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Introduction of a novel prototype bioartificial liver support system utilizing small human hepatocytes in rotary culture.

机译:介绍了一种新型的生物人工肝支持系统原型,该系统利用小型人肝细胞进行了旋转培养。

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The aim of this study was to establish a stand-alone, perfused, rotary cell culture system using small human hepatocytes (SH) for bioartificial liver (BAL) support. SH were grown on cytodex 3 microcarriers (beads) to a maximum density of 1.2 +/- 0.3 x 10(7) cells per mL within 12 days. Size of aggregates formed by up to 15 beads was regulated by rotation speed. Cell function was proven by treatment with ammonia and galactose, and metabolism was analyzed. Treatment strategy was comprised of two phases, namely growth phase and treatment phase. Cells were grown for 6 days and subsequently incubated with ammonia or galactose for 2 days, followed by a 2-day regeneration period and another 2-day treatment phase. Consumption of glucose, release of lactate dehydrogenase, formation of lactate, and production of urea and albumin were determined regularly. Mean galactose consumption was 50 microg per 106 cells per hour, ammonia-induced urea formation was 3.6 microg per 106 cells per hour, and albumin production was 110 ng per 106 cells per hour. All metabolic parameters followed a logarithmic trend and were found to be very stable in the second half of the culture period when cells were treated with ammonia or galactose. Dissolved oxygen (%DO), pH, and temperature were monitored in-stream at intervals of 7 min, and the values were logged. Viability and morphology of cells were monitored via confocal microscopy. Viability was around 95% in controls and 90% during treatment. Promising results were obtained in support of our ongoing efforts to establish a fully autonomous BAL support device utilizing SH as a bridge to transplantation.
机译:这项研究的目的是建立一个使用小型人肝细胞(SH)来支持生物人工肝(BAL)的独立的灌注旋转细胞培养系统。 SH在cytodex 3微载体(珠子)上生长,在12天内达到每毫升1.2 +/- 0.3 x 10(7)个细胞的最大密度。由多达15个珠子形成的聚集体的大小由转速调节。通过用氨和半乳糖处理证明细胞功能,并分析代谢。治疗策略包括两个阶段,即生长阶段和治疗阶段。细胞生长6天,然后与氨水或半乳糖一起温育2天,随后是2天的再生期和另一个2天的处理阶段。定期测定葡萄糖的消耗,乳酸脱氢酶的释放,乳酸的形成以及尿素和白蛋白的产生。平均半乳糖消耗量为每106个细胞每小时50微克,氨诱导的尿素形成为每106个细胞每小时3.6微克,白蛋白产量为每106个细胞每小时110 ng。当用氨或半乳糖处理细胞时,所有代谢参数都遵循对数趋势,并且在培养期的后半段非常稳定。以7分钟的间隔对流中的溶解氧(%DO),pH和温度进行监控,并记录值。通过共聚焦显微镜监测细胞的活力和形态。对照中的生存力约为95%,治疗期间的生存力为90%。获得了可喜的成果,以支持我们为建立利用SH作为移植桥梁的完全自主的BAL支持设备而进行的不懈努力。

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