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缺氧刺激培养的心房心肌细胞中的心钠素基因表达。

Hypoxia stimulates atrial natriuretic peptide gene expression in cultured atrial cardiocytes.

作者信息

Chen Y F, Durand J, Claycomb W C

机构信息

Department of Medicine, University of Alabama at Birmingham 35294-0007, USA.

出版信息

Hypertension. 1997 Jan;29(1 Pt 1):75-82. doi: 10.1161/01.hyp.29.1.75.

DOI:10.1161/01.hyp.29.1.75
PMID:9039084
Abstract

The current study tested the hypothesis that hypoxia stimulates atrial natriuretic peptide (ANP) gene expression and secretion in cultured atrial myocytes (AT-1 cells). AT-1 cells were obtained from a transplantable mouse atrial cardiomyocyte tumor lineage. Confluent AT-1 cells were exposed to hypoxia (1% oxygen) or normoxia (21% oxygen) as controls for 6 hours to 7 days. Medium ANP levels were measured by radioimmunoassay, and intracellular ANP gene transcripts were quantified by Northern and slot blot analyses. Exposure to hypoxia resulted in a significant increase in cellular ANP mRNA levels within 36 hours, which peaked (3.6-fold increase) at 2 days after hypoxic exposure, and produced a time-dependent increase in the release of ANP from AT-1 cells for 2 to 7 days. Transfection studies with recombinant DNA constructs that contained fragments of the -3003/+62 sequence of the ANP promoter and the luciferase reporter gene revealed that the regulatory sequences that mediate the hypoxia-induced increase in transcription are located within a region that extends from -638 to -518 bp to the transcriptional start site of the ANP gene. Gel mobility shift assays demonstrated that hypoxia-inducible nuclear proteins that bound to the 120-bp putative hypoxia-responsive elements of the ANP gene were produced during hypoxic exposure. We have thus defined a 120-bp region within the ANP gene promoter that contains hypoxia-responsive elements that might be responsible for the enhancement of ANP gene expression in atrial myocytes during hypoxic exposure.

摘要

本研究验证了以下假设

缺氧可刺激培养的心房肌细胞(AT-1细胞)中的心钠素(ANP)基因表达及分泌。AT-1细胞取自一种可移植的小鼠心房心肌细胞瘤系。将汇合的AT-1细胞暴露于缺氧环境(1%氧气)或作为对照的常氧环境(21%氧气)中6小时至7天。通过放射免疫测定法测量培养基中的ANP水平,并用Northern印迹法和狭缝印迹分析法对细胞内ANP基因转录本进行定量。暴露于缺氧环境后,36小时内细胞ANP mRNA水平显著升高,在缺氧暴露后2天达到峰值(增加3.6倍),并且在2至7天内AT-1细胞释放ANP呈时间依赖性增加。用含有ANP启动子-3003 / +62序列片段和荧光素酶报告基因的重组DNA构建体进行转染研究表明,介导缺氧诱导转录增加的调控序列位于从ANP基因转录起始位点-638至-518 bp延伸的区域内。凝胶迁移率变动分析表明,在缺氧暴露期间产生了与ANP基因120 bp推定缺氧反应元件结合的缺氧诱导核蛋白。因此,我们确定了ANP基因启动子内一个120 bp的区域,该区域含有缺氧反应元件,可能负责缺氧暴露期间心房肌细胞中ANP基因表达的增强。

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