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成年小鼠表皮角质形成细胞外植体生长伴随分层上皮片的增殖和形成。

Concomitant proliferation and formation of a stratified epithelial sheet by explant outgrowth of epidermal keratinocytes from adult mice.

作者信息

Morris R J, Haynes A C, Fischer S M, Slaga T J

机构信息

University of Texas M. D. Anderson Cancer Center, Department of Carcinogenesis, Smithville 78957.

出版信息

In Vitro Cell Dev Biol. 1991 Nov;27A(11):886-95. doi: 10.1007/BF02630992.

Abstract

A chemically defined medium containing 1.2 mM Ca2+ has been developed for the culture of primary epidermal keratinocytes from untreated adult mice such that proliferation is accompanied by the formation of desmosomes and stratification. Cultured cutaneous explants of 1 mm2 from the backs of untreated, control, and carcinogen-exposed mice all demonstrated epithelial outgrowth within 1 wk, and by 5 wk approached confluence with characteristics of terminal differentiation such as desmosomes and stratification. Addition of 12-O-tetradecanoylphorbol-13-acetate (TPA) to the medium in concentrations of 0.001, 0.01, and 0.1 micrograms/ml resulted in a delay of approximately 1 wk in the outgrowth of the explants compared with the acetone controls and in a 30% decrease in the diameter of the epithelial outgrowth at 3 wk. The inhibition in outgrowth was overcome at higher concentrations (0.5, 1.0, and 10 micrograms/ml TPA). No obvious differences in morphology or in the rate of epidermal outgrowth within a 5-wk interval among explants from normal untreated epidermis, epidermis from mice treated with acetone, or epidermis from mice treated with an initiating application of 7,12-dimethylbenz[a]anthracene were observed. The defined composition of this medium and its ability to support reproducibly and conveniently both proliferation and differentiation of normal as well as treated primary adult murine epidermal cells suggest that it should be useful for a number of studies not previously possible that are relevant to the biology of the skin, to toxicology, and to carcinogenesis in the murine model system.

摘要

一种含有1.2 mM Ca2+的化学成分明确的培养基已被开发出来,用于培养未处理的成年小鼠的原代表皮角质形成细胞,使得细胞增殖伴随着桥粒的形成和分层。从未处理的对照小鼠和接触致癌物的小鼠背部获取的1 mm2皮肤外植体在1周内均显示出上皮细胞生长,到5周时接近汇合,具有终末分化的特征,如桥粒和分层。向培养基中添加浓度为0.001、0.01和0.1微克/毫升的12-O-十四酰佛波醇-13-乙酸酯(TPA),与丙酮对照组相比,外植体的生长延迟约1周,且在3周时上皮生长直径减少30%。在较高浓度(0.5、1.0和10微克/毫升TPA)下,生长抑制被克服。在5周的时间间隔内,未观察到来自正常未处理表皮的外植体、用丙酮处理的小鼠表皮外植体或用起始剂量的7,12-二甲基苯并[a]蒽处理的小鼠表皮外植体在形态或表皮生长速率上有明显差异。这种培养基明确的成分及其能够可重复且方便地支持正常以及处理过的原代成年小鼠表皮细胞的增殖和分化,表明它对于许多以前无法进行的与皮肤生物学、毒理学以及小鼠模型系统中的致癌作用相关的研究应该是有用的。

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