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作 者:崔雪玲[1] 葛敬岩[2] 李晨光[2] 孙洋[2] 牛立慢[2] 刘海岩[2] 柳忠辉[2] 王轶楠[2]
机构地区:[1]吉林大学白求恩医学院遗传学系,长春130021 [2]吉林大学白求恩医学院免疫学系,长春130021
出 处:《中国生物制品学杂志》2012年第2期161-163,167,共4页Chinese Journal of Biologicals
基 金:国家自然科学基金(30801005;30901323;30901329);吉林省科技厅课题(20080160;20090742)
摘 要:目的探讨激活素受体相互作用蛋白(Activin receptor-interacting protein,ARIP)1及2(ARIP1,2)在小鼠巨噬细胞RAW264.7中的表达及作用。方法采用免疫细胞化学染色法检测RAW264.7细胞中ARIP1,2的表达;将质粒CAGA-lux、CMV-gal分别与表达质粒pcDNA3-ARIP1、pcDNA3-ARIP2或空质粒pcDNA3共转染RAW264.7细胞,应用激活素A刺激,检测细胞内报告基因转录荧光素酶的活性;实时定量RT-PCR检测ActRⅡA mRNA的表达。结果免疫细胞化学染色结果显示,小鼠巨噬细胞系RAW264.7细胞表达ARIP1,2;RAW264.7细胞过表达ARIP1,2均能抑制Activin A诱导的特异基因转录;过表达ARIP2可抑制RAW264.7细胞ActRⅡA mRNA的表达,而过表达ARIP1对ActRⅡA mRNA的表达无明显影响。结论 ARIP1,2在小鼠巨噬细胞中共表达,并具有下调激活素信号传导的作用,但其作用方式不同。Objective To investigate the expression and role of activin receptor-interacting proteins 1, 2 (ARIP1, 2) in mouse macrophages. Methods The expression of ARIP1, 2 was determined by immunoeytochemical staining. RAW264. 7 cells were eo-transfected with plasmids CAGA-lnx and CMV-gal, plus plasmids pcDNA3-ARIP1, pcDNA3-ARIP2 or empty plasmid pcDNA3, respectively, then stimulated with activin A, and determined for transcription activity of report gene. The expression of ActR Ⅱ A mRNA was determined by RT-PCR. Results Immunocytochemical staining proved that ARIP1,2 were expressed in RAW264. 7 cells. The overexpressions of ARIP1, 2 inhibited the transcription of specific gene induced by activin A. The overexpression of ARIP2 inhibited, while that of ARIP1 showed no significant effect on the expression of ActR Ⅱ A mRNA in RAW264. 7 ceils. Conclusion ARIP1, 2 were coexpressed in mouse maerophages, which down-regulated the signal transduction of activin by different action modes.
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