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人卵巢细胞的原代培养及mRNA分析

Primary culture and mRNA analysis of human ovarian cells.

作者信息

Dunfield Lesley D., Shepherd Trevor G., Nachtigal Mark W.

机构信息

Department of Pharmacology, Dalhousie University. Halifax, Nova Scotia B3H 4H7. Canada.

出版信息

Biol Proced Online. 2002 Oct 28;4:55-61. doi: 10.1251/bpo34.

Abstract

Established cell lines are invaluable for studying cell and molecular biological questions. A variety of human ovarian cancer (OC) cell lines exist, however, most have acquired significant genetic alterations from their cells of origin, including deletion of important cell cycle regulatory genes. In order to analyze signaling events related to cell cycle control in human OC, we have modified existing protocols for isolating and culturing OC cells from patient ascites fluid and normal ovarian surface epithelial (OSE) cells from benign ovarian tissue sections. These cells maintain an epithelial phenotype and can be manipulated experimentally for several passages before cellular senescence. An example using TGFb1 treatment of OC cells to examine signaling and target gene activation is presented.

摘要

已建立的细胞系对于研究细胞和分子生物学问题非常宝贵。目前存在多种人类卵巢癌(OC)细胞系,然而,大多数细胞系已从其起源细胞获得了显著的基因改变,包括重要细胞周期调控基因的缺失。为了分析与人类OC细胞周期控制相关的信号事件,我们修改了现有方案,用于从患者腹水分离和培养OC细胞,以及从良性卵巢组织切片分离和培养正常卵巢表面上皮(OSE)细胞。这些细胞保持上皮表型,并且在细胞衰老之前可以通过实验操作传代培养几代。本文展示了一个使用TGFb1处理OC细胞以检测信号传导和靶基因激活的实例。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3ee0/145557/1aa7ddc29d47/m34f1lg.jpg

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