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一种基于聚合酶链反应的方法用于检测实验性感染仓鼠体内的华支睾吸虫的开发。

Development of a PCR-based method for the detection of Opisthorchis viverrini in experimentally infected hamsters.

作者信息

Wongratanacheewin S, Pumidonming W, Sermswan R W, Maleewong W

机构信息

Department of Microbiology, Faculty of Medicine, Khon Kaen University, Thailand.

出版信息

Parasitology. 2001 Feb;122(Pt 2):175-80. doi: 10.1017/s0031182001007235.

Abstract

Opisthorchis viverrini infection is an endemic disease that causes a serious public health problem in southeast Asia, especially in northeast Thailand. We have developed a PCR method using a pair of primers named OV-6F/OV-6R for detecting O. viverrini eggs in stool samples and compared it with Stoll's egg-count method. The primers were designed based on the pOV-A6 specific DNA probe sequence which gave a 330 base pair product. The PCR method can detect a single egg in artificially inoculated faeces or as little as 2 x 10(-17) ng of O. viverrini genomic DNA. The method gave 100% sensitivity in all hamster groups except in animals exposed to the lowest intensity of infection (1 metacercaria/hamster). In the first month of infection, the PCR method was more sensitive than using the egg-count method in all infected groups especially in the light infections. The PCR method was also successfully used in monitoring a therapeutic study. Since the PCR method showed no cross-reaction with Heterophyid flukes, it can be useful for specific identification of O. viverrini eggs in stool samples without the risk of false positives. It also has great potential for application in clinical epidemiological studies.

摘要

华支睾吸虫感染是一种地方病,在东南亚尤其是泰国东北部造成严重的公共卫生问题。我们开发了一种PCR方法,使用一对名为OV-6F/OV-6R的引物来检测粪便样本中的华支睾吸虫卵,并将其与斯托尔虫卵计数法进行比较。引物是根据产生330个碱基对产物的pOV-A6特异性DNA探针序列设计的。该PCR方法可以检测人工接种粪便中的单个虫卵,或低至2×10(-17)纳克的华支睾吸虫基因组DNA。除了感染强度最低(1个囊蚴/仓鼠)的动物组外,该方法在所有仓鼠组中均具有100%的灵敏度。在感染的第一个月,PCR方法在所有感染组中比虫卵计数法更灵敏,尤其是在轻度感染组。该PCR方法也成功用于监测一项治疗研究。由于该PCR方法与异形吸虫无交叉反应,因此可用于粪便样本中华支睾吸虫卵的特异性鉴定,而无假阳性风险。它在临床流行病学研究中也有很大的应用潜力。

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