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首页> 外文期刊>Journal of Clinical Microbiology >Genotype-specific RNA probes for direct identification of wild polioviruses by blot hybridization.
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Genotype-specific RNA probes for direct identification of wild polioviruses by blot hybridization.

机译:基因型特异性RNA探针可通过印迹杂交直接鉴定野生脊髓灰质炎病毒。

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We have developed RNA probes for the direct identification of wild poliovirus isolates by blot hybridization. The probes are complementary to sequences of the first 30 to 32 codons of VP1, which evolve more extensively (approximately 1.5-fold) than the rest of VP1. To illustrate our general approach, we describe the design of probes specific to each of four major genotypes recently endemic (1981 to 1991) to the Americas: Andean type 1, Brazil type 1, Brazil type 3, and Central America-Mexico type 3. A wild isolate of each genotype was selected according to molecular and epidemiologic criteria to be representative of the principal lineages in circulation. Variable VP1 sequences of the representative isolates were amplified by the reverse transcriptase PCR and were inserted into a plasmid vector containing a T7 promoter. The in vitro transcripts, labeled with digoxigenin, served as probes. These formed stable hybrids only with RNAs of isolates of the corresponding genotypes. Hybrids were detected by a sensitive chemiluminescence assay, capable under normal diagnostic conditions of detecting specific wild poliovirus sequences in samples containing up to a 100-fold excess of Sabin vaccine strain-related sequences of the same serotype.
机译:我们已经开发了用于通过印迹杂交直接鉴定野生脊髓灰质炎病毒分离株的RNA探针。探针与VP1的前30至32个密码子的序列互补,与VP1的其余密码子相比,其进化范围更大(约1.5倍)。为了说明我们的一般方法,我们描述了针对最近流行于美洲的四种主要基因型(1981年至1991年)的探针的设计:安第斯类型1,巴西类型1,巴西类型3和中美洲-墨西哥类型3。根据分子和流行病学标准选择每种基因型的野生分离株,以代表循环中的主要谱系。通过逆转录酶PCR扩增代表性分离物的可变VP1序列,并将其插入含有T7启动子的质粒载体中。标记有洋地黄毒苷的体外转录本用作探针。这些仅与相应基因型的分离物的RNA形成稳定的杂种。通过灵敏的化学发光测定法检测杂种,该化学发光法能够在正常诊断条件下检测样品中的特定野生脊髓灰质炎病毒序列,该样品中含有多达100倍过量的相同血清型Sabin疫苗菌株相关序列。

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