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首页> 外文期刊>Journal of dairy science >Identification of promoter response elements that mediate propionate induction of bovine cytosolic phosphoenolpyruvate carboxykinase (PCK1) gene transcription
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Identification of promoter response elements that mediate propionate induction of bovine cytosolic phosphoenolpyruvate carboxykinase (PCK1) gene transcription

机译:鉴定促进丙氨酸诱导牛胞质磷酸丙酮酸羧酮(PCK1)基因转录的促进诱导诱导

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摘要

Cytosolic phosphoenolpyruvate carboxykinase (PCK1) is a key enzyme for gluconeogenesis that is positively regulated by propionate in bovines at the transcription level. The specific elements that determine propionate responsiveness within the bovine PCK1 promoter are unknown. In silico promoter analysis of the bovine PCK1 gene revealed several clusters of transcription factor binding sites. In the present study, we determined the essentiality of the putative cyclic AMP response element (CRE) at −94 through −87 bp and the 2 putative hepatic nuclear factor 4α (HNF4α) binding elements at +68 through +72 and −1,078 through −1,074, respectively, in mediating bovine PCK1 promoter responses to propionate and other regulators, including butyrate, cyclic AMP (cAMP), and glucocorticoids. The wild-type bovine PCK1 promoter [PCK1_((WT))] was ligated to a luciferase reporter gene and transfected into rat hepatoma (H4IIE) cells. Activities of PCK1_((WT)) were induced by approximately 2-, 2-, 4-, 8-, 9-, 18-, and 16-fold respectively when exposed to cAMP (as 1.0 mM 8-Br-cAMP), 5.0 μM dexamethasone, cAMP + dexamethasone, 2.5 mM propionate, cAMP + propionate, cAMP + dexamethasone + propionate, and 2.5 mM butyrate. Seven mutants lacking either one single site, 2 of the 3 sites, or all 3 sites, generated by site-directed mutagenesis, were tested. Responses to propionate and all other treatments were completely abolished when CRE at −94 through −87 bp and HNF4α at +68 through +72 bp were both deleted. Our data indicate that these 2 regulatory elements act synergistically to mediate the bovine PCK1 promoter responses to propionate as well as butyrate, cAMP, and dexamethasone. The activation of PCK1 through these regulatory elements serves to activate the metabolic potential of bovine toward gluconeogenesis when the primary substrate for gluconeogenesis, propionate, is also present.
机译:胞质磷烯醇丙酮酸羧基酶(PCK1)是葡糖基因的关键酶,其通过在转录水平的丙酸盐中呈正调节。确定牛PCK1启动子内丙酸响应性的特定元素是未知的。在牛PCK1基因的硅启动子分析中,揭示了几种转录因子结合位点的簇。在本研究中,我们确定了-94至-87bp的推定循环AMP响应元件(CRE)的物质和在+ 68至+72和-1,078的+68至-1,078和-1,078的2调用肝核因子4α(HNF4α)结合元素分别在培养牛PCK1启动子反应对丙酸盐和其他调节剂的1,074中,包括丁酸盐,环状辐射(阵营)和糖皮质激素。将野生型牛PCK1启动子[Pck1_((重量))]连接到荧光素酶报告基因中,并转染成大鼠肝癌(H4IIE)细胞。在暴露于营地时,PCK1 _((WT))的活动分别诱导约2-,2-,4-,8-,9-,18-和16倍(如1.0mm 8-Br-Br-Br-Br-Br-Br-Br-Br-Br)。 5.0μm地塞米松,营地+地塞米松,2.5毫米丙酸盐,营养蛋白+丙酸盐,营地+地塞米松+丙酸盐,2.5毫米丁酸盐。测试了缺少3位点的单个位点的七个突变体,或通过点定向诱变产生的所有3位点的突变体。当CRE在-94至-87bp和HNF4αAT + 68至+ 72bp均删除时,对丙酸酯和所有其他治疗的反应完全消除了。我们的数据表明,这2个监管要素协同介绍牛蛋白PCK1启动子反应,替代丙酸盐以及丁酸盐,营地和地塞米松。通过这些调节元件的PCK1的激活用于当葡糖苷的初级基质也存在时激活牛对葡糖生成的代谢潜力。

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