Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial

Quantitative real-time PCR (qPCR) is an accurate method to quantify Trypanosoma cruzi DNA and can be used to follow-up parasitemia in Chagas disease (CD) patients undergoing chemotherapy. The Benznidazole Evaluation for Interrupting Trypanosomiasis (BENEFIT) study is an international, multicenter, r...

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Fecha de publicación:
2013
Institución:
Universidad del Rosario
Repositorio:
Repositorio EdocUR - U. Rosario
Idioma:
eng
OAI Identifier:
oai:repository.urosario.edu.co:10336/26414
Acceso en línea:
https://doi.org/10.1016/j.actatropica.2012.08.020
https://repository.urosario.edu.co/handle/10336/26414
Palabra clave:
Cardiac chronic
Chagas disease
Molecular diagnosis
Real-time PCRBENEFI
TTrypanosoma cruzi
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oai_identifier_str oai:repository.urosario.edu.co:10336/26414
network_acronym_str EDOCUR2
network_name_str Repositorio EdocUR - U. Rosario
repository_id_str
dc.title.spa.fl_str_mv Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
dc.title.TranslatedTitle.spa.fl_str_mv Hacia el establecimiento de una qPCR consensuada en tiempo real para monitorear la parasitemia por Trypanosoma cruzi en pacientes con miocardiopatía crónica por enfermedad de Chagas: un subestudio del ensayo BENEFIT
title Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
spellingShingle Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
Cardiac chronic
Chagas disease
Molecular diagnosis
Real-time PCRBENEFI
TTrypanosoma cruzi
title_short Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
title_full Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
title_fullStr Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
title_full_unstemmed Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
title_sort Towards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trial
dc.subject.keyword.spa.fl_str_mv Cardiac chronic
Chagas disease
Molecular diagnosis
Real-time PCRBENEFI
TTrypanosoma cruzi
topic Cardiac chronic
Chagas disease
Molecular diagnosis
Real-time PCRBENEFI
TTrypanosoma cruzi
description Quantitative real-time PCR (qPCR) is an accurate method to quantify Trypanosoma cruzi DNA and can be used to follow-up parasitemia in Chagas disease (CD) patients undergoing chemotherapy. The Benznidazole Evaluation for Interrupting Trypanosomiasis (BENEFIT) study is an international, multicenter, randomized, double-blinded and placebo-controlled clinical trial to evaluate the efficacy of benznidazole (BZ) treatment in patients with chronic Chagas cardiomyopathy (CCC). One important question to be addressed concerns the effectiveness of BZ in reducing overall parasite load in CCC patients, even in the absence of parasitological cure. This report describes the evaluation of multiple procedures for DNA extraction and qPCR-based protocols aiming to establish a standardized methodology for the absolute quantification of T. cruzi DNA in Guanidine-EDTA blood (GEB) samples. A panel of five primer sets directed to the T. cruzi nuclear satellite DNA repeats (Sat-DNA) and to the minicircle DNA conserved regions (kDNA) was compared in either SYBR Green or TaqMan systems. Standard curve parameters such as, amplification efficiency, coefficient of determination and intercept were evaluated, as well as different procedures to generate standard samples containing pre-established T. cruzi DNA concentration. Initially, each primer set was assayed in a SYBR Green qPCR to estimate parasite load in GEB samples from chronic Chagas disease patients. The results achieved from Bayesian transmutability analysis elected the primer sets Cruzi1/Cruzi2 (p = 0.0031) and Diaz7/Diaz8 (p = 0.0023) coupled to the QIAamp DNA Kit extraction protocol (silica gel column), as the most suitable for monitoring parasitemia in these patients. Comparison between the parasite burden of 150 GEB samples of BENEFIT patients from Argentina, Brazil and Colombia, prior to drug/placebo administration, was performed using Cruzi1/Cruzi2 primers in a SYBR Green approach. The median parasitemia found in patients from Argentina and Colombia (1.93 and 2.31 parasite equivalents/mL, respectively) was around 20 times higher than the one estimated for the Brazilian patients (0.1 parasite equivalents/mL). This difference could be in part due to the complexity of T. cruzi genetic diversity, which is a factor possibly implicated in different clinical presentations of the disease and/or influencing parasitemia levels in infected individuals from different regions of Latin America. The results of SYBR Green qPCR assays herein presented prove this methodology to be more cost efficient than the alternative use of internal fluorogenic probes. In addition, its sensitivity and reproducibility are shown to be adequate to detect low parasitemia burden in patients with chronic Chagas disease.
publishDate 2013
dc.date.created.spa.fl_str_mv 2013-01
dc.date.accessioned.none.fl_str_mv 2020-08-06T16:21:38Z
dc.date.available.none.fl_str_mv 2020-08-06T16:21:38Z
dc.type.eng.fl_str_mv article
dc.type.coarversion.fl_str_mv http://purl.org/coar/version/c_970fb48d4fbd8a85
dc.type.coar.fl_str_mv http://purl.org/coar/resource_type/c_6501
dc.type.spa.spa.fl_str_mv Artículo
dc.identifier.doi.none.fl_str_mv https://doi.org/10.1016/j.actatropica.2012.08.020
dc.identifier.issn.none.fl_str_mv ISSN: 0001-706X
EISSN: 1873-6254
dc.identifier.uri.none.fl_str_mv https://repository.urosario.edu.co/handle/10336/26414
url https://doi.org/10.1016/j.actatropica.2012.08.020
https://repository.urosario.edu.co/handle/10336/26414
identifier_str_mv ISSN: 0001-706X
EISSN: 1873-6254
dc.language.iso.spa.fl_str_mv eng
language eng
dc.relation.citationEndPage.none.fl_str_mv 31
dc.relation.citationIssue.none.fl_str_mv No. 1
dc.relation.citationStartPage.none.fl_str_mv 23
dc.relation.citationTitle.none.fl_str_mv Acta Tropica
dc.relation.citationVolume.none.fl_str_mv Vol. 125
dc.relation.ispartof.spa.fl_str_mv Acta Tropica, ISSN: 0001-706X;EISSN: 1873-6254, Vol.125, No.1 (2013-01);pp. 23-31
dc.relation.uri.spa.fl_str_mv https://www.sciencedirect.com/sdfe/reader/pii/S0001706X12003063/pdf
dc.rights.coar.fl_str_mv http://purl.org/coar/access_right/c_16ec
dc.rights.acceso.spa.fl_str_mv Restringido (Acceso a grupos específicos)
rights_invalid_str_mv Restringido (Acceso a grupos específicos)
http://purl.org/coar/access_right/c_16ec
dc.format.mimetype.none.fl_str_mv application/pdf
dc.publisher.spa.fl_str_mv Elsevier
dc.source.spa.fl_str_mv Acta Tropica
institution Universidad del Rosario
dc.source.instname.none.fl_str_mv instname:Universidad del Rosario
dc.source.reponame.none.fl_str_mv reponame:Repositorio Institucional EdocUR
repository.name.fl_str_mv Repositorio institucional EdocUR
repository.mail.fl_str_mv edocur@urosario.edu.co
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spelling cc5cb7dd-8436-4c49-b5a0-4cd18a86a30310117161186004e7a760a-e927-4c97-9bd8-a4942eee0c26c9d35941-d90f-46fc-b99d-eb93678b5eca5a3a7164-0060-4144-b60b-e37d54307c2ef2428500-1bed-4573-bb9d-210b32d8f52bb30d8652-aac5-4bca-9171-92d5b16a1d35aae788e6-6f3d-4590-9435-8ed37f10f97c9d5bdca0-a8a4-4129-9dd5-97822696d5476ccfc20a-efa9-4503-9be2-edb3a70fb59a2020-08-06T16:21:38Z2020-08-06T16:21:38Z2013-01Quantitative real-time PCR (qPCR) is an accurate method to quantify Trypanosoma cruzi DNA and can be used to follow-up parasitemia in Chagas disease (CD) patients undergoing chemotherapy. The Benznidazole Evaluation for Interrupting Trypanosomiasis (BENEFIT) study is an international, multicenter, randomized, double-blinded and placebo-controlled clinical trial to evaluate the efficacy of benznidazole (BZ) treatment in patients with chronic Chagas cardiomyopathy (CCC). One important question to be addressed concerns the effectiveness of BZ in reducing overall parasite load in CCC patients, even in the absence of parasitological cure. This report describes the evaluation of multiple procedures for DNA extraction and qPCR-based protocols aiming to establish a standardized methodology for the absolute quantification of T. cruzi DNA in Guanidine-EDTA blood (GEB) samples. A panel of five primer sets directed to the T. cruzi nuclear satellite DNA repeats (Sat-DNA) and to the minicircle DNA conserved regions (kDNA) was compared in either SYBR Green or TaqMan systems. Standard curve parameters such as, amplification efficiency, coefficient of determination and intercept were evaluated, as well as different procedures to generate standard samples containing pre-established T. cruzi DNA concentration. Initially, each primer set was assayed in a SYBR Green qPCR to estimate parasite load in GEB samples from chronic Chagas disease patients. The results achieved from Bayesian transmutability analysis elected the primer sets Cruzi1/Cruzi2 (p = 0.0031) and Diaz7/Diaz8 (p = 0.0023) coupled to the QIAamp DNA Kit extraction protocol (silica gel column), as the most suitable for monitoring parasitemia in these patients. Comparison between the parasite burden of 150 GEB samples of BENEFIT patients from Argentina, Brazil and Colombia, prior to drug/placebo administration, was performed using Cruzi1/Cruzi2 primers in a SYBR Green approach. The median parasitemia found in patients from Argentina and Colombia (1.93 and 2.31 parasite equivalents/mL, respectively) was around 20 times higher than the one estimated for the Brazilian patients (0.1 parasite equivalents/mL). This difference could be in part due to the complexity of T. cruzi genetic diversity, which is a factor possibly implicated in different clinical presentations of the disease and/or influencing parasitemia levels in infected individuals from different regions of Latin America. The results of SYBR Green qPCR assays herein presented prove this methodology to be more cost efficient than the alternative use of internal fluorogenic probes. In addition, its sensitivity and reproducibility are shown to be adequate to detect low parasitemia burden in patients with chronic Chagas disease.application/pdfhttps://doi.org/10.1016/j.actatropica.2012.08.020ISSN: 0001-706XEISSN: 1873-6254https://repository.urosario.edu.co/handle/10336/26414engElsevier31No. 123Acta TropicaVol. 125Acta Tropica, ISSN: 0001-706X;EISSN: 1873-6254, Vol.125, No.1 (2013-01);pp. 23-31https://www.sciencedirect.com/sdfe/reader/pii/S0001706X12003063/pdfRestringido (Acceso a grupos específicos)http://purl.org/coar/access_right/c_16ecActa Tropicainstname:Universidad del Rosarioreponame:Repositorio Institucional EdocURCardiac chronicChagas diseaseMolecular diagnosisReal-time PCRBENEFITTrypanosoma cruziTowards the establishment of a consensus real-time qPCR to monitor Trypanosoma cruzi parasitemia in patients with chronic Chagas disease cardiomyopathy: A substudy from the BENEFIT trialHacia el establecimiento de una qPCR consensuada en tiempo real para monitorear la parasitemia por Trypanosoma cruzi en pacientes con miocardiopatía crónica por enfermedad de Chagas: un subestudio del ensayo BENEFITarticleArtículohttp://purl.org/coar/version/c_970fb48d4fbd8a85http://purl.org/coar/resource_type/c_6501Moreira, Otalicio C.Ramírez, Juan DavidVelázquez, ElsaDías Melo, Myllena F. A.Lima Ferreira, CarolinaGushi, FelipeSosa Estani, SergioMarín Neto, José AntonioMorillo, Carlos A.Britto, Constanza10336/26414oai:repository.urosario.edu.co:10336/264142021-10-05 07:02:22.9https://repository.urosario.edu.coRepositorio institucional EdocURedocur@urosario.edu.co