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互补链特异性2型腺病毒DNA与转化细胞的病毒DNA序列的重新结合。

Reassociation of complementary strand-specific adenovirus type 2 DNA with viral DNA sequences of transformed cells.

作者信息

Johansson K, Pettersson U, Philipson L, Tibbetts C

出版信息

J Virol. 1977 Jul;23(1):29-35. doi: 10.1128/JVI.23.1.29-35.1977.

Abstract

Complementary strand-specific adenovirus DNA, either full length or from restriction enzyme cleavage fragments, was used to estimate the fractional representation and abundance of viral sequences in two adenovirus type 2 (Ad2)-transformed rat cell lines, A2F19 and A2T2C4. The reassociation method introduced is based on the linear relationship, after exhaustive hybridization, between the inverted fraction of hybrid DNA and the molar ratio of probe to cellular DNA in the reaction mixture. The amount of viral DNA in A2F19 cells represents 12 to 14% of the viral genome at a level of around seven copies per diploid cell equivalent. For the cell line A2T2C4, the pattern of integrated viral DNA sequences is more complex. With full-length Ad2 DNA strands as a probe, about 56% of the probe was represented in cellular DNA. When each of the four BamHI fragment strands of Ad2 DNA was used as a probe, the fraction of the viral DNA present also amounted to around 56% with one to five copies from different regions of the viral genome. The results demonstrate the advantage of using strand-specific viral DNA as a probe in reassociation analysis with denatured cell DNA. The method should be useful in any system in which complementary strand separation of viral DNA sequences can be achieved.

摘要

互补链特异性腺病毒DNA,无论是全长的还是限制性内切酶切割片段,都被用于估计两种2型腺病毒(Ad2)转化的大鼠细胞系A2F19和A2T2C4中病毒序列的分数表示和丰度。所介绍的重退火方法基于在彻底杂交后,杂交DNA的反向分数与反应混合物中探针与细胞DNA的摩尔比之间的线性关系。A2F19细胞中病毒DNA的量在每个二倍体细胞当量约有七个拷贝的水平下占病毒基因组的12%至14%。对于细胞系A2T2C4,整合的病毒DNA序列模式更为复杂。以全长Ad2 DNA链作为探针时,约56%的探针存在于细胞DNA中。当使用Ad2 DNA的四个BamHI片段链中的每一个作为探针时,存在的病毒DNA分数也约为56%,来自病毒基因组不同区域的拷贝数为一至五个。结果证明了在与变性细胞DNA的重退火分析中使用链特异性病毒DNA作为探针的优势。该方法在任何能够实现病毒DNA序列互补链分离的系统中都应是有用的。

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Transcription map for adenovirus type 12 DNA.12型腺病毒DNA的转录图谱。
J Virol. 1978 Oct;28(1):227-39. doi: 10.1128/JVI.28.1.227-239.1978.

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