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体外低温低氧期间心脏磷酸果糖激酶磷酸化状态的保守性

Conservation of phosphorylation state of cardiac phosphofructokinase during in vitro hypothermic hypoxia.

作者信息

Pulis R P, Wu B M, Kneteman N M, Churchill T A

机构信息

Surgical-Medical Research Institute, University of Alberta, Edmonton, Alberta, Canada.

出版信息

Am J Physiol Heart Circ Physiol. 2000 Nov;279(5):H2151-8. doi: 10.1152/ajpheart.2000.279.5.H2151.

DOI:10.1152/ajpheart.2000.279.5.H2151
PMID:11045948
Abstract

We investigated the metabolic effects of buffering agents alpha-amino-4-imidazole-propionic acid (Histidine), N, N-bis(2-hydroxyethyl)glycine (bicine), N, N-bis(2-hydroxyethyl)-2-aminoethanesulfonic acid (BES) on anaerobic energy production (via glycolysis) and conservation of key regulatory enzyme activity, and phosphofructokinase (PFK) throughout prolonged hypothermic hypoxia in porcine hearts. Hearts from 35 to 40 kg pigs were flushed with one of the following five solutions: St. Thomas' Hospital solution (STHS); modified University of Wisconsin (UW) solution; and three solutions containing modified UW plus 90 mM of histidine, bicine, or BES. The hearts were then stored at 4 degrees C for 10 h. After 10 h of hypothermic hypoxia, lactate values were 6.7-12.9 micromol/g higher than control; this reflected an increase in anaerobic end product of 35-67%. The consequences of enhanced anaerobic metabolism were higher ATP, total adenylate, Energy Charge, and ATP/ADP ratios in most of the buffered groups after 4-10 h cold storage; effectiveness of the buffers employed correlated with buffering capacity (BES proved to be the most effective). PFK remained activated throughout most of the 10-h period in hearts stored with buffers and did not undergo the rapid inactivation experienced by hearts stored in STHS. Conservation of PFK integrity with buffering agents was not related to a pH-mediated event; changes in kinetic parameters suggested that this protection was due to an irreversible posttranslational modification, specifically a dephosphorylation event.

摘要

我们研究了缓冲剂α-氨基-4-咪唑丙酸(组氨酸)、N,N-双(2-羟乙基)甘氨酸(二乙醇胺)、N,N-双(2-羟乙基)-2-氨基乙磺酸(BES)对猪心脏在长时间低温缺氧状态下无氧能量产生(通过糖酵解)以及关键调节酶活性和磷酸果糖激酶(PFK)活性维持的代谢影响。用以下五种溶液之一对体重35至40千克猪的心脏进行灌注:圣托马斯医院溶液(STHS);改良威斯康星大学(UW)溶液;以及三种含有改良UW加90 mM组氨酸、二乙醇胺或BES的溶液。然后将心脏在4℃下保存10小时。低温缺氧10小时后,乳酸值比对照组高6.7 - 12.9微摩尔/克;这反映出无氧终产物增加了35% - 67%。在4 - 10小时的冷藏后,大多数缓冲组中增强的无氧代谢导致ATP、总腺苷酸、能荷以及ATP/ADP比值升高;所使用缓冲剂的有效性与缓冲能力相关(事实证明BES最有效)。在使用缓冲剂保存的心脏中,PFK在10小时的大部分时间里都保持激活状态,没有经历STHS保存的心脏所出现的快速失活。缓冲剂对PFK完整性的维持与pH介导的事件无关;动力学参数的变化表明这种保护是由于不可逆的翻译后修饰,具体是去磷酸化事件。

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