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首页> 外文期刊>Journal of Virological Methods >Specific detection of small ruminant lentiviral nucleic acid sequences located in the proviral long terminal repeat and leader-gag regions using real-time polymerase chain reaction.
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Specific detection of small ruminant lentiviral nucleic acid sequences located in the proviral long terminal repeat and leader-gag regions using real-time polymerase chain reaction.

机译:使用实时聚合酶链反应特异性检测位于前病毒长末端重复序列和前导序列区域中的小反刍动物慢病毒核酸序列。

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摘要

Real-time polymerase chain reaction (RT-PCR) detection of proviral nucleic acid sequences of small ruminant lentiviruses (SRLV) in blood samples was developed and evaluated. Priming oligonucleotides were designed on the highly conserved 5' untranslated leader-gag region while those on the long terminal repeat (LTR) assay were derived from literature. DNA was extracted from the buffycoat interlayer of centrifuged blood samples. Real-time PCR was performed by means of LightCycler technology (Roche Applied Science) using melting temperature analysis (SYBR Green I) for detection. Results were compared with those of serology using samples from Dutch sheep and goat flocks with known SRLV statuses, with sequential samples from a natural transmission experiment and samples from different regions in Norway, France, Spain and Italy. Real-time PCR testing, especially the application of oligonucleotides for priming the leader-gag region appeared promising in detecting SRLV specific proviral DNA in blood samples from both sheep and goats.
机译:实时聚合酶链反应(RT-PCR)检测血液样本中的小反刍动物慢病毒(SRLV)的前病毒核酸序列已开发并评估。在高度保守的5'非翻译前导-gag区域上设计了引物寡核苷酸,而在长末端重复(LTR)测定中的引物寡核苷酸则来自文献。从离心血样的血沉棕黄层夹层中提取DNA。实时PCR通过LightCycler技术(罗氏应用科学公司(Roche Applied Science))使用熔融温度分析(SYBR Green I)进行检测。将结果与血清学的结果进行了比较,使用的样本来自具有已知SRLV状态的荷兰绵羊和山羊群,具有自然传播实验的顺序样本,以及来自挪威,法国,西班牙和意大利不同地区的样本。实时PCR测试,特别是寡核苷酸用于引发前导gag区域的应用,在检测绵羊和山羊血液样本中的SRRV特异性前病毒DNA方面似乎很有希望。

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