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Effects of Extracts from Tiaozhi Granule and Its Components on Expression of Scavenger Receptor Class B Type I

机译:调脂冲剂及其成分对Ⅰ型清道夫受体表达的影响

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摘要

Sera from the rats with different drug treatments (atorvastatin, Tiaozhi granule, or its extracts) were collected. LO-2 cells or HepG2 cells were pretreated with different sera as the following groups randomly: (1) blank control group, (2) positive control group (atorvastatin group), (3) Tiaozhi granule water extract groups, (4) Tiaozhi granule alcohol extract groups, and (5) alcohol extracts for each component: Pollen Typhae Angustifoliae, Curcuma longa L., and Rhizoma Alismatis. LO-2 cells were cotransfected with plasmid carrying SR-BI and pRL-TK promoter genes. Promoter activity was measured by the luciferase reporter gene assay. The mRNA and protein expressions of SR-BI were examined using real-time PCR and western blot analyses. Our results show that promoter activity and mRNA and protein expression levels of the SR-BI were significantly upregulated by Tiaozhi granules alcohol or water extracts in a dose-dependent manner. Pollen Typhae Angustifoliae alcohol extract with a high dosage could also increase SR-BI activity and expression, but not the extracts from Curcuma longa L. and Rhizoma Alismatis. Both Tiaozhi granule alcohol and water extracts can upregulate SR-BI gene expression. Among the components, Pollen Typhae Angustifoliae are important for the regulatory effect coordinating with Curcuma longa L. and Rhizoma Alismatis.
机译:收集不同药物处理的大鼠(阿托伐他汀,调脂颗粒或其提取物)的血清。将LO-2细胞或HepG2细胞用不同的血清随机分为以下几组:(1)空白对照组,(2)阳性对照组(阿托伐他汀组),(3)调脂冲剂水提物组,(4)调脂冲剂酒精提取物组,以及(5)每种成分的酒精提取物:花粉香蒲,姜黄和姜。 LO-2细胞用携带SR-BI和pRL-TK启动子基因的质粒共转染。启动子活性通过荧光素酶报道基因测定来测量。 SR-BI的mRNA和蛋白质表达使用实时PCR和蛋白质印迹分析进行了检查。我们的结果表明,调脂颗粒酒精或水提取物以剂量依赖性方式显着上调了SR-BI的启动子活性以及mRNA和蛋白表达水平。高剂量的花粉香蒲醇提取物也可以增加SR-BI活性和表达,但不能提高姜黄和香根草的提取物。调脂颗粒酒精和水提取物均可上调SR-BI基因的表达。在花粉中,香蒲花粉对于与姜黄和甜叶菊协调作用的调节作用很重要。

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