首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Detection of hepatitis B virus DNA in serum by polymerase chain reaction amplification and microtiter sandwich hybridization.
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Detection of hepatitis B virus DNA in serum by polymerase chain reaction amplification and microtiter sandwich hybridization.

机译:通过聚合酶链反应扩增和微量滴定夹心杂交检测血清中的乙型肝炎病毒DNA。

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摘要

We have developed a microtiter sandwich hybridization assay for the detection of polymerase chain reaction (PCR)-amplified hepatitis B virus (HBV) sequences. This assay utilizes an enzyme-linked immunosorbent assay-like format in which cloned DNA containing a sequence complementary to half of one PCR product strand is immobilized in microtiter wells. A biotin-labeled DNA sequence complementary to the other portion of the same PCR product strand is used as the probe. The DNAs from 69 hepatitis B surface antigen-positive serum samples and 16 antigen-negative control samples were amplified by the PCR procedure, and the product was detected by Southern and sandwich hybridization. Both detection procedures were capable of detecting as few as five copies of HBV DNA. Compared with Southern hybridization, the sandwich hybridization assay exhibited a sensitivity of 100% and a specificity of 95% for the detection of amplified HBV sequences. Unlike Southern hybridization, however, the sandwich hybridization assay employs a nonradioactive probe and allows easy handling of large numbers of samples. DNA was detected in 74% of the antigen-positive samples. All of the antigen-negative samples (healthy blood donors) were negative for HBV DNA by both procedures.
机译:我们已经开发了一种微量滴定夹心杂交测定法,用于检测聚合酶链反应(PCR)扩增的乙型肝炎病毒(HBV)序列。该测定利用酶联免疫吸附测定样形式,其中将含有与一条PCR产物链的一半互补的序列的克隆DNA固定在微量滴定孔中。与相同PCR产物链的其他部分互补的生物素标记的DNA序列用作探针。通过PCR程序从69个乙型肝炎表面抗原阳性血清样本和16个抗原阴性对照样本中扩增DNA,并通过Southern和三明治杂交检测产物。两种检测方法均能够检测到多达五个拷贝的HBV DNA。与Southern杂交相比,三明治杂交检测对扩增的HBV序列的检测灵敏度为100%,特异性为95%。但是,与Southern杂交不同,夹心杂交测定采用非放射性探针,可轻松处理大量样品。在74%的抗原阳性样本中检测到DNA。通过这两种方法,所有抗原阴性样品(健康献血者)的HBV DNA均为阴性。

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