Performance of a Stool-Based Quantitative PCR Assay for the Diagnosis of Tuberculosis in Adolescents and Adults: A Multinational, Prospective Diagnostic Accuracy Study

Authors

Alexander Kay
Anca Vasiliu
Lucia Carratala-Castro
Bariki Mtafya
Jose Euberto Mendez Reyes
Nontobeko Maphalala
Shilzia Munguambe
Durbbin Mulengwa
Tara Ness
Belen Saavedra
Jason Bacha
Gugu Maphalala
Rojelio Mejia
Godwin Mtetwa
Sozinho Acacio
Patricia Manjate
Edson Mambuque
Nosisa Shiba
Nokwanda Kota
Mangaliso Ziyane
Nyanda Elias Ntinginya
Christoph Lange
H Lester Kirchner
Andrew R DiNardo
Alberto L Garcia-Basteiro
Anna Maria Mandalakas
Stool4TB Global Partnership

Publication Date

5-1-2024

Journal

Lancet Microbe

DOI

10.1016/S2666-5247(23)00391-9

PMID

38461830

PMCID

PMC11142891

PubMedCentral® Posted Date

6-1-2024

PubMedCentral® Full Text Version

Author MSS

Published Open-Access

yes

Keywords

Humans, Adolescent, Feces, Adult, Prospective Studies, Mycobacterium tuberculosis, Female, Male, Sensitivity and Specificity, Real-Time Polymerase Chain Reaction, Young Adult, Tuberculosis, Sputum, Middle Aged, Child, Tanzania, DNA, Bacterial, Mozambique

Abstract

BACKGROUND: Despite increasing availability of rapid molecular tests for the diagnosis of tuberculosis in high-burden settings, many people with tuberculosis are undiagnosed. Reliance on sputum as the primary specimen for tuberculosis diagnostics contributes to this diagnostic gap. We evaluated the diagnostic accuracy and additive yield of a novel stool quantitative PCR (qPCR) assay for the diagnosis of tuberculosis in three countries in Africa with high tuberculosis burdens.

METHODS: We undertook a prospective diagnostic accuracy study in Eswatini, Mozambique, and Tanzania from Sept 21, 2020, to Feb 2, 2023, to compare the diagnostic accuracy for tuberculosis of a novel stool qPCR test with the current diagnostic standard for Mycobacterium tuberculosis DNA detection from sputum and stool, Xpert-MTB/RIF Ultra (Xpert Ultra). Sputum, stool, and urine samples were provided by a cohort of participants, aged 10 years or older, diagnosed with tuberculosis. Participants with tuberculosis (cases) were enrolled within 72 h of treatment initiation for tuberculosis diagnosed clinically or following laboratory confirmation. Participants without tuberculosis (controls) consisted of household contacts of the cases who did not develop tuberculosis during a 6-month follow-up. The performance was compared with a robust composite microbiological reference standard (CMRS).

FINDINGS: The cohort of adolescents and adults (n=408) included 268 participants with confirmed or clinical tuberculosis (cases), 147 (55%) of whom were living with HIV, and 140 participants (controls) without tuberculosis. The sensitivity of the novel stool qPCR was 93·7% (95% CI 87·4-97·4) compared with participants with detectable growth on M tuberculosis culture, and 88·1% (81·3-93·0) compared with sputum Xpert Ultra. The stool qPCR had an equivalent sensitivity as sputum Xpert Ultra (94·8%, 89·1-98·1) compared with culture. Compared with the CMRS, the sensitivity of the stool qPCR was higher than the current standard for tuberculosis diagnostics on stool, Xpert Ultra (80·4%, 73·4-86·2 vs 73·5%, 66·0-80·1; p=0·025 on paired comparison). The qPCR also identified 17-21% additional tuberculosis cases compared to sputum Xpert Ultra or sputum culture. In controls without tuberculosis, the specificity of the stool qPCR was 96·9% (92·2-99·1).

INTERPRETATION: In this study, a novel qPCR for the diagnosis of tuberculosis from stool specimens had a higher accuracy in adolescents and adults than the current diagnostic PCR gold standard on stool, Xpert-MTB/RIF Ultra, and equivalent sensitivity to Xpert-MTB/RIF Ultra on sputum.

FUNDING: National Institutes of Health (NIH) Allergy and Infectious Diseases, and NIH Fogarty International Center.

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