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用牛GLUT4 cDNA片段评估犊牛肌肉中胰岛素敏感性葡萄糖转运体转录水平。

Insulin-sensitive glucose transporter transcript levels in calf muscles assessed with a bovine GLUT4 cDNA fragment.

作者信息

Hocquette J F, Graulet B, Castiglia-Delavaud C, Bornes F, Lepetit N, Ferre P

机构信息

INRA, Laboratoire Croissance et Métabolismes des Herbivores, Theix, France.

出版信息

Int J Biochem Cell Biol. 1996 Jul;28(7):795-806. doi: 10.1016/1357-2725(96)00013-1.

Abstract

Previous studies have shown that the expression of the insulin-sensitive glucose transporter (GLUT4) is lower in oxidative muscles than in glycolytic muscles in bovines and goats in contrast to observations in rats. Additional experiments in this work provide very strong arguments that the immunoreactive band detected does represent GLUT4 protein, which further validates our previous results. Therefore, to determine the level of regulation, the main objective of the present study was to measure GLUT4 mRNA amounts in various bovine muscles. A 241-bp fragment of the bovine GLUT4 cDNA was cloned by polymerase chain reaction (PCR). It shares 80-90% sequence identity with related sequences in other species. This PCR-amplified bovine GLUT4 probe was used to determine the distribution of GLUT4 mRNA in bovine tissues in comparison with that of GLUT1 mRNA. Moreover, GLUT4 mRNA amounts were quantified by Northern-blot analysis in heart and seven skeletal muscles with various oxidative and glycolytic activities from seven ruminant calves. GLUT4 mRNA was detected by Northern-blot analysis only in calf insulin-sensitive tissues. In contrast, GLUT1 mRNA was detected in all tissues studied except liver. GLUT4 mRNA amount was the highest in masseter and heart, which are oxidative muscles (1.67 +/- 0.16 and 1.53 +/- 0.19 units/g wet tissue weight, respectively) and the lowest in glycolytic or oxido-glycolytic muscles (0.31 +/- 0.04 to 1.00 +/- 0.09 units/g wet tissue weight; SEM, n = 7). These data and our previous results provide evidence for translational and/or post-translational control mechanisms of bovine GLUT4 protein expression in a muscle type-specific manner.

摘要

先前的研究表明,与大鼠的观察结果相反,牛和山羊的氧化型肌肉中胰岛素敏感性葡萄糖转运体(GLUT4)的表达低于糖酵解型肌肉。本研究中的其他实验提供了非常有力的证据,证明检测到的免疫反应条带确实代表GLUT4蛋白,这进一步验证了我们先前的结果。因此,为了确定调节水平,本研究的主要目的是测量各种牛肌肉中GLUT4 mRNA的含量。通过聚合酶链反应(PCR)克隆了牛GLUT4 cDNA的一个241bp片段。它与其他物种的相关序列具有80-90%的序列同一性。将该PCR扩增的牛GLUT4探针用于确定牛组织中GLUT4 mRNA的分布,并与GLUT1 mRNA的分布进行比较。此外,通过Northern印迹分析对来自7头反刍动物犊牛的心脏和7种具有不同氧化和糖酵解活性的骨骼肌中的GLUT4 mRNA含量进行了定量。通过Northern印迹分析仅在犊牛胰岛素敏感组织中检测到GLUT4 mRNA。相比之下,除肝脏外,在所有研究的组织中均检测到GLUT1 mRNA。GLUT4 mRNA含量在咬肌和心脏中最高,这两种肌肉都是氧化型肌肉(分别为1.67±0.16和1.53±0.19单位/g湿组织重量),在糖酵解型或氧化-糖酵解型肌肉中最低(0.31±0.04至1.00±0.09单位/g湿组织重量;标准误,n = 7)。这些数据和我们先前的结果为牛GLUT4蛋白表达的翻译和/或翻译后控制机制提供了肌肉类型特异性的证据。

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