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心肌分化的生化方面。脱氧核糖核酸合成以及细胞核和细胞质中的脱氧核糖核酸聚合酶活性。

Biochemical aspects of cardiac muscle differentiation. Deoxyribonucleic acid synthesis and nuclear and cytoplasmic deoxyribonucleic acid polymerase activity.

作者信息

Claycomb W C

出版信息

J Biol Chem. 1975 May 10;250(9):3229-35.

PMID:235544
Abstract

DNA synthesis and DNA polymerase activity have been measured in terminally differentiating cardiac muscle of the rat. Incorporation of [3H]thymidine into DNA essentially ceases by the 17th day of postnatal development. Cardiac muscle of neonatal rats contains at least two molecular species of DNA polymerase: a 3.5 S DNA polymerase that can be extracted from nuclei with 0.2 m potassium phosphate and a 6 to 8 S soluble cytoplasmic DNA polymerase. The nuclear DNA polymerase in crude extracts has a pH optimum of 9.0 and is more active with native DNA than with denatured DNA as the primer-template. The cytoplasmic DNA polymerase in crude extracts has a pH optimum of 7.5 and is more active with denatured DNA. The activity of the 6 to 8 S cytoplasmic DNA polymerase decreases 80-fold from day 1 to day 17 after birth, which correlates temporally with the reduced rate of DNA synthesis. The activity of the 3.5 S nuclear DNA polymerase remains relatively constant throughout postnatal development. Mixing experiments (assay of neonatal enzyme extracts with adult enzyme extracts) gave additive results, suggesting that the decline in 6 to 8 S DNA polymerase activity apparently is not due to the presence of absence of soluble activators or inhibitors at different times during development. These studies may provide a system which can be used to investigate the control of DNA synthesis and cellular proliferation during the terminal stages of cardiac muscle differentiation.

摘要

已对大鼠终末分化心肌中的DNA合成及DNA聚合酶活性进行了测定。出生后第17天,[3H]胸苷掺入DNA的过程基本停止。新生大鼠心肌中至少含有两种DNA聚合酶分子类型:一种3.5S的DNA聚合酶,可用0.2m磷酸钾从细胞核中提取;另一种6至8S的可溶性细胞质DNA聚合酶。粗提物中的核DNA聚合酶最适pH为9.0,以天然DNA作为引物模板时比变性DNA更具活性。粗提物中的细胞质DNA聚合酶最适pH为7.5,对变性DNA更具活性。出生后第1天到第17天,6至8S细胞质DNA聚合酶的活性下降了80倍,这在时间上与DNA合成速率降低相关。3.5S核DNA聚合酶的活性在出生后发育过程中保持相对恒定。混合实验(用成年酶提取物检测新生酶提取物)得到了相加结果,表明6至8S DNA聚合酶活性的下降显然不是由于发育过程中不同时间存在或不存在可溶性激活剂或抑制剂所致。这些研究可能提供一个可用于研究心肌分化末期DNA合成及细胞增殖调控的系统。

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