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体外合成的腺病毒信使核糖核酸的特性

Properties of adenovirus messenger ribonucleic Acid synthesized in vitro.

作者信息

Warren R J

机构信息

Department of Microbiology, Saint Louis University School of Medicine, Saint Louis, Missouri 63110.

出版信息

J Virol. 1969 Sep;4(3):231-9. doi: 10.1128/JVI.4.3.231-239.1969.

Abstract

Adenovirus deoxyribonucleic acid (DNA) was used as template for the in vitro synthesis of viral-specific ribonucleic acid (RNA). When the kinetics of the reaction were compared by using native and heat-denatured DNA templates, the latter synthesized RNA at a slower rate. The fate of the DNA after acting as template and physical characteritstics of the RNA product were studied. The DNA template, according to its sedimentation rate, was not significantly degraded by the Micrococcus lysodeicticus RNA polymerase. The products of the RNA polymerase reaction had the following properties. (i) Hybridization experiments revealed a high degree of complementarity (50 to 70%) for its homologous DNA. (ii) A very low complementarity (6 to 7%) was found for its heterologous DNA. (iii) The sedimentation rate of the synthetic RNA in a sucrose gradient was 5 to 10S when native DNA was used as the template. When heat-denatured DNA was used, the resulting RNA product, free of the template, sedimented at a rate of 3 to 16S. A rapidly sedimenting (>30S) DNA-RNA complex resulted when denatured DNA was the template. The DNA moiety of the complex was sensitive to 125 mug of deoxyribonuclease per ml. The RNA of the complex, however, was fully refractory to 50 mug of ribonuclease per ml. When the adenovirus DNA was sonically treated and then used as template, the RNA product sedimented at 3 to 9S. The heat-denatured sonically treated DNA template yielded a DNA-RNA complex that also sedimented at an unusually fast rate (>18S).

摘要

腺病毒脱氧核糖核酸(DNA)被用作病毒特异性核糖核酸(RNA)体外合成的模板。当使用天然和热变性的DNA模板比较反应动力学时,后者合成RNA的速度较慢。研究了DNA作为模板后的命运以及RNA产物的物理特性。根据其沉降速率,溶壁微球菌RNA聚合酶并未使DNA模板发生显著降解。RNA聚合酶反应的产物具有以下特性。(i)杂交实验表明,其与同源DNA具有高度互补性(50%至70%)。(ii)发现其与异源DNA的互补性非常低(6%至7%)。当使用天然DNA作为模板时,合成RNA在蔗糖梯度中的沉降速率为5至10S。当使用热变性DNA时,得到的不含模板的RNA产物沉降速率为3至16S。当以变性DNA为模板时,会形成一种快速沉降(>30S)的DNA-RNA复合物。该复合物的DNA部分对每毫升125微克的脱氧核糖核酸酶敏感。然而,该复合物的RNA对每毫升50微克的核糖核酸酶完全耐受。当对腺病毒DNA进行超声处理后用作模板时,RNA产物沉降在3至9S。经超声处理的热变性DNA模板产生的DNA-RNA复合物沉降速率也异常快(>18S)。

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