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机构地区:[1]汕头大学医学院微生物学教研室,中山医科大学微生物学教研室
出 处:《中华微生物学和免疫学杂志》1994年第6期426-429,共4页Chinese Journal of Microbiology and Immunology
基 金:CMB基金;卫生部医学重点科技项目资金
摘 要:用地高辛配基(Digoxigenin,Dig)、生物素(Biotin,Bio)和辣根过氧化物酶(Horseradishperoxidase,HRP)分别标记登革病毒2型(Denguevirustype2,Dv2)的cDNA,制备三种非同位素标记探针,与感染DV2的C6/36细胞上清中病毒核酸做斑点杂交。结果表明:三种标记探针均只与DV2-RNA呈强阳性杂交反应,显示DV2型特异性;Dig-探针最灵敏,可检出DV2-RNA的最小量为0.1pg,其次为HRP-探针(可检出0.3pg)和Bio-探针(可检出1~3pg)。用PCR技术制备探针并同步标记比其他方法简便、快速,只需少量模板数小时内可获得足够量的标记探针,是值得推广使用的标记探针制备方法。igoxigenin,biotin and horseradish peroxidase(HRP) were used to prepare nonisotope labelled DV2-cDNAproberespectively. These probes were used to detect DV-RNA extracted from DV2 infected supernatant of C6/36cell. The results of cDNA : RNA dot blot hybridization showed that these nonisotope labelled probes were highlyspecific. The digoxigenin labelled probe was the most sensitive among the three kinds fo probes and the tiny amount(0.1pof DV2-RNA was detectable.The amount of 0.3pg and 1-3pg DV2-RNA can be detected byHRP and bi-otin labelled probes,respectively.Our results suggest that a large amount of labelled probes can be obtaint using a small quantity of templatewith labelling method.The preparation of labelled probes with PCR may have great value in producing labelledprobes.The modified NaI method for extracting DV-RNA was more convenient and much faster.
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