大鼠库普弗细胞的分离与原代培养。

Isolation and primary culture of rat Kupffer cells.

作者信息

Olynyk J K, Clarke S L

机构信息

University Department of Medicine, Fremantle Hospital, Western Australia, Australia.

出版信息

J Gastroenterol Hepatol. 1998 Aug;13(8):842-5. doi: 10.1111/j.1440-1746.1998.tb00746.x.

DOI:10.1111/j.1440-1746.1998.tb00746.x

PMID:9736181

Abstract

The aim of this study was to describe a reproducible method for the isolation, purification and primary culture of rat Kupffer cells. Kupffer cells were isolated following sequential pronase/collagenase digestion of the liver and enrichment of a non-parenchymal cell fraction by a single-density gradient centrifugation step using 30% metrizamide. Kupffer cells were isolated and further purified from this cell fraction by centrifugal elutriation. Kupffer cells were isolated at 1017 g at 48-110 mL/min. All Kupffer cell fractions exhibited phagocytosis of 3 microm latex beads. Kupffer cell fractions isolated at 48 and 60 mL/min were predominantly ED2 negative while later fractions (80-110 mL/min) were ED2 positive. Kupffer cells were adherent in culture after 2 h. This method for Kupffer cell isolation resulted in a yield of 80-120 x 10(6) Kupffer cells per liver.

摘要

本研究的目的是描述一种可重复的大鼠库普弗细胞分离、纯化和原代培养方法。通过用链霉蛋白酶/胶原酶对肝脏进行顺序消化，并使用30%的甲泛葡胺通过单密度梯度离心步骤富集非实质细胞部分来分离库普弗细胞。通过离心淘洗从该细胞部分中分离并进一步纯化库普弗细胞。在48 - 110 mL/分钟的流速下，以1017 g的离心力分离库普弗细胞。所有库普弗细胞部分均表现出对3微米乳胶珠的吞噬作用。在48和60 mL/分钟流速下分离的库普弗细胞部分主要为ED2阴性，而后来的部分（80 - 110 mL/分钟）为ED2阳性。库普弗细胞在培养2小时后贴壁。这种库普弗细胞分离方法每只肝脏可产生80 - 120×10⁶个库普弗细胞。

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大鼠库普弗细胞的分离与原代培养。

Isolation and primary culture of rat Kupffer cells.

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