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A role for microwave processing in the dry preservation of mammalian cells

机译:微波处理在哺乳动物细胞干保存中的作用

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Dry preservation involves removing water from samples so that degradative biochemical processes are slowed and extended storage is possible. Recently this approach has been explored as a method for preserving living mammalian cells. The current work explores the use of microwave processing to enhance evaporation rates and to improve drying uniformity, thereby overcoming some of the challenges in this field. Mouse macrophage cells (J774) were pre-incubated in full complement media containing 50 mM trehalose, for 18-h, to allow for endocytosis of trehalose. Droplets of experimental and control (no intracellular trehalose) cell suspensions were placed on coverslips in a microwave cavity. Water was evaporated using intermittent microwave heating (600 W, 30 s intervals). Samples were dried to various moisture levels, rehydrated, and then survival was assessed after a 45-min recovery period using Calcein-AM/PI fluorescence and Trypan Blue exclusion assays. The metabolic activity of dried cells (4.3 gH(2)O/gdw) was assessed after rehydration using a resazurin reduction assay. Apoptosis levels were also measured. Post-rehydration survival correlated with the final moisture content achieved, consistent with other drying methods. Intracellular trehalose provided protection against injury associated with moisture loss. Metabolic assays revealed normal growth in surviving cells, and these survival levels were consistent with results from apoptosis assays (P > 0.05). Brightfield and fluorescence images of microwave-dried samples revealed a uniform distribution of cells within the dried matrix and profilometry analysis demonstrated that solids were uniformly distributed throughout the sample. Microwave-processing successfully facilitated rapid and uniform dehydration of cell-based samples.
机译:干燥保存涉及从样品中除去水,从而减慢降解性生化过程并可能延长存储时间。最近,已经探索了这种方法作为保存活的哺乳动物细胞的方法。当前的工作探索了使用微波处理来提高蒸发速率并改善干燥均匀性,从而克服了该领域的一些挑战。将小鼠巨噬细胞(J774)在含有50 mM海藻糖的全补体培养基中预孵育18小时,以允许海藻糖内吞。将实验和对照(无细胞内海藻糖)细胞悬液的液滴置于微波腔中的盖玻片上。使用间歇微波加热(600 W,30 s间隔)蒸发水。将样品干燥至各种水分含量,再水化,然后在45分钟的恢复期后使用钙黄绿素-AM / PI荧光和锥虫蓝排除法评估存活率。使用刃天青素还原试验在补液后评估干细胞的代谢活性(4.3 gH(2)O / gdw)。还测量了细胞凋亡水平。补液后的存活率与最终获得的水分含量相关,与其他干燥方法一致。细胞内海藻糖可防止水分流失造成的伤害。代谢测定显示存活细胞正常生长,这些存活水平与凋亡测定的结果一致(P> 0.05)。微波干燥样品的明场和荧光图像显示干燥基质中细胞的均匀分布,轮廓分析表明固体在整个样品中均匀分布。微波处理成功地促进了基于细胞的样品的快速且均匀的脱水。

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