Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease

This work evaluated a serial blood sampling procedure to enhance the sensitivity of duplex real-time quantitative PCR (qPCR) for baseline detection and quantification of parasitic loads and posttreatment identification of failure in the context of clinical trials for treatment of chronic Chagas dise...

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Autores principales: Parrado, Rudy, Ramirez, Juan Carlos, de la Barra, Anabelle, Alonso-Vega, Cristina, Juiz, Natalia, Ortiz, Lourdes, Illanes, Daniel, Torrico, Faustino, Gascon, Joaquim, Alves, Fabiana, Flevaud, Laurence, Garcia, Lineth, Schijman, Alejandro G., Ribeiro, Isabela
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Society for Microbiology 2019
Materias:
Analytical Procedures
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6355557/
https://www.ncbi.nlm.nih.gov/pubmed/30509941
http://dx.doi.org/10.1128/AAC.01191-18
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author Parrado, Rudy
Ramirez, Juan Carlos
de la Barra, Anabelle
Alonso-Vega, Cristina
Juiz, Natalia
Ortiz, Lourdes
Illanes, Daniel
Torrico, Faustino
Gascon, Joaquim
Alves, Fabiana
Flevaud, Laurence
Garcia, Lineth
Schijman, Alejandro G.
Ribeiro, Isabela
author_facet Parrado, Rudy
Ramirez, Juan Carlos
de la Barra, Anabelle
Alonso-Vega, Cristina
Juiz, Natalia
Ortiz, Lourdes
Illanes, Daniel
Torrico, Faustino
Gascon, Joaquim
Alves, Fabiana
Flevaud, Laurence
Garcia, Lineth
Schijman, Alejandro G.
Ribeiro, Isabela
author_sort Parrado, Rudy
collection PubMed
description This work evaluated a serial blood sampling procedure to enhance the sensitivity of duplex real-time quantitative PCR (qPCR) for baseline detection and quantification of parasitic loads and posttreatment identification of failure in the context of clinical trials for treatment of chronic Chagas disease, namely, DNDi-CH-E1224-001 (ClinicalTrials.gov registration no. NCT01489228) and the MSF-DNDi PCR Sampling Optimization Study (NCT01678599). Patients from Cochabamba (n = 294), Tarija (n = 257), and Aiquile (n = 220) were enrolled. Three serial blood samples were collected at each time point, and qPCR triplicates were tested for each sample. The first two samples were collected during the same day and the third one 7 days later. A patient was considered PCR positive if at least one qPCR replicate was detectable. Cumulative results of multiple samples and qPCR replicates enhanced the proportion of pretreatment sample positivity from 54.8% to 76.2%, 59.5% to 77.8%, and 73.5% to 90.2% in Cochabamba, Tarija, and Aiquile cohorts, respectively. This strategy increased the detection of treatment failure from 72.9% to 91.7%, 77.8% to 88.9%, and 42.9% to 69.1% for E1224 low-, short-, and high-dosage regimens, respectively, and from 4.6% to 15.9% and 9.5% to 32.1% for the benznidazole arm in the DNDi-CH-E1224-001 and MSF-DNDi studies, respectively. The addition of the third blood sample and third qPCR replicate in patients with nondetectable PCR results in the first two samples gave a small, non-statistically significant improvement in qPCR positivity. No change in clinical sensitivity was seen with a blood volume increase from 5 to 10 ml. The monitoring of patients treated with placebo in the DNDi-CH-E1224-001 trial revealed fluctuations in parasitic loads and occasionally nondetectable results. In conclusion, a serial sampling strategy enhanced PCR sensitivity to detecting treatment failure during follow-up and has the potential for improving recruitment capacity in Chagas disease trials, which require an initial positive qPCR result for patient admission.
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spelling pubmed-63555572019-02-01 Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease Parrado, Rudy Ramirez, Juan Carlos de la Barra, Anabelle Alonso-Vega, Cristina Juiz, Natalia Ortiz, Lourdes Illanes, Daniel Torrico, Faustino Gascon, Joaquim Alves, Fabiana Flevaud, Laurence Garcia, Lineth Schijman, Alejandro G. Ribeiro, Isabela Antimicrob Agents Chemother Analytical Procedures This work evaluated a serial blood sampling procedure to enhance the sensitivity of duplex real-time quantitative PCR (qPCR) for baseline detection and quantification of parasitic loads and posttreatment identification of failure in the context of clinical trials for treatment of chronic Chagas disease, namely, DNDi-CH-E1224-001 (ClinicalTrials.gov registration no. NCT01489228) and the MSF-DNDi PCR Sampling Optimization Study (NCT01678599). Patients from Cochabamba (n = 294), Tarija (n = 257), and Aiquile (n = 220) were enrolled. Three serial blood samples were collected at each time point, and qPCR triplicates were tested for each sample. The first two samples were collected during the same day and the third one 7 days later. A patient was considered PCR positive if at least one qPCR replicate was detectable. Cumulative results of multiple samples and qPCR replicates enhanced the proportion of pretreatment sample positivity from 54.8% to 76.2%, 59.5% to 77.8%, and 73.5% to 90.2% in Cochabamba, Tarija, and Aiquile cohorts, respectively. This strategy increased the detection of treatment failure from 72.9% to 91.7%, 77.8% to 88.9%, and 42.9% to 69.1% for E1224 low-, short-, and high-dosage regimens, respectively, and from 4.6% to 15.9% and 9.5% to 32.1% for the benznidazole arm in the DNDi-CH-E1224-001 and MSF-DNDi studies, respectively. The addition of the third blood sample and third qPCR replicate in patients with nondetectable PCR results in the first two samples gave a small, non-statistically significant improvement in qPCR positivity. No change in clinical sensitivity was seen with a blood volume increase from 5 to 10 ml. The monitoring of patients treated with placebo in the DNDi-CH-E1224-001 trial revealed fluctuations in parasitic loads and occasionally nondetectable results. In conclusion, a serial sampling strategy enhanced PCR sensitivity to detecting treatment failure during follow-up and has the potential for improving recruitment capacity in Chagas disease trials, which require an initial positive qPCR result for patient admission. American Society for Microbiology 2019-01-29 /pmc/articles/PMC6355557/ /pubmed/30509941 http://dx.doi.org/10.1128/AAC.01191-18 Text en Copyright © 2019 Parrado et al. https://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Analytical Procedures
Parrado, Rudy
Ramirez, Juan Carlos
de la Barra, Anabelle
Alonso-Vega, Cristina
Juiz, Natalia
Ortiz, Lourdes
Illanes, Daniel
Torrico, Faustino
Gascon, Joaquim
Alves, Fabiana
Flevaud, Laurence
Garcia, Lineth
Schijman, Alejandro G.
Ribeiro, Isabela
Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease
title Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease
title_full Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease
title_fullStr Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease
title_full_unstemmed Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease
title_short Usefulness of Serial Blood Sampling and PCR Replicates for Treatment Monitoring of Patients with Chronic Chagas Disease
title_sort usefulness of serial blood sampling and pcr replicates for treatment monitoring of patients with chronic chagas disease
topic Analytical Procedures
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6355557/
https://www.ncbi.nlm.nih.gov/pubmed/30509941
http://dx.doi.org/10.1128/AAC.01191-18
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