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细胞活力的原位评估。

In situ assessment of cell viability.

作者信息

Yang H, Acker J, Chen A, McGann L

机构信息

Department of Laboratory Medicine and Pathology, University of Alberta, Edmonton, Canada.

出版信息

Cell Transplant. 1998 Sep-Oct;7(5):443-51. doi: 10.1177/096368979800700503.

Abstract

Cryobiological studies of tissues often require the simultaneous assessment of tissue structure and in situ cellular function. Localization of damage during cryopreservation occurs as a consequence of tissue structure and morphology and as a result of biophysical constraints imposed by diffusion and heat transfer. This study used five experimental model tissue systems: cells in suspension, cells attached to a substrate, a monolayer of cells attached to a substrate, porcine corneas, and intact porcine articular cartilage to examine the efficacy of assessing cell recovery using a novel fluorescent stain (SYTO-13). A graded freezing protocol was used to induce varying degrees of tissue damage. Recovery was assessed in the different tissue model systems using SYTO with ethidium bromide, fluorescein diacetate (FDA) with ethidium bromide, and 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide (MTT). In each of the tissue model systems, the SYTO/EB assessment technique was shown to be equally effective as the existing techniques for the determination of cell recovery. In addition, the properties of fluorescence intensity and rate of release for SYTO were significantly better than those obtained using FDA. Assessment of in situ cell viability was clearly demonstrated using porcine corneas and articular cartilage. The SYTO/EB assay is superior to the existing techniques used for the localization of cell damage in tissues after cryopreservation.

摘要

组织的低温生物学研究通常需要同时评估组织结构和原位细胞功能。冷冻保存过程中的损伤定位是组织结构和形态的结果,也是扩散和热传递所施加的生物物理限制的结果。本研究使用了五种实验模型组织系统:悬浮细胞、附着于基质的细胞、附着于基质的单层细胞、猪角膜和完整的猪关节软骨,以检验使用新型荧光染料(SYTO-13)评估细胞恢复的效果。采用分级冷冻方案诱导不同程度的组织损伤。使用SYTO与溴化乙锭、荧光素二乙酸酯(FDA)与溴化乙锭以及3-(4,5-二甲基噻唑-2-基)-2,5-二苯基四氮唑溴盐(MTT)在不同的组织模型系统中评估恢复情况。在每个组织模型系统中,SYTO/EB评估技术在确定细胞恢复方面与现有技术同样有效。此外,SYTO的荧光强度和释放速率特性明显优于使用FDA获得的特性。使用猪角膜和关节软骨清楚地证明了原位细胞活力的评估。SYTO/EB检测优于冷冻保存后用于组织中细胞损伤定位的现有技术。

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