Development and comparative evaluation of two antigen detection tests for Visceral Leishmaniasis

被引:39
作者
Vallur, Aarthy C. [1 ]
Tutterrow, Yeung L. [1 ]
Mohamath, Raodoh [1 ]
Pattabhi, Sowmya [1 ]
Hailu, Asrat [2 ]
Abdoun, Asim O. [3 ]
Ahmed, Abdalla E. [3 ]
Mukhtar, Maowia [3 ]
Salam, Md Abdus [4 ]
Almeida, Meirielly Lima [5 ]
Almeida, Roque P. [5 ]
Mondal, Dinesh [6 ]
Albertini, Audrey [7 ]
Ghalib, Hashim [1 ]
Duthie, Malcolm S. [1 ]
Reed, Steven G. [1 ]
机构
[1] Infect Dis Res Inst, Seattle, WA 98102 USA
[2] Univ Addis Ababa, Dept Microbiol Immunol & Parasitol, Addis Ababa, Ethiopia
[3] Univ Khartoum, Inst Endem Dis, Khartoum, Sudan
[4] Rajshahi Med Coll, Dept Microbiol, Rajshahi, Bangladesh
[5] Univ Fed Sergipe, Dept Med, Aracaju, Sergipe, Brazil
[6] Int Ctr Diarrhoeal Dis Res, Dhaka, Bangladesh
[7] FIND, Geneva, Switzerland
关键词
Diagnosis; Leishmania; Antigen; Treatment; Antibody; Kala azar; Infection; LATEX AGGLUTINATION-TEST; KALA-AZAR; SODIUM STIBOGLUCONATE; DIAGNOSIS; URINE; MILTEFOSINE;
D O I
10.1186/s12879-015-1125-3
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Background: Visceral leishmaniasis (VL) can be fatal without timely diagnosis and treatment. Treatment efficacies vary due to drug resistance, drug toxicity and co-morbidities. It is important to monitor treatment responsiveness to confirm cure and curtail relapse. Currently, microscopy of spleen, bone marrow or lymph node biopsies is the only definitive method to evaluate cure. A less invasive test for treatment success is a high priority for VL management. Methods: In this study, we describe the development of a capture ELISA based on detecting Leishmania donovani antigens in urine samples and comparison with the Leishmania Antigen ELISA, also developed for the same purpose. Both were developed as prototype kits and tested on patient urine samples from Sudan, Ethiopia, Bangladesh and Brazil, along with appropriate control samples from endemic and non-endemic regions. Sensitivity and specificity were assessed based on accurate detection of patients compared to control samples. One- Way ANOVA was used to assess the discrimination capacity of the tests and Cohen's kappa was used to assess their correlation. Results: The Leishmania Antigen Detect (TM) ELISA demonstrated >90 % sensitivity on VL patient samples from Sudan, Bangladesh and Ethiopia and 88 % on samples from Brazil. The Leishmania Antigen ELISA was comparable in performance except for lower sensitivity on Sudanese samples. Both were highly specific. To confirm utility in monitoring treatment, urine samples were collected from VL patients at days 0, 30 and 180 post-treatment. For the Leishmania Antigen Detect (TM) ELISA, positivity was high at day 0 at 95 %, falling to 21 % at day 30. At day 180, all samples were negative, corresponding well with clinical cure. A similar trend was also seen for the Leishmania Antigen ELISA albeit; with lower positivity of 91 % at Day 0 and more patients, remaining positive at Days 30 and 180. Discussion: The Leishmania Antigen Detect (TM) and the Leishmania Antigen ELISAs are standardized, user-friendly, quantitative and direct tests to detect Leishmania during acute VL as well as to monitor parasite clearance during treatment. They are a clear improvement over existing options. Conclusion: The ELISAs provide a non-invasive method to detect parasite antigens during acute infection and monitor its clearance upon cure, filling an unmet need in VL management. Further refinement of the tests with more samples from endemic regions will define their utility in monitoring treatment.
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页数:10
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