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Detection of cytomegalovirus in the meconium of infected newborns by polymerase chain reaction.

机译:通过聚合酶链反应检测感染的新生儿胎粪中的巨细胞病毒。

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摘要

OBJECTIVE: Congenital cytomegalovirus (CMV) infection is a leading cause of hearing loss and mental retardation throughout the world. Detection of the CMV DNA by polymerase chain reaction (PCR) offers a sensitive, rapid, and specific means of identification. Meconium, the stool formed in utero, may be an ideal specimen for CMV detection. The objective of this study was to develop a PCR-based methodology for the detection of CMV in the meconium of neonates. METHODS: Meconium was collected from 10 newborn infants (seven with positive viral cultures and three uninfected infants born to CMV-seropositive mothers). For each, DNA was isolated from meconium by organic extraction and attachment to a DNA-binding matrix, and PCR was performed using amplimers specific for the major intermediate early (MIE) and late antigenic (LA) regions of CMV. RESULTS: Gel electrophoresis demonstrated an anticipated PCR product of 250 base pairs (bp) corresponding to the MIE region of CMV in all infected and positive control meconium samples. Furthermore, a single band of 150 bp corresponding to the LA region of CMV was also amplified in several of the infected infants. Conversely, no amplification of these antigenic regions was noted in either uninfected infants born to CMV-seropositive mothers or negative controls. CONCLUSIONS: CMV is present within the meconium of infected neonates and is readily detectable by PCR.
机译:目的:先天性巨细胞病毒(CMV)感染是全世界听力丧失和智力低下的主要原因。通过聚合酶链反应(PCR)对CMV DNA的检测提供了灵敏,快速和特异性的鉴定手段。胎粪是子宫内形成的粪便,可能是检测CMV的理想标本。这项研究的目的是开发一种基于PCR的方法来检测新生儿胎粪中的CMV。方法:从10例新生儿中收集了胎粪(其中7例病毒培养阳性,而3例CMV血清阳性母亲出生的未感染婴儿)。对于每种化合物,都通过有机萃取从胎粪中分离出DNA并将其附着在DNA结合基质上,并使用对CMV的主要中间早期(MIE)和晚期抗原性(LA)区具有特异性的扩增子进行PCR。结果:凝胶电泳显示,在所有感染和阳性对照胎粪样本中,预期的250个碱基对(bp)的PCR产物对应于CMV的MIE区。此外,在一些被感染的婴儿中,对应于CMV的LA区域的150bp的单条带也被扩增。相反,在CMV血清阳性母亲出生的未感染婴儿或阴性对照中,未观察到这些抗原区域的扩增。结论:CMV存在于被感染的新生儿的胎粪中,并易于通过PCR检测。

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