Selection of Antigens and Development of Prototype Tests for Point-of-Care Leprosy Diagnosis

Author:

Duthie Malcolm S.12345,Ireton Greg C.12345,Kanaujia Ganga V.12345,Goto Wakako12345,Liang Hong12345,Bhatia Ajay12345,Busceti Jean Marie12345,Macdonald Murdo12345,Neupane Kapil Dev12345,Ranjit Chaman12345,Sapkota Bishwa Raj12345,Balagon Marivic12345,Esfandiari Javan12345,Carter Darrick12345,Reed Steven G.12345

Affiliation:

1. Infectious Disease Research Institute, 1124 Columbia St., Suite 400, Seattle, Washington 98104

2. ChemBio Diagnostic Systems Inc., 3661 Horseblock Road, Medford, New York 11763

3. Mycobacterial Research Laboratory, Anandaban Hospital, Kathmandu, Nepal

4. Leonard Wood Memorial Center for Leprosy Research, Cebu City, Philippines

5. Protein AI, 1102 Columbia St., Seattle, Washington 98104

Abstract

ABSTRACT Leprosy can be a devastating chronic infection that causes nerve function impairment and associated disfigurement. Despite the recent reduction in the number of registered worldwide leprosy cases as a result of the widespread use of multidrug therapy, the number of new cases detected each year remains relatively stable. The diagnosis of leprosy is currently based on the appearance of clinical signs and requires expert clinical, as well as labor-intensive and time-consuming laboratory or histological, evaluation. For the purpose of developing an effective, simple, rapid, and low-cost diagnostic alternative, we have analyzed the serologic antibody response to identify Mycobacterium leprae proteins that are recognized by leprosy patients. More than 100 recombinant antigens were analyzed in a protein array format to select those with discriminatory properties for leprosy diagnosis. As expected, multibacillary leprosy patients recognized more antigens with stronger antibody responses than paucibacillary leprosy patients. Our data indicate, however, that multibacillary patients can be distinguished from paucibacillary patients, and both of these groups can be segregated from endemic control groups. We went on to confirm the diagnostic properties of antigens ML0405 and ML2331 and the LID-1 fusion construct of these two proteins by enzyme-linked immunosorbent assay. We then demonstrated the performance of these antigens in rapid test formats with a goal of developing a point-of-care diagnostic test. A serological diagnostic test capable of identifying and allowing treatment of leprosy could reduce transmission, prevent functional disabilities and stigmatizing deformities, and facilitate leprosy eradication.

Publisher

American Society for Microbiology

Subject

Microbiology (medical),Clinical Biochemistry,Immunology,Immunology and Allergy

Reference24 articles.

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4. Simple and Fast Lateral Flow Test for Classification of Leprosy Patients and Identification of Contacts with High Risk of Developing Leprosy

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