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唾液标本采集、处理及储存方案对通过聚合酶链反应检测丙型肝炎病毒(HCV)RNA的影响。

The effect of saliva specimen collection, handling and storage protocols on hepatitis C virus (HCV) RNA detection by PCR.

作者信息

Roy K M, Bagg J, McCarron B

机构信息

Infection Research Group, University of Glasgow Dental School, Scotland.

出版信息

Oral Dis. 1999 Apr;5(2):123-7. doi: 10.1111/j.1601-0825.1999.tb00076.x.

Abstract

OBJECTIVES

Commercial assays can now be adapted to detect salivary anti-hepatitis C virus (HCV) antibodies, increasing the potential of saliva as a non-invasive diagnostic specimen suited to surveillance and epidemiological studies. However, current diagnostic algorithms involve confirmation of HCV infection by RT-PCR. Manipulation and storage conditions of serum can influence the stability of viral RNA. This study examined whether varying specimen collection, handling and storage protocols also affected subsequent HCV RNA detection by RT-PCR applied to saliva specimens.

METHODS

Whole unstimulated saliva, together with saliva samples collected in two commercially available devices (Salivette and Omnisal) were obtained from 50 HCV seropositive intravenous drug users. The specimens were subjected to a number of handling and storage conditions, including heat treatment and prolonged storage, then examined for HCV RNA by RT-PCR using primers derived from the 5' non-coding region (5'NCR).

RESULTS

HCV RNA was detected in saliva samples from 25 (50%) of the patients. No single collection device or handling procedure identified all the subjects with HCV RNA positive saliva though whole saliva yielded the greatest number of positive results.

CONCLUSIONS

Collection and processing of saliva specimens for RT-PCR analysis is complex. At present, detection of salivary HCV RNA by PCR is not sufficiently sensitive for use as a diagnostic tool in epidemiological studies.

摘要

目的

目前商业检测方法可用于检测唾液中的抗丙型肝炎病毒(HCV)抗体,这增加了唾液作为适合监测和流行病学研究的非侵入性诊断标本的潜力。然而,当前的诊断算法涉及通过逆转录聚合酶链反应(RT-PCR)来确认HCV感染。血清的处理和储存条件会影响病毒RNA的稳定性。本研究探讨了不同的标本采集、处理和储存方案是否也会影响随后应用于唾液标本的RT-PCR检测HCV RNA的结果。

方法

从50名HCV血清学阳性的静脉吸毒者中获取未刺激的全唾液,以及用两种市售装置(Salivette和Omnisal)采集的唾液样本。对标本进行多种处理和储存条件,包括热处理和长时间储存,然后使用源自5'非编码区(5'NCR)的引物通过RT-PCR检测HCV RNA。

结果

在25名(50%)患者的唾液样本中检测到HCV RNA。尽管全唾液产生的阳性结果数量最多,但没有一种单一的采集装置或处理程序能识别出所有HCV RNA阳性唾液的受试者。

结论

用于RT-PCR分析的唾液标本的采集和处理很复杂。目前,通过PCR检测唾液中的HCV RNA在流行病学研究中用作诊断工具时不够灵敏。

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