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单管巢式聚合酶链反应在结核病诊断中的应用

Single-tube nested PCR in the diagnosis of tuberculosis.

作者信息

Chan C M, Yuen K Y, Chan K S, Yam W C, Yim K H, Ng W F, Ng M H

机构信息

Department of Microbiology, University of Hong Kong.

出版信息

J Clin Pathol. 1996 Apr;49(4):290-4. doi: 10.1136/jcp.49.4.290.

DOI:10.1136/jcp.49.4.290
PMID:8655703
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC500452/
Abstract

AIMS

To evaluate the usefulness of a single-tube nested polymerase chain reaction (PCR) assay in the diagnosis of tuberculosis in 1497 pulmonary and 536 extrapulmonary specimens.

METHODS

A single-tube nested PCR, utilising two sets of primers with different melting temperatures (88 degrees C for external primers; 70 degrees C for internal primers) to augment sensitivity and specificity without increasing the risk of amplicon contamination, was evaluated. Specimens were initially tested for the repetitive IS6110 sequences and if negative, retested for the universal 38 kilodalton sequence and for inhibitors. dUTP/Uracil-N-glycosylase and Instagene treatment were used to minimise contamination and the effect of inhibitors, respectively.

RESULTS

Using culture as the gold standard, the overall sensitivity of the assay was 89% for pulmonary and 42% for extrapulmonary specimens. Sensitivity varied greatly with respect to sample type (92% for follow up specimens from a chest hospital and 70% for non-follow up specimens from a general hospital). The smear positivity rates were 15% for extrapulmonary specimens, and 69% and 45%, respectively, for follow up and non-follow up specimens from pulmonary sites. Specificity was 99.7%. Inhibitors were present more frequently in extrapulmonary than in pulmonary specimens (13.4% v 2.7%).

CONCLUSION

Despite the high sensitivity of the PCR assay for the diagnosis of tuberculosis in pulmonary specimens, it was less effective in the extrapulmonary samples. This is probably because of the lower bacterial load in extrapulmonary specimens, the presence of more inhibitors adversely affecting the PCR assay and the higher volume of specimens used for culture.

摘要

目的

评估单管巢式聚合酶链反应(PCR)检测法在1497份肺部标本和536份肺外标本结核病诊断中的实用性。

方法

评估了一种单管巢式PCR,它使用两组具有不同解链温度的引物(外部引物为88℃;内部引物为70℃)来提高敏感性和特异性,同时不增加扩增子污染风险。标本首先检测重复性IS6110序列,若为阴性,则重新检测通用的38千道尔顿序列及抑制剂。分别使用dUTP/尿嘧啶-N-糖基化酶和InstaGene处理来尽量减少污染和抑制剂的影响。

结果

以培养作为金标准,该检测法对肺部标本的总体敏感性为89%,对肺外标本为42%。敏感性因样本类型差异很大(胸科医院的随访标本为92%,综合医院的非随访标本为70%)。肺外标本的涂片阳性率为15%,肺部标本的随访和非随访标本的涂片阳性率分别为69%和45%。特异性为99.7%。肺外标本中抑制剂的出现频率高于肺部标本(13.4%对2.7%)。

结论

尽管PCR检测法对肺部标本结核病诊断具有高敏感性,但对肺外标本的效果较差。这可能是因为肺外标本中的细菌载量较低、存在更多对PCR检测有不利影响的抑制剂以及用于培养的标本量较大。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e32c/500452/706c388873d9/jclinpath00241-0022-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e32c/500452/706c388873d9/jclinpath00241-0022-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e32c/500452/706c388873d9/jclinpath00241-0022-a.jpg

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