Validation of the NAT Chagas IVD Kit for the Detection and Quantification of Trypanosoma cruzi in Blood Samples of Patients with Chagas Disease

Author:

Moreira Otacilio C.1ORCID,Fernandes Alice Gomes2,Gomes Natalia Lins da Silva1,dos Santos Carolina Messias2,Jacomasso Thiago3ORCID,Costa Alexandre Dias Tavares4ORCID,Nascimento Lucas de O. Rossetti3,Hasslocher-Moreno Alejandro Marcel5,do Brasil Pedro Emmanuel Alvarenga Americano5,Morello Luis Gustavo34,Marchini Fabricio Klerynton34,Krieger Marco Aurelio4,Britto Constança2ORCID

Affiliation:

1. Real Time PCR Platform RPT09A, Laboratory of Molecular Virology and Parasitology, Oswaldo Cruz Institute/Fiocruz, Rio de Janeiro 21040-900, Brazil

2. Laboratory of Molecular Biology and Endemic Diseases, Oswaldo Cruz Institute/Fiocruz, Rio de Janeiro 21040-900, Brazil

3. Instituto de Biologia Molecular do Paraná, Curitiba 81350-010, Brazil

4. Laboratory for Applied Science and Technology in Health, Carlos Chagas Institute/Fiocruz, Curitiba 81310-020, Brazil

5. Laboratory of Clinical Research in Chagas Disease, Evandro Chagas National Institute of Infectious Diseases/Fiocruz, Rio de Janeiro 21040-360, Brazil

Abstract

In the absence of validated biomarkers to control the cure of Chagas disease, PCR-based diagnosis is being used as the main tool for an early indication of therapeutic failure. However, since it is considered a technique of complex reproducibility, mainly due to difficulties in establishing accurate controls to guarantee the quality of the reaction, the use of PCR for Chagas disease diagnosis is restricted to specialized centers. In an effort to disseminate the molecular diagnosis of Chagas disease and its applications, new diagnostic kits based on qPCR have been made available in the market in recent years. Here, we show the results of the validation of the NAT Chagas kit (Nucleic Acid Test for Chagas Disease) for the detection and quantification of T. cruzi in blood samples of patients suspected of Chagas disease infection. The kit, composed of a TaqMan duplex reaction targeting the T. cruzi satellite nuclear DNA and an exogenous internal amplification control, presented a reportable range from 104 to 0.5 parasite equivalents/mL and a limit of detection (LOD) of 0.16 parasite equivalents/mL of blood. In addition, the NAT Chagas kit detected T. cruzi belonging to all six discrete typing units (DTUs—TcI to TcVI), similarly to the in-house real-time PCR performed with commercial reagents, which has been selected as the best performance assay in the international consensus for the validation of qPCR for Chagas disease. In the clinical validation presented here, the kit showed 100% sensitivity and 100% specificity when compared to the consensus in-house real-time PCR assay. Thus, the NAT Chagas kit, which is produced entirely in Brazil under the international standards of good manufacturing practices (GMP), appears as an excellent alternative to enable the molecular diagnosis of Chagas disease in public and private diagnostic centers, as well as to facilitate the monitoring of patients under etiological treatment participating in clinical trials.

Funder

Coordination for the Improvement of Higher Education Personnel

Departamento de Ciência e Tecnologia—Ministério da Saúde (DECIT)/Conselho Nacional de Desenvolvimento Científico e Tecnológico

NFiocruz

CNPq1D and FAPERJ

CNPq research 1B and FAPERJ

Publisher

MDPI AG

Subject

Paleontology,Space and Planetary Science,General Biochemistry, Genetics and Molecular Biology,Ecology, Evolution, Behavior and Systematics

Reference58 articles.

1. World Health Organization (2022, November 29). Chagas Disease (American Trypanosomiasis). Available online: https://www.who.int/health-topics/chagas-disease.

2. Pinazo Delgado, M.J., and Gascón, J. (2020). Chagas Disease, Springer.

3. American Trypanosomiasis (Chagas Disease);Rassi;Infect. Dis. Clin. N. Am.,2012

4. Chagas Disease in Europe: A Long Way to Go;Antinori;Eur. J. Intern. Med.,2018

5. Chagas Disease in the United States: A Public Health Approach;Bern;Clin. Microbiol. Rev.,2019

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