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丙二醛生成和抗坏血酸减少与离体缺血后大鼠心脏的再灌注有关。

Malondialdehyde production and ascorbate decrease are associated to the reperfusion of the isolated postischemic rat heart.

作者信息

Tavazzi B, Lazzarino G, Di Pierro D, Giardina B

机构信息

Department of Experimental Medicine, II University of Rome, Italy.

出版信息

Free Radic Biol Med. 1992;13(1):75-8. doi: 10.1016/0891-5849(92)90167-f.

Abstract

Isolated Langendorff-perfused rat hearts after 20 min of normoxic perfusion in the presence of 2.5 mM Ca++ and 11 mM glucose were subjected to 30 min of global normothermic ischemia followed by 30 min of normoxic reperfusion with the starting buffer. At the end of each perfusion condition, hearts were freeze-clamped and deproteinized by 0.6 M HClO4. Two-hundred microL of the neutralized tissue extracts were analyzed by a recently developed high-performance liquid chromatography (HPLC) method for the simultaneous determination of malondialdehyde (MDA), ascorbic acid, and adenine nucleotides. By means of this analytical technique, it was possible to demonstrate that MDA is undetectable in control hearts. In contrast, 30 min of ischemia induced a modest production of MDA (0.012 mumol/g dw), while a large amount of MDA (0.103 mumol/g dw) was observed in reperfused hearts. Values referring to ascorbic acid showed that the concentration of this antioxidant progressively decreased from 1.190 (control hearts) to 0.837 (ischemic hearts) and to 0.595 mumol/g dw (reperfused hearts). The overall conclusions of this study are that reperfusion induces an oxidative stress to the isolated myocardium, a decrease of ascorbate, and an increase of lipid peroxidation. Therefore, by means of a proper analytical method, MDA may represent a valid biochemical parameter to demonstrate the relationship between myocardial reperfusion and a detectable tissue damage.

摘要

在含有2.5 mM钙离子和11 mM葡萄糖的条件下进行20分钟常氧灌注后,对离体Langendorff灌注大鼠心脏进行30分钟全心常温缺血,随后用起始缓冲液进行30分钟常氧再灌注。在每个灌注条件结束时,将心脏冷冻钳夹并用0.6 M高氯酸脱蛋白。用最近开发的高效液相色谱(HPLC)方法分析200微升中和后的组织提取物,以同时测定丙二醛(MDA)、抗坏血酸和腺嘌呤核苷酸。通过这种分析技术,可以证明在对照心脏中检测不到MDA。相比之下,30分钟的缺血诱导了适度的MDA产生(0.012微摩尔/克干重),而在再灌注心脏中观察到大量的MDA(0.103微摩尔/克干重)。抗坏血酸的值表明,这种抗氧化剂的浓度从1.190(对照心脏)逐渐降低到0.837(缺血心脏),再到0.595微摩尔/克干重(再灌注心脏)。本研究的总体结论是,再灌注会对离体心肌诱导氧化应激、抗坏血酸盐减少以及脂质过氧化增加。因此,通过适当的分析方法,MDA可能是一个有效的生化参数,用于证明心肌再灌注与可检测到的组织损伤之间的关系。

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