南方医科大学学报
南方醫科大學學報
남방의과대학학보
JOURNAL OF SOUTHERN MEDICAL UNIVERSITY
2014年
6期
787-791
,共5页
Toll样受体4%肾素血管紧张素系统%脂肪细胞
Toll樣受體4%腎素血管緊張素繫統%脂肪細胞
Toll양수체4%신소혈관긴장소계통%지방세포
Toll-like receptor 4%renin-angiotensin system%3T3-L1 adipose cells
目的:探讨Toll样受体4(TLR4)信号通路在脂肪细胞肾素-血管紧张素系统(RAS)激活的参与机制。方法诱导3T3-L1细胞分化为脂肪细胞,予TLR4特异性激动剂LPS干预,分为对照组、10、100、1000 ng/ml LPS组,应用RT-PCR法、Western-blot法测定TLR4、AGT、ATlR mRNA及蛋白表达并使用免疫荧光双染色法观察NF-κB p65亚基核转位变化;另设10μmol/L厄贝沙坦(AT1R阻滞剂)预处理+100 ng/ml LPS组,观察NF-κB p65亚基核转位情况。结果 LPS干预呈时间依赖性及浓度依赖性升高3T3-L1脂肪细胞TLR4、AGT和AT1R的mRNA表达水平;LPS干预12 h后,TLR4、AGT、AT1R蛋白表达亦呈浓度依赖性升高;各浓度LPS处理组NF-κB p65亚基核转位较对照组明显增强,而10μmol/L厄贝沙坦预处理减弱该效应。结论 TLR4信号通路激活后,上调AGT与AT1R的mRNA及蛋白表达,并激活NF-κB;预先阻断RAS减弱NF-κB的激活。提示TLR4信号激动可激活脂肪细胞局部RAS。
目的:探討Toll樣受體4(TLR4)信號通路在脂肪細胞腎素-血管緊張素繫統(RAS)激活的參與機製。方法誘導3T3-L1細胞分化為脂肪細胞,予TLR4特異性激動劑LPS榦預,分為對照組、10、100、1000 ng/ml LPS組,應用RT-PCR法、Western-blot法測定TLR4、AGT、ATlR mRNA及蛋白錶達併使用免疫熒光雙染色法觀察NF-κB p65亞基覈轉位變化;另設10μmol/L阨貝沙坦(AT1R阻滯劑)預處理+100 ng/ml LPS組,觀察NF-κB p65亞基覈轉位情況。結果 LPS榦預呈時間依賴性及濃度依賴性升高3T3-L1脂肪細胞TLR4、AGT和AT1R的mRNA錶達水平;LPS榦預12 h後,TLR4、AGT、AT1R蛋白錶達亦呈濃度依賴性升高;各濃度LPS處理組NF-κB p65亞基覈轉位較對照組明顯增彊,而10μmol/L阨貝沙坦預處理減弱該效應。結論 TLR4信號通路激活後,上調AGT與AT1R的mRNA及蛋白錶達,併激活NF-κB;預先阻斷RAS減弱NF-κB的激活。提示TLR4信號激動可激活脂肪細胞跼部RAS。
목적:탐토Toll양수체4(TLR4)신호통로재지방세포신소-혈관긴장소계통(RAS)격활적삼여궤제。방법유도3T3-L1세포분화위지방세포,여TLR4특이성격동제LPS간예,분위대조조、10、100、1000 ng/ml LPS조,응용RT-PCR법、Western-blot법측정TLR4、AGT、ATlR mRNA급단백표체병사용면역형광쌍염색법관찰NF-κB p65아기핵전위변화;령설10μmol/L액패사탄(AT1R조체제)예처리+100 ng/ml LPS조,관찰NF-κB p65아기핵전위정황。결과 LPS간예정시간의뢰성급농도의뢰성승고3T3-L1지방세포TLR4、AGT화AT1R적mRNA표체수평;LPS간예12 h후,TLR4、AGT、AT1R단백표체역정농도의뢰성승고;각농도LPS처리조NF-κB p65아기핵전위교대조조명현증강,이10μmol/L액패사탄예처리감약해효응。결론 TLR4신호통로격활후,상조AGT여AT1R적mRNA급단백표체,병격활NF-κB;예선조단RAS감약NF-κB적격활。제시TLR4신호격동가격활지방세포국부RAS。
Objective To investigate the role of Toll-like receptor 4 (TLR4) signaling pathway in the activation of rennin-angiotensin system (RAS) in adipose cells. Methods 3T3- L1 cells induced with isobutylmethylxanthine, insulin and dexamethasone to differentiate into adipocytes were stimulated by LPS with or without irbesartan pretreatment. The expression levels of TLR4, angiotensinogen (AGT) and angiotensin II receptor type 1 (ATlR) mRNA in 3T3-L1 cells was determined by RT-PCR, and their protein expressions were detected with Western-blotting. Immunofluorescence double staining was used to observe the traslocation of NF-κB p65 subunit in the cells. Results Stimulation with LPS dose-and time-dependently increased the mRNA and protein expressions of TLR4, AGT and AT1R. LPS exposure resulted in enhanced translocation of NF-κB p65 subunit in the adipose cells, which was attenuated by irbesartan pretreatment. Conclusion Activation of TLR4 signaling pathway may trigger the activation of local RAS in adipose cells.
