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首页> 外文期刊>Journal of Virological Methods >In vitro cultivation and cryopreservation of duck embryonic hepatocytes
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In vitro cultivation and cryopreservation of duck embryonic hepatocytes

机译:鸭胚胎肝细胞的体外培养和冷冻保存

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Hepatitis B-virucidal testing of biocides in quantitative suspension tests using duck hepatitis B virus (DHBV) requires primary duck embryonic hepatocytes for viral propagation. To improve the test system and availability of these cells, commercial culture plates with different growth surfaces were tested for cell cultivation and different approaches for cryopreservation of hepatocyte suspension were examined. After 12 days of culture, the largest amounts of hepatocytes were grown in CellBIND and TTP plates and CellBIND surface showed the lowest tendency of monolayer detachment nearly comparable with collagen 1-coated CELLCOAT plates. For cryopreservation of hepatocyte suspension, the use of growth medium supplemented with fetal calf serum (FCS) and dimethyl sulfoxide (ME sub(2)SO), FCS supplemented with ME sub(2)SO or cryosafe-1 as cryoprotective agents provided the highest rates of surviving cells after thawing. The freezing-thawing process did not significantly reduce the susceptibility of hepatocytes to infection with DHBV. In conclusion, plates without collagen 1 such as CellBIND are recommended for cultivation of primary duck embryonic hepatocytes in infectivity experiments of DHBV for virucidal testing of biocides. The use of cryopreserved hepatocytes is possible when freshly isolated cells from the liver of duck embryos are not available.
机译:在使用鸭乙型肝炎病毒(DHBV)进行的定量悬浮液测试中,对乙肝病毒进行杀生物剂杀伤性测试需要原代鸭胚肝细胞进行病毒繁殖。为了改善测试系统和这些细胞的可用性,测试了具有不同生长表面的商业培养板进行细胞培养,并研究了冷冻保存肝细胞悬液的不同方法。培养12天后,最大数量的肝细胞在CellBIND和TTP平板中生长,CellBIND表面显示出最低的单层分离趋势,几乎与胶原1涂层CELLCOAT平板相当。对于肝细胞悬液的冷冻保存,使用添加了胎牛血清(FCS)和二甲基亚砜(ME sub(2)SO),添加有ME sub(2)SO或cryosafe-1的FCS作为冷冻保护剂的生长培养基提供了最高的保护解冻后存活细胞的比率。冻融过程并未显着降低肝细胞对DHBV感染的敏感性。总之,在DHBV的感染性实验中,建议使用不含胶原蛋白1的板(如CellBIND)培养原代鸭胚胎肝细胞,以进行杀生物剂的杀伤性测试。当无法从鸭胚肝脏中分离出新鲜分离的细胞时,可以使用冷冻保存的肝细胞。

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