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首页> 外文期刊>Journal of viral hepatitis. >A novel primer-extension assay for the detection of a G to A mutation in the distal precore region of hepatitis B virus DNA.
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A novel primer-extension assay for the detection of a G to A mutation in the distal precore region of hepatitis B virus DNA.

机译:一种新的引物 - 延伸测定,用于检测乙型肝炎病毒DNA远端前部区域中的突变。

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摘要

The roles of genetic heterogeneity of the hepatitis B virus (HBV) precore gene in the pathogenesis of HBV infection are unclear. Various methods have been used to detect nucleotide (nt) 1896 precore mutants. We established a new primer-extension assay to facilitate the detection of these mutants. This assay is based upon the fact that there is no adenine in the distal precore region of wild-type HBV. Polymerase chain reaction (PCR)-amplified template DNA was denatured and annealed to the [gamma-32P]-labelled primer. During primer extension in the presence of DNA polymerase and dCTP, dGTP, dTTP and ddATP, the reaction terminates if there is a nucleotide A. When mixtures of different ratios of wild-type and nt 1896 precore mutants were analysed in the primer-extension assay, correlation between the percentage known amounts and the percentage measured amounts of nt 1896 precore mutants was excellent (r2=0. 9669). When the primer-extension assay and direct sequencing were compared in hepatitis B e antigen (HBeAg)-positive and -negative chronic active hepatitis B patients, the primer-extension assay detected a greater number of nt 1896 precore mutants than direct sequencing and thus most HBV infections were found to be mixed infections. In conclusion, the primer-extension assay is a reliable and sensitive method for the detection of nt 1896 precore mutants.
机译:乙型肝炎病毒(HBV)预态基因在HBV感染的发病机制中的遗传异质性的作用尚不清楚。已经使用各种方法来检测核苷酸(NT)1896的预突变体。我们建立了一种新的底漆 - 延伸测定,以促进这些突变体的检测。该测定基于野生型HBV的远端前部区域中没有腺嘌呤的事实。聚合酶链式反应(PCR) - 取出的模板DNA被变性并退火给γ-32P -Labelled底漆。在DNA聚合酶和DCTP存在下的引物延伸期间,如果存在核苷酸A,则反应终止反应。在引物 - 延伸测定中分析不同比例的野生型和NT 1896预突变体的混合物时,已知量百分比与NT 1896的测量量之间的相关性优异(R2 = 0.9669)。在乙型肝炎抗原(HBEAG) - 阳性和阴性慢性活性乙型肝炎患者中比较引物 - 延伸测定和直接测序时,引物 - 延伸测定检测到比直接测序更大数量的NT 1896突变体,因此发现HBV感染是混合感染。总之,引物 - 延伸测定是一种可靠敏感的方法,用于检测NT 1896预突变体。

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