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9-(2-羟乙氧甲基)鸟嘌呤三磷酸对纯化的人及单纯疱疹病毒诱导的DNA聚合酶的抑制作用。对引物-模板功能的影响。

Inhibition of purified human and herpes simplex virus-induced DNA polymerases by 9-(2-hydroxyethoxymethyl)guanine triphosphate. Effects on primer-template function.

作者信息

Derse D, Cheng Y C, Furman P A, St Clair M H, Elion G B

出版信息

J Biol Chem. 1981 Nov 25;256(22):11447-51.

PMID:6271750
Abstract

The inhibition of highly purified herpes simplex virus (HSV)-induced and host cell DNA polymerases by the triphosphate form of 9-(2-hydroxyethoxymethyl)guanine (acyclovir; acycloguanosine) was examined. Acyclovir triphosphate (acyclo-GTP) competitively inhibited the incorporation of dGMP into DNA, catalyzed by HSV DNA polymerase; apparent Km and Ki values of dGTP and acyclo-GTP were 0.15 microM and 0.003 microM, respectively. HeLa DNA polymerase alpha was also competitively inhibited; Km and Ki values of dGTP and acyclo-GTP were 1.2 microM and 0.18 microM, respectively. In contrast, HeLa DNA polymerase beta was insensitive to the analogue. The "limited" DNA synthesis observed when dGTP was omitted from HSV or alpha DNA polymerase reactions was inhibited by acyclo-GTP in a concentration-dependent manner. Prior incubation of activated DNA, acyclo-GTP, and DNA polymerase (alpha or HSV resulted in a marked decrease in the utilization of the primer-template in subsequent DNA polymerase reactions. This decreased ability of preincubated primer-templates to support DNA synthesis was dependent on acyclo-GTP, enzyme concentration, and the time of prior incubation. Acyclo-GMP-terminated DNA was found to inhibit HSV DNA polymerase-catalyzed DNA synthesis. Kinetic experiments with variable concentrations of activated DNA and fixed concentrations of acyclo-GMP-terminated DNA revealed a noncompetitive inhibition of HSV-1 DNA polymerase. The apparent Km of 3'-hydroxyl termini was 1.1 X 10(-7) M, the Kii and Kis of acyclo-GMP termini in activated DNA were 8.8 X 10(-8) M and 2.1 X 10(-9) M, respectively. Finally, 14C-labeled acyclo-GMP residues incorporated into activated DNA by HSV-1 DNA polymerase could not be excised by the polymerase-associated 3',5'-exonuclease activity.

摘要

研究了9-(2-羟乙氧甲基)鸟嘌呤(阿昔洛韦;无环鸟苷)的三磷酸形式对高度纯化的单纯疱疹病毒(HSV)诱导的和宿主细胞DNA聚合酶的抑制作用。阿昔洛韦三磷酸(无环-GTP)竞争性抑制HSV DNA聚合酶催化的dGMP掺入DNA;dGTP和无环-GTP的表观Km和Ki值分别为0.15μM和0.003μM。HeLa DNA聚合酶α也受到竞争性抑制;dGTP和无环-GTP的Km和Ki值分别为1.2μM和0.18μM。相比之下,HeLa DNA聚合酶β对该类似物不敏感。当从HSV或α DNA聚合酶反应中省略dGTP时观察到的“有限”DNA合成被无环-GTP以浓度依赖的方式抑制。预先孵育活化的DNA、无环-GTP和DNA聚合酶(α或HSV)导致随后的DNA聚合酶反应中引物模板的利用率显著降低。预孵育的引物模板支持DNA合成的能力下降取决于无环-GTP、酶浓度和预先孵育的时间。发现无环-GMP末端的DNA抑制HSV DNA聚合酶催化的DNA合成。用可变浓度的活化DNA和固定浓度的无环-GMP末端DNA进行的动力学实验显示对HSV-1 DNA聚合酶有非竞争性抑制作用。3'-羟基末端的表观Km为1.1×10(-7)M,活化DNA中无环-GMP末端的Kii和Kis分别为8.8×10(-8)M和2.1×10(-9)M。最后,HSV-1 DNA聚合酶掺入活化DNA中的14C标记的无环-GMP残基不能被与聚合酶相关的3',5'-外切核酸酶活性切除。

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