Evaluation of in-house PCR for diagnosis of smear-negative pulmonary tuberculosis in Kampala, Uganda

Lydia Nakiyingi,Ponsiano Ocama,Harriet Mayanja-Kizza,Fred A Katabazi,Moses L Joloba,Joseph B Sempa,David P Kateete,William Worodria,Achilles Katamba,Laurence Huang,Benon B Asiimwe

doi:10.1186/1756-0500-5-487

Abstract

BackgroundNucleic acid amplification tests (NAATs) have offered hope for rapid diagnosis of tuberculosis (TB). However, their efficiency with smear-negative samples has not been widely studied in low income settings. Here, we evaluated in-house PCR assay for diagnosis of smear-negative TB using Lowenstein-Jensen (LJ) culture as the baseline test. Two hundred and five pulmonary TB (PTB) suspects with smear-negative sputum samples, admitted on a short stay emergency ward at Mulago Hospital in Kampala, Uganda, were enrolled. Two smear-negative sputum samples were obtained from each PTB suspect and processed simultaneously for identification of MTBC using in-house PCR and LJ culture.ResultsSeventy two PTB suspects (35%, 72/205) were LJ culture positive while 128 (62.4%, 128/205) were PCR-positive. The sensitivity and specificity of in-house PCR for diagnosis of smear-negative PTB were 75% (95% CI 62.6-85.0) and 35.9% (95% CI 27.2-45.3), respectively. The positive and negative predictive values were 39% (95% CI 30.4-48.2) and 72.4% (95% CI 59.1-83.3), respectively, while the positive and negative likelihood ratios were 1.17 (95% CI 0.96-1.42) and 0.70 (95% CI 0.43-1.14), respectively. One hundred and seventeen LJ culture-negative suspects (75 PCR-positive and 42 PCR-negative) were enrolled for follow-up at 2 months. Of the PCR-positive suspects, 45 (60%, 45/75) were still alive, of whom 29 (64.4%, 29/45) returned for the follow-up visit; 15 (20%, 15/75) suspects died while another 15 (20%, 15/75) were lost to follow-up. Of the 42 PCR-negative suspects, 22 (52.4%, 22/42) were still alive, of whom 16 (72.7%, 16/22) returned for follow-up; 11 (26.2%, 11/42) died while nine (21.4%, 9/42) were lost to follow-up. Overall, more PCR-positive suspects were diagnosed with PTB during follow-up visits but the difference was not statistically significant (27.6%, 8/29 vs. 25%, 4/16, p = 0.9239). Furthermore, mortality was higher for the PCR-negative suspects but the difference was also not statistically significant (26.2% vs. 20% p = 0.7094).ConclusionIn-house PCR correlates poorly with LJ culture for diagnosis of smear-negative PTB. Therefore, in-house PCR may not be adopted as an alternative to LJ culture.

Highlights

Nucleic acid amplification tests (NAATs) have offered hope for rapid diagnosis of tuberculosis (TB)
Accurate diagnosis is crucial for efficient management of TB patients [3]; TB diagnosis remains a challenge in resource limited settings (RLS) where the disease is complicated by Human immunodeficiency virus (HIV) co-infection
Using LJ culture as the base-line test, this study evaluated in-house Polymerase chain reaction (PCR) for rapid diagnosis of smear-negative

Summary

Introduction

Nucleic acid amplification tests (NAATs) have offered hope for rapid diagnosis of tuberculosis (TB). Their efficiency with smear-negative samples has not been widely studied in low income settings. Two hundred and five pulmonary TB (PTB) suspects with smear-negative sputum samples, admitted on a short stay emergency ward at Mulago Hospital in Kampala, Uganda, were enrolled. Two smear-negative sputum samples were obtained from each PTB suspect and processed simultaneously for identification of MTBC using in-house PCR and LJ culture. Accurate diagnosis is crucial for efficient management of TB patients [3]; TB diagnosis remains a challenge in resource limited settings (RLS) where the disease is complicated by HIV co-infection. Solid cultures are used as confirmatory tests but are expensive, lengthy (up to 8 weeks) and not widely available in RLS [11]

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Results

Discussion

Conclusion