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大鼠脑缺血后蛋白质合成的变化:低温的影响。

Postischaemic changes in protein synthesis in the rat brain: effects of hypothermia.

作者信息

Bergstedt K, Hu B R, Wieloch T

机构信息

Laboratory for Experimental Brain Research, Lund University, Lund Hospital, Sweden.

出版信息

Exp Brain Res. 1993;95(1):91-9. doi: 10.1007/BF00229658.

DOI:10.1007/BF00229658
PMID:8405256
Abstract

Protein synthesis, measured as [14C]-leucine incorporation into proteins, was studied in the normothermic rat brain following 15 min of transient cerebral ischaemia and 1 h, 24 h and 48 h of recirculation, and in the hypothermic (33 degrees C) brain following 1 h and 48 h of recirculation. Ischaemia was induced by bilateral common carotid occlusion combined with hypotension. Following normothermic ischaemia, incorporation of [14C]-leucine was depressed by 40-80% at 1 h of recirculation in all brain regions studied. At 48 h postischaemia, incorporation returned to normal or above normal levels in the inner layers of neocortex, the CA3 region, the striatum and the dentate gyrus, while in the outer layers of neocortex and in the hippocampal CA1 region the incorporation was persistently decreased by 26% and 40% respectively. At 24 and 48 h postischaemia, protein synthesis in the CA1 region and the striatum could be attributed to proliferating microglia. Intra-ischaemic hypothermia ameliorated the persistent depression of protein synthesis in the CA1 region at 48 h postischaemia, and a two-fold increase compared to the normothermic group was observed both in the CA1 region and the striatum. In the cortex, eucaryotic initiation factor 2 activity transiently decreased at 30 min postischaemia. In animals subjected to intra-ischaemic hypothermia, the eucaryotic initiation factor 2 activity was reduced by 50% of control at 30 min of recirculation compared with 77% in normothermic animals. We conclude that the postischaemic depression of protein synthesis is in part caused by a decrease in eucaryotic initiation factor 2 activity.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

以[¹⁴C]-亮氨酸掺入蛋白质来衡量蛋白质合成,在短暂性脑缺血15分钟及再灌注1小时、24小时和48小时后的常温大鼠脑中进行了研究,以及在再灌注1小时和48小时后的低温(33℃)脑中进行了研究。缺血通过双侧颈总动脉闭塞联合低血压诱导。常温缺血后,在所有研究的脑区,再灌注1小时时[¹⁴C]-亮氨酸掺入量降低了40%-80%。缺血后48小时,新皮层内层、CA3区、纹状体和齿状回的掺入量恢复到正常或高于正常水平,而新皮层外层和海马CA1区的掺入量分别持续降低26%和40%。缺血后24小时和48小时,CA1区和纹状体中的蛋白质合成可归因于增殖的小胶质细胞。缺血期间低温改善了缺血后48小时CA1区蛋白质合成的持续抑制,并且在CA1区和纹状体中均观察到与常温组相比增加了两倍。在皮层中,真核起始因子2活性在缺血后30分钟短暂降低。在进行缺血期间低温的动物中,再灌注30分钟时真核起始因子2活性比对照组降低了50%,而常温动物中为77%。我们得出结论,缺血后蛋白质合成抑制部分是由真核起始因子2活性降低引起的。(摘要截短至250字)

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