New approach for the identification of potentially toxigenic Corynebacterium sp. using a multiplex PCR assay

Sunarno; Khariri; Fauzul Muna; Kambang Sariadji; Yuni Rukminiati; Dwi Febriyana; Tati Febrianti; Ratih Dian Saraswati; Ida Susanti; Nelly Puspandari; Anis Karuniawati; Amarila Malik; Amin Soebandrio

doi:10.1016/j.mimet.2021.106198

New approach for the identification of potentially toxigenic Corynebacterium sp. using a multiplex PCR assay

J Microbiol Methods. 2021 May:184:106198. doi: 10.1016/j.mimet.2021.106198. Epub 2021 Mar 10.

Authors

Affiliations

¹ Centre for Research and Development of Biomedical and Basic Health Technology, National Institute of Health Research and Development, Ministry of Health, Jakarta, Indonesia. Electronic address: no_nar@yahoo.com.
² Centre for Research and Development of Biomedical and Basic Health Technology, National Institute of Health Research and Development, Ministry of Health, Jakarta, Indonesia.
³ Faculty of Medicine, Universitas Indonesia, Jakarta, Indonesia.
⁴ Division of Microbiology and Biotechnology Pharmacy, Faculty of Pharmacy, Universitas Indonesia, Depok, Indonesia.
⁵ Faculty of Medicine, Universitas Indonesia, Jakarta, Indonesia; Eijkman Institute for Molecular Biology, Jakarta, Indonesia.

PMID: 33713727
DOI: 10.1016/j.mimet.2021.106198

Abstract

In diphtheria laboratory examinations, the PCR test can be applied to isolates and clinical specimens. This study aimed to develop a PCR assay to identify the species and toxigenicity of diphtheria-causing bacteria, including the prediction of some NTTB types. Seven reference isolates, four synthetic DNA samples, 36 stored isolates, and 487 clinical samples used for PCR optimization. The PCR results was confirmed by DNA sequence analysis. The results of the PCR examination of the 7 reference isolates and 36 stored isolates were similar to the results obtained using conventional methods as gold standard, both for diphtheria-causing and non-diphtheria-causing bacteria. The validation of the PCR results using DNA sequence analysis showed that there was no mispriming or misamplification. The multiplex PCR assay developed in this study could correctly identify the species and toxigenicity of diphtheria-causing bacteria, including the prediction of some NTTB types not yet covered by established PCR methods.

Keywords: Diphtheria; PCR; Potentially toxigenic Corynebacterium; dtxR gene.

Publication types

Evaluation Study

MeSH terms

Bacterial Proteins / genetics
Bacterial Typing Techniques / methods*
Corynebacterium / classification
Corynebacterium / genetics
Corynebacterium / isolation & purification*
Corynebacterium Infections / microbiology*
DNA Primers / genetics
Diphtheria / microbiology
Humans
Multiplex Polymerase Chain Reaction / methods*

Substances

Bacterial Proteins
DNA Primers