维生素E和EDTA提高低温治疗的疗效-细胞凋亡的影响。

In vitro & molecular toxicology Pub Date : 1999-01-01
Mathew, Hollister, Addona, Baust, Van Buskirk RG
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引用次数: 0

摘要

工程组织和新细胞株的出现要求我们探索可以在不使用冷冻保存的情况下将这些细胞和组织储存在接近假死状态的解决方案。低温溶液ViaSpan(杜邦默克制药公司,Wilmington, DE), HypoThermosol (crymedical Sciences, Rockville, MD), HypoThermosol添加乙二胺四乙酸(EDTA)或维生素E, HypoThermosol添加凋亡蛋白酶抑制剂,在4℃下测试其冷保护Madin Darby犬肾(MDCK)细胞的能力。Alamar Blue是一种无毒的代谢指标,用于测量细胞活力。低温防护效果依次为:维生素E + EDTA低温溶胶>维生素E低温溶胶> EDTA低温溶胶> ViaSpan低温溶胶> Dulbecco's Modified Eagle's Medium (DMEM)。膜完整性测试支持Alamar Blue数据,EDTA和维生素E赋予低温溶胶的冷藏能力。低温保存1 - 6天后死亡的MDCK细胞从基质中分离出来,在37℃下放置后收集其DNA。将这些DNA与在相同培养物中低温保存后存活的贴壁细胞中提取的DNA进行比较。低温保存1 ~ 4天死亡的细胞凝胶电泳显示DNA阶梯,表明细胞通过凋亡死亡,即程序性细胞死亡。然而,在冷藏5至6天后收获的死亡细胞具有随机分裂的DNA,表明坏死细胞死亡。添加凋亡蛋白酶抑制剂的低温溶胶比碱性低温溶胶具有更好的冷保护细胞的能力。这些数据表明,在未来的冷藏配方中应考虑抑制细胞凋亡。
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Vitamin E and EDTA Improve the Efficacy of Hypothermosol-Implication of Apoptosis.

The emergence of engineered tissues and new cell strains has called for the need to explore solutions that can be used to store these cells and tissues in a state of near suspended animation without using cryopreservation. The ability of the hypothermic solutions ViaSpan (DuPont Merck Pharmaceutical Company, Wilmington, DE), HypoThermosol (Cryomedical Sciences, Rockville, MD), HypoThermosol supplemented with either ethylenediaminetetraacetic acid (EDTA) or Vitamin E and HypoThermosol supplemented with apoptosis protease inhibitors were tested for their abilities to cold-protect Madin Darby Canine Kidney (MDCK) cells at 4 degrees C. Alamar Blue, a nontoxic metabolic indicator was used to measure cell viability. The order of cold protection was HypoThermosol with Vitamin E and EDTA > HypoThermosol with Vitamin E > HypoThermosol with EDTA > HypoThermosol > ViaSpan > Dulbecco's Modified Eagle's Medium (DMEM). Membrane integrity tests supported the Alamar Blue data that EDTA and Vitamin E conferred a benefit to the cold-storage capabilities of HypoThermosol. MDCK cells that died subsequent to 1 to 6 days cold-storage detached from the substratum and their DNA was harvested after being placed at 37 degrees C. This DNA was compared to DNA retrieved from adherent cells in the same cultures that survived the cold-storage regime. Gel electrophoresis of cells dying due to 1 to 4 days of cold-storage showed a DNA ladder indicating that cells died through apoptosis, programmed cell death. Dead cells harvested at 5 to 6 days of cold storage, however, had randomly cleaved DNA indicative of necrotic cell death. HypoThermosol supplemented with apoptosis protease inhibitors was better able to cold-protect cells than the base HypoThermosol. These data suggest that the inhibition of apoptosis should be considered in the future cold-storage formulations.

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