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通过Dispase灌注从成年大鼠分离肝细胞的制备及原代培养。

Preparation and primary culture of liver cells isolated from adult rats by dispase perfusion.

作者信息

Wahid S, Miyazaki M, Sato J

出版信息

Acta Med Okayama. 1984 Jun;38(3):251-60. doi: 10.18926/AMO/30360.

Abstract

The dispase perfusion technique was used to isolate liver cells from adult rats. The optimum conditions for obtaining many isolated liver cells with high viability were an enzyme concentration of 2000 U/ml, a pH of 7.5 and a perfusion time of 20 min. The population of isolated liver cells prepared with dispase consisted of 43.6% cells with diameters less than 20 micron and 56.4% cells with diameters above 20 micron. The isolated liver cells were cultured in basal culture medium either supplemented with or without dexamethasone (1 X 10(-5)M) and insulin (10 micrograms/ml). The addition of hormones to the culture medium improved the attachment efficiency of the isolated liver cells and delayed the disappearance of mature hepatocytes. Epithelial-like clear cells proliferated early in primary culture even in the presence of hormones. Therefore, functioning mature hepatocytes and proliferating epithelial-like clear cells coexisted well in the hormone-containing medium. Furthermore, the number of cultured cells reached a maximal level earlier in the presence of hormones than in the absence of hormones. The level of TAT activity in primary cultured cells was higher up to 3 days after inoculation in the presence of hormones than in their absence. No difference between G6Pase activity in primary cultured cells in the presence of hormones and that in the absence of hormones was found.

摘要

采用分散酶灌注技术从成年大鼠中分离肝细胞。获得大量高活力分离肝细胞的最佳条件是酶浓度为2000 U/ml、pH值为7.5、灌注时间为20分钟。用分散酶制备的分离肝细胞群体由直径小于20微米的细胞(占43.6%)和直径大于20微米的细胞(占56.4%)组成。分离的肝细胞在基础培养基中培养,培养基中添加或不添加地塞米松(1×10⁻⁵M)和胰岛素(10微克/毫升)。向培养基中添加激素可提高分离肝细胞的贴壁效率,并延缓成熟肝细胞的消失。即使在有激素存在的情况下,上皮样透明细胞在原代培养早期也会增殖。因此,在含激素的培养基中,功能正常的成熟肝细胞和增殖的上皮样透明细胞能很好地共存。此外,与无激素时相比,有激素存在时培养细胞的数量更早达到最高水平。接种后3天内,有激素存在时原代培养细胞中的TAT活性水平高于无激素时。未发现有激素存在时与无激素时原代培养细胞中的G6Pase活性有差异。

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Effects of hormones on the activity of glucose-6-phosphatase in primary cultures of rat hepatocytes.
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