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医院重症监护病房环境表面 A 组轮状病毒检测。

Group A rotavirus detection on environmental surfaces in a hospital intensive care unit.

机构信息

Laboratory of Comparative and Environmental Virology, Oswaldo Cruz Institute, Oswaldo Cruz Foundation, Ministry of Health, Rio de Janeiro, Brazil.

出版信息

Am J Infect Control. 2012 Aug;40(6):544-7. doi: 10.1016/j.ajic.2011.07.017. Epub 2011 Oct 22.

DOI:10.1016/j.ajic.2011.07.017
PMID:22018841
Abstract

BACKGROUND

Environmental surfaces can play a role in the spread of pathogens, such as enteric viruses, within a hospital. This study assessed the level of contamination of group A rotavirus (RV-A) on environmental surfaces samples from an adult intensive care unit in a hospital in Rio de Janeiro, Brazil.

METHODS

A total of 504 environmental surface samples were obtained from multiple sites in the intensive care unit, including flushing buttons, telephones, and alcohol gel supports. Nested and quantitative reverse-transcriptase polymerase chain reaction (RT-PCR) were used to detect and quantify RV-A levels through partial amplification of VP6 and NSP3 genes, respectively, and the viability of the viruses detected was assessed by MA-104 cell integrated cell culture/RT-PCR.

RESULTS

RV-A was detected by nested RT-PCR in 14% of the samples (73 of 504), with viral loads ranging from 3.4 genomic copies/mL to 2.9 × 10(3) genomic copies/mL. The nucleotide sequence of the amplicons obtained from nested RT-PCR confirmed that the positive samples were RV-A. Moreover, 3 of 10 strains investigated demonstrated viability by integrated cell culture/RT-PCR.

CONCLUSION

The detection of RV-A on environmental surface samples indicates a need for improvements to hospital cleaning procedures to reduce viral contamination, and suggests, as reported previously, that RV-A can be used as a biomarker to assess contamination in hospitals.

摘要

背景

环境表面可能在医院内肠道病毒等病原体的传播中发挥作用。本研究评估了巴西里约热内卢一家医院成人重症监护病房环境表面样本中 A 组轮状病毒(RV-A)的污染水平。

方法

从重症监护病房的多个地点共采集了 504 个环境表面样本,包括冲洗按钮、电话和酒精凝胶支架。巢式和定量逆转录聚合酶链反应(RT-PCR)分别用于通过部分扩增 VP6 和 NSP3 基因来检测和定量 RV-A 水平,并且通过 MA-104 细胞整合细胞培养/RT-PCR 来评估检测到的病毒的存活能力。

结果

通过巢式 RT-PCR 在 14%的样本(504 个中的 73 个)中检测到 RV-A,病毒载量范围从 3.4 个基因组拷贝/mL 到 2.9×10(3)个基因组拷贝/mL。从巢式 RT-PCR 获得的扩增子的核苷酸序列证实阳性样本为 RV-A。此外,通过整合细胞培养/RT-PCR 检测到 10 株中的 3 株具有活力。

结论

在环境表面样本中检测到 RV-A 表明需要改进医院清洁程序以减少病毒污染,并表明如先前报道的那样,RV-A 可作为评估医院污染的生物标志物。

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