中国医师杂志
中國醫師雜誌
중국의사잡지
JOURNAL OF CHINESE PHYSICIAN
2013年
8期
1028-1031
,共4页
吕天旻%朱千东%张启瑜%俞富祥
呂天旻%硃韆東%張啟瑜%俞富祥
려천민%주천동%장계유%유부상
四氯化碳/毒性%疾病模型,动物%肝硬化,实验性/病理学%大鼠,Sprague-Dawley%胞间信号肽类和蛋白质类/遗传学
四氯化碳/毒性%疾病模型,動物%肝硬化,實驗性/病理學%大鼠,Sprague-Dawley%胞間信號肽類和蛋白質類/遺傳學
사록화탄/독성%질병모형,동물%간경화,실험성/병이학%대서,Sprague-Dawley%포간신호태류화단백질류/유전학
Carbon tetrachloride/toxicity%Disease models,animal%Liver cirrhosis,experimental/pathology%Rats,Sprague-Dawley%Intercellular signaling peptides and proteins/genetics
目的 探讨脂肪特异性蛋白27(Fsp27)基因对活体肝纤维化进程的调节作用.方法 分离原代肝星状细胞(HSCs),采用PCR技术检测在原代HSCs及活化HSCs中的Fsp27基因表达;构建携带Fsp27目的基因的慢病毒;建立肝纤维化模型;慢病毒转染模型鼠肝脏,对实验大鼠行肝脏病理切片检查,采用ELISA法和放射免疫法分别检测肝脏及血浆纤维蛋白含量.结果 Fsp27基因在原代HSCs及活化HSCs中表达差异有统计学意义(P<0.01);成功构建了Fsp27基因的慢病毒载体;成功建立了肝纤维化活体模型;Fsp27基因慢病毒成功转染大鼠肝脏,Fsp27基因减轻了肝脏的纤维化程度.结论 Fsp27基因具有延缓活体肝纤维化进程的作用.
目的 探討脂肪特異性蛋白27(Fsp27)基因對活體肝纖維化進程的調節作用.方法 分離原代肝星狀細胞(HSCs),採用PCR技術檢測在原代HSCs及活化HSCs中的Fsp27基因錶達;構建攜帶Fsp27目的基因的慢病毒;建立肝纖維化模型;慢病毒轉染模型鼠肝髒,對實驗大鼠行肝髒病理切片檢查,採用ELISA法和放射免疫法分彆檢測肝髒及血漿纖維蛋白含量.結果 Fsp27基因在原代HSCs及活化HSCs中錶達差異有統計學意義(P<0.01);成功構建瞭Fsp27基因的慢病毒載體;成功建立瞭肝纖維化活體模型;Fsp27基因慢病毒成功轉染大鼠肝髒,Fsp27基因減輕瞭肝髒的纖維化程度.結論 Fsp27基因具有延緩活體肝纖維化進程的作用.
목적 탐토지방특이성단백27(Fsp27)기인대활체간섬유화진정적조절작용.방법 분리원대간성상세포(HSCs),채용PCR기술검측재원대HSCs급활화HSCs중적Fsp27기인표체;구건휴대Fsp27목적기인적만병독;건립간섬유화모형;만병독전염모형서간장,대실험대서행간장병리절편검사,채용ELISA법화방사면역법분별검측간장급혈장섬유단백함량.결과 Fsp27기인재원대HSCs급활화HSCs중표체차이유통계학의의(P<0.01);성공구건료Fsp27기인적만병독재체;성공건립료간섬유화활체모형;Fsp27기인만병독성공전염대서간장,Fsp27기인감경료간장적섬유화정도.결론 Fsp27기인구유연완활체간섬유화진정적작용.
Objective To investigate the influence of fat-specific protein 27 (Fsp27) gene on the regulation of liver fibrogenesis in vivo.Methods Hepatic stellate cells (HSCs) were isolated from rat liver.Fsp27 gene was detected in primary HSCs and activated HSCs by real-time quantitative PCR (RTqPCR).Lentiviral vector carrying Fsp27 gene was constructed.The model of liver fibrosis was established by infusing carbon tetrachloride (CC14).The rats with liver fibrogenesis were infected by the virus.Liver sections were made to observe the structure and form of liver histocytes.The content of fibrous protein in liver and serum was detected by enzyme-linked immunosorbent assay (ELISA) and radioimmunoassay.Resukts HSCs were isolated and cultured successfully.The difference of Fsp27 gene between primary HSCs and activated HSCs was significant(P < 0.01).The model of liver fibrosis was achieved.After infecting the model rats,we found the fibrosis level in treatment group was lower compared with control group.Conclusions Fsp27 treatment can decrease collagen deposition in the liver and inhibit the formation of fibrosis.
