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利用蓖麻毒素A亚基筛选法纯化培养的原代大鼠肝细胞。

Purification of cultured primary rat hepatocytes using selection with ricin A subunit.

作者信息

Johnston D E, Jasuja R

机构信息

Department of Medicine, New England Medical Center, Boston, Massachusetts.

出版信息

Hepatology. 1994 Aug;20(2):436-44.

PMID:8045505
Abstract

We had found several methods of hepatocyte isolation to be inadequate for removing Kupffer and endothelial cells and so developed a method of selectively killing these nonparenchymal cells in hepatocyte cultures using the known selective uptake and toxicity of the protein synthesis inhibitor ricin and its A chain by nonparenchymal cells. Kupffer cells were quantitated with the Ku-1 monoclonal antibody. Endothelial and Kupffer cells were identified by means of fluorescence microscopy after uptake of fluorescent-labeled, acetylated low-density lipoprotein. Freshly isolated hepatocyte suspensions contained 21% +/- 1.2% (mean +/- S.E.M.) as many nonparenchymal cells as hepatocytes (n = 12), including 7.6% +/- 1.0% as many Kupffer cells as hepatocytes (n = 10). In monolayers of hepatocytes maintained up to 48 hr in serum-free medium, 3% to 7% of cells were Ku-1 positive, and 2% to 11% took up fluorescence-labeled, acetylated low-density lipoprotein. Purification of hepatocytes using Percoll densitygradient centrifugation, elutriation rotor or other means was only partially effective. Hepatocyte monolayers in serum-free medium were incubated with various concentrations of ricin A chain for 1 hr, then washed and studied up to 48 hr later. Optimal treatment with 1.0 ng/ml ricin A chain resulted in decreased nonparenchymal cells 24 hr later and nearly complete loss of Kupffer and endothelial cells at 48 hr. Hepatocyte morphology and protein synthesis were unchanged. Ricin A chain can be used to eliminate Kupffer and endothelial cells from hepatocyte cultures.

摘要

我们发现几种肝细胞分离方法在去除库普弗细胞和内皮细胞方面并不充分,因此开发了一种方法,利用蛋白质合成抑制剂蓖麻毒素及其A链被非实质细胞的已知选择性摄取和毒性,在肝细胞培养物中选择性杀死这些非实质细胞。用Ku-1单克隆抗体对库普弗细胞进行定量。在摄取荧光标记的乙酰化低密度脂蛋白后,通过荧光显微镜鉴定内皮细胞和库普弗细胞。新鲜分离的肝细胞悬液中,非实质细胞数量是肝细胞的21%±1.2%(平均值±标准误)(n = 12),其中库普弗细胞数量是肝细胞的7.6%±1.0%(n = 10)。在无血清培养基中维持长达48小时的肝细胞单层中,3%至7%的细胞为Ku-1阳性,2%至11%的细胞摄取荧光标记的乙酰化低密度脂蛋白。使用Percoll密度梯度离心、淘洗转子或其他方法纯化肝细胞仅部分有效。将无血清培养基中的肝细胞单层与不同浓度的蓖麻毒素A链孵育1小时,然后洗涤并在48小时后进行研究。用1.0 ng/ml蓖麻毒素A链进行最佳处理,24小时后非实质细胞数量减少,48小时时库普弗细胞和内皮细胞几乎完全消失。肝细胞形态和蛋白质合成未改变。蓖麻毒素A链可用于从肝细胞培养物中消除库普弗细胞和内皮细胞。

相似文献

1
Purification of cultured primary rat hepatocytes using selection with ricin A subunit.利用蓖麻毒素A亚基筛选法纯化培养的原代大鼠肝细胞。
Hepatology. 1994 Aug;20(2):436-44.
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Stimulation of prostaglandin synthesis in cultured liver cells by CCl4.四氯化碳对培养肝细胞中前列腺素合成的刺激作用。
Hepatology. 1996 Sep;24(3):677-84. doi: 10.1002/hep.510240334.
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Isolated Kupffer cells, endothelial cells and hepatocytes as investigative tools for liver research.分离的库普弗细胞、内皮细胞和肝细胞作为肝脏研究的工具。
Fed Proc. 1981 Aug;40(10):2460-8.
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Lab Invest. 1981 Dec;45(6):567-74.
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Increased nitric oxide synthase activity as a cause of mitochondrial dysfunction in rat hepatocytes: roles for tumor necrosis factor alpha.一氧化氮合酶活性增加作为大鼠肝细胞线粒体功能障碍的一个原因:肿瘤坏死因子α的作用
Hepatology. 1996 Nov;24(5):1185-92. doi: 10.1002/hep.510240534.
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Morphogenetic events in mixed cultures of rat hepatocytes and nonparenchymal cells maintained in biological matrices in the presence of hepatocyte growth factor and epidermal growth factor.在肝细胞生长因子和表皮生长因子存在的情况下,维持于生物基质中的大鼠肝细胞与非实质细胞混合培养物中的形态发生事件。
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[The role of Kupffer cells in regulating protein synthesis in hepatocytes].
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Kupffer cells and not liver sinusoidal endothelial cells prevent lentiviral transduction of hepatocytes.库普弗细胞而非肝窦内皮细胞可阻止慢病毒转导肝细胞。
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[The role of hepatocytes, Kupffer, and endothelial cells of the liver in blood lipoprotein metabolism].[肝细胞、库普弗细胞及肝内皮细胞在血液脂蛋白代谢中的作用]
Biokhimiia. 1994 Mar;59(3):353-9.

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