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促有丝分裂激素诱导的细胞内信息:表皮生长因子诱导的DNA复制激活剂的测定及部分特性分析

Mitogenic hormone-induced intracellular message: assay and partial characterization of an activator of DNA replication induced by epidermal growth factor.

作者信息

Das M

出版信息

Proc Natl Acad Sci U S A. 1980 Jan;77(1):112-6. doi: 10.1073/pnas.77.1.112.

Abstract

This paper explores the pathway from nuclear quiescence to mitogenesis. It describes an in vitro assay for an activator of DNA replication induced by epidermal growth factor (EGF) in responsive cells. Cytoplasmic extracts from EGF-treated 3T3 cells were found to contain substances that can stimulate DNA synthesis in isolated nuclei from spleen cells of adult frogs. Extracts from untreated resting 3T3 cells lack this activity, and EGF itself is incapable of stimulating DNA synthesis in these cell-free systems. The extract-induced stimulation of incorporation of [3H]dTTP into nuclear DNA is ATP dependent and requires the presence of the four deoxyribonucleoside triphosphates, suggesting the occurrence of replication rather than repair synthesis. This cell-free assay has been used to obtain some initial insights into the mechanism of induction and biochemical characterization of the intermediate in EGF action. Half-maximal induction of the active intracellular substance is achieved at about 0.08 nM EGF, a concentration that correlates well with the concentration required for half-maximal mitogenesis. Studies on the biochemical characteristics of this active substance strongly suggest that the activity is associated with a protein. The activity is nondialyzable and sensitive to trypsin and heat. Sucrose gradient centrifugation of the extract revealed three peaks of activity with molecular weights of 46,000, 110,000, and 270,000 (sedimentation coefficients: 3.7 S, 6.6 S, and 12 S, respectively). These results indicate that receptor-EGF interaction at the cell surface leads to the intracellular generation of protein that are capable of stimulating quiescent nuclei into activity.

摘要

本文探讨了从核静止到有丝分裂发生的途径。它描述了一种在响应细胞中由表皮生长因子(EGF)诱导的DNA复制激活剂的体外测定方法。发现经EGF处理的3T3细胞的细胞质提取物含有能刺激成年青蛙脾细胞分离核中DNA合成的物质。未经处理的静止3T3细胞的提取物缺乏这种活性,并且EGF本身在这些无细胞系统中不能刺激DNA合成。提取物诱导的[3H]dTTP掺入核DNA的刺激是ATP依赖性的,并且需要四种脱氧核糖核苷三磷酸的存在,这表明发生的是复制而不是修复合成。这种无细胞测定方法已被用于初步了解EGF作用中间体的诱导机制和生化特性。活性细胞内物质的半最大诱导在约0.08 nM EGF时实现,该浓度与半最大有丝分裂发生所需的浓度相关性良好。对这种活性物质的生化特性研究强烈表明该活性与一种蛋白质相关。该活性不可透析,对胰蛋白酶和热敏感。提取物的蔗糖梯度离心显示出三个活性峰,分子量分别为46,000、110,000和270,000(沉降系数分别为3.7 S、6.6 S和12 S)。这些结果表明,细胞表面的受体-EGF相互作用导致细胞内产生能够刺激静止核进入活性状态的蛋白质。

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