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在存在核糖体RNA的情况下,斑点杂交试验检测临床标本中轮状病毒的特异性。

Specificity of dot hybridization assay in the presence of rRNA for detection of rotaviruses in clinical specimens.

作者信息

Eiden J, Sato S, Yolken R

机构信息

Department of Pediatrics, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205.

出版信息

J Clin Microbiol. 1987 Sep;25(9):1809-11. doi: 10.1128/jcm.25.9.1809-1811.1987.

DOI:10.1128/jcm.25.9.1809-1811.1987
PMID:2821066
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC269341/
Abstract

Nucleic acid hybridization is used to identify viral genomic sequences in clinical and environmental samples. However, RNA virus genomes have been reported to hybridize to mammalian rRNA from uninfected cells under stringent conditions, and caution has therefore been advised in the use of nucleic acid probes for detection of RNA viruses. To evaluate the effect of rRNA on a diagnostic assay for an RNA virus, we tested the specificity of a rotavirus dot hybridization assay with clinical specimens which contained eucaryotic rRNA. The cDNA probe used in this assay contained sequences complementary to all 11 rotavirus genes. Preliminary experiments indicated that hybridization between rRNA and the cDNA probe occurred only with greater than 50 ng of rRNA, and this interaction was easily distinguished from the hybridization of the rotavirus probe with homologous or heterologous strains of the same rotavirus group. When 95 clinical specimens were tested, the rotavirus dot hybridization assay had a specificity of 98.8%. The predictive value of a negative test was 94.2%, although nearly all of the specimens contained rRNA and also reacted with an rRNA probe. Although the specificity of all dot hybridization assays should be individually evaluated, we conclude that our dot hybridization assay for rotaviruses is highly specific even in the presence of quantities of rRNA that may be anticipated in extracts of fecal specimens.

摘要

核酸杂交用于鉴定临床和环境样本中的病毒基因组序列。然而,据报道,在严格条件下,RNA病毒基因组会与未感染细胞的哺乳动物rRNA杂交,因此在使用核酸探针检测RNA病毒时需谨慎。为评估rRNA对RNA病毒诊断检测的影响,我们用含有真核rRNA的临床标本测试了轮状病毒斑点杂交检测的特异性。该检测中使用的cDNA探针包含与所有11个轮状病毒基因互补的序列。初步实验表明,rRNA与cDNA探针之间的杂交仅在rRNA含量超过50 ng时才会发生,并且这种相互作用很容易与轮状病毒探针与同一轮状病毒组的同源或异源毒株的杂交区分开来。当对95份临床标本进行检测时,轮状病毒斑点杂交检测的特异性为98.8%。阴性检测的预测值为94.2%,尽管几乎所有标本都含有rRNA并且也与rRNA探针发生反应。尽管所有斑点杂交检测的特异性都应单独评估,但我们得出结论,即使存在粪便标本提取物中可能预期的大量rRNA,我们的轮状病毒斑点杂交检测仍具有高度特异性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3a23/269341/a5e01ceaa22c/jcm00093-0252-b.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3a23/269341/36b4a8f1ec50/jcm00093-0252-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3a23/269341/a5e01ceaa22c/jcm00093-0252-b.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3a23/269341/36b4a8f1ec50/jcm00093-0252-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3a23/269341/a5e01ceaa22c/jcm00093-0252-b.jpg

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本文引用的文献

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A dot hybridisation assay for detection of rotavirus.一种用于检测轮状病毒的斑点杂交试验。
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RNA virus genomes hybridize to cellular rRNAs and to each other.RNA病毒基因组与细胞rRNA以及它们彼此之间发生杂交。
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Poliovirus genome RNA hybridizes specifically to higher eukaryotic rRNAs.脊髓灰质炎病毒基因组RNA与高等真核生物的核糖体RNA特异性杂交。
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Detection of rotaviruses by nucleic acid hybridization with cloned DNA of simian rotavirus SA11 genes.用猿猴轮状病毒SA11基因的克隆DNA进行核酸杂交检测轮状病毒
J Infect Dis. 1985 Aug;152(2):293-300. doi: 10.1093/infdis/152.2.293.