Evaluation of Loopamp Leishmania detection kit for the diagnosis of cutaneous leishmaniasis in Ethiopia

被引:1
|
作者
Taye, Behailu [1 ,2 ]
Melkamu, Roma [3 ]
Tajebe, Fitsumbrhan [1 ]
Ibarra-Meneses, Ana Victoria [4 ]
Adane, Desalegn [3 ]
Atnafu, Saba [3 ]
Adem, Mohammed [1 ]
Adane, Gashaw [1 ]
Kassa, Mekibib [3 ]
Asres, Mezgebu Silamsaw [3 ]
van Griensven, Johan [5 ]
van Henten, Saskia [5 ]
Pareyn, Myrthe [5 ]
机构
[1] Univ Gondar, Dept Immunol & Mol Biol, Gondar, Ethiopia
[2] Dilla Univ, Dept Med Lab Sci, Dilla, Ethiopia
[3] Univ Gondar, Leishmaniasis Res & Treatment Ctr, Gondar, Ethiopia
[4] Univ Montreal, Fac Med Vet, Dept Pathol & Microbiol, St Hyacinthe, PQ, Canada
[5] Inst Trop Med, Dept Clin Sci, Antwerp, Belgium
来源
PARASITES & VECTORS | 2024年 / 17卷 / 01期
关键词
Cutaneous leishmaniasis; Molecular diagnosis; Leishmania aethiopica; LAMP; SPLICED-LEADER RNA;
D O I
10.1186/s13071-024-06475-3
中图分类号
R38 [医学寄生虫学]; Q [生物科学];
学科分类号
07 ; 0710 ; 09 ; 100103 ;
摘要
Background Cutaneous leishmaniasis (CL) in Ethiopia and some parts of Kenya is predominantly caused by Leishmania aethiopica. While skin-slit (SS) microscopy is routinely used for CL diagnosis, more sensitive molecular tests are available. The Loopamp (TM) Leishmania detection kit (Loopamp) is a robust loop-mediated isothermal amplification (LAMP) assay with the potential for implementation in primary healthcare facilities. In this study, we comparatively assessed the diagnostic accuracy of four methods currently used to diagnose CL: Loopamp, kinetoplast DNA (kDNA) PCR, spliced leader RNA (SL-RNA) PCR and SS microscopy. Methods A study on 122 stored tape disc samples of suspected CL patients was conducted in Gondar, northwestern Ethiopia. Routine SS microscopy results were obtained from all patients. Total nucleic acids were extracted from the tapes and subjected to PCR testing targeting kDNA and SL-RNA, and Loopamp. Diagnostic accuracy was calculated with SS microscopy as a reference test. The limit of detection (LoD) of Loopamp and kDNA PCR were determined for cultured L. aethiopica and Leishmania donovani. Results Of the 122 patients, 64 (52.5%) were identified as CL cases based on SS microscopy. Although the PCR tests showed a sensitivity of 95.3% (95% confidence interval [CI] 91.6-99.1), Loopamp only had 48.4% (95% CI 39.6-57.3) sensitivity and 87.9% (95% CI 82.1-93.7) specificity. The LoD of Loopamp for L. donovani was 100-fold lower (20 fg/mu l) than that for L. aethiopica (2 pg/mu l). Conclusions The Loopamp (TM) Leishmania detection kit is not suitable for the diagnosis of CL in Ethiopia, presumably due to a primer mismatch with the L. aethiopica 18S rRNA target. Further research is needed to develop a simple and sensitive point-of-care test that allows the decentralization of CL diagnosis in Ethiopia.
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