基于四维无标记定量蛋白质组学研究,葛花解酒地黄汤通过调节脂质和胆汁酸代谢以及发挥抗氧化作用改善小鼠酒精性脂肪肝。

Han Min, Y I Xu, You Shaowei, W U Xueli, Wang Shuoshi, H E Diancheng
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引用次数: 0

摘要

目的采用蛋白质组学方法分析葛花解酒滴丸(GJDD)对酒精性脂肪活症(AFLD)的作用及分子机制:方法:将雄性C57BL/6J小鼠随机分为4组:对照组、模型组、GJDD组和白藜芦醇组。在Lieber-DeCarli经典方法基础上通过胃内注射酒精一次成功制备AFLD模型后,分别给GJDD组和白藜芦醇组胃内注射GJDD(4900 mg/kg)和白藜芦醇(400 mg/kg),每天一次,连续9 d。采用4D无标记定量蛋白质组方法测定和量化各实验组肝组织中的蛋白质表达。根据蛋白表达差异倍数筛选差异表达蛋白,然后进行基因本体分类和京都基因组百科全书通路富集分析。最后,通过靶向蛋白质组学定量技术验证了对照组、模型组和 GJDD 组差异共表达蛋白的表达情况:结果:在ORO的半定量分析中,AFLD小鼠的各种脂肪变性(ToS、MaS和MiS)均高于GJDD或白藜芦醇处理的小鼠。4D无标记蛋白质组学分析结果显示,共鉴定出4513个蛋白质,其中3763个蛋白质被定量,946个差异表达蛋白质被筛选。与对照组相比,模型组肝脏组织中有145个蛋白质上调,148个蛋白质下调。此外,与模型组相比,GJDD 组肝脏组织中有 92 个蛋白质上调,135 个蛋白质下调。在每两组(模型组与对照组、GJDD 组与模型组、GJDD 组与对照组)之间发现了 15 个差异共表达蛋白,它们参与了许多生物学过程。其中,11个差异共表达的关键蛋白(Aox3、H1-5、Fabp5、Ces3a、Nudt7、Serpinb1a、Fkbp11、Rpl22l1、Keg1、Acss2和Slco1a1)经靶向蛋白质组学定量技术进一步鉴定,其表达模式与4D无标记蛋白质组学分析结果一致:我们的研究提供了基于蛋白质组学的证据,证明 GJDD 可通过调节肝脏蛋白表达缓解 AFLD,这可能是通过调节脂质代谢、胆汁酸代谢和发挥抗氧化应激作用实现的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Gehua Jiejiu Dizhi decoction ameliorates alcoholic fatty liver in mice by regulating lipid and bile acid metabolism and with exertion of antioxidant stress based on 4DLabel-free quantitative proteomic study.

Objective: To analyze the effect and molecular mechanism of Gehua Jiejiu Dizhi decoction (, GJDD) on alcoholic fatty live disease (AFLD) by using proteomic methods.

Methods: The male C57BL/6J mouse were randomly divided into four groups: control group, model group, GJDD group and resveratrol group. After the AFLD model was successfully prepared by intragastric administration of alcohol once on the basis of the Lieber-DeCarli classical method, the GJDD group and resveratrol group were intragastrically administered with GJDD (4900 mg/kg) and resveratrol (400 mg/kg) respectively, once a day for 9 d. The fat deposition of liver tissue was observed and evaluated by oil red O (ORO) staining. 4DLabel-free quantitative proteome method was used to determine and quantify the protein expression in liver tissue of each experimental group. The differentially expressed proteins were screened according to protein expression differential multiples, and then analyzed by Gene ontology classification and Kyoto Encyclopedia of Genes and Genomes pathway enrichment. Finally, expression validation of the differentially co-expressed proteins from control group, model group and GJDD group were verified by targeted proteomics quantification techniques.

Results: In semiquantitative analyses of ORO, all kinds of steatosis (ToS, MaS, and MiS) were evaluated higher in AFLD mice compared to those in GJDD or resveratrol-treated mice. 4DLabel-free proteomics analysis results showed that a total of 4513 proteins were identified, of which 3763 proteins were quantified and 946 differentially expressed proteins were screened. Compared with the control group, 145 proteins were up-regulated and 148 proteins were down-regulated in the liver tissue of model group. In addition, compared with the model group, 92 proteins were up-regulated and 135 proteins were down-regulated in the liver tissue of the GJDD group. 15 differentially co-expressed proteins were found between every two groups (model group vs control group, GJDD group vs model group and GJDD group vs control group), which were involved in many biological processes. Among them, 11 differentially co-expressed key proteins (Aox3, H1-5, Fabp5, Ces3a, Nudt7, Serpinb1a, Fkbp11, Rpl22l1, Keg1, Acss2 and Slco1a1) were further identified by targeted proteomic quantitative technology and their expression patterns were consistent with the results of 4D label-free proteomic analysis.

Conclusions: Our study provided proteomics-based evidence that GJDD alleviated AFLD by modulating liver protein expression, likely through the modulation of lipid metabolism, bile acid metabolism and with exertion of antioxidant stress.

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