Molecular Diagnosis of Leishmaniasis in Spain: Development and Validation of Ready-To-Use Gel-Form Nested and Real-Time PCRs To Detect Leishmania spp

Carmen Chicharro; Javier Nieto; Silvia Miguelañez; Emilia Garcia; Sheila Ortega; Ana Peña; Jose Miguel Rubio; Maria Flores-Chavez

doi:10.1128/spectrum.03354-22

Molecular Diagnosis of Leishmaniasis in Spain: Development and Validation of Ready-To-Use Gel-Form Nested and Real-Time PCRs To Detect Leishmania spp

Microbiol Spectr. 2023 Jun 15;11(3):e0335422. doi: 10.1128/spectrum.03354-22. Epub 2023 Apr 4.

Authors

Carmen Chicharro^{1

2

3}, Javier Nieto^{1

2

3}, Silvia Miguelañez^{1

3}, Emilia Garcia^{1

3}, Sheila Ortega¹, Ana Peña¹, Jose Miguel Rubio^{1

2}, Maria Flores-Chavez^{1

4}

Affiliations

¹ Reference and Research Laboratory for Parasitology, National Centre for Microbiology, Instituto de Salud Carlos III (ISCIII), Madrid, Spain.
² Centro de Investigación Biomédica en Red de Enfermedades Infecciosas (CIBERINFEC-ISCIII), Madrid, Spain.
³ WHO Collaborating Center for Leishmaniasis (WHOCCLeish), Madrid, Spain.
⁴ Fundación Mundo Sano, Madrid, Spain.

Abstract

Leishmaniasis is an endemic parasitic disease in at least 98 countries. In Spain, it is considered a zoonosis caused by Leishmania infantum, with an annual incidence of 0.62 cases/100,000 inhabitants. The predominant clinical manifestations are the cutaneous (CL) and visceral forms (VL), and the diagnosis is performed by parasitological, serological, and molecular tests. At the WHO Collaborating Center for Leishmaniasis (WHOCCLeish), routine diagnostic tests are based on a nested PCR (Ln-PCR), culture, and serological tests. To simplify our PCR protocol, we aimed to develop and validate a ready-to-use nested gel-form PCR (LeishGelPCR) and a duplex real-time PCR (qPCR) that allowed simultaneous detection of Leishmania and mammalian DNA as an internal control (Leish-qPCR). Clinical validation was performed in 200 samples from the WHOCCLeish collection; 92 and 85 out of 94 and 87 samples were positive by LeishGelPCR and Leish-qPCR, respectively, showing a sensitivity of 98% in both approaches. The specificity was 100% for LeishGelPCR and 98% for Leish-qPCR. The limits of detection of both protocols were similar (0.5 and 0.2 parasites/reaction). Parasite loads in VL and CL forms were similar, although high loads were observed when invasive samples were tested. In conclusion, LeishGelPCR and Leish-qPCR showed excellent performance in the diagnosis of leishmaniasis. These new forms of 18S rRNA gene PCR are equivalent to Ln-PCR and can be introduced in the algorithm for CL and VL diagnosis. IMPORTANCE Although the gold standard for diagnosis of leishmaniasis is the microscopic observation of amastigotes, molecular techniques are becoming a cost-efficient alternative. Currently, PCR is a routine resource that is used in many reference microbiology laboratories. In this article, we have described two ways to improve the reproducibility and usability of the molecular detection of Leishmania spp. These new approaches could be introduced even in middle- and low-resource laboratories; one is a ready-to-use gel-form system of a nested PCR and the other is a real-time PCR. We show why molecular diagnosis is the best methodology to confirm a clinical suspicion of leishmaniasis with higher sensitivity than traditional methods, thus facilitating early diagnosis and timely treatment of human leishmaniasis.

Keywords: gel system; leishmaniasis; molecular diagnosis; nested PCR; parasite load; qPCR; sensitivity; specificity.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
DNA, Protozoan / analysis
DNA, Protozoan / genetics
Humans
Leishmania* / genetics
Leishmaniasis* / diagnosis
Mammals
Real-Time Polymerase Chain Reaction / methods
Reproducibility of Results
Sensitivity and Specificity
Spain

Substances

DNA, Protozoan