Vavvas D, Apazidis A, Saha A K, Gamble J, Patel A, Kemp B E, Witters L A, Ruderman N B
Department of Physiology and Diabetes and Metabolism Unit, Evans Department of Medicine, Boston University Medical Center, Boston, Massachusetts 02118, USA.
J Biol Chem. 1997 May 16;272(20):13255-61. doi: 10.1074/jbc.272.20.13255.
The concentration of malonyl-CoA, a negative regulator of fatty acid oxidation, diminishes acutely in contracting skeletal muscle. To determine how this occurs, the activity and properties of acetyl-CoA carboxylase beta (ACC-beta), the skeletal muscle isozyme that catalyzes malonyl-CoA formation, were examined in rat gastrocnemius-soleus muscles at rest and during contractions induced by electrical stimulation of the sciatic nerve. To avoid the problem of contamination of the muscle extract by mitochondrial carboxylases, an assay was developed in which ACC-beta was first purified by immunoprecipitation with a monoclonal antibody. ACC-beta was quantitatively recovered in the immunopellet and exhibited a high sensitivity to citrate (12-fold activation) and a Km for acetyl-CoA (120 microM) similar to that reported for ACC-beta purified by other means. After 5 min of contraction, ACC-beta activity was decreased by 90% despite an apparent increase in the cytosolic concentration of citrate, a positive regulator of ACC. SDS-polyacrylamide gel electrophoresis of both homogenates and immunopellets from these muscles showed a decrease in the electrophoretic mobility of ACC, suggesting that phosphorylation could account for the decrease in ACC activity. In keeping with this notion, citrate activation of ACC purified from contracting muscle was markedly depressed. In addition, homogenization of the muscles in a buffer free of phosphatase inhibitors and containing the phosphatase activators glutamate and MgCl2 or treatment of immunoprecipitated ACC-beta with purified protein phosphatase 2A abolished the decreases in both ACC-beta activity and electrophoretic mobility caused by contraction. The rapid decrease in ACC-beta activity after the onset of contractions (50% by 20 s) and its slow restoration to initial values during recovery (60-90 min) were paralleled temporally by reciprocal changes in the activity of the alpha2 but not the alpha1 isoform of 5'-AMP-activated protein kinase (AMPK). In conclusion, the results suggest that the decrease in ACC activity during muscle contraction is caused by an increase in its phosphorylation, most probably due, at least in part, to activation of the alpha2 isoform of AMPK. They also suggest a dual mechanism for ACC regulation in muscle in which inhibition by phosphorylation takes precedence over activation by citrate. These alterations in ACC and AMPK activity, by diminishing the concentration of malonyl-CoA, could be responsible for the increase in fatty acid oxidation observed in skeletal muscle during exercise.
丙二酰辅酶A是脂肪酸氧化的负调节因子,其在收缩的骨骼肌中的浓度会急剧下降。为了确定其发生机制,研究了乙酰辅酶A羧化酶β(ACC-β)的活性和特性,ACC-β是催化丙二酰辅酶A形成的骨骼肌同工酶,在大鼠比目鱼肌-腓肠肌处于静息状态以及坐骨神经电刺激诱导收缩期间进行了检测。为避免线粒体羧化酶污染肌肉提取物的问题,开发了一种检测方法,其中ACC-β首先通过用单克隆抗体进行免疫沉淀来纯化。ACC-β在免疫沉淀颗粒中被定量回收,并且对柠檬酸表现出高敏感性(12倍激活),对乙酰辅酶A的Km值(120μM)与通过其他方法纯化的ACC-β报道的值相似。收缩5分钟后,尽管ACC的正向调节因子柠檬酸的胞质浓度明显增加,但ACC-β活性仍下降了90%。对这些肌肉的匀浆和免疫沉淀颗粒进行SDS-聚丙烯酰胺凝胶电泳显示,ACC的电泳迁移率降低,表明磷酸化可能是ACC活性下降的原因。与此观点一致的是,从收缩肌肉中纯化的ACC的柠檬酸激活明显受到抑制。此外,在不含磷酸酶抑制剂且含有磷酸酶激活剂谷氨酸和MgCl2的缓冲液中匀浆肌肉,或用纯化的蛋白磷酸酶2A处理免疫沉淀的ACC-β,消除了收缩引起的ACC-β活性和电泳迁移率的下降。收缩开始后ACC-β活性迅速下降(20秒时下降50%),恢复期间缓慢恢复到初始值(60 - 90分钟),在时间上与5'-AMP激活蛋白激酶(AMPK)的α2亚型而非α1亚型活性的反向变化平行。总之,结果表明肌肉收缩期间ACC活性的下降是由其磷酸化增加引起的,最可能至少部分是由于AMPK的α2亚型的激活。它们还表明肌肉中ACC调节存在双重机制,其中磷酸化抑制优先于柠檬酸激活。ACC和AMPK活性的这些改变,通过降低丙二酰辅酶A的浓度,可能是运动期间骨骼肌中脂肪酸氧化增加的原因。
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