尼替卡酮体外抑制髓过氧化物酶,提高实验性心脏移植缺血8 h后的功能表现。

A E Vento, O J Rämö, A T Nemlander, M Ahotupa, E Nissinen, A Holopainen, S P Mattila
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引用次数: 2

摘要

尼替卡酮(NC)已被证明对langendorff制剂大鼠心脏功能恢复有有益作用。本研究旨在评估NC对心脏移植中移植物保存的影响以及NC在抑制粒细胞浸润中的作用。在+4℃条件下,将供心灌注于对照组(C组,n = 26)或添加林格液的NC(50微米)中(NC组,n = 18),保存8 h。行异位心脏移植。两组大鼠分别在主动脉钳释放后10分钟或60分钟处死,并获得组织样本进行抗氧化能力、髓过氧化物酶活性和脂质过氧化测定。体外研究使用叠氮化钠或尼替卡酮来抑制分离的人白细胞的髓过氧化物酶(MPO)活性。nc组有61%的移植物开始跳动,而对照组为46%。使用任意的功能表现量表,对照组中只有33%(4/12)的移植物被归类为功能良好,而nc组为82% (9/11)
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Nitecapone inhibits myeloperoxidase in vitro and enhances functional performance after 8 h of ischemia in experimental heart transplantation.

Nitecapone (NC) has been shown to have beneficial effects on the functional recovery of rat hearts in Langendorff-preparation. The present study was executed to evaluate the effect of NC on preservation of grafts in heart transplantation and the role of NC in the inhibition of granulocyte infiltration. Donor hearts were perfused and stored at +4 degrees C for 8 h in either Ringer solution in the control-group (C-group, n = 26) or in NC (50 microM) added Ringer solution (NC-group, n = 18). The heterotopic heart transplantation was performed. The rats in both groups were killed at either 10 min or 60 min after release of the aortic clamp and tissue samples were obtained for antioxidative capacity, myeloperoxidase activity, and lipid peroxidation measurements. In vitro studies were performed using sodium azide or nitecapone to inhibit myeloperoxidase (MPO) activity of isolated human leukocytes. A total of 61% of the grafts began to beat in the NC-group, compared to 46% in the control group. Using an arbitrary scale of functional performance, only 33% (4/12) of the grafts were classified as well functioning in the control group, compared to 82% (9/11) in the NC-group (P<0.05). MPO activity was equal in both groups after 10 min but significantly lower after 60 min in the NC-group as compared to the control group (P<0.05). In vitro studies demonstrated that NC inhibits 50% of purified MPO activity at a concentration of 10 microM. NC did not significantly affect lipid peroxidation or the preservation of endogenous antioxidants. Since NC inhibited myeloperoxidase both in vitro and in vivo, it seems that the positive effects of NC on graft preservation may be mediated via the inhibition of granulocyte infiltration.

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