胡彬1,2,3 王赫2,3 晏贤春2,3 蒋芳2,3 王清明2,3 杨俊涛2,3△.高脂培养抑制LPS诱导的HSC-T6 细胞活化*[J].,2014,14(8):1420-1422 |
高脂培养抑制LPS诱导的HSC-T6 细胞活化* |
The Fat Culture Inhabited LPS-Induced Activation of HSCs-T6 Cells* |
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DOI: |
中文关键词: 游离脂肪酸 肝星形细胞 LPS 肝纤维化 |
英文关键词: Free fatty acids HSC-T6 LPS Liver fibrosis |
基金项目:国家自然科学基金项目(31000405);国家高技术研究发展计划(2012AA020201); |
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中文摘要: |
摘要目的:鉴定高脂培养对肝星形细胞活化的影响。方法:培养HSC-T6 细胞系,加入含有游离脂肪酸的高脂培养基处理,利用
LPS 处理活化,通过检测α-SMA 的表达分析星形细胞的活化程度,通过Q-PCR分析HSCs 细胞胶原的表达,通过Q-PCR实验分
析LPS相关通路靶基因表达情况情况。结果:高脂培养能够抑制LPS 诱导的HSC-T6 细胞增殖,降低HSC-T6 细胞α-SMA 和胶
原I和TIMP-1 表达的水平,Q-PCR 的分析表明,高脂培养能够抑制HSCs活化后的NF-κB 通路下游靶基因MCP-1 和IL-6 的表
达。结论:在体外培养实验中,高脂培养能够抑制LPS诱导的HSC-T6 细胞活化。 |
英文摘要: |
ABSTRACT Objective:To investigate the effect of high-fat medium on the activition of hepatic stellate cells. Methods:HSC-T6
cell line was cultured, and treated with high-fat medium which containing free fatty acid, activated with LPS. The degree of activation
was analyzed by detecting α-SMA expression. The expression of collagen-I and TIMP-1 was analyzed by Q-PCR, and the activation of
transcription factor which related to LPS pathway was analyzed by Q-PCR assay. Results:High-fat medium was able to inhibit the
activation of HSC-T6 cells which induced by LPS, reduced the expression of collagen level in the HSC-T6 cells. Q-PCR analysis showed
that the high-fat medium inhibited the expression of MCP-1 and IL-6 which were the target genes of NF-κB in activated HSCs.
Conclusion:In vitro culture experiments, high-fat mediumcan inhibit the activation of HSC-T6 cells which induced by LPS. |
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