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影响暴露于低温环境下哺乳动物细胞存活的因素。IV. 铁螯合作用的影响。

Factors influencing survival of mammalian cells exposed to hypothermia. IV. Effects of iron chelation.

作者信息

Zieger M A, Glofcheski D J, Lepock J R, Kruuv J

机构信息

Guelph-Waterloo Program for Graduate Work in Physics, University of Waterloo, Ontario, Canada.

出版信息

Cryobiology. 1990 Aug;27(4):452-64. doi: 10.1016/0011-2240(90)90022-v.

Abstract

Survival of V-79 Chinese hamster cells was assessed by colony growth assay after hypothermic exposure in the presence of iron chelators. At 5 degrees C, maximum protection from hypothermic damage was achieved with a 50 microM concentration of the intracellular ferric iron chelator Desferal. A 3-hr prehypothermic incubation with 50 microM Desferal followed by replacement with chelator-free medium at 5 degrees C also provided some protection. This was not observed when the extracellular chelator DETA-PAC (50 microM) was used prior to cold storage. Treating 5 degrees C-stored cells with Desferal just prior to rewarming was ineffective, but treating cells with Desferal during hypothermia exposure after a significant period of unprotected cold exposure ultimately increased the surviving fraction. Submaximal protection during hypothermia was achieved to various degrees with extracellular chelators at 5 degrees C, including 50 microM DETAPAC and 110 microM EDTA. EGTA (110 microM) had little effect. The sensitization of cells at 5 degrees C with 200 microM FeCl3 could be reduced or eliminated with Desferal in accordance with a 1:1 binding ratio. At 10 degrees C, 50 microM Desferal, 50 microM DETAPAC, and 110 microM EDTA were as or less effective in protecting cells than at 5 degrees C. An Arrhenius plot of cell inactivation rates shows a break at 7-8 degrees C, corresponding to maximum survival for control cells and cells in 50 microM Desferal; however, the amount of protection offered by the chelator increases with decreasing temperature below about 19 degrees C, and sensitization increases above that point. It has not previously been shown that iron chelators protect against cellular hypothermia damage which is uncomplicated by previous or simultaneous ischemia. This may be relevant to the low-temperature storage of transplant organs, in which iron of intracellular origin and in the perfusate may be active and damaging.

摘要

在存在铁螯合剂的情况下,通过集落生长试验评估V - 79中国仓鼠细胞在低温暴露后的存活率。在5℃时,细胞内三价铁螯合剂去铁胺浓度为50μM时,可实现对低温损伤的最大保护。在5℃下用50μM去铁胺进行3小时的低温预孵育,然后换成无螯合剂培养基,也能提供一定保护。在冷藏前使用细胞外螯合剂DETA - PAC(50μM)时未观察到这种情况。在复温前立即用去铁胺处理5℃保存的细胞无效,但在长时间无保护的冷暴露后,在低温暴露期间用去铁胺处理细胞最终增加了存活分数。在5℃时,细胞外螯合剂包括50μM DETAPAC和110μM EDTA在不同程度上实现了低温期间的亚最大保护。EGTA(110μM)几乎没有效果。根据1:1的结合比例,用50μM去铁胺可降低或消除200μM FeCl3对5℃细胞的致敏作用。在10℃时,50μM去铁胺、50μM DETAPAC和110μM EDTA对细胞的保护作用与在5℃时相同或更差。细胞失活率的阿伦尼乌斯图在7 - 8℃处出现断点,对应于对照细胞和处于50μM去铁胺中的细胞的最大存活率;然而,螯合剂提供的保护量随着温度降至约19℃以下而增加,在该温度以上致敏作用增加。以前尚未表明铁螯合剂可防止细胞低温损伤,这种损伤未因先前或同时存在的缺血而复杂化。这可能与移植器官的低温保存有关,其中细胞内来源的铁和灌注液中的铁可能具有活性并造成损害。

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