CAJ | 학술논문

目的观察糖基化终末产物(advanced glycation end products,AGEs)对人腹膜间皮细胞(human peritoneal mesothelial cell,HPMC)分泌单核细胞趋化蛋白1(monocyte chemoattractant protein-1,MCP1)的作用及细胞内活性氧族(reactive oxygen species,ROS)在其中的作用.方法分别用不同浓度的糖基化人血清白蛋白(advanced glycation end products-human serum albumin,AGE-HSA)及抗氧化剂N-乙酰-L-半胱氨酸(N-acetyl-L-cysteine,NAC)作用于细胞,用逆转录多聚酶链反应(RT-PCR)法和酶联免疫吸附法(ELISA)测定HPMC中MCP-1的表达;再以氧化敏感的荧光染料2,7-二氢二氯荧光素(2.7-dichlorofluorescin,DCFH)染色,流式细胞仪测定ROS强度.结果 AGE-HSA能使细胞内ROS水半明显升高,呈现浓度依赖效应;AGE-HSA同时以时效和量效方式促进HPMC中MCP-1的表达;而NAC能够明显抑制AGE-HSA 所导致的细胞内ROS升高,同时抑制HPMC中MCP-1的分泌.结论 AGE-HSA 可能部分通过诱导细胞内ROS,促进HPMC 表达MCP-1.
목적 관찰당기화종말산물(advanced glycation end products,AGEs)대인복막간피세포(human peritoneal mesothelial cell,HPMC)분비단핵세포추화단백1(monocyte chemoattractant protein-1,MCP1)적작용급세포내활성양족(reactive oxygen species,ROS)재기중적작용.방법 분별용불동농도적당기화인혈청백단백(advanced glycation end products-human serum albumin,AGE-HSA)급항양화제N-을선-L-반광안산(N-acetyl-L-cysteine,NAC)작용우세포,용역전록다취매련반응(RT-PCR)법화매련면역흡부법(ELISA)측정HPMC중MCP-1적표체;재이양화민감적형광염료2,7-이경이록형광소(2.7-dichlorofluorescin,DCFH)염색,류식세포의측정ROS강도.결과 AGE-HSA능사세포내ROS수반명현승고,정현농도의뢰효응;AGE-HSA동시이시효화량효방식촉진HPMC중MCP-1적표체;이NAC능구명현억제AGE-HSA 소도치적세포내ROS승고,동시억제HPMC중MCP-1적분비.결론 AGE-HSA 가능부분통과유도세포내ROS,촉진HPMC 표체MCP-1.