Detection of katG Ser315Thr substitution in respiratory specimens from patients with isoniazid-resistant Mycobacterium tuberculosis using PCR-RFLP

doi:10.1099/jmm.0.05223-0

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Detection of katG Ser315Thr substitution in respiratory specimens from patients with isoniazid-resistant Mycobacterium tuberculosis using PCR-RFLP

Eric Tung-Yiu Leung¹, Kai-Man Kam², Agatha Chiu², Pak-Leung Ho^1,3, Wing-Hong Seto¹, Kwok-Yung Yuen^1,4 and Wing-Cheong Yam¹

¹Department of Microbiology, The University of Hong Kong, University Pathology Building, Queen Mary Hospital, Pokfulam Road, Hong Kong SAR, China ²Tuberculosis Reference Laboratory and Public Health Laboratory, Department of Health, Hong Kong SAR, China ^3,4Centre of Infection³ and HKU-Pasteur Research Centre⁴, Faculty of Medicine, The University of Hong Kong, Hong Kong SAR, China

Correspondence Wing-Cheong Yam wcyam{at}hkucc.hku.hk

Received February 17, 2003
Accepted August 7, 2003

Mutations in the katG locus of catalase peroxidase in Mycobacteriumtuberculosis (MTB) account for major isoniazid (INH) resistance.In the South China region, a collection of 906 respiratory specimensand 142 MTB isolates was used to evaluate the sensitivity andspecificity of a PCR-RFLP method for the detection of INH resistance-associatedmutations. Except for four catalase-negative MTB isolates, katGPCR for a 620-bp amplicon was successful for all purified MTBisolates. For respiratory specimens, diagnostic sensitivityand specificity of katG PCR was 85 and 100 %. Subsequent RFLPof the katG amplicons by MspI digestion identified that 51 %of INH-resistant MTB were associated with the Thr315 phenotype,and that codon 463 was a polymorphic site with no linkage toINH resistance. The Arg463 wild-type MTB isolates predominantin the Western world were replaced by isolates carrying Leu463in the South China region. RFLP patterns of katG amplicons fromrespiratory specimens were identical to those of the correspondingMTB cultured colonies. This method has potential applicationfor rapid diagnosis of INH resistance due to katG Ser315Thrmutation.

Abbreviations: AFB, acid-fast bacilli; INH, isoniazid; MOTT,Mycobacterium sp. other than tuberculosis; MTB, Mycobacteriumtuberculosis.

INTRODUCTION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Tuberculosis remains a global threat to public health. The problemis further complicated by the emergence of multidrug-resistanttuberculosis as a consequence of the widespread use and incautiousadministration of antibiotics (WHO, 2000). Rapid diagnosis andappropriate chemotherapy become the first priorities in controllinggrowing epidemics. Nowadays, isoniazid (INH), ethambutol, rifampicin,pyrazinamide and streptomycin are important components of first-lineanti-tubercular regimens. INH has a much more complex resistancemechanism than the other four compounds. Several studies haverevealed different putative molecular targets of INH, includingcatalase peroxidase (katG) (van Soolingen et al., 2000), enoyl-acylreductase (inhA) (Basso et al., 1998), alkyl-hydroperoxide reductase(ahpC) (Sherman et al., 1996), ß-ketoacyl-acyl carrierprotein synthase (kasA) (Mdluli et al., 1998) and NADH dehydrogenase(ndh) (Lee et al., 2001). However, a predominant mutation inthe katG locus, Ser315Thr, accounts for more than 50 % of INH-resistancephenotypes, according to earlier reports (Musser et al., 1996;van Soolingen et al., 2000). Mycobacterial strains lacking theentire katG gene would also exhibit an INH-resistant phenotype(Heym et al., 1995).

In this study, we developed a simple PCR-RFLP method for directdetection of katG Ser315Thr-associated INH-resistant Mycobacteriumtuberculosis (MTB) in clinical isolates and respiratory specimens.A total of 906 respiratory specimens and 142 MTB isolates wereused to evaluate the specificity and sensitivity of this assay.Results were compared with commercial and in-house PCR assaysfor MTB, anti-mycobacterial susceptibility testing and DNA sequencing.

METHODS

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Specimens and isolates.

Between December 1999 and February 2002, 906 respiratory specimens(828 expectorated sputum and 78 bronchoalveolar lavage samples)collected from patients suffering from chest symptoms and/orchest radiographic infiltrates of undetermined origin included675 patients from Queen Mary Hospital and 231 out-patients ofPolyclinics of the Department of Health in Hong Kong. An additional142 clinical isolates of MTB were collected from three majorcities in the Pearl River delta of the South China region ofChina: Hong Kong (96 isolates), Macau (27 isolates) and Guangzhou(19 isolates). Specimens were processed for direct smear followedby concentration for acid-fast bacilli (AFB) culture as describedpreviously (Nolte & Metchock, 1995). After concentration,digested sediments were divided equally for AFB culture andsubsequent PCR assays. Cultures positive for AFB were identifiedusing the AccuProbe hybridization assay (Gen-Probe) and conventionalbiochemical tests. Catalase test for MTB was performed accordingto the method of Nolte & Metchock (1995). Antimicrobialsusceptibility testing was performed using the proportionalmethod (NCCLS, 2000).

DNA extraction for PCR.

For the digested sediments, the Roche Cobas Amplicor extractionprotocol was adopted as described previously (Yam et al., 1998;Yuen et al., 1997). A final volume of 200 µl DNA extractwas used for subsequent PCRs (undiluted extract). For samplesrequiring further DNA concentration and purification, 100 µlDNA extract was further purified using mini-columns (gel extractionkit; Qiagen) according to the manufacturer's instructions and30 µl purified DNA was eluted (3x concentrated extract).For purified culture of MTB on Lowenstein–Jensen medium,a uniform bacterial suspension (McFarland standard no. 1) wasmade in 0.1 M Tris/HCl, pH 7.5. For the MTB standard strainRv37, the bacterial suspension was further diluted from 10^-3to 10^-10 for colony counting using Middlebrook agar plates.All bacterial suspensions were subsequently heated at 100 °Cfor 30 min, frozen at -80 °C, thawed at 80 °C and centrifugedat 15 000 g for 10 min; the supernatant was used directly forsubsequent PCR assays. For the MTB standard strain Rv37, serialdilutions of heated extract were used for determination of analyticalsensitivity of the IS6110 and katG PCR assays.

PCR assays for MTB 16S rRNA and IS6110.

The Cobas Amplicor MTB test (Roche) uses genus Mycobacterium-specificbiotinylated primers to amplify a sequence of 584 bp withina 1500-bp region encoding the 16S rRNA of MTB (Yuen et al., 1997).An internal control was incorporated in each reactionto monitor PCR inhibitors. A manual one-tube nested PCR forIS6110 was performed as described previously (Chan et al., 1996;Yam et al., 1998; Yuen et al., 1997).

PCR-RFLP for katG.

Each PCR contained 10 µl DNA extract. Primers katG904(5'-AGCTCGTATGGCACCGGAAC-3', forward primer, positions 904–923)and katG1523 (5'-TTGACCTCCCACCCGACTTG-3', reverse primer, positions1523–1502) (Uhl et al., 1996) were used to amplify a 620-bpfragment of katG. Each 100 µl reaction contained 10 mMTris/HCl (pH 8.3), 50 mM KCl, 2 mM MgCl₂, 0.15 mM dNTPs, 0.2µM each primer and 2 U AmpliTaq Gold polymerase (PerkinElmer). To activate the Taq polymerase, the mixture was firstincubated at 94 °C for 12 min. Subsequent temperature cyclingfor 45 cycles started at 94 °C for 1 min, 60 °C for1 min and 72 °C for 1 min. A 10 µl aliquot of thePCR product was electrophoresed for 1 h through 2 % agarosegel in 1x TBE. For samples positive for the 620-bp fragmentof katG, a 5 µl aliquot of the PCR product was digestedusing 2 U MspI restriction endonuclease (Amersham PharmaciaBiotech) in a 10 µl reaction at 37 °C for 4 h, followedby electrophoresis in a 6 % polyacrylamide gel. In this study,the INH-resistance mutation in katG codon 315 (Ser, AGC $<-$ Thr,ACC) and polymorphic variation in codon 463 (Arg, CGG or Leu,CTG) were identified by RFLP using MspI digestion (restrictionsite C ${uparrow}$ CGG).

DNA sequencing of 620-bp katG amplicons.

To verify the point mutations detected by PCR-RFLP, 620-bp katGamplicons of 20 randomly selected MTB isolates (10 INH-susceptibleand 10 INH-resistant) were sequenced using BigDye technologyand an ABI 377 Genetic Analyzer (Applied Biosystems).

RESULTS AND DISCUSSION

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Among 906 respiratory specimens shown in Table 1, 233 were culture-positivefor MTB and 35 were culture-positive for ‘Mycobacteriumsp. other than tuberculosis’ (MOTT), while the remaining638 were culture-negative for Mycobacterium. Of 187 samplesthat were AFB smear-positive and culture-positive for MTB, 161(86 %) were positive for katG PCR, whereas IS6110 PCR and RochePCR provided 100 % sensitivity for direct detection of MTB inthese specimens. This result is concordant with an experimenton analytical sensitivity that showed that IS6110 PCR was 10times more sensitive than the katG PCR (Fig. 1). End-point detectionof MTB for IS6110 PCR and katG PCR was found to be 1.5 and 15c.f.u., respectively. Using a simple column-elution concentrator,all 187 AFB smear-positive specimens and 11/46 (24 %) AFB smear-negativespecimens were positive for katG PCR. A total of 233 specimenswere subsequently confirmed to be culture-positive for MTB,all of which were found to be catalase-positive. A specificityof 100 % was exhibited for the three PCR assays on 906 respiratoryspecimens with diagnostic sensitivity of 92 % for IS6110 PCR,86 % for Roche PCR and 85 % for katG PCR. The katG PCR is highlyspecific for MTB, in that none of the specimens with MOTT orthose that were culture-positive for other respiratory bacterialpathogens showed a positive result. By Roche PCR, 4.8 % specimensoverall were detected to contain PCR inhibitors (data not shown).

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Table 1. Comparative sensitivities and specificities of three PCR assays for detection of MTB IS6110 PCR and Roche PCR were performed with undiluted extract. Values are number positive/total (% positive).

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Fig. 1. Analytical sensitivity of IS6110 PCR (lanes A–F) and katG PCR (a–f) with serial dilutions of MTB Rv37 extracts. Lanes: A, a, 10^-5; B, b, 10^-6; C, c, 10^-7; D, d, 10^-8; E, e, 10^-9; F, f, 10^-10; M, molecular size marker ${phi}$ X174.

The katG amplicons were further analysed by RFLP using MspIdigestion (Table 2) and four distinct RFLP patterns were generated(Fig. 2). All RFLP patterns of katG amplicons from the 198 respiratoryspecimens were identical to those of the corresponding MTB isolates,indicating that katG PCR provides reliable detection in clinicalspecimens. Four catalase-negative MTB isolates were katG PCR-negativeand confirmed INH-resistant by susceptibility testing. Theseisolates confer INH resistance by partial or complete deletionof katG, accounting for the negative katG PCR result (Heym et al., 1995).Among the 375 MTB isolates (233 isolates from respiratoryspecimens and 142 isolates from purified culture), the proportionalmethod identified 273 INH-susceptible and 102 INH-resistantMTB isolates. Of the 102 INH-resistant isolates (Hong Kong,71 isolates; Macau, 19; Guangzhou, 12), 52 (51 %) isolates exhibitedphenotype Thr315 (RFLP patterns C and D). The remaining 50 (49%) resistant isolates showed phenotype Ser315 (RFLP patternsA and B). There was no documentation of an outbreak during thestudy period, and all RFLP patterns were distributed randomlyamong isolates from the three cities (data not shown). Thr315is 100 % specific for INH resistance, since no susceptible isolatesexhibited Thr315. Automated DNA sequencing of the 620-bp katGamplicons from 10 randomly selected INH-susceptible isolates(four isolates of RFLP pattern A and six isolates of RFLP patternB) and 10 INH-resistant isolates (two, one, three and four isolates,respectively, of RFLP patterns A–D) verified 100 % sequenceaccuracy of the point mutations detected by PCR-RFLP. DNA sequencingalso revealed no mutation other than Ser/Thr315 and Arg/Leu463within the 620-bp katG amplicons for the 20 isolates. Arg463and Leu463 were identified in 20 % (20/102) and 80 % (82/102), respectively, of the resistant isolates. Codon 463 is a polymorphicsite that does not contribute to INH resistance (van Doorn et al., 2001).In this study, Leu463 was the predominant wild-typeMTB isolate in the South China region, replacing the major Arg463wild-type found in the Western world (Cockerill et al., 1995).

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Table 2. PCR-RFLP patterns of 620-bp katG fragments for 375 MTB isolates after MspI digestion DNA fragments smaller than 30 bp are not shown.

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Fig. 2. RFLP patterns of katG amplicons after MspI digestion. Lanes: 1, 3, 4, 7, 9 and 10, pattern B; 2, pattern A; 5, pattern C; 6 and 8, pattern D; M, molecular size marker ${phi}$ X174. Details of RFLP patterns are given in Table 2.

Previous findings showed rapid detection of INH resistance inpurified MTB colonies using a real-time PCR assay (Garcia de Viedma et al., 2002)or allele-specific PCR assay (Mokrousov et al., 2002):this is the first report of direct detectionof INH resistance-associated mutations of MTB in clinical specimenswith highly specific results. Our protocol requires a simplelaboratory set-up suitable for a diagnostic microbiology serviceand the turnaround time can be shortened from 8–10 weeksto 3 days. In routine practice, respiratory specimens positivefor IS6110 or Roche PCR should be subjected to subsequent katGPCR. For katG PCR-positive samples, RFLP should be applied toidentify the Ser315Thr substitution. For katG PCR-negative samples,routine mycobacterial culture should be monitored regularlyso that MTB colonies identified can be used directly for katGPCR-RFLP. The proposed diagnostic algorithm would possibly shortenthe turnaround time for identification of INH-resistant MTBassociated with katG Ser315Thr substitution. However, this PCR-RFLPmethod only detected 51 % of all INH-resistant MTB in this study.The remaining resistant isolates possibly acquired the INH-resistantphenotype by accumulation of novel mutations in katG or knownmutations of other gene loci, such as inhA or ahpC (Basso et al., 1998;Lee et al., 2001; Mdluli et al., 1998; Sherman et al., 1996).Further understanding of INH-resistance mechanismsin MTB will facilitate the development of PCR-based protocolsfor rapid diagnosis of the pathogen in clinical specimens.

ACKNOWLEDGEMENTS

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

This work was done in partial fulfilment of the requirementsof the MPhil degree of the University of Hong Kong by E. T.-Y.L. We thank Dr P. K. Ip, Director of Public Health Laboratory,Macau, and Dr Y. K. Tam, Director of Medical Laboratory, Chestand Lung Hospital, Guangzhou, for the provision of Mycobacteriumtuberculosis isolates from patients suffering from pulmonarytuberculosis.

REFERENCES

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INTRODUCTION
METHODS
RESULTS AND DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Basso, L. A., Zheng, R., Musser, J. M., Jacobs, W. R., Jr & Blanchard, J. S. (1998). Mechanisms of isoniazid resistance in Mycobacterium tuberculosis: enzymatic characterization of enoyl reductase mutants identified in isoniazid-resistant clinical isolates. J Infect Dis 178, 769–775.[Medline]

Chan, C. M., Yuen, K. Y., Chan, K. S., Yam, W. C., Yim, K. H., Ng, W. F. & Ng, M. H. (1996). Single-tube nested PCR in the diagnosis of tuberculosis. J Clin Pathol 49, 290–294.[Abstract/Free Full Text]

Cockerill, F. R., III, Uhl, J. R., Temesgen, Z., Zhang, Y., Stockman, L., Roberts, G. D., Williams, D. L. & Kline, B. C. (1995). Rapid identification of a point mutation of the Mycobacterium tuberculosis catalase-peroxidase (katG) gene associated with isoniazid resistance. J Infect Dis 171, 240–245.[Medline]

Garcia de Viedma, D., del Sol Diaz Infantes, M., Lasala, F., Chaves, F., Alcala, L. & Bouza, E. (2002). New real-time PCR able to detect in a single tube multiple rifampin resistance mutations and high-level isoniazid resistance mutations in Mycobacterium tuberculosis. J Clin Microbiol 40, 988–995.[Abstract/Free Full Text]

Heym, B., Alzari, P. M., Honore, N. & Cole, S. T. (1995). Missense mutations in the catalase-peroxidase gene, katG, are associated with isoniazid resistance in Mycobacterium tuberculosis. Mol Microbiol 15, 235–245.[Medline]

Lee, A. S. G., Teo, A. S. M. & Wong, S. Y. (2001). Novel mutations in ndh in isoniazid-resistant Mycobacterium tuberculosis isolates. Antimicrob Agents Chemother 45, 2157–2159.[Abstract/Free Full Text]

Mdluli, K., Slayden, R. A., Zhu, Y., Ranaswamy, S., Pan, X., Mead, D., Crane, D. D., Musser, J. M. & Barry, C. E., III (1998). Inhibition of a Mycobacterium tuberculosis ß-ketocyl ACP synthase by isoniazid. Science 280, 1607–1610.[Abstract/Free Full Text]

Mokrousov, I., Otten, T., Filipenka, M., Vyazovaya, A., Chrapov, E., Limeschenko, E., Steklova, L., Vyshnevskiy, B. & Narvskaya, O. (2002). Detection of isoniazid-resistant Mycobacterium tuberculosis strains by a multiplex allele-specific PCR assay targeting katG codon 315 variation. J Clin Microbiol 40, 2509–2512.[Abstract/Free Full Text]

Musser, J. M., Kapur, V., Williams, D. L., Kreiswirth, B. N., van Soolingen, D. & van Embden, J. D. (1996). Characterization of the catalase-peroxidase gene (katG) and inhA locus in isoniazid-resistant and -susceptible strains of Mycobacterium tuberculosis by automated DNA sequencing: restricted array of mutations associated with drug resistance. J Infect Dis 173, 196–202.[Medline]

NCCLS (2000). Susceptibility Testing of Mycobacteria, Nocardia and other Aerobic Actinomycetes. Tentative Standard MT24-T2, vol. 20, 26. Villanova, PA: National Committee for Clinical Laboratory Standards.

Nolte, F. S. & Metchock, B. (1995). Mycobacterium. In Manual of Clinical Microbiology, 6th edn, pp. 400–437. Edited by P. R. Murray, E. J. Baron, M. A. Pfaller, F. C. Tenover & R. H. Yolken. Washington, DC: American Society for Microbiology.

Sherman, D. R., Mdluli, K., Hickey, M. J., Arain, T. M., Morris, S. L., Barry, C. E., III & Stover, C. K. (1996). Compensatory ahpC gene expression in isoniazid-resistant Mycobacterium tuberculosis. Science 272, 1641–1643.[Abstract]

Uhl, J. R., Sandhu, G. S., Kline, B. C. & Cockerill, F. R., III (1996). PCR-RFLP. Point mutations in catalase-peroxidase gene (KatG) of Mycobacterium tuberculosis associated with isoniazid resistance. In PCR Protocols for Emerging Infectious Diseases, pp. 144–149. Edited by D. H. Persing. Washington, DC: American Society for Microbiology.

van Doorn, H. R., Kuijper, E. J., van der Ende, A., Welten, A. G., van Soolingen, D., de Haas, P. E. & Dankert, J. (2001). The susceptibility of Mycobacterium tuberculosis to isoniazid and the Arg $<-$ Leu mutation at codon 463 of katG are not associated. J Clin Microbiol 39, 1591–1594.[Abstract/Free Full Text]

van Soolingen, D., de Haas, P. E. W., van Doorn, H. R., Kuijper, E., Rinder, H. & Borgdorff, M. W. (2000). Mutations at amino acid position 315 of the katG gene are associated with high-level resistance to isoniazid, other drug resistance, and successful transmission of Mycobacterium tuberculosis in the Netherlands. J Infect Dis 182, 1788–1790.[CrossRef][Medline]

WHO (2000). Anti-tuberculosis Drug Resistance in the World, report no. 2, Prevalence and Trends. WHO/IUATLD Global Project on Anti-tuberculosis Drug Resistance Surveillance. Geneva: World Health Organization.

Yam, W. C., Yuen, K. Y. & Seto, W. H. (1998). Direct detection of Mycobacterium tuberculosis in respiratory specimens using an automated DNA amplification assay and a single tube nested polymerase chain reaction (PCR). Clin Chem Lab Med 36, 597–599.[CrossRef][Medline]

Yuen, K. Y., Yam, W. C., Wong, L. P. & Seto, W. H. (1997). Comparison of two automated DNA amplification systems with a manual one-tube nested PCR assay for diagnosis of pulmonary tuberculosis. J Clin Microbiol 35, 1385–1389.[Abstract]

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