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膳食多不饱和脂肪酸会干扰L型丙酮酸激酶基因转录的胰岛素/葡萄糖激活作用。

Dietary polyunsaturated fatty acids interfere with the insulin/glucose activation of L-type pyruvate kinase gene transcription.

作者信息

Liimatta M, Towle H C, Clarke S, Jump D B

机构信息

Department of Physiology, Michigan State University, East Lansing 48824.

出版信息

Mol Endocrinol. 1994 Sep;8(9):1147-53. doi: 10.1210/mend.8.9.7838147.

DOI:10.1210/mend.8.9.7838147
PMID:7838147
Abstract

L-type pyruvate kinase (L-PK) is a key glycolytic enzyme regulating the flux of metabolites through the pyruvate-phosphoenolpyruvate cycle (1). The regulation of L-PK is complex involving both hormones and nutrients. We have found that feeding rats diets containing polyunsaturated fatty acids (PUFA) significantly inhibits hepatic pyruvate kinase enzyme activity (> 60%) and suppresses mRNAPK abundance (> 70%). Studies with primary hepatocytes indicate that PUFA act directly on hepatocytes. Specifically, arachidonic (20:4, omega 6) and eicosapentaenoic (20:5, omega 3) acid suppressed both mRNAPK llevels and the activity of a transfected PKCAT (-4300/+12) fusion gene by > 70%. This is due to an inhibition of the insulin/glucose-mediated transactivation of L-PKCAT. Deletion analysis localized PUFA-regulated cis-acting elements to a region within the L-PK proximal promoter, i.e. between -197 and -96 base pairs. This region binds two transcription factors involved in the hormone/nutrient regulation of L-PK gene transcription, i.e. a major late transcription factor-like factor and HNF-4. Linker scanning mutation analysis localized the PUFA-regulated cis-acting elements to the vicinity of the HNF-4 binding site. Thus, PUFA-regulated factors abrogate the insulin/glucose activation of L-PK gene transcription by targeting the HNF-4 elements. These studies suggest that PUFA may have significant effects on hepatic carbohydrate metabolism by inhibiting the L-PK side of the pyruvate-phosphoenolpyruvate cycle.

摘要

L型丙酮酸激酶(L-PK)是一种关键的糖酵解酶,可调节代谢物通过丙酮酸-磷酸烯醇丙酮酸循环的通量(1)。L-PK的调节很复杂,涉及激素和营养物质。我们发现,给大鼠喂食含有多不饱和脂肪酸(PUFA)的饮食会显著抑制肝丙酮酸激酶的酶活性(>60%),并抑制mRNA PK丰度(>70%)。对原代肝细胞的研究表明,PUFA直接作用于肝细胞。具体而言,花生四烯酸(20:4,ω-6)和二十碳五烯酸(20:5,ω-3)使mRNA PK水平和转染的PKCAT(-4300/+12)融合基因的活性均降低>70%。这是由于胰岛素/葡萄糖介导的L-PKCAT反式激活受到抑制。缺失分析将PUFA调节的顺式作用元件定位到L-PK近端启动子内的一个区域,即-197至-96碱基对之间。该区域结合了两个参与L-PK基因转录的激素/营养调节的转录因子,即一个主要晚期转录因子样因子和肝细胞核因子-4(HNF-4)。接头扫描突变分析将PUFA调节的顺式作用元件定位到HNF-4结合位点附近。因此,PUFA调节因子通过靶向HNF-4元件消除了L-PK基因转录的胰岛素/葡萄糖激活。这些研究表明,PUFA可能通过抑制丙酮酸-磷酸烯醇丙酮酸循环的L-PK一侧对肝脏碳水化合物代谢产生显著影响。

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