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Validation of a single-step, single-tube reverse transcription loop-mediated isothermal amplification assay for rapid detection of SARS-CoV-2 RNA.
Lee, Jean Y H; Best, Nickala; McAuley, Julie; Porter, Jessica L; Seemann, Torsten; Schultz, Mark B; Sait, Michelle; Orlando, Nicole; Mercoulia, Karolina; Ballard, Susan A; Druce, Julian; Tran, Thomas; Catton, Mike G; Pryor, Melinda J; Cui, Huanhuan L; Luttick, Angela; McDonald, Sean; Greenhalgh, Arran; Kwong, Jason C; Sherry, Norelle L; Graham, Maryza; Hoang, Tuyet; Herisse, Marion; Pidot, Sacha J; Williamson, Deborah A; Howden, Benjamin P; Monk, Ian R; Stinear, Timothy P.
Afiliação
  • Lee JYH; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Best N; Department of Infectious Diseases, Monash Health, Clayton, Victoria, Australia.
  • McAuley J; GenWorks Pty Ltd, Thebarton, South Australia, Australia.
  • Porter JL; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Seemann T; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Schultz MB; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Sait M; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Orlando N; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Mercoulia K; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Ballard SA; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Druce J; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Tran T; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Catton MG; Victorian Infectious Diseases Reference Laboratory, Melbourne Health at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Pryor MJ; Victorian Infectious Diseases Reference Laboratory, Melbourne Health at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Cui HL; Victorian Infectious Diseases Reference Laboratory, Melbourne Health at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Luttick A; 360Biolabs, Melbourne, Victoria, Australia.
  • McDonald S; 360Biolabs, Melbourne, Victoria, Australia.
  • Greenhalgh A; 360Biolabs, Melbourne, Victoria, Australia.
  • Kwong JC; GenWorks Pty Ltd, Thebarton, South Australia, Australia.
  • Sherry NL; GenWorks Pty Ltd, Thebarton, South Australia, Australia.
  • Graham M; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Hoang T; Department of Infectious Diseases, Austin Health, Heidelberg, Victoria, Australia.
  • Herisse M; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Pidot SJ; Department of Infectious Diseases, Austin Health, Heidelberg, Victoria, Australia.
  • Williamson DA; Department of Microbiology, Monash Health, Clayton, Victoria, Australia.
  • Howden BP; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Monk IR; Microbiological Diagnostic Unit Public Health Laboratory, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
  • Stinear TP; Department of Microbiology and Immunology, University of Melbourne at the Peter Doherty Institute for Infection and Immunity, Melbourne, Victoria, Australia.
J Med Microbiol ; 69(9): 1169-1178, 2020 Sep.
Article em En | MEDLINE | ID: mdl-32755529
ABSTRACT
Introduction. The SARS-CoV-2 pandemic of 2020 has resulted in unparalleled requirements for RNA extraction kits and enzymes required for virus detection, leading to global shortages. This has necessitated the exploration of alternative diagnostic options to alleviate supply chain issues.Aim. To establish and validate a reverse transcription loop-mediated isothermal amplification (RT- LAMP) assay for the detection of SARS-CoV-2 from nasopharyngeal swabs.Methodology. We used a commercial RT-LAMP mastermix from OptiGene in combination with a primer set designed to detect the CDC N1 region of the SARS-CoV-2 nucleocapsid (N) gene. A single-tube, single-step fluorescence assay was implemented whereby 1 µl of universal transport medium (UTM) directly from a nasopharyngeal swab could be used as template, bypassing the requirement for RNA purification. Amplification and detection could be conducted in any thermocycler capable of holding 65 °C for 30 min and measure fluorescence in the FAM channel at 1 min intervals.Results. Assay evaluation by assessment of 157 clinical specimens previously screened by E-gene RT-qPCR revealed assay sensitivity and specificity of 87 and 100%, respectively. Results were fast, with an average time-to-positive (Tp) for 93 clinical samples of 14 min (sd±7 min). Using dilutions of SARS-CoV-2 virus spiked into UTM, we also evaluated assay performance against FDA guidelines for implementation of emergency-use diagnostics and established a limit-of-detection of 54 Tissue Culture Infectious Dose 50 per ml (TCID50 ml-1), with satisfactory assay sensitivity and specificity. A comparison of 20 clinical specimens between four laboratories showed excellent interlaboratory concordance; performing equally well on three different, commonly used thermocyclers, pointing to the robustness of the assay.Conclusion. With a simplified workflow, The N1 gene Single Tube Optigene LAMP assay (N1-STOP-LAMP) is a powerful, scalable option for specific and rapid detection of SARS-CoV-2 and an additional resource in the diagnostic armamentarium against COVID-19.
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Texto completo: 1 Coleções: 01-internacional Base de dados: MEDLINE Assunto principal: Pneumonia Viral / Infecções por Coronavirus / Técnicas de Amplificação de Ácido Nucleico Tipo de estudo: Diagnostic_studies / Guideline Limite: Humans Idioma: En Revista: J Med Microbiol Ano de publicação: 2020 Tipo de documento: Article País de afiliação: Austrália
Texto completo
Imprimir
XML
PubMed Links
Buscar no Google

Texto completo: 1 Coleções: 01-internacional Base de dados: MEDLINE Assunto principal: Pneumonia Viral / Infecções por Coronavirus / Técnicas de Amplificação de Ácido Nucleico Tipo de estudo: Diagnostic_studies / Guideline Limite: Humans Idioma: En Revista: J Med Microbiol Ano de publicação: 2020 Tipo de documento: Article País de afiliação: Austrália