Rifampin-Isoniazid Oligonucleotide Typing: an Alternative Format for Rapid Detection of Multidrug-Resistant Mycobacterium tuberculosis

Author:

Hernández-Neuta Iván1,Varela Andrés1,Martin Anandi2,von Groll Andrea2,Jureen Pontus3,López Beatriz4,Imperiale Belén5,Šķenders Ģirts6,Ritacco Viviana4,Hoffner Sven3,Morcillo Nora5,Palomino Juan Carlos2,Del Portillo Patricia1

Affiliation:

1. Corporacion CorpoGen, Carrera 5 No. 66A-34, Bogotá, Colombia

2. Mycobacteriology Unit, Institute of Tropical Medicine, Nationalestraat 155, Antwerp, Belgium

3. Swedish Institute for Infectious Disease Control, 171 82 Solna, Sweden

4. Instituto Nacional de Enfermedades Infecciosas ANLIS C. G. Malbrán, Velez Sarsfield 563, Buenos Aires, Argentina

5. Hospital Dr. Cetrángolo, Italia 1750, Buenos Aires, Argentina

6. State Agency of Tuberculosis and Lung Diseases, Riga, Latvia

Abstract

ABSTRACT A reverse line blot DNA hybridization format for rapid detection of multidrug-resistant tuberculosis was developed. Simultaneous detection of rifampin and isoniazid resistance in clinical isolates of Mycobacterium tuberculosis was based on the same amplification/reverse hybridization principle of the widely used spoligotyping. The test involved probing nine DNA regions that are targets of common drug resistance-associated mutations in the genes rpoB , katG , and inhA . Addition of quaternary amine tetramethyl ammonium chloride to the hybridization buffer promoted multiple hybrid formations at a single annealing temperature irrespective of the different GC contents of probes. The assay was standardized using 20 well-documented strains from the Institute of Tropical Medicine (Belgium) and evaluated blindly in a central laboratory with 100 DNA samples that were obtained from cultured clinical isolates and shipped dried from three other countries. Compared with drug susceptibility testing, both sensitivity and specificity for rifampin resistance detection were 93.0% while for isoniazid the values were 87.7% and 97.7%, respectively. Compared with sequencing and GenoType MTBDRplus methods, sensitivity and specificity reached 96.4% and 95.5% for rifampin and 92.7% and 100% for isoniazid. Altogether, 40/45 (89%) multidrug-resistant isolates were correctly identified. Advantages of this in-house development include versatility, capacity to run up to 41 samples by triplicate in a single run, and reuse of the membrane at least 10 times. These features substantially reduce cost per reaction and make the assay an attractive tool for use in reference laboratories of countries that have a high burden of multidrug-resistant tuberculosis but that cannot afford expensive commercial tests because of limited resources.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

Reference33 articles.

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2. Bostanabad, S. Z., L. P. Titov, A. Bahrmand, and S. A. Nojoumi. 2008. Detection of mutation in isoniazid-resistant Mycobacterium tuberculosis isolates from tuberculosis patients in Belarus. Indian J. Med. Microbiol. 26 : 143-147.

3. Performance of the Genotype MTBDR Line Probe Assay for Detection of Resistance to Rifampin and Isoniazid in Strains of Mycobacterium tuberculosis with Low- and High-Level Resistance

4. Bwanga, F., S. Hoffner, M. Haile, and M. L. Joloba. 2009. Direct susceptibility testing for multi drug resistant tuberculosis: a meta-analysis. BMC Infect. Dis. 9 : 67.

5. Canetti, G., W. Fox, A. Khomenko, H. T. Mahler, N. K. Menon, D. A. Mitchison, N. Rist, and N. A. Smelev. 1969. Advances in techniques of testing mycobacterial drug sensitivity, and the use of sensitivity tests in tuberculosis control programmes. Bull. World Health Organ. 41 : 21-43.

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