原位PCR:方案和应用。

G J Nuovo
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引用次数: 55

摘要

许多研究小组现在已经发表了基于pcr扩增DNA和cDNA原位检测的数据。与标准的原位杂交或PCR一样,影响原位PCR结果的变量包括固定物的类型和固定时间、蛋白酶消化以及扩增溶液和寡聚探针混合物的组成。原位PCR领域的新研究者应该首先尝试将报告分子直接掺入石蜡包埋的组织切片中。虽然在这些条件下会产生非特异性DNA合成,但人们可以建立在细胞核内合成DNA的信心,并认识到蛋白酶消化时间对RT原位PCR成功的重要性。这是一个有争议的说法,pcr扩增的DNA和cDNA的原位检测将对许多不同的领域产生非常强烈的影响,如肿瘤发生,胚胎学,RNA转运和病毒性疾病的检测,因为它已经对我们对HIV-1感染发病机制的理解产生了很大的影响。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
In situ PCR: protocols and applications.

Many groups have now published data based on the in situ detection of PCR-amplified DNA and cDNA. As with standard in situ hybridization or PCR, variables that can affect in situ PCR results include type of fixative and time of fixation, protease digestion, and the composition of the amplifying solution and oligoprobe cocktail. Investigators new to the field of in situ PCR should first try direct incorporation of the reporter molecule into paraffin-embedded tissue sections. Although nonspecific DNA synthesis is generated under these conditions, one can develop the confidence of synthesizing DNA inside the nucleus and appreciate the importance of protease digestion time to successful RT in situ PCR. It is an arguable statement that the in situ detection of PCR-amplified DNA and cDNA will have a very strong impact on many diverse fields, such as oncogenesis, embryology, RNA trafficking, and detection of viral diseases, as it already has on our understanding of the pathogenesis of HIV-1 infection.

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