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作 者:张黔桓[1] 邓春玉[1] 饶芳[1] 刘晓颖[1] 麦丽萍[1] 朱杰宁[1] 谭虹虹[1] 吴书林[1]
机构地区:[1]广东省人民医院心内科,广东省心血管病研究所,广东广州510080
出 处:《中国病理生理杂志》2013年第6期982-987,共6页Chinese Journal of Pathophysiology
基 金:广东省自然科学基金资助项目(No.10151008002000011)
摘 要:目的:采用基因沉默技术抑制小鼠HL-1心肌细胞桥粒斑蛋白(DSP)基因表达以明确DSP与缝隙连接蛋白43(Cx43)的结构和功能关系。方法:用基因沉默技术抑制DSP基因的表达,Western blotting和流式细胞术检测HL-1细胞DSP和Cx43蛋白的表达,用双免疫荧光方法检测DSP与Cx43蛋白的表达与定位情况,并用划痕标记染料示踪技术检测细胞缝隙连接通讯状况。结果:与空白组和对照组相比,siRNA-DSP组的DSP和Cx43蛋白表达量降低(P<0.05)。免疫荧光检测发现空白组和对照组DSP与Cx43蛋白存在共定位情况,而siRNA-DSP组DSP和Cx43蛋白共定位遭到破坏,Cx43蛋白出现再分布,在细胞内检测到Cx43蛋白,并且划痕标记染料示踪技术检测发现siRNA-DSP组Lucifer yellow通过HL-1细胞缝隙连接的传输功能降低。结论:DSP表达抑制不仅使Cx43出现再分布,而且影响缝隙连接传导功能。AIM: To evaluate the content, distribution, and function of connexin 43 (Cx43) gap junctions in mouse HL-1 myocardial cells under the condition of desmoplakin (DSP) silencing. METHODS: The technique of RNA interference was used to inhibit the protein expression of DSP in HL-1 cells. The protein expression of DSP and Cx43 was analyzed by Western blotting and flow cytometry. The immunofluorescence staining was used to detect the distribution and co-localization of DSP and Cx43. The techniques of scrape loading and dye transfer were also used to determine the function of Cx43 gap junctions. RESULTS: Compared with non-treatment group and negative control group, the protein expression of DSP and Cx43 was reduced ( P 〈 0.05 ). Co-localization to the site of cell-cell contact was apparent in untreated and control conditions, but loss of DSP expression induced by siRNA-DSP correlated with a drastic redistribution of Cx43. In- stead, Cx43 was found mostly within the intracellular space. The results of dye transfer assay indicated a significant de- crease in the function of Cx43 gap junctions of the ceils treated with siRNA-DSP. CONCLUSION : Inhibition of DSP ex- pression induces redistribution of Cx43 and decrease in dye coupling between ceils.
关 键 词:缝隙连接蛋白43 桥粒斑蛋白 基因沉默 HL-1细胞
分 类 号:R542.2[医药卫生—心血管疾病]
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