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人肝癌细胞系中生长激素对人生长激素结合蛋白产生的调节作用

Regulation of human growth hormone-binding protein production by human growth hormone in a hepatoma cell line.

作者信息

Mullis P E, Holl R W, Lund T, Eblé A, Brickell P M

机构信息

Department of Paediatric Endocrinology, Children's Hospital, University of Bern, Inselspital, Switzerland.

出版信息

Mol Cell Endocrinol. 1995 Jun;111(2):181-90. doi: 10.1016/0303-7207(95)03567-q.

Abstract

The mechanism by which growth hormone-binding protein (GH-BP) is generated in humans remains unclear. To address this question, we analysed human GH-receptor/GH-BP gene expression in a human hepatoma cell line (HuH7). Northern hybridisation showed that HuH7 cells contain a single mRNA species hybridising with a probe for the sequences encoding the extracellular domain of the hGH-receptor/GH-BP. These data were confirmed by solution hybridisation methods. Thereafter, the cells were treated with r-hGH at physiological (12.5, 25, 50 ng/ml) and supra-physiological (150, 500 ng/ml) concentrations over the period of 48 h. At intervals, RNase protection assays were performed to determine GH-receptor/GH-BP mRNA levels, nuclear run-on assays were carried out to determine whether changes in mRNA levels represented changes in transcription rate, and a radio-ligand binding assay was performed to measure levels of GH-BP in the medium. We found that the r-hGH-regulated changes in GH-receptor/GH-BP mRNA levels detected with the probe for sequences encoding the extracellular domain of human GH-receptor/GH-BP were identical to those previously detected using a probe for the sequences encoding the transmembrane/intracellular domain of the human GH-receptor. In addition, we found that r-hGH had a rapid effect on the levels of GH-BP in the culture medium, which differed from its effect on the GH-receptor/GH-BP mRNA levels. Furthermore, lowering of temperature resulted in a decrease of GH-BP released into the medium implying that enzymes may be involved in the releasing mechanism. These data support the idea that GH-receptor and GH-BP are encoded by a single mRNA species in humans. In addition, they suggest that GH-BP levels are not an accurate reflection of GH-receptor/GH-BP mRNA levels, but that GH-BP production is subject to r-hGH-dependent post-transcriptional regulation, perhaps at the level of post-translational cleavage of the full-length GH-receptor protein. The notion that GH-BP measurements might represent GH-receptor status at the functional level must therefore be taken with caution.

摘要

人类生长激素结合蛋白(GH - BP)的产生机制尚不清楚。为解决这一问题,我们分析了人肝癌细胞系(HuH7)中的人GH受体/GH - BP基因表达。Northern杂交显示,HuH7细胞含有一种单一的mRNA,可与编码hGH受体/GH - BP细胞外结构域序列的探针杂交。这些数据通过溶液杂交方法得到证实。此后,在48小时内,用生理浓度(12.5、25、50 ng/ml)和超生理浓度(150、500 ng/ml)的重组人生长激素(r - hGH)处理细胞。每隔一段时间进行核糖核酸酶保护试验以测定GH受体/GH - BP mRNA水平,进行细胞核连续转录分析以确定mRNA水平的变化是否代表转录速率的变化,并进行放射性配体结合试验以测量培养基中GH - BP的水平。我们发现,用编码人GH受体/GH - BP细胞外结构域序列的探针检测到的r - hGH调节的GH受体/GH - BP mRNA水平变化与先前使用编码人GH受体跨膜/细胞内结构域序列的探针检测到的变化相同。此外,我们发现r - hGH对培养基中GH - BP的水平有快速影响,这与其对GH受体/GH - BP mRNA水平的影响不同。此外,降低温度导致释放到培养基中的GH - BP减少,这意味着酶可能参与了释放机制。这些数据支持了人类中GH受体和GH - BP由单一mRNA编码的观点。此外,它们表明GH - BP水平并非GH受体/GH - BP mRNA水平的准确反映,而是GH - BP的产生受到r - hGH依赖的转录后调控,可能在全长GH受体蛋白的翻译后切割水平。因此,必须谨慎看待GH - BP测量可能代表功能水平上GH受体状态的观点。

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