Utility of the Loop-Mediated Isothermal Amplification Assay for the Diagnosis of Visceral Leishmaniasis from Blood Samples in Ethiopia

Hagos, Dawit Gebreegzabher; Kiros, Yazezew Kebede; Abdulkader, Mahmud; Arefaine, Zekarias Gessessew; Nigus, Etsay; Schallig, Henk H.D.F.; Wolday, Dawit

doi:10.4269/ajtmh.21-0334

Cited by 4 publications

(5 citation statements)

References 43 publications

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“…The LAMP assay was performed using the LoopAmp Leishmania kit as per the manufacturer's instructions (Eiken Chemical Co., Tokyo, Japan) [44]. The kit uses 6 primers that target conserved Leishmania gene segments kDNA and 18S rRNA, respectively [13]. The LAMP assay utilized Bst polymerase, which has auto-DNA denaturing and amplification properties [33].…”

Section: Laboratory Analysis Of Blood Samplesmentioning

confidence: 99%

“…In most VL-endemic, resource-limited countries, the diagnosis of VL relies on a combination of the patient's clinical presentation and rapid serological tests and/or microscopy of Giemsa-stained tissue aspirates [12][13][14]. Despite its poor performance and risky specimen collection procedures, microscopy is often still used as the reference standard for VL diagnoses in many endemic countries.…”

Section: Introductionmentioning

confidence: 99%

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Comparison of the Diagnostic Performances of Five Different Tests in Diagnosing Visceral Leishmaniasis in an Endemic Region of Ethiopia

Hagos,

Kiros,

Abdulkader

et al. 2024

Diagnostics

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The lack of accurate and feasible diagnostic tests poses a significant challenge to visceral leishmaniasis (VL) healthcare services in endemic areas. To date, various VL diagnostic tests have been or are being developed, and their diagnostic performances need to be assessed. In the present study, the diagnostic performances of rk39 RDT, the direct agglutination test (DAT), microscopy, loop-mediated isothermal amplification (LAMP), and miniature direct-on-blood polymerase chain reaction–nucleic acid lateral flow immunoassay (mini-dbPCR-NALFIA) were assessed using quantitative polymerase chain reaction (qPCR) as the reference test in an endemic region of Ethiopia. In this study, 235 suspected VL cases and 104 non-endemic healthy controls (NEHCs) were recruited. Among the suspected VL cases, 144 (61.28%) tested positive with qPCR. The sensitivities for rk39 RDT, DAT, microscopy, LAMP assay, and mini-dbPCR-NALFIA were 88.11%, 96.50%, 76.58%, 94.33%, and 95.80%, respectively. The specificities were 83.33%, 97.96%, 100%, 97.38%, and 98.92% for rk39 RDT, DAT, microscopy, LAMP assay, and mini-dbPCR-NALFIA, respectively. In conclusion, rk39 RDT and microscopy exhibited lower sensitivities, while DAT demonstrated excellent performance. LAMP and mini-dbPCR-NALFIA showed excellent performances with feasibility for implementation in remote endemic areas, although the latter requires further evaluation in such regions.

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Section: Laboratory Analysis Of Blood Samplesmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Comparison of the Diagnostic Performances of Five Different Tests in Diagnosing Visceral Leishmaniasis in an Endemic Region of Ethiopia

Hagos,

Kiros,

Abdulkader

et al. 2024

Diagnostics

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“…Such algorithm would prioritize bone marrow samples, and patients with splenomegaly and especially low WBC values to be tested as they have a higher chance of being PCR positive. Alternatively, an affordable and simple test (e.g., loopmediated isothermal amplification [28] or a novel RDT) on a non-invasive sample like peripheral blood would be very useful to include in the diagnostic algorithm in VL endemic areas for early diagnosis and treatment of VL patients.…”

Section: Plos Neglected Tropical Diseasesmentioning

confidence: 99%

PCR for detection of Leishmania donovani from microscopically negative tissue smears of suspected patients in Gondar, Ethiopia

Melkamu

Berhane²,

Jacobs³

et al. 2023

PLoS Negl Trop Dis

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Background As untreated visceral leishmaniasis (VL) is fatal, reliable diagnostics are pivotal for accurate treatment allocation. The current diagnostic algorithm for VL in Ethiopia, which is based on the rK39 rapid diagnostic test and microscopy of tissue smears, lacks sensitivity. This probably leads to missed cases and patients not receiving treatment. Methodology We conducted a retrospective study on stored microscopically negative spleen and bone marrow smears from suspected VL patients collected at the Leishmaniasis Research and Treatment Center (LRTC) in Gondar, northern Ethiopia between June 2019 and November 2020. Sociodemographic, clinical and treatment data were collected and samples were tested by real-time PCR targeting kinetoplast DNA. Principle findings Among the 191 eligible samples (135 spleen and 56 bone marrow) with a microscopically negative and valid PCR result, 119 (62.3%) were positive by PCR, although Ct values for some were high (median 33.0). Approximately three quarters of these undiagnosed primary VL (77.3%) and relapse (69.6%) patients did not receive antileishmanial treatment. Of the 56 microscopically negative bone marrow samples, 46 (82.1%) were PCR positive, which is considerably higher compared to the microscopically negative spleen samples, for which 73 out of 135 (54.1%) were PCR positive. The odds of being PCR positive were significantly higher for bone marrow aspirates and higher when white blood cell values were lower and splenomegaly (in cm) was more pronounced. Conclusions This study demonstrates that a lot of suspected VL patients remain undiagnosed and untreated. This indicates the urgent need for better diagnostics for VL in the East-African region. The outcomes of PCR positive should be closely monitored and treatment should be provided if the patient deteriorates. In resource limited settings, implementation of PCR on bone marrow aspirate smears of patients with low WBC values and splenomegaly could lead to considerable improvements in patient management.

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“…The LAMP assay was performed using LoopAmp Leishmania kit (Eiken Chemical Co., Tokyo, Japan) [44]. The kit employed 6 primers that target conserved Leishmania gene segment [13]: kDNA and 18S rRNA. LAMP assay utilized Bst polymerase, which has auto-DNA denaturing and amplification properties [33].…”

Section: Laboratory Analysis Of Blood Samplesmentioning

confidence: 99%

“…In most VL-endemic resource-limited countries, the diagnosis of VL relies on a combination of the patient's clinical presentation and rapid serological tests and/or microscopy of Giemsa-stained tissue aspirate/s [12][13][14]. Despite its poor performance and risky specimen collection procedures, microscopy is still often used as the reference standard for VL diagnosis in many endemic countries.…”

Section: Introductionmentioning

confidence: 99%

Comparison of the Diagnostic Performance of Five Different Tests to Diagnose Visceral Leishmaniasis in an Endemic Region of Ethiopia

Hagos,

Kiros,

Mahmud

et al. 2023

Preprint

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The lack of accurate and feasible diagnostic tests poses a significant challenge to visceral leish-maniasis (VL) healthcare services in endemic areas. To date, various VL diagnostic tests have been or are being developed, and their diagnostic performance needs to be assessed.. In the present study, the diagnostic performance of rk39RDT, Direct Agglutination Test (DAT), Microscopy, Loop Mediated Isothermal Amplification (LAMP), and miniature direct-on-blood polymerase chain reaction - nucleic acid lateral flow immunoassay (mini-dbPCR-NALFIA) was assessed using quantitative polymerase chain reaction (qPCR) as reference test in an endemic region of Ethiopia. In this study, 235 patients VL suspected patients and 104 non-endemic healthy controls (NEHC) were recruited. Among the VL-suspected patients, 144(61.28%) tested positive with qPCR. Sensi-tivities for rk39 RDT, DAT, Microscopy, LAMP assay, and mini-dbPCR-NALFIA were 88.11%, 96.50%, 76.58%, 94.33%, and 95.80%, respectively. Specificities were 83.33%, 97.96%, 100%, 97.38%, and 98.92% for rk39 RDT, DAT, Microscopy, LAMP assay, and mini-dbPCR-NALFIA, respectively. In conclusion, Rk39 RDT and microscopy exhibited lower sensitivity, while DAT demonstrated excellent performance. LAMP and mini-dbPCR-NALFIA showed excellent perfor-mance with feasibility to implement in remote endemic areas, although the latter requires further evaluation in such regions.

show abstract

Utility of the Loop-Mediated Isothermal Amplification Assay for the Diagnosis of Visceral Leishmaniasis from Blood Samples in Ethiopia

Cited by 4 publications

References 43 publications

Comparison of the Diagnostic Performances of Five Different Tests in Diagnosing Visceral Leishmaniasis in an Endemic Region of Ethiopia

Comparison of the Diagnostic Performances of Five Different Tests in Diagnosing Visceral Leishmaniasis in an Endemic Region of Ethiopia

PCR for detection of Leishmania donovani from microscopically negative tissue smears of suspected patients in Gondar, Ethiopia

Comparison of the Diagnostic Performance of Five Different Tests to Diagnose Visceral Leishmaniasis in an Endemic Region of Ethiopia

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