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对经多种应激处理的A549细胞中HSF-1磷酸化的分析。

Analysis of HSF-1 phosphorylation in A549 cells treated with a variety of stresses.

作者信息

Mivechi N F, Koong A C, Giaccia A J, Hahn G M

机构信息

Department of Radiation Oncology, Cancer Biology Research Laboratory, Stanford, CA 94305.

出版信息

Int J Hyperthermia. 1994 May-Jun;10(3):371-9. doi: 10.3109/02656739409010281.

DOI:10.3109/02656739409010281
PMID:7930803
Abstract

In the absence of stress, heat shock transcription factor-1 (HSF-1) exists as a monomer. After the treatment of cells with variety of stresses, HSF-1 forms a trimer and binds to the heat shock element (HSE), a motif consisting of three consecutive NGAAN sequences located in an inverted orientation upstream of the heat shock genes. HSF-1 is then phosphorylated causing transactivation of heat shock mRNAs. Treatment of cells with some of the stresses has been shown to increase HSF binding to HSE without detectably increasing the synthesis of heat shock mRNAs. Here we used antibody specific to HSF-1 to detect its phosphorylation status following exposure of A549, a human lung carcinoma cell line to a variety of stresses in order to correlate HSF-1 phosphorylation with its transactivation ability. Our studies show that HSF-1 is phosphorylated following heat shock (43 degrees C for 1 h), hypoxia (5 h exposure to 0.02% oxygen), 8% ethanol (1 h exposure at 37 degrees C), or 200 microM sodium arsenite (1 h exposure at 37 degrees C). All such stresses have previously been shown to increase the synthesis of heat shock proteins (hsps). However, there are no detectable increases in HSF-1 phosphorylation after the treatment of cells with X-irradiation (2-8 Gy) or 100 microM canavanine, an amino acid analogue (1 h exposure at 37 degrees C). Treatment of cells with X-irradiation increases HSF binding to HSE without increasing the synthesis of hsps, while treatment of cells with canavanine has been shown to increase the synthesis of hsps.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在无应激状态下,热休克转录因子1(HSF-1)以单体形式存在。用多种应激因素处理细胞后,HSF-1形成三聚体并与热休克元件(HSE)结合,HSE是位于热休克基因上游反向排列的由三个连续的NGAAN序列组成的基序。随后HSF-1被磷酸化,导致热休克mRNA的反式激活。已表明用某些应激因素处理细胞可增加HSF与HSE的结合,但未检测到热休克mRNA的合成有明显增加。在此,我们使用HSF-1特异性抗体检测人肺癌细胞系A549暴露于多种应激因素后其磷酸化状态,以便将HSF-1磷酸化与其反式激活能力相关联。我们的研究表明,热休克(43℃处理1小时)、缺氧(暴露于0.02%氧气5小时)、8%乙醇(37℃暴露1小时)或200μM亚砷酸钠(37℃暴露1小时)后HSF-1被磷酸化。所有这些应激因素此前均已表明可增加热休克蛋白(hsps)的合成。然而,用X射线照射(2 - 8 Gy)或100μM刀豆氨酸(一种氨基酸类似物,37℃暴露1小时)处理细胞后,未检测到HSF-1磷酸化有明显增加。用X射线照射处理细胞可增加HSF与HSE的结合,但不增加hsps的合成,而用刀豆氨酸处理细胞已表明可增加hsps的合成。(摘要截短于250字)

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