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培养的肝癌细胞中苯丙氨酸羟化酶周转的测定。

Measurement of phenylalanine hydroxylase turnover in cultured hepatoma cells.

作者信息

Baker R E, Shiman R

出版信息

J Biol Chem. 1979 Oct 10;254(19):9633-9.

PMID:489556
Abstract

A substantially new method has been developed to measure protein turnover. Its basis is the notion that in labeling experiments a secreted protein can be used to determine the specific radioactivity of the intracellular amino acid precursor pool. To measure protein turnover in the Reuber hepatoma H4 cell line, cultures were labeled with [3H]leucine for specified periods after which phenylalanine hydroxylase was isolated and its leucine specific radioactivity determined. Serum albumin secreted by the cultures was also isolated and used to estimate the leucine precursor pool specific radioactivity. The protein half-life of phenylalanine hydroxylase could them be calculated. Experiments performed at long and short labeling times and with high and low concentrations of leucine in the medium yielded equivalent results. Phenylalanine hydroxylase half-life in the H4 cells was investigated under both normal and hydrocortisone-induced growth conditions. Average half-lives of 7.4 and 8.2 h were found for induced and uninduced cultures, respectively. Although these measured enzyme half-lives were not essentially different, the steady state level of phenylalanine hydroxylase was increased 6.2-fold upon hydrocortisone induction, from 0.076 to 0.47 microgram/10(6) cells. The results demonstrated that hydrocortisone induces phenylalanine hydroxylase in the H4 cells by causing an increase in the rate of enzyme synthesis.

摘要

一种全新的测量蛋白质周转率的方法已被开发出来。其依据是这样一种理念:在标记实验中,一种分泌蛋白可用于确定细胞内氨基酸前体池的比放射性。为了测量鲁伯肝癌H4细胞系中的蛋白质周转率,在特定时间段内用[³H]亮氨酸标记培养物,之后分离出苯丙氨酸羟化酶并测定其亮氨酸比放射性。培养物分泌的血清白蛋白也被分离出来,用于估计亮氨酸前体池的比放射性。然后可以计算苯丙氨酸羟化酶的蛋白质半衰期。在长标记时间和短标记时间以及培养基中亮氨酸浓度高和低的情况下进行的实验都得到了相同的结果。在正常和氢化可的松诱导的生长条件下研究了H4细胞中苯丙氨酸羟化酶的半衰期。诱导培养物和未诱导培养物的平均半衰期分别为7.4小时和8.2小时。尽管这些测量的酶半衰期没有本质差异,但氢化可的松诱导后苯丙氨酸羟化酶的稳态水平增加了6.2倍,从0.076微克/10⁶个细胞增加到0.47微克/10⁶个细胞。结果表明,氢化可的松通过增加酶的合成速率来诱导H4细胞中的苯丙氨酸羟化酶。

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