppression(2006), Centre National de la Recherche Scientifique (CNRS)-Université Toulouse III - Paul Sabatier (UT3), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées, and Institut Pasteur [Paris]
- Subjects
MESH: Phagocytes/metabolism ,Time Factors ,MESH: Antigen Presentation/physiology ,PHTHIOCEROL DIESTER ,HUMAN MONOCYTES ,MESH: Cricetinae ,MESH: Antigens, Bacterial/genetics ,Microbiology/Innate Immunity ,PHENOLIC GLYCOLIPID-1 ,Protein Engineering ,MESH: Mycobacterium leprae/genetics ,MESH: Glycolipids/metabolism ,ACTIVATION ,Infectious Diseases/Bacterial Infections ,MESH: Glycolipids/genetics ,MESH: Cricetulus ,Cricetinae ,MESH: Animals ,TUBERCULOSIS COMPLEX ,CD11B/CD18 ,[SDV.BDD]Life Sciences [q-bio]/Development Biology ,lcsh:QH301-705.5 ,Mycobacterium leprae ,Cells, Cultured ,MESH: Immune Evasion/immunology ,MESH: Glycolipids/physiology ,Antigen Presentation ,Phagocytes ,0303 health sciences ,Mycobacterium bovis ,Genetics and Genomics/Functional Genomics ,MESH: Mycobacterium bovis/genetics ,VIRULENCE FACTORS ,DENDRITIC CELLS ,RECEPTORS ,BIOSYNTHESIS ,Recombinant Proteins ,3. Good health ,MESH: Recombinant Proteins/chemistry ,MESH: Immunity, Innate/physiology ,Microbiology/Cellular Microbiology and Pathogenesis ,MESH: Cells, Cultured ,Research Article ,MESH: Immunity, Innate/genetics ,lcsh:Immunologic diseases. Allergy ,MESH: Antigens, Bacterial/metabolism ,MESH: Recombinant Proteins/metabolism ,Phagocytosis ,Immunology ,MESH: Immune Evasion/genetics ,Context (language use) ,MESH: Phagocytes/immunology ,[SDV.BC]Life Sciences [q-bio]/Cellular Biology ,CHO Cells ,Biology ,Models, Biological ,Microbiology ,MESH: Antigen Presentation/genetics ,03 medical and health sciences ,MESH: Antigens, Bacterial/physiology ,Cricetulus ,Glycolipid ,Immune system ,MESH: CHO Cells ,Virology ,Genetics ,Animals ,Humans ,MESH: Recombinant Proteins/genetics ,Molecular Biology ,Tropism ,Immune Evasion ,030304 developmental biology ,Antigens, Bacterial ,MESH: Humans ,030306 microbiology ,MESH: Time Factors ,MESH: Models, Biological ,biology.organism_classification ,Immunity, Innate ,In vitro ,MESH: Mycobacterium bovis/metabolism ,lcsh:Biology (General) ,Parasitology ,Glycolipids ,lcsh:RC581-607 ,MESH: Protein Engineering/methods - Abstract
The species-specific phenolic glycolipid 1 (PGL-1) is suspected to play a critical role in the pathogenesis of leprosy, a chronic disease of the skin and peripheral nerves caused by Mycobacterium leprae. Based on studies using the purified compound, PGL-1 was proposed to mediate the tropism of M. leprae for the nervous system and to modulate host immune responses. However, deciphering the biological function of this glycolipid has been hampered by the inability to grow M. leprae in vitro and to genetically engineer this bacterium. Here, we identified the M. leprae genes required for the biosynthesis of the species-specific saccharidic domain of PGL-1 and reprogrammed seven enzymatic steps in M. bovis BCG to make it synthesize and display PGL-1 in the context of an M. leprae-like cell envelope. This recombinant strain provides us with a unique tool to address the key questions of the contribution of PGL-1 in the infection process and to study the underlying molecular mechanisms. We found that PGL-1 production endowed recombinant BCG with an increased capacity to exploit complement receptor 3 (CR3) for efficient invasion of human macrophages and evasion of inflammatory responses. PGL-1 production also promoted bacterial uptake by human dendritic cells and dampened their infection-induced maturation. Our results therefore suggest that M. leprae produces PGL-1 for immune-silent invasion of host phagocytic cells., Author Summary Mycobacterium leprae, the causative agent of leprosy, is a chronic human disease responsible for irreversible peripheral nerve damage and deformities. Lepromatous leprosy, the most severe form of the disease, is accompanied by T-cell unresponsiveness, suggesting that M. leprae has evolved strategies to modulate host immune responses. However, the molecular mechanisms of M. leprae infection remain poorly understood, mainly because this bacterium has been to date impossible to grow in vitro. The present study reports an innovative approach to study the contribution of a phenolic glycolipid (PGL-1) specific of M. leprae in the cross-talk of the pathogen with host cells. We reprogrammed a biosynthetic pathway in a surrogate host, M. bovis BCG, to make it synthesize and display PGL-1 in the context of a mycobacterial envelope. Using this novel microbial tool, we found that PGL-1 production enhances the cellular invasiveness of BCG and promotes the entry via complement receptor 3-mediated phagocytosis. Bacterial uptake via this route was associated with reduced inflammatory responses in infected human macrophages. In addition, we showed that PGL-1 production inhibited the infection-induced maturation of human dendritic cells. Our findings thus provide new insights into the contribution and molecular mechanisms of action of PGL-1 in leprosy pathogenesis.
- Published
- 2010