Dieni Christopher A, Storey Kenneth B
Institute of Biochemistry and Department of Chemistry, Carleton University, 1125 Colonel By Drive, Ottawa, Ontario, K1S 5B6, Canada.
BMC Biochem. 2008 Apr 22;9:12. doi: 10.1186/1471-2091-9-12.
The wood frog, Rana sylvatica, is one of a few vertebrate species that have developed natural freeze tolerance, surviving days or weeks with 65-70% of its total body water frozen in extracellular ice masses. Frozen frogs exhibit no vital signs and their organs must endure multiple stresses, particularly long term anoxia and ischemia. Maintenance of cellular energy supply is critical to viability in the frozen state and in skeletal muscle, AMP deaminase (AMPD) plays a key role in stabilizing cellular energetics. The present study investigated AMPD control in wood frog muscle.
Wood frog AMPD was subject to multiple regulatory controls: binding to subcellular structures, protein phosphorylation, and effects of allosteric effectors, cryoprotectants and temperature. The percentage of bound AMPD activity increased from 20 to 35% with the transition to the frozen state. Bound AMPD showed altered kinetic parameters compared with the free enzyme (S0.5 AMP was reduced, Hill coefficient fell to approximately 1.0) and the transition to the frozen state led to a 3-fold increase in S0.5 AMP of the bound enzyme. AMPD was a target of protein phosphorylation. Bound AMPD from control frogs proved to be a low phosphate form with a low S0.5 AMP and was phosphorylated in incubations that stimulated PKA, PKC, CaMK, or AMPK. Bound AMPD from frozen frogs was a high phosphate form with a high S0.5 AMP that was reduced under incubation conditions that stimulated protein phosphatases. Frog muscle AMPD was activated by Mg.ATP and Mg.ADP and inhibited by Mg.GTP, KCl, NaCl and NH4Cl. The enzyme product, IMP, uniquely inhibited only the bound (phosphorylated) enzyme from muscle of frozen frogs. Activators and inhibitors differentially affected the free versus bound enzyme. S0.5 AMP of bound AMPD was also differentially affected by high versus low assay temperature (25 vs 5 degrees C) and by the presence/absence of the natural cryoprotectant (250 mM glucose) that accumulates during freezing.
Maintenance of long term viability under the ischemic conditions in frozen muscle requires attention to the control of cellular energetics. Differential regulatory controls on AMPD by mechanisms including binding to muscle proteins, actions allosteric effectors, glucose and temperature effects and reversible phosphorylation adjust enzyme function for an optimal role in controlling cellular adenylate levels in ischemic frozen muscle. Stable modification of AMPD properties via freeze-responsive phosphorylation may contribute both to AMPD control and to coordinating AMPD function with other enzymes of energy metabolism in cold ischemic muscle.
林蛙(Rana sylvatica)是少数已进化出天然耐冻能力的脊椎动物物种之一,能在全身65 - 70%的水分在细胞外结成冰团的情况下存活数天或数周。处于冰冻状态的林蛙没有生命体征,其器官必须承受多种压力,尤其是长期的缺氧和缺血。维持细胞能量供应对于冰冻状态下的生存能力至关重要,在骨骼肌中,AMP脱氨酶(AMPD)在稳定细胞能量代谢方面发挥着关键作用。本研究调查了林蛙肌肉中AMPD的调控机制。
林蛙AMPD受到多种调控:与亚细胞结构结合、蛋白质磷酸化以及变构效应剂、冷冻保护剂和温度的影响。随着转变为冰冻状态,结合态AMPD活性的百分比从20%增加到35%。与游离酶相比,结合态AMPD的动力学参数发生了变化(S0.5 AMP降低,希尔系数降至约1.0),并且向冰冻状态的转变导致结合态酶的S0.5 AMP增加了3倍。AMPD是蛋白质磷酸化的靶点。来自对照林蛙的结合态AMPD被证明是一种低磷酸化形式,具有较低的S0.5 AMP,并且在刺激PKA、PKC、CaMK或AMPK的孵育过程中会发生磷酸化。来自冰冻林蛙的结合态AMPD是一种高磷酸化形式,具有较高的S0.5 AMP,在刺激蛋白磷酸酶的孵育条件下其S0.5 AMP会降低。林蛙肌肉AMPD被Mg.ATP和Mg.ADP激活,被Mg.GTP、KCl、NaCl和NH4Cl抑制。该酶的产物IMP仅特异性抑制来自冰冻林蛙肌肉的结合态(磷酸化)酶。激活剂和抑制剂对游离酶和结合态酶的影响不同。结合态AMPD的S0.5 AMP也受到高低测定温度(25℃对5℃)以及冷冻过程中积累的天然冷冻保护剂(250 mM葡萄糖)的存在与否的不同影响。
在冰冻肌肉的缺血条件下维持长期生存能力需要关注细胞能量代谢的调控。通过包括与肌肉蛋白结合、变构效应剂作用、葡萄糖和温度效应以及可逆磷酸化等机制对AMPD进行差异调控,可调节酶的功能,使其在控制缺血冰冻肌肉中的细胞腺苷酸水平方面发挥最佳作用。通过冷冻响应性磷酸化对AMPD特性进行稳定修饰可能有助于AMPD的调控,并使AMPD功能与冷缺血肌肉中其他能量代谢酶协调。
Zotero 插件