猪肝细胞球体制冷保存用于肝细胞球型生物人工肝。
Cold storage of porcine hepatocyte spheroids for spheroid bioartificial liver.
机构信息
Laboratory of Pathology, Key Laboratory of Transplant Engineering and Immunology, NHFPC, West China Hospital, Sichuan University, Chengdu, China.
Department of Surgery, Mayo Clinic, Rochester, Minnesota.
出版信息
Xenotransplantation. 2019 Jul;26(4):e12512. doi: 10.1111/xen.12512. Epub 2019 Apr 10.
BACKGROUND AND AIMS
Cell-based therapies for liver disease such as bioartificial liver rely on a large quantity and high quality of hepatocytes. Cold storage was previously shown to be a better way to preserve the viability and functionality of hepatocytes during transportation rather than freezing, but this was only proved at a lower density of rat hepatocytes spheroids. The purpose of this study was to optimize conditions for cold storage of high density of primary porcine hepatocyte spheroids.
METHODS
Porcine hepatocytes were isolated by a three-step perfusion method; hepatocyte spheroids were formed by a 24 hours rocked culture technique. Hepatocyte cell density was 5 × 10 /mL in 1000 mL spheroid forming medium. Spheroids were then maintained in rocked culture at 37°C (control condition) or cold stored at 4°C for 24, 48 or 72 hours in four different cold storage solutions: histidine-tryptophan-ketoglutarate (HTK) alone; HTK + 1 mM deferoxamine (DEF); HTK + 5 mM N-acetyl-L-cysteine (NAC); and HTK + 1 mM DEF + 5 mM NAC. The viability, ammonia clearance, albumin production, gene expression, and functional activity of cytochrome P450 enzymes were measured after recovery from the cold storage.
RESULTS
In this study, we observed that cold-induced injury was reduced by the addition of the iron chelator. Viability of HTK + DEF group hepatocyte spheroids was increased compared with other cold storage groups (P < 0.05). Performance metrics of porcine hepatocyte spheroids cold stored for 24 hours were similar to those in control conditions. The hepatocyte spheroids in control conditions started to lose their ability to clear ammonia while production of albumin was still active at 48 and 72 hours (P < 0.05). In contrast, the viability and functionality of hepatocyte spheroids including ammonia clearance and albumin secretion were preserved in HTK + DEF group at both 48- and 72-hour time points (P < 0.05).
CONCLUSIONS
The beneficial effects of HTK supplemented with DEF were more obvious after cold storage of high density of porcine hepatocyte spheroids for 72 hours. The porcine hepatocyte spheroids were above the cutoff criteria for use in a spheroid-based bioartificial liver.
背景与目的
细胞疗法治疗肝病(如生物人工肝)需要大量高质量的肝细胞。先前的研究表明,与冷冻相比,低温保存是在运输过程中更好地保持肝细胞活力和功能的方法,但这仅在较低密度的大鼠肝细胞球状体中得到证实。本研究的目的是优化高浓度原代猪肝细胞球状体低温保存的条件。
方法
采用三步灌流法分离猪肝细胞;采用 24 小时摇床培养技术形成肝细胞球状体。在 1000 毫升的球状体形成培养基中,肝细胞密度为 5×10 /mL。然后将球状体在 37°C 的摇床培养(对照条件)或在 4°C 下冷存 24、48 或 72 小时,在四种不同的低温保存液中:单独的组氨酸-色氨酸-酮戊二酸(HTK);HTK+1mM 去铁胺(DEF);HTK+5mM N-乙酰-L-半胱氨酸(NAC);和 HTK+1mM DEF+5mM NAC。从低温保存中恢复后,测量细胞活力、氨清除率、白蛋白产量、基因表达和细胞色素 P450 酶的功能活性。
结果
在这项研究中,我们观察到添加铁螯合剂可减少冷诱导损伤。与其他低温保存组相比,HTK+DEF 组的肝细胞球状体活力增加(P<0.05)。24 小时低温保存的猪肝细胞球状体的性能指标与对照条件相似。在 48 小时和 72 小时时,对照条件下的肝细胞球状体开始失去清除氨的能力,而白蛋白的产生仍很活跃(P<0.05)。相比之下,HTK+DEF 组的肝细胞球状体的活力和功能,包括氨清除率和白蛋白分泌,在 48 小时和 72 小时时均得到保留(P<0.05)。
结论
在对高浓度猪肝细胞球状体进行 72 小时低温保存后,HTK 补充 DEF 的有益效果更为明显。猪肝细胞球状体达到了基于球状体的生物人工肝使用的截止标准。
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