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Continuous observation of heat shock protein 70 expression in its kinetics study

机译:连续观察热休克蛋白70在其动力学研究中的表达

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The kinetics study of heat shock protein 70 (HSP70) expression is essential to any clinical application of HSP70. HSP70 expression was visualized continuously in cultured bovine aortic endothelial cells (BAECs) on a culture dish adaptable heating stage with green fluorescent protein (GFP) as a reporter. BAECs were transfected with a DNA vector, HSP/sub p/-HSP70-GFP, which has HSP70 promoter followed by HSP70 gene and GFP gene. Cloning was used to construct this vector. Western Blot analysis of transfected and heated cells showed the fusion protein expression. Transfected cells were heated on the stage at 42/spl deg/C and post-heated at 37/spl deg/C on the same stage for varied time periods. The expression of the fusion protein, HSP70-GFP, and its localization were visualized by GFP with a fluorescence microscope. HSP70 expression kinetics can be measured by quantitative analysis of serial fluorescence images captured over different heating and post-heating times. This is a much more efficient method to study HSP70 expression kinetics than the discontinuous steps of cell heating, cell lysis and Western Blot analysis. The kinetics data from continuous observation of HSP70 expression will be compared with our endogenous HSP70 expression kinetics study.
机译:热休克蛋白70(HSP70)表达的动力学研究对于HSP70的任何临床应用都是必不可少的。在培养皿适应性加热阶段,以绿色荧光蛋白(GFP)为报告基因,在培养的牛主动脉内皮细胞(BAEC)中连续观察HSP70表达。用DNA载体HSP / sub p / -HSP70-GFP转染BAEC,其具有HSP70启动子,随后是HSP70基因和GFP基因。克隆被用于构建该载体。转染和加热的细胞的蛋白质印迹分析显示融合蛋白表达。将转染的细胞在载物台上以42 / spl deg / C加热,并在同一载物台上以37 / spl deg / C后加热不同的时间段。用荧光显微镜通过GFP观察融合蛋白HSP70-GFP的表达及其定位。 HSP70表达动力学可以通过对在不同加热时间和加热后时间捕获的连续荧光图像进行定量分析来测量。与不连续的细胞加热,细胞裂解和蛋白质印迹分析步骤相比,这是一种研究HSP70表达动力学的更有效的方法。连续观察HSP70表达的动力学数据将与我们的内源性HSP70表达动力学研究进行比较。

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