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中等钙浓度决定永生化培养胸腺上皮细胞(TECs)中角蛋白中间丝的密度和分布。

Medium calcium concentration determines keratin intermediate filament density and distribution in immortalized cultured thymic epithelial cells (TECs).

作者信息

Sands Sandra S, Meek William D, Hayashi Jun, Ketchum Robert J

机构信息

Oklahoma State University Center for Health Sciences, College of Osteopathic Medicine, Department of Anatomy and Cell Biology, 1111 W. 17th Street, Tulsa, OK 74107, USA.

出版信息

Microsc Microanal. 2005 Aug;11(4):283-92. doi: 10.1017/S1431927605050282.

Abstract

Isolation and culture of thymic epithelial cells (TECs) using conventional primary tissue culture techniques under conditions employing supplemented low calcium medium yielded an immortalized cell line derived from the LDA rat (Lewis [Rt1l] cross DA [Rt1a]) that could be manipulated in vitro. Thymi were harvested from 4-5-day-old neonates, enzymically digested using collagenase (1 mg/ml, 37 degrees C, 1 h) and cultured in low calcium WAJC404A medium containing cholera toxin (20 ng/ml), dexamethasone (10 nM), epidermal growth factor (10 ng/ml), insulin (10 mug/ml), transferrin (10 mug/ml), 2% calf serum, 2.5% Dulbecco's Modified Eagle's Medium (DMEM), and 1% antibiotic/antimycotic. TECs cultured in low calcium displayed round to spindle-shaped morphology, distinct intercellular spaces (even at confluence), and dense reticular-like keratin patterns. In high calcium (0.188 mM), TECs formed cobblestone-like confluent monolayers that were resistant to trypsinization (0.05%) and displayed keratin intermediate filaments concentrated at desmosomal junctions between contiguous cells. Changes in cultured TEC morphology were quantified by an analysis of desmosome/membrane relationships in high and low calcium media. Desmosomes were significantly increased in the high calcium medium. These studies may have value when considering the growth conditions of cultured primary cell lines like TECs.

摘要

使用传统的原代组织培养技术,在添加低钙培养基的条件下分离和培养胸腺上皮细胞(TECs),得到了一种源自LDA大鼠(Lewis [Rt1l] 与DA [Rt1a] 的杂交种)的永生化细胞系,该细胞系可在体外进行操作。从4至5日龄的新生大鼠中采集胸腺,用胶原酶(1 mg/ml,37℃,1小时)进行酶消化,并在含有霍乱毒素(20 ng/ml)、地塞米松(10 nM)、表皮生长因子(10 ng/ml)、胰岛素(10 μg/ml)、转铁蛋白(10 μg/ml)、2%小牛血清、2.5% Dulbecco改良 Eagle培养基(DMEM)和1%抗生素/抗真菌剂的低钙WAJC404A培养基中培养。在低钙条件下培养的TECs呈现圆形到纺锤形的形态,细胞间有明显的间隙(即使在汇合时),以及密集的网状角蛋白模式。在高钙(0.188 mM)条件下,TECs形成鹅卵石样的汇合单层,对胰蛋白酶消化(0.05%)具有抗性,并显示角蛋白中间丝集中在相邻细胞之间的桥粒连接处。通过分析高钙和低钙培养基中桥粒/膜的关系,对培养的TEC形态变化进行了量化。高钙培养基中的桥粒显著增加。在考虑像TECs这样的原代培养细胞系的生长条件时,这些研究可能具有价值。

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