Possible drug resistance in Mycobacterium leprae strains from Venezuela and three other South American countries was surveyed by molecular methods. None of the 230 strains from new leprosy cases exhibited drug resistance-associated mutations. However, two of the three strains from relapsed cases contained dapsone resistance mutations, and one strain also harbored a rifampin resistance mutation. Single nucleotide polymorphism analysis of these strains revealed five subtypes: 3I (73.8%), 4P (11.6%), 1D (6.9%), 4N (6%), and 4O (1.7%).The success of leprosy control programs relies heavily upon multidrug therapy (MDT) (rifampin, dapsone, and clofazimine). Therefore, it is important that drug resistance trends be monitored periodically and Mycobacterium leprae strains genotyped in order to understand transmission patterns and genetic diversity. In the present study, strains of M. leprae from Bolivia, Brazil, Uruguay, and Venezuela were genotyped using single nucleotide polymorphism (SNP) analysis (17, 18), and their drug resistance-determining regions (DRDRs) in the rpoB, folP1, and gyrA genes were sequenced. In parallel, a real-time PCR assay that targets the most frequent sites of drug resistance in rpoB and folP1 was established.A total of 233 M. leprae strains were obtained from patient biopsy specimens or from slit skin smears; the majority of the patients were from Venezuela (n ϭ 197), and the remainder were from Bolivia (n ϭ 10), Brazil (n ϭ 24), and Uruguay (n ϭ 2). Reference DNA from drug-susceptible strains TN, Br4923, NHDP63, and Thai53 was used as a control for the sequencing and the real-time PCR-based TaqMan assay. A known rifampinresistant strain, 85054 (French West Indies), with an rpoB mutation (Ser425Leu) (8), was included as a positive control. This strain also has a dapsone resistance mutation (Pro55Leu) in folP1.DNA extraction from skin biopsy specimens/slit skin samples was carried out by the "freeze-boiling" method as described previously (24), followed by PCR amplification and DNA sequencing (18). Primers used for analyzing the drug resistance-associated loci are shown in Table 1. The sequences, obtained from an ABI 3130xl genetic analyzer (Applied Biosystems, Life Technologies Corporation, CA), were aligned against the sequences of the TN reference strain using CodonCode Aligner software (Dedham, MA) to identify polymorphisms. SNP genotyping was done as described previously (17, 18). The frequency of SNP7614 (presence of "T" at this position in subtype 3I strains) (18) was also determined.TaqMan probe assays using real-time PCR were performed in triplicate. Each 20-l reaction mixture contained 100 nM probe, 200 nM primers (Table 2) in 1ϫ TaqMan PCR master mix (Applied Biosystems, CA), and 2 l of DNA. PCR mixtures were subjected to thermal cycling for 2 min at 50°C and 10 min at 95°C followed by 40 cycles of 15 s at 95°C and 1 min at 60°C with a 7900HT Fast real-time PCR system (Applied Biosystems, CA). An increase in fluorescence indicates perfect complementarity between template and probe. ...
