Pilot study of a rapid and minimally instrumented sputum sample preparation method for molecular diagnosis of tuberculosis

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作者
Tanya M. Ferguson
Kris M. Weigel
Annie Lakey Becker
Delia Ontengco
Masahiro Narita
Ilya Tolstorukov
Robert Doebler
Gerard A. Cangelosi
Angelika Niemz
机构
[1] Claremont BioSolutions,Department of Environmental and Occupational Health Sciences
[2] LLC,undefined
[3] University of Washington,undefined
[4] Seattle Biomedical Research Institute,undefined
[5] University of Santo Tomas Graduate School,undefined
[6] Keck Graduate Institute of Applied Life Sciences,undefined
[7] Public Health - Seattle & King County,undefined
[8] TB Control Program,undefined
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Nucleic acid amplification testing (NAAT) enables rapid and sensitive diagnosis of tuberculosis (TB), which facilitates treatment and mitigates transmission. Nucleic acid extraction from sputum constitutes the greatest technical challenge in TB NAAT for near-patient settings. This report presents preliminary data for a semi-automated sample processing method, wherein sputum is disinfected and liquefied, followed by PureLyse® mechanical lysis and solid-phase nucleic acid extraction in a miniaturized, battery-operated bead blender. Sputum liquefaction and disinfection enabled a >104 fold reduction in viable load of cultured Mycobacterium tuberculosis (M.tb) spiked into human sputum, which mitigates biohazard concerns. Sample preparation via the PureLyse® method and a clinically validated manual method enabled positive PCR-based detection for sputum spiked with 104 and 105 colony forming units (cfu)/mL M.tb. At 103 cfu/mL sputum, four of six and two of six samples amplified using the comparator and PureLyse® method, respectively. For clinical specimens from TB cases and controls, the two methods provided 100% concordant results for samples with [inline-graphic not available: see fulltext]1 mL input volume (N = 41). The semi-automated PureLyse® method therefore performed similarly to a validated manual comparator method, but is faster, minimally instrumented and can be integrated into TB molecular diagnostic platforms designed for near-patient low-resource settings.
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