Combined Species Identification, Genotyping, and Drug Resistance Detection of Mycobacterium tuberculosis Cultures by MLPA on a Bead-Based Array

Bergval, Indra; Sengstake, Sarah; Brankova, Nadia; Levterova, Victoria; Abadia, Edgar; Tadumaze, Nino; Bablishvili, Nino; Akhalaia, Maka; Tuin, Kiki; Schuitema, A. R. J.; Panaiotov, Stefan; Bachiyska, Elizabeta; Kantardjiev, Todor; Zwaan, Rina de; Schürch, Anita C.; Soolingen, Dick van; Hoog, Anja van t.; Cobelens, Frank; Aspindzelashvili, Rusudan; Sola, Christophe; Klatser, P. R.; Anthony, Richard

doi:10.1371/journal.pone.0043240

Cited by 50 publications

(79 citation statements)

References 74 publications

(107 reference statements)

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“…Results are in progress (Gomgnimbou et al, unpublished data). Because methods developed with the Luminex 200 or MagPix system are highly flexible, local improvements are possible (33). This flexibility will also allow us to adapt a panel of new drug resistance targets, including different markers for different regions.…”

Section: Discussionmentioning

confidence: 99%

Tuberculosis-Spoligo-Rifampin-Isoniazid Typing: an All-in-One Assay Technique for Surveillance and Control of Multidrug-Resistant Tuberculosis on Luminex Devices

et al. 2013

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e As a follow-up of the "spoligoriftyping" development, we present here an extension of this technique which includes the detection of isoniazid resistance-associated mutations in a new 59-plex assay, i.e., tuberculosis-spoligo-rifampin-isoniazid typing (TB-SPRINT), running on microbead-based multiplexed systems. This assay improves the synergy between clinical microbiology and epidemiology by providing (i) mutation-based prediction of drug resistance profiles for patient treatment and (ii) genotyping data for tuberculosis (TB) surveillance. This third-generation microbead-based high-throughput assay for TB runs on the Luminex 200 system and on the recently launched MagPix system (Luminex, Austin, TX). Spoligotyping patterns obtained by the TB-SPRINT method were 100% (n ‫؍‬ 85 isolates; 3,655/3,655 spoligotype data points) concordant with those obtained by microbead-based and membrane-based spoligotyping. Genetic drug susceptibility typing provided by the TB-SPRINT method was 100% concordant with resistance locus sequencing (n ‫؍‬ 162 for rpoB gene sequencing and n ‫؍‬ 76 for katG and inhA sequencing). Considering phenotypic drug susceptibility testing (DST) as the reference method, the sensitivity and specificity of TB-SPRINT regarding Mycobacterium tuberculosis complex (n ‫؍‬ 162 isolates) rifampin resistance were both 100%, and those for isoniazid resistance were 90.4% (95% confidence interval, 85 to 95%) and 100%, respectively. Used routinely in national TB reference and specialized laboratories, the TB-SPRINT assay should simultaneously improve personalized medicine and epidemiological surveillance of multidrug-resistant (MDR) TB. This assay is expected to play an emerging role in public health in countries with heavy burdens of MDR TB and/or HIV/TB coinfection. Application of this assay directly to biological samples, as well as development for extensively drug-resistant (XDR) TB detection by inclusion of second-line antituberculosis drug-associated mutations, is under development. With bioinformatical methods and data mining to reduce the number of targets to the most informative ones, locally adapted formats of this technique can easily be developed everywhere.

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Section: Discussionmentioning

confidence: 99%

Tuberculosis-Spoligo-Rifampin-Isoniazid Typing: an All-in-One Assay Technique for Surveillance and Control of Multidrug-Resistant Tuberculosis on Luminex Devices

et al. 2013

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“…Therefore, this study suggests that providing PTBTHs with relevant health education and encouraging a willingness to be supervised can help improve their sputum disposal. This might be explained by the fact that patients who have received health education are better able to manage TBrelated waste on their own (25). More relevant health education must be developed so that PTBTHs are better able to manage TB-related waste on their own.…”

Section: Discussionmentioning

confidence: 99%

A cross-sectional study of sputum handling by and supervision of patients with pulmonary tuberculosis treated at home in China

Мэй¹

2012

Biosci Trends

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“…However, the number of known genes and mutations conferring resistance to first-and second-line drugs greatly exceeds the multiplexing capacity of these platforms, which may limit their clinical efficacy in the treatment and control of multidrug-resistant or extensively drug-resistant TB. Planar and suspension microarrays are well suited to address the multiple-gene, multiple-mutation challenge of diagnosing drug-resistant TB (4)(5)(6)(7)(8)(9)(10)(11)(12), but clinical adoption of microarray technology is hampered by poor reproducibility (13)(14)(15), complex workflows, and/or extensive user subjectivity and involvement in image and data analysis (16). In order to translate microarrays into efficacious TB diagnostics at the point of need, it is therefore necessary to simplify user interaction with the technology while retaining the ability to detect multiple genes and multiple mutations in a timely manner.…”

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Simplified Microarray System for Simultaneously Detecting Rifampin, Isoniazid, Ethambutol, and Streptomycin Resistance Markers in Mycobacterium tuberculosis

et al. 2014

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bWe developed a simplified microarray test for detecting and identifying mutations in rpoB, katG, inhA, embB, and rpsL and compared the analytical performance of the test to that of phenotypic drug susceptibility testing (DST). The analytical sensitivity was estimated to be at least 110 genome copies per amplification reaction. The microarray test correctly detected 95.2% of mutations for which there was a sequence-specific probe on the microarray and 100% of 96 wild-type sequences. M ycobacterium tuberculosis infects one-third of the world's population, with approximately nine million new cases and two million deaths attributable to the disease each year (1). Early case detection and rapid treatment are considered the most effective control strategies to reduce M. tuberculosis transmission (2), especially in cases involving multidrug-resistant (MDR) or extensively drug-resistant (XDR) M. tuberculosis. Culture-based methods remain the gold standard for diagnosing drug-resistant M. tuberculosis but can take several weeks or months to complete. Thus, nucleic acid-based drug susceptibility tests are becoming increasingly attractive as diagnostic tools in order to initiate individualized, patient-appropriate treatment in a timely manner.Technologies such as Cepheid's GeneXpert and Hain line probe assays reduce the time to diagnosis for many tuberculosis (TB) patients, provide a rapid read-out indicating resistance to rifampin or selected mutations conferring resistance to other firstor second-line drugs, and illustrate the potential to deploy molecular tests closer to the point of need (3). However, the number of known genes and mutations conferring resistance to first-and second-line drugs greatly exceeds the multiplexing capacity of these platforms, which may limit their clinical efficacy in the treatment and control of multidrug-resistant or extensively drug-resistant TB. Planar and suspension microarrays are well suited to address the multiple-gene, multiple-mutation challenge of diagnosing drug-resistant TB (4-12), but clinical adoption of microarray technology is hampered by poor reproducibility (13-15), complex workflows, and/or extensive user subjectivity and involvement in image and data analysis (16). In order to translate microarrays into efficacious TB diagnostics at the point of need, it is therefore necessary to simplify user interaction with the technology while retaining the ability to detect multiple genes and multiple mutations in a timely manner. The objectives of this study were to develop a gel element microarray test for MDR TB at a level of coverage surpassing what is currently available with WHO-endorsed molecular platforms, estimate the analytical specificity of the test on M. tuberculosis isolates of known genotype and phenotype, and compare the performance of the test to that of conventional drug susceptibility testing as a precursor to integrating the method into an entirely closed-amplicon consumable (17, 18) and sample-to-answer system. MATERIALS AND METHODSIsolates and positive control...

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Combined Species Identification, Genotyping, and Drug Resistance Detection of Mycobacterium tuberculosis Cultures by MLPA on a Bead-Based Array

Cited by 50 publications

References 74 publications

Tuberculosis-Spoligo-Rifampin-Isoniazid Typing: an All-in-One Assay Technique for Surveillance and Control of Multidrug-Resistant Tuberculosis on Luminex Devices

Tuberculosis-Spoligo-Rifampin-Isoniazid Typing: an All-in-One Assay Technique for Surveillance and Control of Multidrug-Resistant Tuberculosis on Luminex Devices

A cross-sectional study of sputum handling by and supervision of patients with pulmonary tuberculosis treated at home in China

Simplified Microarray System for Simultaneously Detecting Rifampin, Isoniazid, Ethambutol, and Streptomycin Resistance Markers in Mycobacterium tuberculosis

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