Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test

There is a growing awareness that molecular diagnostics for detect-to-treat applications will soon need a highly multiplexed mutation detection and identification capability. In this study, we converted an open-amplicon microarray hybridization test for multidrug-resistant (MDR) Mycobacterium tuberc...

Descripción completa

Detalles Bibliográficos
Autores principales: Linger, Yvonne, Knickerbocker, Christopher, Sipes, David, Golova, Julia, Franke, Molly, Calderon, Roger, Lecca, Leonid, Thakore, Nitu, Holmberg, Rebecca, Qu, Peter, Kukhtin, Alexander, Murray, Megan B., Cooney, Christopher G., Chandler, Darrell P.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Society for Microbiology 2018
Materias:
Mycobacteriology and Aerobic Actinomycetes
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5824040/
https://www.ncbi.nlm.nih.gov/pubmed/29305543
http://dx.doi.org/10.1128/JCM.01652-17
_version_ 1783301981123641344
author Linger, Yvonne
Knickerbocker, Christopher
Sipes, David
Golova, Julia
Franke, Molly
Calderon, Roger
Lecca, Leonid
Thakore, Nitu
Holmberg, Rebecca
Qu, Peter
Kukhtin, Alexander
Murray, Megan B.
Cooney, Christopher G.
Chandler, Darrell P.
author_facet Linger, Yvonne
Knickerbocker, Christopher
Sipes, David
Golova, Julia
Franke, Molly
Calderon, Roger
Lecca, Leonid
Thakore, Nitu
Holmberg, Rebecca
Qu, Peter
Kukhtin, Alexander
Murray, Megan B.
Cooney, Christopher G.
Chandler, Darrell P.
author_sort Linger, Yvonne
collection PubMed
description There is a growing awareness that molecular diagnostics for detect-to-treat applications will soon need a highly multiplexed mutation detection and identification capability. In this study, we converted an open-amplicon microarray hybridization test for multidrug-resistant (MDR) Mycobacterium tuberculosis into an entirely closed-amplicon consumable (an amplification microarray) and evaluated its performance with matched sputum and sediment extracts. Reproducible genotyping (the limit of detection) was achieved with ∼25 M. tuberculosis genomes (100 fg of M. tuberculosis DNA) per reaction; the estimated shelf life of the test was at least 18 months when it was stored at 4°C. The test detected M. tuberculosis in 99.1% of sputum extracts and 100% of sediment extracts and showed 100% concordance with the results of real-time PCR. The levels of concordance between M. tuberculosis and resistance-associated gene detection were 99.1% and 98.4% for sputum and sediment extracts, respectively. Genotyping results were 100% concordant between sputum and sediment extracts. Relative to the results of culture-based drug susceptibility testing, the test was 97.1% specific and 75.0% sensitive for the detection of rifampin resistance in both sputum and sediment extracts. The specificity for the detection of isoniazid (INH) resistance was 98.4% and 96.8% for sputum and sediment extracts, respectively, and the sensitivity for the detection of INH resistance was 63.6%. The amplification microarray reported the correct genotype for all discordant phenotype/genotype results. On the basis of these data, primary sputum may be considered a preferred specimen for the test. The amplification microarray design, shelf life, and analytical performance metrics are well aligned with consensus product profiles for next-generation drug-resistant M. tuberculosis diagnostics and represent a significant ease-of-use advantage over other hybridization-based tests for diagnosing MDR tuberculosis.
format Online
Article
Text
id pubmed-5824040
institution National Center for Biotechnology Information
language English
publishDate 2018
publisher American Society for Microbiology
record_format MEDLINE/PubMed
spelling pubmed-58240402018-03-05 Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test Linger, Yvonne Knickerbocker, Christopher Sipes, David Golova, Julia Franke, Molly Calderon, Roger Lecca, Leonid Thakore, Nitu Holmberg, Rebecca Qu, Peter Kukhtin, Alexander Murray, Megan B. Cooney, Christopher G. Chandler, Darrell P. J Clin Microbiol Mycobacteriology and Aerobic Actinomycetes There is a growing awareness that molecular diagnostics for detect-to-treat applications will soon need a highly multiplexed mutation detection and identification capability. In this study, we converted an open-amplicon microarray hybridization test for multidrug-resistant (MDR) Mycobacterium tuberculosis into an entirely closed-amplicon consumable (an amplification microarray) and evaluated its performance with matched sputum and sediment extracts. Reproducible genotyping (the limit of detection) was achieved with ∼25 M. tuberculosis genomes (100 fg of M. tuberculosis DNA) per reaction; the estimated shelf life of the test was at least 18 months when it was stored at 4°C. The test detected M. tuberculosis in 99.1% of sputum extracts and 100% of sediment extracts and showed 100% concordance with the results of real-time PCR. The levels of concordance between M. tuberculosis and resistance-associated gene detection were 99.1% and 98.4% for sputum and sediment extracts, respectively. Genotyping results were 100% concordant between sputum and sediment extracts. Relative to the results of culture-based drug susceptibility testing, the test was 97.1% specific and 75.0% sensitive for the detection of rifampin resistance in both sputum and sediment extracts. The specificity for the detection of isoniazid (INH) resistance was 98.4% and 96.8% for sputum and sediment extracts, respectively, and the sensitivity for the detection of INH resistance was 63.6%. The amplification microarray reported the correct genotype for all discordant phenotype/genotype results. On the basis of these data, primary sputum may be considered a preferred specimen for the test. The amplification microarray design, shelf life, and analytical performance metrics are well aligned with consensus product profiles for next-generation drug-resistant M. tuberculosis diagnostics and represent a significant ease-of-use advantage over other hybridization-based tests for diagnosing MDR tuberculosis. American Society for Microbiology 2018-02-22 /pmc/articles/PMC5824040/ /pubmed/29305543 http://dx.doi.org/10.1128/JCM.01652-17 Text en Copyright © 2018 Linger et al. https://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Mycobacteriology and Aerobic Actinomycetes
Linger, Yvonne
Knickerbocker, Christopher
Sipes, David
Golova, Julia
Franke, Molly
Calderon, Roger
Lecca, Leonid
Thakore, Nitu
Holmberg, Rebecca
Qu, Peter
Kukhtin, Alexander
Murray, Megan B.
Cooney, Christopher G.
Chandler, Darrell P.
Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test
title Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test
title_full Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test
title_fullStr Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test
title_full_unstemmed Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test
title_short Genotyping Multidrug-Resistant Mycobacterium tuberculosis from Primary Sputum and Decontaminated Sediment with an Integrated Microfluidic Amplification Microarray Test
title_sort genotyping multidrug-resistant mycobacterium tuberculosis from primary sputum and decontaminated sediment with an integrated microfluidic amplification microarray test
topic Mycobacteriology and Aerobic Actinomycetes
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5824040/
https://www.ncbi.nlm.nih.gov/pubmed/29305543
http://dx.doi.org/10.1128/JCM.01652-17
work_keys_str_mv AT lingeryvonne genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT knickerbockerchristopher genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT sipesdavid genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT golovajulia genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT frankemolly genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT calderonroger genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT leccaleonid genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT thakorenitu genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT holmbergrebecca genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT qupeter genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT kukhtinalexander genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT murraymeganb genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT cooneychristopherg genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest
AT chandlerdarrellp genotypingmultidrugresistantmycobacteriumtuberculosisfromprimarysputumanddecontaminatedsedimentwithanintegratedmicrofluidicamplificationmicroarraytest

Ejemplares similares