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枯草芽孢杆菌噬菌体SPP1 DNA的结构与其转染活性的关系

Structure of Bacillus subtilis bacteriophage SPP1 DNA in relation to its transfection activity.

作者信息

Humphreys G O, Trautner T A

出版信息

J Virol. 1981 Feb;37(2):574-9. doi: 10.1128/JVI.37.2.574-579.1981.

Abstract

The availability of a detailed restriction map of SPP1 DNA allowed defined manipulations of such molecules. These were performed to investigate structural requirements for SPP1 transfection. (i) The transfection activity of SPP1 DNA was destroyed by degradation with restriction enzymes. Biological activity could be regenerated when transfection was performed with a combination of two different restriction endonuclease digests, provided that such digests generated widely overlapping DNA fragments. (ii) Unique DNA molecules were constructed from the natural population of circularly permuted SPP1 DNA molecules by using genetic engineering techniques. Such molecules had the same specific transfection activity as did the circularly permuted SPP1 DNA. These results are discussed in the context of current models of DNA processing in transfection.

摘要

SPP1 DNA详细限制图谱的可得性使得对这类分子进行特定操作成为可能。进行这些操作是为了研究SPP1转染的结构要求。(i) SPP1 DNA的转染活性通过用限制酶降解而被破坏。当用两种不同的限制内切酶消化产物组合进行转染时,生物活性可以再生,前提是这些消化产物产生广泛重叠的DNA片段。(ii) 通过使用基因工程技术,从环状排列的SPP1 DNA分子的天然群体构建独特的DNA分子。这类分子具有与环状排列的SPP1 DNA相同的特定转染活性。在当前转染中DNA处理模型的背景下讨论了这些结果。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/147f/171044/bd8fd53e4a34/jvirol00002-0053-a.jpg

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Transfection in B. subtilis.枯草芽孢杆菌中的转染
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