Postgenomic Approach To Identify Novel Mycobacterium leprae Antigens with Potential To Improve Immunodiagnosis of Infection

Author:

Geluk Annemieke1,Klein Michèl R.1,Franken Kees L. M. C.1,van Meijgaarden Krista E.1,Wieles Brigitte1,Pereira Kelly Cristina2,Bührer-Sékula Samira3,Klatser Paul R.3,Brennan Patrick J.4,Spencer John S.4,Williams Diana L.5,Pessolani Maria C. V.6,Sampaio Elizabeth P.2,Ottenhoff Tom H. M.1

Affiliation:

1. Departments of Immunohematology and Blood Transfusion, Leiden University Medical Center, The Netherlands

2. Department of Immunology, Oswaldo Cruz Institute, FIOCRUZ, Manguinhos, Rio de Janeiro, Brazil

3. Royal Tropical Institute, Amsterdam, The Netherlands

4. Microbiology, Immunology and Pathology, Colorado State University, Ft. Collins, Colorado

5. Molecular Biology, Laboratory Research Branch, National Hansen's Disease Programs, Louisiana State University, Baton Rouge, Louisiana

6. Laboratory of Cellular Microbiology and Leprosy Laboratory, Laboratory of Immunology

Abstract

ABSTRACT Early detection of Mycobacterium leprae infection is considered an important component of strategies aiming at reducing transmission of infection, but currently available diagnostic tools often lack sufficient sensitivity and specificity to reach this goal. Recent comparative genomics have revealed the presence of 165 M. leprae genes with no homologue in M. tuberculosis . We selected 17 of these genes for further study. All 17 genes were found to be expressed at the mRNA level in M. leprae from infected mice and from a multibacillary leprosy patient. Additional comparative genomic analyses of all currently available mycobacterial genome databases confirmed 12 candidate genes to be unique to M. leprae , whereas 5 genes had homologues in mycobacteria other than M. tuberculosis . Evaluation of the immunogenicity of all 17 recombinant proteins in PBMC from 127 Brazilians showed that five antigens (ML0576, ML1989, ML1990, ML2283, and ML2567) induced significant gamma interferon levels in paucibacillary leprosy patients, reactional leprosy patients, and exposed healthy controls but not in most multibacillary leprosy patients, tuberculosis patients, or endemic controls. Importantly, among exposed healthy controls 71% had no detectable immunoglobulin M antibodies to the M. leprae -specific PGL-I but responded to one or more M. leprae antigen(s). Collectively, the M. leprae proteins identified are expressed at the transcriptome level and can efficiently activate T cells of M. leprae -exposed individuals. These proteins may provide new tools to develop tests for specific diagnosis of M. leprae infection and may enhance our understanding of leprosy and its transmission.

Publisher

American Society for Microbiology

Subject

Infectious Diseases,Immunology,Microbiology,Parasitology

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