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对内部聚合酶链反应用于诊断HIV感染且有肺部浸润患者的分枝杆菌病的前瞻性评估。

Prospective evaluation of in-house polymerase chain reaction for diagnosis of mycobacterial diseases in patients with HIV infection and lung infiltrates.

作者信息

Schijman A G, Losso M H, Montoto M, Saez C B, Smayevsky J, Benetucci J A

机构信息

Laboratorios BioCiencia-Grupo CentraLab, Buenos Aires, Argentina.

出版信息

Int J Tuberc Lung Dis. 2004 Jan;8(1):106-13.

Abstract

SETTING

Rapid diagnosis of tuberculosis (TB) in AIDS is critical for optimal treatment to reduce mycobacterial dissemination, HIV-1 replication and mortality. The inadequate sensitivity of Ziehl-Neelsen staining and its inability to distinguish atypical mycobacteria delays accurate diagnosis.

OBJECTIVE

To evaluate the polymerase chain reaction (PCR) for diagnosis of TB in bronchoalveolar lavage (BAL), blood and extra-pulmonary samples from patients with AIDS and pulmonary infiltrates.

DESIGN

Specimens from 103 HIV-1-infected patients were prospectively analysed using bacteriological methods and IS6110-PCR. Smear-positive samples were also tested using 16S ribosomal-DNA-PCR to identify Mycobacterium avium complex (MAC) infections. Gold standard diagnosis relied on positive cultures or treatment outcome.

RESULTS

Thirty-four patients exhibited TB, one TB and MAC and four MAC. The sensitivity of IS6110-PCR was 100% in smear-positive samples, 81.8% in smear-negative BAL, 66.7% in extra-pulmonary samples and 42.9% in blood. Its specificity was 97.1% in BAL and 100% in extra-pulmonary and blood specimens. The 16S rDNA-PCR identified M. avium from all smear-positive samples that grew MAC.

CONCLUSIONS

IS6110-PCR proved useful in evaluating episodes with probable clinical diagnosis of pulmonary or mixed TB and negative smears, whereas 16S rDNA-PCR would be helpful for prompt differential diagnosis of MAC in smear-positive specimens.

摘要

背景

对艾滋病患者的结核病(TB)进行快速诊断对于优化治疗以减少分枝杆菌播散、HIV-1复制及死亡率至关重要。萋尼氏染色敏感性不足且无法区分非典型分枝杆菌,从而延误了准确诊断。

目的

评估聚合酶链反应(PCR)用于诊断艾滋病合并肺部浸润患者支气管肺泡灌洗(BAL)液、血液及肺外样本中的结核病。

设计

前瞻性分析103例HIV-1感染患者的样本,采用细菌学方法及IS6110-PCR。涂片阳性样本还采用16S核糖体DNA-PCR检测以鉴定鸟分枝杆菌复合群(MAC)感染。金标准诊断依赖于培养阳性或治疗结果。

结果

34例患者患有结核病,1例同时患有结核病和MAC,4例患有MAC。IS6110-PCR在涂片阳性样本中的敏感性为100%,在涂片阴性的BAL液中为81.8%,在肺外样本中为66.7%,在血液中为42.9%。其在BAL液中的特异性为97.1%,在肺外及血液样本中为100%。16S rDNA-PCR从所有培养出MAC的涂片阳性样本中鉴定出鸟分枝杆菌。

结论

IS6110-PCR被证明有助于评估临床诊断可能为肺结核或混合型结核且涂片阴性的病例,而16S rDNA-PCR有助于对涂片阳性样本中的MAC进行快速鉴别诊断。

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