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大鼠肝脏在热缺血和冷缺血期间的糖酵解与能量代谢:调节酶磷酸果糖激酶激活的证据

Glycolysis and energy metabolism in rat liver during warm and cold ischemia: evidence of an activation of the regulatory enzyme phosphofructokinase.

作者信息

Churchill T A, Cheetham K M, Fuller B J

机构信息

University Department of Surgery, Royal Free Hospital School of Medicine, London, United Kingdom.

出版信息

Cryobiology. 1994 Oct;31(5):441-52. doi: 10.1006/cryo.1994.1054.

DOI:10.1006/cryo.1994.1054
PMID:7988153
Abstract

The current study was undertaken so that the effects of both ischemia and ischemia + hypothermia could be examined in mammalian liver. Particular reference was made to the function of glycolysis, which is the only mechanism for energy production under these conditions. The response of adenylate pools reflected the energy imbalance created during warm ischemia within minutes of organ isolation. ATP levels and energy charge values for control (freshly isolated) livers were 1.20 +/- 0.07 and 0.49 +/- 0.02 mumol/g. Within 5 min of warm ischemia, ATP levels had dropped well below control values and by 30 min warm ischemia, ATP, AMP, and E.C. values were 0.21, 2.01, and 0.17 mumol/g, respectively. Cold ischemic livers (flushed with Marshall's citrate solution and stored on ice) exhibited similar, but more protracted, patterns of adenylate depletion (ATP and ADP) and accumulation (AMP). In both warm and cold ischemic livers, levels of fructose-6-phosphate (F6P) and fructose-1,6-bisphosphate (F1,6P2) indicated a marked activation of glycolysis at the phosphofructokinase (PFK) locus after a certain time of ischemia. Although the activations occurred at different times (30 min and 10 h for warm and cold ischemic livers, respectively), the patterns of change in levels of glycolytic metabolites associated with the PFK-catalyzed reaction were similar; levels of F6P dropped and F1,6P2 increased. Changes in metabolite levels (phosphoenol pyruvate and pyruvate) associated with another key suspect regulatory enzyme, pyruvate kinase, indicated no role in regulatory control of glycolysis during warm or cold ischemia. The activation of PFK at 30 min and 10 h of warm and cold ischemia, respectively, may reflect the accumulating effects of loss of intracellular homeostasis, which leads to impending irreversible damage.

摘要

进行当前这项研究是为了能够在哺乳动物肝脏中检测缺血及缺血+低温的影响。特别关注了糖酵解的功能,糖酵解是这些条件下唯一的能量产生机制。腺苷酸池的反应反映了器官分离后数分钟内热缺血期间产生的能量失衡。对照(新鲜分离)肝脏的ATP水平和能量电荷值分别为1.20±0.07和0.49±0.02μmol/g。热缺血5分钟内,ATP水平已大幅降至对照值以下,热缺血30分钟时,ATP、AMP和E.C.值分别为0.21、2.01和0.17μmol/g。冷缺血肝脏(用马歇尔柠檬酸盐溶液冲洗并保存在冰上)表现出类似但更持久的腺苷酸消耗(ATP和ADP)和积累(AMP)模式。在热缺血和冷缺血肝脏中,6-磷酸果糖(F6P)和1,6-二磷酸果糖(F1,6P2)水平均表明在缺血一定时间后磷酸果糖激酶(PFK)位点的糖酵解显著激活。尽管激活发生在不同时间(热缺血和冷缺血肝脏分别为30分钟和10小时),但与PFK催化反应相关的糖酵解代谢物水平的变化模式相似;F6P水平下降而F1,6P2水平上升。与另一种关键的可疑调节酶丙酮酸激酶相关的代谢物水平(磷酸烯醇丙酮酸和丙酮酸)变化表明,在热缺血或冷缺血期间,丙酮酸激酶在糖酵解的调节控制中不起作用。热缺血和冷缺血分别在30分钟和10小时时PFK的激活可能反映了细胞内稳态丧失的累积效应,这会导致即将发生的不可逆损伤。

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