Title
Estimation of pyrazinamidase activity using a cell-free in vitro synthesis of pnca and its association with pyrazinamide susceptibility in Mycobacterium tuberculosis
Date Issued
01 January 2018
Access level
open access
Resource Type
journal article
Author(s)
Bernard C.
Gandy L.
Capton E.
Boudjelloul R.
Brossier F.
Veziris N.
Sougakoff W.
Publisher(s)
Wolters Kluwer Medknow Publications
Abstract
Background: The main mechanism of resistance to PZA in Mycobacterium tuberculosis relies on mutations on its pyrazinamidase/nicotinamidase. Recently, a rapid colorimetric test relying on the PCR-based in vitro-synthesized-PZase assay has been reported for PZase activity determination from clinical M. tuberculosis isolates but the assay has not been compared with other tests to evaluate PZA susceptibility in M. tuberculosis isolates. Methods: In this study, we have used the PCR-based in vitro-synthesized-PZase assay to analyze the specific pyrazinamidase (PZase) activity of PncA mutants and have correlated the results to the PZA susceptibility phenotype determined by culture in acidic agar medium at pH 6.0. A set of 23 clinical isolates displaying mutated pncA genes (11 PZA-resistant and 12 PZA-susceptible) and 55 PZA-susceptible clinical strains displaying a wild-type pncA gene were tested. Results: Among the 23 mutants tested, 4 corresponded to mutations not reported before (I5T, Y99S, T142R and P77L+V131G). Of the 11 PncA mutants expressed from PZA-resistant clinical isolates, 9 were expressed in vitro at yields > 50% relative to the wild type enzyme. Among them, 6 enzymes (T47P, H51P, H51R, H57D, L85R and T142R) showed no detectable activity, while the relative activities for the 3 others, V9A (27%), G97D (10%) and A146V (28%) were low compared to the wild-type PZase. The remaining two mutants, I5T and V9G, presented very low relative expression (5%) and relative activities values of 12 and 1%, respectively. Twelve mutants were expressed from PZA-susceptible isolates. Their expression was similar to the wild type enzyme and behaved as active pyrazinamidase with specific relative activities ranging from 34 to 314%. Finally, discrepant results were observed for two mutants, V7A and P62T. Conclusion: Thus, this study provides the proof of concept that the PCR-based in vitro-synthesized-PZase assay represents a promising rapid approach for the evaluation of PZA susceptibility based on the estimation of the relative PZase activity from clinical isolates.
Start page
16
End page
25
Volume
7
Issue
1
Language
English
OCDE Knowledge area
Enfermedades infecciosas
Biotecnología relacionada con la salud
Subjects
Scopus EID
2-s2.0-85043683663
PubMed ID
Source
International Journal of Mycobacteriology
ISSN of the container
2212-5531
Sponsor(s)
This work was supported by the Université Pierre et Marie Curie (UPMC) and by the Institut National de la Santé et de la Recherche Médicale (INSERM) (grant UPMC‑INSERM UMRS1135). D.R. was supported by a scholarship of the Franco‑Peruvian Doctoral School in Life Sciences.
We thank G. Millot for his technical assistance. This work was supported by the Université Pierre et Marie Curie (UPMC) and by the Institut National de la Santé et de la Recherche Médicale (INSERM) (grant UPMC-INSERM UMRS1135). D.R. was supported by a scholarship of the Franco-Peruvian Doctoral School in Life Sciences.
Sources of information:
Directorio de Producción Científica
Scopus