Molecular identification of Leishmania tropica and L. infantum isolated from cutaneous human leishmaniasis samples in central Morocco

M Echchakery; C Chicharro; S Boussaa; J Nieto; S Ortega; E Carrillo; J Moreno; A Boumezzough

doi:10.4103/0972-9062.308804

Molecular identification of Leishmania tropica and L. infantum isolated from cutaneous human leishmaniasis samples in central Morocco

J Vector Borne Dis. 2020 Jan-Mar;57(1):71-77. doi: 10.4103/0972-9062.308804.

Authors

M Echchakery¹, C Chicharro², S Boussaa³, J Nieto², S Ortega², E Carrillo², J Moreno², A Boumezzough¹

Affiliations

¹ Microbial Biotechnologies, Agrosciences and Environment Laboratory (BioMAgE), Faculty of Sciences Semlalia, Cadi Ayyad University, Marrakech, Morocco.
² National Center of Microbiology, Institute of Health Carlos III (WHO Collaborating Centre for Leishmaniasis, Parasitology Service), Majadahonda, Madrid, Spain.
³ Microbial Biotechnologies, Agrosciences and Environment Laboratory (BioMAgE), Faculty of Sciences Semlalia, Cadi Ayyad University; ISPITS-Higher Institute of Nursing and Technical Health Occupations, Marrakesh, Morocco.

PMID: 33818459
DOI: 10.4103/0972-9062.308804

Abstract

Background & objectives: Cutaneous leishmaniasis (CL) in Marrakesh-Safi region located in the central-south part of Morocco is a public health problem. This study assessed the efficiency of a microscopic examination method in establishing the diagnosis of CL and PCR for the characterization and identification of the circulating Leishmania strains in different CL foci of the study area.

Methods: A total of 297 smears obtained from cutaneous lesions of suspected patients with CL were stained with May-Grünwald Giemsa (MGG) for microscopic examination. For each positive smear, genomic DNA was extracted and PCR-analysed, targeting the small subunit ribosomal ribonucleic acid (ssu rRNA) gene to detect Leishmania DNA. Then, the internal transcribed spacer 1 (ITS1) was amplified and sequenced in order to identify the Leishmania species. The sensitivity and specificity of the conventional microscopy with ssu rRNA gene were compared by Leishmania nested PCR (LnPCR) and ITS1 gene by ITS-PCR.

Results: A total of 257 smears were positive in the microscopic examination, i.e. the detection rate of amastigotes by optical microscopy was 86.53% (257/297). The LnPCR was found to have a specificity and a sensitivity of 100%, each. Interestingly, the sequencing results showed that 99.61% (256/257) of the isolates had Leishmania tropica and 0.39% (1/257) had L. infantum infection.

Interpretation & conclusion: Though, classical microscopic examination is useful and economical, it is not sensitive enough, especially in endemic regions where several Leishmania species coexist. In such situations, PCR constitutes a complementary method for the identification of the causal species. The results indicate that both the L. tropica (dominant) and L. infantum are the causative agents of CL in the Marrakesh-Safi region. The rate of CL infection is high in Imintanout, and Chichaoua provinces. Hence, early diagnosis and prompt treatment of CL patients is necessary to prevent its extension to neighboring localities.

Keywords: Cutaneous leishmaniasis; ITS-PCR; L. tropica; Leishmania infantum; LnPCR; Morocco; microscopic examination.

MeSH terms

Adolescent
Adult
Child
Child, Preschool
DNA, Protozoan / genetics*
Female
Humans
Infant
Leishmania infantum / genetics*
Leishmania infantum / isolation & purification
Leishmania tropica / genetics*
Leishmania tropica / isolation & purification
Leishmaniasis, Cutaneous / diagnosis*
Leishmaniasis, Cutaneous / epidemiology
Leishmaniasis, Cutaneous / parasitology*
Male
Microscopy / methods
Microscopy / standards
Middle Aged
Morocco / epidemiology
Pathology, Molecular / methods
Pathology, Molecular / standards
Sensitivity and Specificity
Young Adult

Substances

DNA, Protozoan