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作 者:秦鄂德[1] 杨佩英[1] 于曼[1] 徐品芳 司炳银[1] 阎国珍[1]
机构地区:[1]军事医学科学院微生物流行病研究所
出 处:《中华实验和临床病毒学杂志》1995年第1期56-58,共3页Chinese Journal of Experimental and Clinical Virology
基 金:国家自然科学基金
摘 要:利用特异抗体吸附的登革病毒,经含TritonX-100的裂解缓冲液处理,释放出基因组RNA,在同一管中进行逆转录聚合酶链扩增反应。采用这种方法利用保守性引物可检测出登革1型、2型和4型病毒参考株及我国海南岛登革2型病毒分离株的基因组序列,扩增产物约为550bp。用32P-标记的分子克隆的登革2型病毒基因探针进行Southern印迹杂交分析证实了扩增产物的特异性。利用这种技术还可从感染后24h的C6/36细胞培养上清中检测出登革病毒基因组序列。而明显的细胞病变作用(CPE)在感染后96h才可观察到。Dengue virions associated by their specific antibodies were treated with a buffer solution containing Triton X-100 to release viral RNAs, and then a reverse transcriptase-polymerase chain reaction (RT-PCR) of viral RNA was carried out in a single reaction vessel, By using this method, the sequences of classical of dengue type, 1,2,and 4 virused and dengue type 2 virus isolated from human sear in Hainan Island were detected by using consensus primers for NS1 genes of all 4 dengue serotypes in the RTPCR. The amplified product was about 550bp in length. the specificity was verified by performing the Southern blot hybridization of the ammplified product ot 32P-labeled cDNA probes specific for the dengue type 2 virus. The sequence of dengue-2 viral RNA could also be detected from the infected culture fluid of C6/36 cells 24hrs after virus inocalation. The clear cytopathic effect (CPF) could be observed with naked eye 96hrs after inoculation.
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