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使用微载体大规模培养人视网膜色素上皮细胞。

Mass cultivation of human retinal pigment epithelial cells with microcarrier.

作者信息

Kuriyama S, Nakano T, Yoshimura N, Ohuchi T, Moritera T, Honda Y

机构信息

Departement of Ophthalmology, Kyoto University Faculty of Medicine, Japan.

出版信息

Ophthalmologica. 1992;205(2):89-95. doi: 10.1159/000310319.

Abstract

Microcarrier cell culture permits mass cultivation of anchorage-dependent cells. In this study, mass cultivation of human retinal pigment epithelial (RPE) cells was studied using Cytodex 3 (Pharmacia) as a microcarrier. Human RPE cells were established from aborted fetuses and cultured in Dulbecco's modified Eagle's Medium (DMEM). After the 3rd-5th passages, RPE cells were suspended in 50 ml of DMEM in a spinner flask at a density of 2 x 10(5)/ml, and Cytodex 3 was added to the spinner flask at a bead density of 10 mg/ml. Cultures were maintained at 20-50 rpm (final speed) on a magnetic stirrer, and DMEM was added up to 100 ml. Fifty milliliters of DMEM were decanted and replaced with fresh DMEM every 2 days. After 1 week, a cell density of 10(6)/ml DMEM was obtained. Phase contrast microscopy showed bridging formation between microcarriers, which suggests tight cell adhesion. Microcarrier cell culture has a variety of advantages which include greater cell production, use of less medium and less risk of contamination compared to the conventional monolayer culture technique, and it also allows passaging without using proteases. Using this culture system, greater possibilities for wider application of new cell cultures can be expected.

摘要

微载体细胞培养可实现贴壁依赖性细胞的大规模培养。在本研究中,使用Cytodex 3(Pharmacia公司)作为微载体对人视网膜色素上皮(RPE)细胞进行大规模培养。人RPE细胞取自流产胎儿,在杜氏改良 Eagle 培养基(DMEM)中培养。在第3至5代后,将RPE细胞以2×10⁵/ml的密度悬浮于50 ml DMEM中,置于转瓶中,并以10 mg/ml的珠密度向转瓶中加入Cytodex 3。在磁力搅拌器上以20 - 50 rpm(最终速度)维持培养,并将DMEM补充至100 ml。每2天倾析50 ml DMEM并用新鲜DMEM替换。1周后,获得了10⁶/ml DMEM的细胞密度。相差显微镜显示微载体之间形成桥接,这表明细胞紧密粘附。与传统的单层培养技术相比,微载体细胞培养具有多种优点,包括更高的细胞产量、更少的培养基使用量和更低的污染风险,并且它还允许在不使用蛋白酶的情况下传代。使用这种培养系统,可以预期新细胞培养物更广泛应用的更大可能性。

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