微重力模拟条件下酿酒酵母菌活性氧和谷胱甘肽测定方法的验证

T. Hammond, P. Allen, H. Birdsall
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引用次数: 4

摘要

太空飞行对酵母的影响与诱导极低细胞内氧化还原状态和诱导大量谷胱甘肽外排的药物高度一致。这些结果提出了重要的问题。太空飞行过程中还原的氧化还原状态能否在地面模拟中重现和调制?这是否允许定义独特的药物途径,因为低氧化还原电位状态反映了许多药物代谢的线粒体的亲电特性?不幸的是,氧化还原状态及其主要细胞决定因素-谷胱甘肽-的测定方法是多种多样的,通常是细胞类型特异性的。目前,一个公认的氧化还原探针设置酵母的研究是不可用的。本文验证了酵母中谷胱甘肽和活性氧状态的荧光探针,以支持微重力和药物代谢的机制研究。过多的荧光试剂用于活性氧和谷胱甘肽使得所有替代品的直接比较不切实际。这些试剂测量活性氧和各种硫醇的生理环境,而不是特定的单个分子。我们报道,在酵母中,单氯比曼(mBCL)和2 ',7 ' -二氯二氢荧光素二乙酸酯(DC-FDA)分别适用于谷胱甘肽和活性氧的荧光和流式细胞术研究。这两种染料具有低背景荧光,可预测的负载,良好的保留率,并且对酿酒酵母没有急性毒性。这两种染料与其他荧光和生化分析结果一致。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Validation of Assays for Reactive Oxygen Species and Glutathione in Saccharomyces cerevisiae during Microgravity Simulation
ABSTRACT The effects of spaceflight on yeast have high concordance with agents that induce a very low intracellular redox state and induce a massive efflux of glutathione. These results raise important issues. Can the reduced redox state during spaceflight be reproduced and modulated in ground-based simulations? Will this allow definition of unique drug pathways as a low redox potential state mirrors the electrophilic properties of mitochondria where many drugs are metabolized? Unfortunately, assays for redox status and its major cellular determinant—glutathione—are diverse and often cell-type-specific. Currently, an accepted redox probe set for yeast studies is not available. This paper validates fluorescent probes for glutathione and reactive oxygen status in yeast to support mechanistic studies of microgravity and drug metabolism. The plethora of fluorescent reagents for reactive oxygen species and glutathione makes head-to-head comparisons of all the alternatives impractical. These reagents measure the physiological milieu of reactive oxygen species and diverse thiols, rather than specific individual molecules. We report that in yeast, monochlorobimane (mBCL) and 2’,7’-dichlorodihydrofluorescein diacetate (DC-FDA) are suitable for fluorometric and flow cytometry studies of glutathione and reactive oxygen species, respectively. Both dyes have low background fluorescence, predictable loading, good retention, and are not acutely toxic to Saccharomyces cerevisiae. Both dyes show concordance with other fluorescent and biochemical assays of reactive oxygen species.
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