从子宫切除标本中建立原代人子宫内膜基质细胞的两种方法。
Two methods for establishing primary human endometrial stromal cells from hysterectomy specimens.
作者信息
Jividen Kasey, Movassagh Mercedeh Javanbakht, Jazaeri Amir, Li Hui
机构信息
Department of Pathology, University of Virginia.
Department of Obstetrics & Gynecology, University of Virginia.
出版信息
J Vis Exp. 2014 May 23(87):51513. doi: 10.3791/51513.
Abstract
Many efforts have been devoted to establish in vitro cell culture systems. These systems are designed to model a vast number of in vivo processes. Cell culture systems arising from human endometrial samples are no exception. Applications range from normal cyclic physiological processes to endometrial pathologies such as gynecological cancers, infectious diseases, and reproductive deficiencies. Here, we provide two methods for establishing primary endometrial stromal cells from surgically resected endometrial hysterectomy specimens. The first method is referred to as "the scraping method" and incorporates mechanical scraping using surgical or razor blades whereas the second method is termed "the trypsin method." This latter method uses the enzymatic activity of trypsin to promote the separation of cells and primary cell outgrowth. We illustrate step-by-step methodology through digital images and microscopy. We also provide examples for validating endometrial stromal cell lines via quantitative real time polymerase chain reactions (qPCR) and immunofluorescence (IF).
摘要
人们为建立体外细胞培养系统付出了诸多努力。这些系统旨在模拟大量的体内过程。源自人子宫内膜样本的细胞培养系统也不例外。其应用范围涵盖从正常的周期性生理过程到子宫内膜病变,如妇科癌症、传染病和生殖缺陷等。在此,我们提供两种从手术切除的子宫切除标本中建立原代子宫内膜基质细胞的方法。第一种方法称为“刮除法”,采用手术刀片或剃须刀片进行机械刮除,而第二种方法称为“胰蛋白酶法”。后一种方法利用胰蛋白酶的酶活性来促进细胞分离和原代细胞生长。我们通过数字图像和显微镜展示了逐步的方法。我们还提供了通过定量实时聚合酶链反应(qPCR)和免疫荧光(IF)验证子宫内膜基质细胞系的示例。
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