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含有5-巯基取代嘧啶的多核苷酸:对病毒DNA聚合酶的抑制作用及其生物学意义。

Polynucleotides containing 5-mercapto-substituted pyrimidines: inhibition of viral DNA polymerases and the biological implication.

作者信息

Chandra P, Ebener U, Bardos T J, Chakrabarti P, Ho Y K, Mikulski A J, Zsindely A

出版信息

Ann N Y Acad Sci. 1975 Aug 8;255:532-43. doi: 10.1111/j.1749-6632.1975.tb29256.x.

Abstract

Partially thiolated polycytidylic acids MPC I-III, containing 1.7%, 3.5% and 8.6% 5-mercaptocytidylate units, respectively) inhibited the DNA polymerase of Friend leukemia virus (FLV) in the endogenic reaction as well as in the presence of poly(A)-(dT)14 or poly[d(a-T)] templates; the inhibitory activities were directly related to the percent of thiolation. Various partially thiolated RNA and DNA isolates from Ehrlich ascites cells (containing one 5-mercaptopyrimidine nucleotide/50-100 nucleotide units) also inhibited the DNA polymerases of FLV in the endogenic reaction, and also in the presence of the synthetic templates. The thiolated DNA was the most active, but the thiolated tRNA also showed substantial inhibitory effects, while the thiolated ribosomal RNA was less effective. In a bacterial DNA polymerase (E. coli-K12, using denatured DNA as template), MPC I-III showed no activity. By contrast, MPC III and several partially thiolated nucleic acid isolates significantly inhibited a regenerating rat liver DNA polymerase (I) system; among those tested, the thiolated DNA from Ehrlich ascites cells showed the highest activity. Kinetic analysis of the inhibitory action of this thiolated DNA in the rat liver enzyme system, using as template the corresponding unmodified DNA, demonstrated that the thiolated DNA acts as a competitive inhibitor of the template, with a Ki/Km ratio of 0.5.

摘要

部分硫醇化的聚胞苷酸MPC I - III(分别含有1.7%、3.5%和8.6%的5 - 巯基胞苷酸单元)在内源反应中以及在存在聚(A) - (dT)14或聚[d(A - T)]模板的情况下,均可抑制弗氏白血病病毒(FLV)的DNA聚合酶;抑制活性与硫醇化百分比直接相关。从艾氏腹水癌细胞中分离得到的各种部分硫醇化的RNA和DNA(含有1个5 - 巯基嘧啶核苷酸/50 - 100个核苷酸单元)在内源反应中以及在存在合成模板的情况下,也能抑制FLV的DNA聚合酶。硫醇化的DNA活性最强,但硫醇化的tRNA也显示出显著的抑制作用,而硫醇化的核糖体RNA效果较差。在一种细菌DNA聚合酶(大肠杆菌 - K12,以变性DNA为模板)中,MPC I - III无活性。相比之下,MPC III和几种部分硫醇化的核酸分离物显著抑制再生大鼠肝DNA聚合酶(I)系统;在测试的样品中,来自艾氏腹水癌细胞的硫醇化DNA活性最高。以相应的未修饰DNA为模板,对该硫醇化DNA在大鼠肝酶系统中的抑制作用进行动力学分析表明,硫醇化DNA作为模板的竞争性抑制剂,Ki/Km比值为0.5。

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