Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis

Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis

Abstract Background The characterization of Leishmania species is important for clinical management of the diseases and the epidemiological control of the parasite distribution. Most of the published polymerase chain reaction (PCR) amplification methods lack the ability to identify all species compl...

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Main Authors: Mahmoud Nateghi Rostami, Fatemeh Darzi, Mahin Farahmand, Mohsen Aghaei, Parviz Parvizi
Format: Article
Language:English
Published: BMC 2020-08-01
Series:Parasites & Vectors
Subjects:
Leishmania
PCR
ITS
Diagnosis
Cutaneous leishmaniasis
Online Access:http://link.springer.com/article/10.1186/s13071-020-04261-5
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spelling doaj-4265b7a14bab4e4fa4a61190b5e048b52020-11-25T03:43:33ZengBMCParasites & Vectors1756-33052020-08-0113111210.1186/s13071-020-04261-5Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasisMahmoud Nateghi Rostami0Fatemeh Darzi1Mahin Farahmand2Mohsen Aghaei3Parviz Parvizi4Laboratory of Host-Parasite Interactions, Department of Parasitology, Pasteur Institute of IranLaboratory of Host-Parasite Interactions, Department of Parasitology, Pasteur Institute of IranLaboratory of Host-Parasite Interactions, Department of Parasitology, Pasteur Institute of IranQom University of Medical SciencesMolecular Systematics Laboratory, Department of Parasitology, Pasteur Institute of IranAbstract Background The characterization of Leishmania species is important for clinical management of the diseases and the epidemiological control of the parasite distribution. Most of the published polymerase chain reaction (PCR) amplification methods lack the ability to identify all species complexes, have low performance and usually need post-PCR procedures. There is a need for improving the diagnosis of CL by development of an accurate affordable PCR method to identify all Leishmania species in clinical specimens. Methods We designed an optimized a PCR amplifying the internal transcribed spacer 2 sequence of the ribosomal RNA gene (ITS2) aligned from different strains of CL-causing Leishmania species in the Old World. The performance of the method was evaluated on lesion samples from several CL suspected patients and the limit of detection (LOD) was determined on DNA of promastigotes from reference strains. Results The universal PCR enabled simultaneous discrimination of L. major, L. tropica and L. infantum using one primer pair in one reaction. Stained smear microscopy and Novy-MacNeal-Nicolle (NNN) medium culture alone detected 77.27% (17/22) and 72.73% (16/22) of the positive CL samples, respectively. The PCR assay showed 100% sensitivity (22/22) (95% CI: 84.56–100%) and 100% specificity (3/3) (95% CI: 29.24–100%) for species identification on isolates from lesion scraping/exudate and 100% sensitivity (13/13) (95% CI: 75.29–100%) and 100% specificity (11/11) (95% CI: 71.51–100%) for species identification on biopsy samples of CL patients, while being capable to successfully amplify as little as 0.01–0.1 pg of Leishmania DNA from cultured promastigotes. Conclusions We present a validated easy-to-use affordable universal PCR assay to identify the most common Old World Leishmania species causing CL. This PCR assay could be used as a sensitive/specific technique to diagnose CL-causing Leishmania species in clinical samples with high accuracy.http://link.springer.com/article/10.1186/s13071-020-04261-5LeishmaniaPCRITSDiagnosisCutaneous leishmaniasis
collection DOAJ
language English
format Article
sources DOAJ
author Mahmoud Nateghi Rostami
Fatemeh Darzi
Mahin Farahmand
Mohsen Aghaei
Parviz Parvizi
spellingShingle Mahmoud Nateghi Rostami
Fatemeh Darzi
Mahin Farahmand
Mohsen Aghaei
Parviz Parvizi
Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis
Parasites & Vectors
Leishmania
PCR
ITS
Diagnosis
Cutaneous leishmaniasis
author_facet Mahmoud Nateghi Rostami
Fatemeh Darzi
Mahin Farahmand
Mohsen Aghaei
Parviz Parvizi
author_sort Mahmoud Nateghi Rostami
title Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis
title_short Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis
title_full Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis
title_fullStr Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis
title_full_unstemmed Performance of a universal PCR assay to identify different Leishmania species causative of Old World cutaneous leishmaniasis
title_sort performance of a universal pcr assay to identify different leishmania species causative of old world cutaneous leishmaniasis
publisher BMC
series Parasites & Vectors
issn 1756-3305
publishDate 2020-08-01
description Abstract Background The characterization of Leishmania species is important for clinical management of the diseases and the epidemiological control of the parasite distribution. Most of the published polymerase chain reaction (PCR) amplification methods lack the ability to identify all species complexes, have low performance and usually need post-PCR procedures. There is a need for improving the diagnosis of CL by development of an accurate affordable PCR method to identify all Leishmania species in clinical specimens. Methods We designed an optimized a PCR amplifying the internal transcribed spacer 2 sequence of the ribosomal RNA gene (ITS2) aligned from different strains of CL-causing Leishmania species in the Old World. The performance of the method was evaluated on lesion samples from several CL suspected patients and the limit of detection (LOD) was determined on DNA of promastigotes from reference strains. Results The universal PCR enabled simultaneous discrimination of L. major, L. tropica and L. infantum using one primer pair in one reaction. Stained smear microscopy and Novy-MacNeal-Nicolle (NNN) medium culture alone detected 77.27% (17/22) and 72.73% (16/22) of the positive CL samples, respectively. The PCR assay showed 100% sensitivity (22/22) (95% CI: 84.56–100%) and 100% specificity (3/3) (95% CI: 29.24–100%) for species identification on isolates from lesion scraping/exudate and 100% sensitivity (13/13) (95% CI: 75.29–100%) and 100% specificity (11/11) (95% CI: 71.51–100%) for species identification on biopsy samples of CL patients, while being capable to successfully amplify as little as 0.01–0.1 pg of Leishmania DNA from cultured promastigotes. Conclusions We present a validated easy-to-use affordable universal PCR assay to identify the most common Old World Leishmania species causing CL. This PCR assay could be used as a sensitive/specific technique to diagnose CL-causing Leishmania species in clinical samples with high accuracy.
topic Leishmania
PCR
ITS
Diagnosis
Cutaneous leishmaniasis
url http://link.springer.com/article/10.1186/s13071-020-04261-5
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