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Molecular characteristic of treatment failure clinical isolates of Leishmania major. / Eslami, Gilda; Hatefi, Samira; Ramezani, Vahid et al.

In: PeerJ, Vol. 9, 10969, 11.03.2021.

Research output: Contribution to journalArticlepeer-review

Harvard

Eslami, G, Hatefi, S, Ramezani, V, Tohidfar, M, Churkina, TV, Orlov, YL, Hosseini, SS, Boozhmehrani, MJ & Vakili, M 2021, 'Molecular characteristic of treatment failure clinical isolates of Leishmania major', PeerJ, vol. 9, 10969. https://doi.org/10.7717/peerj.10969

APA

Eslami, G., Hatefi, S., Ramezani, V., Tohidfar, M., Churkina, T. V., Orlov, Y. L., Hosseini, S. S., Boozhmehrani, M. J., & Vakili, M. (2021). Molecular characteristic of treatment failure clinical isolates of Leishmania major. PeerJ, 9, [10969]. https://doi.org/10.7717/peerj.10969

Vancouver

Eslami G, Hatefi S, Ramezani V, Tohidfar M, Churkina TV, Orlov YL et al. Molecular characteristic of treatment failure clinical isolates of Leishmania major. PeerJ. 2021 Mar 11;9:10969. doi: 10.7717/peerj.10969

Author

Eslami, Gilda ; Hatefi, Samira ; Ramezani, Vahid et al. / Molecular characteristic of treatment failure clinical isolates of Leishmania major. In: PeerJ. 2021 ; Vol. 9.

BibTeX

@article{7bb77792e8594bbc8f588cc3d03b0ba5,
title = "Molecular characteristic of treatment failure clinical isolates of Leishmania major",
abstract = "Background: Leishmaniasis is a prevalent tropical disease caused by more than 20 Leishmania species (Protozoa, Kinetoplastida and Trypanosomatidae). Among different clinical forms of the disease, cutaneous leishmaniasis is the most common form, with an annual 0.6-1 million new cases reported worldwide. This disease's standard treatment is pentavalent antimonial (SbV) that have been used successfully since the first half of the 20th century as a first-line drug. However, treatment failure is an increasing problem that is persistently reported from endemic areas. It is important to define and standardize tests for drug resistance in cutaneous leishmaniasis. SbV must be reduced to its trivalent active form (SbIII). This reduction occurs within the host macrophage, and the resultant SbIIIenters amastigotes via the aquaglyceroporin1 (AQP1) membrane carrier. Overexpression of AQP1 results in hypersensitivity of the parasites to SbIII, but resistant phenotypes accompany reduced expression, inactivation mutations, or deletion of AQP1. Hence, in this study, a phylogenetic analysis using barcode gene COXII and kDNA minicircle and expression analysis of AQP1 were performed in treatment failure isolates to assess the isolates' molecular characteristics and to verify possible association with drug response. Methods: Samples in this study were collected from patients with cutaneous leishmaniasis referred to the Diagnosis Laboratory Center in Isfahan Province, Iran, from October 2017 to December 2019. Among them, five isolates (code numbers 1-5) were categorized as treatment failures. The PCR amplification of barcode gene COXII and kDNA minicircle were done and subsequently analyzed using MEGA (10.0.5) to perform phylogenetics analysis of Treatment failures (TF) and Treatment response (TR) samples. Relative quantification of the AQP1 gene expression of TF and TR samples was assessed by real-time PCR. Results: All samples were classified as L. major. No amplification failure was observed in the cases of barcode gene COXII and kDNA minicircle amplification. Having excluded the sequences with complete homology using maximum parsimony with the Bootstrap 500 method, four major groups were detected to perform phylogenetic analysis using COXII. The phylogenetic analysis using the barcode target of minicircle showed that all five treatment failure isolates were grouped in a separate sub-clade. Conclusions: We concluded that the barcode gene COXII and the minicircle kDNA were suitable for identification, differentiation and phylogenetic analysis in treatment failure clinical isolates of Leishmania major. Also, AQP1 gene expression analyses showed that treatment failure isolates had less expression than TR isolates. The isolate with TF and overexpression of the AQP1 gene of other molecular mechanisms such as overexpression of ATP-binding cassette may be involved in the TR, such as overexpression of ATP-binding cassette which requires further research. ",
keywords = "Clinical isolates, COXII, Gene expression, Leishmania, Leishmaniasis, Minicircle kDNA, Parasitology, Phylogenetic analysis, Treatment failure",
author = "Gilda Eslami and Samira Hatefi and Vahid Ramezani and Masoud Tohidfar and Churkina, {Tatyana V.} and Orlov, {Yuriy L.} and Hosseini, {Saeedeh Sadat} and Boozhmehrani, {Mohammad Javad} and Mahmood Vakili",
note = "Publisher Copyright: {\textcopyright} 2021 Eslami et al. Copyright: Copyright 2021 Elsevier B.V., All rights reserved.",
year = "2021",
month = mar,
day = "11",
doi = "10.7717/peerj.10969",
language = "English",
volume = "9",
journal = "PeerJ",
issn = "2167-8359",
publisher = "PeerJ",

}

RIS

TY - JOUR

T1 - Molecular characteristic of treatment failure clinical isolates of Leishmania major

AU - Eslami, Gilda

AU - Hatefi, Samira

AU - Ramezani, Vahid

AU - Tohidfar, Masoud

AU - Churkina, Tatyana V.

AU - Orlov, Yuriy L.

AU - Hosseini, Saeedeh Sadat

AU - Boozhmehrani, Mohammad Javad

AU - Vakili, Mahmood

N1 - Publisher Copyright: © 2021 Eslami et al. Copyright: Copyright 2021 Elsevier B.V., All rights reserved.

PY - 2021/3/11

Y1 - 2021/3/11

N2 - Background: Leishmaniasis is a prevalent tropical disease caused by more than 20 Leishmania species (Protozoa, Kinetoplastida and Trypanosomatidae). Among different clinical forms of the disease, cutaneous leishmaniasis is the most common form, with an annual 0.6-1 million new cases reported worldwide. This disease's standard treatment is pentavalent antimonial (SbV) that have been used successfully since the first half of the 20th century as a first-line drug. However, treatment failure is an increasing problem that is persistently reported from endemic areas. It is important to define and standardize tests for drug resistance in cutaneous leishmaniasis. SbV must be reduced to its trivalent active form (SbIII). This reduction occurs within the host macrophage, and the resultant SbIIIenters amastigotes via the aquaglyceroporin1 (AQP1) membrane carrier. Overexpression of AQP1 results in hypersensitivity of the parasites to SbIII, but resistant phenotypes accompany reduced expression, inactivation mutations, or deletion of AQP1. Hence, in this study, a phylogenetic analysis using barcode gene COXII and kDNA minicircle and expression analysis of AQP1 were performed in treatment failure isolates to assess the isolates' molecular characteristics and to verify possible association with drug response. Methods: Samples in this study were collected from patients with cutaneous leishmaniasis referred to the Diagnosis Laboratory Center in Isfahan Province, Iran, from October 2017 to December 2019. Among them, five isolates (code numbers 1-5) were categorized as treatment failures. The PCR amplification of barcode gene COXII and kDNA minicircle were done and subsequently analyzed using MEGA (10.0.5) to perform phylogenetics analysis of Treatment failures (TF) and Treatment response (TR) samples. Relative quantification of the AQP1 gene expression of TF and TR samples was assessed by real-time PCR. Results: All samples were classified as L. major. No amplification failure was observed in the cases of barcode gene COXII and kDNA minicircle amplification. Having excluded the sequences with complete homology using maximum parsimony with the Bootstrap 500 method, four major groups were detected to perform phylogenetic analysis using COXII. The phylogenetic analysis using the barcode target of minicircle showed that all five treatment failure isolates were grouped in a separate sub-clade. Conclusions: We concluded that the barcode gene COXII and the minicircle kDNA were suitable for identification, differentiation and phylogenetic analysis in treatment failure clinical isolates of Leishmania major. Also, AQP1 gene expression analyses showed that treatment failure isolates had less expression than TR isolates. The isolate with TF and overexpression of the AQP1 gene of other molecular mechanisms such as overexpression of ATP-binding cassette may be involved in the TR, such as overexpression of ATP-binding cassette which requires further research.

AB - Background: Leishmaniasis is a prevalent tropical disease caused by more than 20 Leishmania species (Protozoa, Kinetoplastida and Trypanosomatidae). Among different clinical forms of the disease, cutaneous leishmaniasis is the most common form, with an annual 0.6-1 million new cases reported worldwide. This disease's standard treatment is pentavalent antimonial (SbV) that have been used successfully since the first half of the 20th century as a first-line drug. However, treatment failure is an increasing problem that is persistently reported from endemic areas. It is important to define and standardize tests for drug resistance in cutaneous leishmaniasis. SbV must be reduced to its trivalent active form (SbIII). This reduction occurs within the host macrophage, and the resultant SbIIIenters amastigotes via the aquaglyceroporin1 (AQP1) membrane carrier. Overexpression of AQP1 results in hypersensitivity of the parasites to SbIII, but resistant phenotypes accompany reduced expression, inactivation mutations, or deletion of AQP1. Hence, in this study, a phylogenetic analysis using barcode gene COXII and kDNA minicircle and expression analysis of AQP1 were performed in treatment failure isolates to assess the isolates' molecular characteristics and to verify possible association with drug response. Methods: Samples in this study were collected from patients with cutaneous leishmaniasis referred to the Diagnosis Laboratory Center in Isfahan Province, Iran, from October 2017 to December 2019. Among them, five isolates (code numbers 1-5) were categorized as treatment failures. The PCR amplification of barcode gene COXII and kDNA minicircle were done and subsequently analyzed using MEGA (10.0.5) to perform phylogenetics analysis of Treatment failures (TF) and Treatment response (TR) samples. Relative quantification of the AQP1 gene expression of TF and TR samples was assessed by real-time PCR. Results: All samples were classified as L. major. No amplification failure was observed in the cases of barcode gene COXII and kDNA minicircle amplification. Having excluded the sequences with complete homology using maximum parsimony with the Bootstrap 500 method, four major groups were detected to perform phylogenetic analysis using COXII. The phylogenetic analysis using the barcode target of minicircle showed that all five treatment failure isolates were grouped in a separate sub-clade. Conclusions: We concluded that the barcode gene COXII and the minicircle kDNA were suitable for identification, differentiation and phylogenetic analysis in treatment failure clinical isolates of Leishmania major. Also, AQP1 gene expression analyses showed that treatment failure isolates had less expression than TR isolates. The isolate with TF and overexpression of the AQP1 gene of other molecular mechanisms such as overexpression of ATP-binding cassette may be involved in the TR, such as overexpression of ATP-binding cassette which requires further research.

KW - Clinical isolates

KW - COXII

KW - Gene expression

KW - Leishmania

KW - Leishmaniasis

KW - Minicircle kDNA

KW - Parasitology

KW - Phylogenetic analysis

KW - Treatment failure

UR - http://www.scopus.com/inward/record.url?scp=85102451740&partnerID=8YFLogxK

U2 - 10.7717/peerj.10969

DO - 10.7717/peerj.10969

M3 - Article

C2 - 33763300

AN - SCOPUS:85102451740

VL - 9

JO - PeerJ

JF - PeerJ

SN - 2167-8359

M1 - 10969

ER -

ID: 28089358