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肌酸作为暴露于高渗应激下的肌肉细胞中的一种相容性渗透剂。

Creatine as a compatible osmolyte in muscle cells exposed to hypertonic stress.

作者信息

Alfieri Roberta R, Bonelli Mara A, Cavazzoni Andrea, Brigotti Maurizio, Fumarola Claudia, Sestili Piero, Mozzoni Paola, De Palma Giuseppe, Mutti Antonio, Carnicelli Domenica, Vacondio Federica, Silva Claudia, Borghetti Angelo F, Wheeler Kenneth P, Petronini Pier Giorgio

机构信息

Department of Biochemistry, School of Life Sciences, JMS Building, University of Sussex, Brighton BN1 9QG, UK.

出版信息

J Physiol. 2006 Oct 15;576(Pt 2):391-401. doi: 10.1113/jphysiol.2006.115006. Epub 2006 Jul 27.

Abstract

Exposure of C2C12 muscle cells to hypertonic stress induced an increase in cell content of creatine transporter mRNA and of creatine transport activity, which peaked after about 24 h incubation at 0.45 osmol (kg H(2)O)(-1). This induction of transport activity was prevented by addition of either cycloheximide, to inhibit protein synthesis, or of actinomycin D, to inhibit RNA synthesis. Creatine uptake by these cells is largely Na(+) dependent and kinetic analysis revealed that its increase under hypertonic conditions resulted from an increase in V(max) of the Na(+)-dependent component, with no significant change in the K(m) value of about 75 mumol l(-1). Quantitative real-time PCR revealed a more than threefold increase in the expression of creatine transporter mRNA in cells exposed to hypertonicity. Creatine supplementation significantly enhanced survival of C2C12 cells incubated under hypertonic conditions and its effect was similar to that obtained with the well known compatible osmolytes, betaine, taurine and myo-inositol. This effect seemed not to be linked to the energy status of the C2C12 cells because hypertonic incubation caused a decrease in their ATP content, with or without the addition of creatine at 20 mmol l(-1) to the medium. This induction of creatine transport activity by hypertonicity is not confined to muscle cells: a similar induction was shown in porcine endothelial cells.

摘要

将C2C12肌细胞暴露于高渗应激下,可诱导肌酸转运蛋白mRNA的细胞含量及肌酸转运活性增加,在0.45 osmol(kg H₂O)⁻¹下孵育约24小时后达到峰值。添加放线菌酮(以抑制蛋白质合成)或放线菌素D(以抑制RNA合成)可阻止这种转运活性的诱导。这些细胞对肌酸的摄取在很大程度上依赖于Na⁺,动力学分析表明,在高渗条件下其增加是由于Na⁺依赖性成分的Vmax增加,而Kₘ值约75 μmol l⁻¹无显著变化。定量实时PCR显示,暴露于高渗环境的细胞中肌酸转运蛋白mRNA的表达增加了三倍多。补充肌酸可显著提高在高渗条件下孵育的C2C12细胞的存活率,其效果与著名的相容性渗透剂甜菜碱、牛磺酸和肌醇相似。这种作用似乎与C2C12细胞的能量状态无关,因为高渗孵育会导致其ATP含量降低,无论培养基中是否添加20 mmol l⁻¹的肌酸。高渗对肌酸转运活性的这种诱导并不局限于肌细胞:在猪内皮细胞中也显示出类似的诱导作用。

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