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Changes in expression of serine biosynthesis and integrated stress response genes during myogenic differentiation of C2C12 cells

机译:C2C12细胞成肌分化过程中丝氨酸生物合成和整合应激反应基因表达的变化

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摘要

Skeletal muscle is a highly metabolic and dynamic tissue that is formed through the complex and well-organised process of myogenesis. Although there is a good understanding about the role of the Muscle Regulatory Factors during myogenesis, little is known about the potential interplay of other metabolic proteins. The aim of this study was to determine the endogenous mRNA expression profile for a novel group of genes, recently associated with β2-adrenergic agonist (BA) induced muscle hypertrophy in pigs [1], during myogenic differentiation in C2C12 cells and their response to dibutyryl cyclic-AMP (dbcAMP). These genes included mitochondrial phosphoenolpyruvate carboxykinase (PCK2/PEPCK-M), genes involved in serine biosynthesis (Phosphoglycerate dehydrogenase, PHGDH; Phosphoserine aminotransferase-1, PSAT1; Phosphoserine phosphatase, PSPH) and those involved in an integrated stress response (Asparagine synthetase, ASNS; Sestrin-2, SESN2; and Activating transcription factor-5, ATF5).A coordinated peak in endogenous PCK2, PHGDH, PSAT1, PSPH, ASNS, ATF5 and SESN2 mRNA expression was observed at day 2 of differentiation (P < 0.001) in C2C12 cells, which coincided with the peak in myogenin mRNA. Myotube hypertrophy was induced with dbcAMP (1 mM) treatment from day 0, thereby mimicking the in vivo BA response. Although dbcAMP treatment from day 0 induced larger myotubes and increased both myosin heavy chain-IIB (MyHC-IIB) and pyruvate carboxylase (PC) mRNA, the expression of PCK2, PHGDH, PSAT1 and ASNS mRNA were all unaffected. Treatment with dbcAMP from day 4 increased MyHC-IIB mRNA, however this was less dramatic compared to the response observed following treatment from day 0, but there was no effect on PC mRNA. There was also no effect of dbcAMP treatment from day 4 on PCK2, PHGDH, PSAT1 and ASNS mRNA.To conclude, the coordinated day 2 peak in endogenous expression of PCK2, PHGDH, PSAT1, PSPH, ASNS, ATF5 and SESN2 mRNA may relate to a shift in biosynthetic demand required to initiate myogenic differentiation. However, dbcAMP had no effect on the expression of these genes in vitro suggesting that the effects observed in BA-treated pigs might be via other signalling pathways from the activation of the β2-adrenergic receptor, but independent of cAMP, or that there are species differences in the response.
机译:骨骼肌是一种高度代谢和动态的组织,是通过复杂且组织良好的成肌过程形成的。尽管对肌肉调节因子在肌发生过程中的作用有很好的了解,但对其他代谢蛋白的潜在相互作用知之甚少。这项研究的目的是确定一组新基因的内源性mRNA表达谱,这些基因最近与β2-肾上腺素能激动剂(BA)诱导的猪肌肉肥大有关[1],在C2C12细胞成肌分化及其对二丁酰的反应中循环AMP(dbcAMP)。这些基因包括线粒体磷酸烯醇丙酮酸羧激酶(PCK2 / PEPCK-M),参与丝氨酸生物合成的基因(磷酸甘油酸脱氢酶,PHGDH;磷酸丝氨酸氨基转移酶-1,PSAT1;磷酸丝氨酸磷酸酶,PSPH)以及参与综合应激反应(天冬酰胺)的基因在分化的第二天观察到内源性PCK2,PHGDH,PSAT1,PSPH,ASNS,ATF5和SESN2 mRNA表达的协调峰(P <0.001)。 C2C12细胞,与肌生成素mRNA的峰重合。从第0天起,用dbcAMP(1μmM)处理诱导肌管肥大,从而模拟体内BA反应。尽管从第0天开始的dbcAMP治疗诱导了更大的肌管,并增加了肌球蛋白重链IIB(MyHC-IIB)和丙酮酸羧化酶(PC)mRNA,但PCK2,PHGDH,PSAT1和ASNS mRNA的表达均不受影响。从第4天开始用dbcAMP处理增加了MyHC-IIB mRNA,但是与从第0天开始治疗后观察到的反应相比,这种变化不那么明显,但是对PC mRNA没有影响。从第4天开始dbcAMP处理对PCK2,PHGDH,PSAT1和ASNS mRNA的影响也没有影响。总而言之,PCK2,PHGDH,PSAT1,PSPH,ASNS,ATF5和SESN2 mRNA的内源表达的第2天协调峰可能与开始生肌分化所需的生物合成需求的变化。但是,dbcAMP在体外对这些基因的表达没有影响,这表明在BA治疗的猪中观察到的影响可能是通过β2-肾上腺素能受体激活的其他信号途径,但与cAMP无关,或者存在物种反应的差异。

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