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首页> 外文期刊>Methods: A Companion to Methods in Enzymology >The utility of in situ detection, including RT in situ PCR, of viral nucleic acid and the co-localization of the cytokine response to the study of viral pathogenesis.
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The utility of in situ detection, including RT in situ PCR, of viral nucleic acid and the co-localization of the cytokine response to the study of viral pathogenesis.

机译:病毒核酸的原位检测(包括RT原位PCR)和对病毒发病机制研究的细胞因子应答共定位的实用性。

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摘要

This manuscript focuses on the detection of viral nucleic acids by in situ based methodologies. The optimal protocol depends on the virus. We will describe protocols for viral RNA detection by reverse transcriptase (RT) in situ PCR. We will also directly compare this method to the detection of viral RNA using standard in situ hybridization with locked nucleic acid (LNA) probes. Most DNA viruses are associated with high viral copy number and, thus, can be detected by standard in situ hybridization. Retroviral provirus is an exception as the single integrated DNA is best detected by PCR in situ hybridization. We will also describe protocols for the co-localization of viral DNA and RNA with host cytokines. Our protocol typically has the protein immunohistochemistry as the second step, with the key features being pretreatment step, antibody concentration, co-labeling analyses with a computer-based system, and co-analyzes with serial sections.
机译:该手稿着重于通过基于原位的方法对病毒核酸的检测。最佳协议取决于病毒。我们将描述通过逆转录酶(RT)原位PCR进行病毒RNA检测的方案。我们还将直接比较此方法与使用标准的原位杂交技术与锁定核酸(LNA)探针检测病毒RNA的比较。大多数DNA病毒与高病毒拷贝数相关,因此可以通过标准的原位杂交进行检测。逆转录病毒前病毒是一个例外,因为单个整合的DNA最好通过PCR原位杂交来检测。我们还将描述病毒DNA和RNA与宿主细胞因子共定位的协议。我们的方案通常将蛋白质免疫组织化学作为第二步,其关键特征是预处理步骤,抗体浓度,与基于计算机的系统进行的共同标记分析以及与连续切片的共同分析。

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