The Development of a Multiplex PCR Assay for Fast and Cost-Effective Identification of the Five Most Significant Pathogenic Prototheca Species-Reference-Cited by-同舟云学术

The Development of a Multiplex PCR Assay for Fast and Cost-Effective Identification of the Five Most Significant Pathogenic Prototheca Species

Published:2023-08-07 Issue:8 Volume:12 Page:1018
ISSN:2076-0817
Container-title:Pathogens
language:en
Short-container-title:Pathogens

Author:

Vasco-Julio David¹²³^ORCID,Huilca-Ibarra María¹,Ledesma Yanua¹^ORCID,Echeverria Gustavo⁴⁵⁶^ORCID,Guerrero-Freire Salome⁶⁷^ORCID,Jagielski Tomasz⁸^ORCID,Bastidas-Caldes Carlos¹⁹^ORCID,de Waard Jacobus H.¹^ORCID

Affiliation:

1. One Health Research Group, Universidad de Las Américas, Quito 170530, Ecuador

2. Posgrado en Ciencias Biológicas, Universidad Nacional Autónoma de México, Unidad de Posgrado, Edificio D, Circuito de Posgrados, Ciudad Universitaria, Coyoacán C.P. 04510, Mexico

3. Centro de Investigación Sobre Enfermedades Infecciosas, Instituto Nacional de Salud Pública, Cuernavaca C.P. 62050, Mexico

4. Instituto de Investigación en Zoonosis-CIZ, Universidad Central del Ecuador, Quito 170518, Ecuador

5. División Investigación y Desarrollo, BioGENA, Quito 170509, Ecuador

6. Programa de Doctorado, Facultad de Ciencias Veterinarias, Universidad de Buenos Aires, Buenos Aires C1063ACV, Argentina

7. Group of Emerging and Neglected Diseases, Ecoepidemiology and Biodiversity, Health Sciences Faculty, Universidad Internacional SEK, Quito 170521, Ecuador

8. Department of Medical Microbiology, Institute of Microbiology, Faculty of Biology, University of Warsaw, 02-096 Warsaw, Poland

9. INABIO—Instituto Nacional de Biodiversidad, Parque La Carolina, Quito 170135, Ecuador

Abstract

A multiplex PCR system (m-PCR) has been developed to accurately differentiate the five most important pathogenic Prototheca species, including the three species associated with infection in dairy cattle (P. ciferrii, P. blaschkeae, and P. bovis) and the two species associated with human infections (P. wickerhamii and P. cutis). The method is low-cost since it employs a simple “heat-shock” method in a TE buffer for DNA extraction. Furthermore, it requires only primers, a Taq polymerase, an agarose gel, and a molecular weight marker for identification. The method was based on published Prototheca cytochrome B sequences and was evaluated using reference strains from each of the five Prototheca species. The validity of the method was confirmed by identifying 50 strains isolated from milk samples. The specificity was tested in silico and with experimental PCR trials, showing no cross-reactions with other Prototheca species, as well as with bacteria, fungi, cows, algae, animals, or humans. The method could detect mixed infections involving two or three Prototheca species, providing a rapid test that delivers results within three hours.

Funder

Universidad de Las Americas

Publisher

MDPI AG

Subject

Infectious Diseases,Microbiology (medical),General Immunology and Microbiology,Molecular Biology,Immunology and Allergy

Link

https://www.mdpi.com/2076-0817/12/8/1018/pdf

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