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作为分化和细胞外钙离子浓度的函数,体内和体外小鼠角质形成细胞中组成型细胞色素P-450表达的调节。

Modulation of constitutive cytochrome P-450 expression in vivo and in vitro in murine keratinocytes as a function of differentiation and extracellular Ca2+ concentration.

作者信息

Reiners J J, Cantu A R, Pavone A

机构信息

University of Texas M.D. Anderson Cancer Center, Science Park-Research Division, Smithville 78957.

出版信息

Proc Natl Acad Sci U S A. 1990 Mar;87(5):1825-9. doi: 10.1073/pnas.87.5.1825.

DOI:10.1073/pnas.87.5.1825
PMID:2308941
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC53576/
Abstract

A procedure was developed for the per cell estimation of cytochrome P-450-dependent monooxygenase activities in cultures and whole cell suspensions of murine epidermal keratinocytes (MEKs). Murine keratinocytes cultured in medium containing less than or equal to 0.04 mM Ca2+ can be induced to differentiate by raising medium Ca2+ concentrations to 1.2 mM. The per cell activities of the monooxygenases 7-ethoxyresorufin O-deethylase (7-ER) and 7-ethoxycoumarin O-deethylase (7-EC) were elevated greater than or equal to 2090% and approximately 460%, respectively, within 13-24 hr of Ca2+ shift. These increases could be completely suppressed by supplementation of culture medium with actinomycin D or cycloheximide immediately prior to Ca2+ shift. After prolonged culture in low Ca2+ medium, some MEKs detached from the monolayer. These detached cells had the characteristics of differentiating MEKs but did not have elevated 7-EC or 7-ER activities. Percoll gradient centrifugation of freshly isolated dorsal skin MEKs was used to prepare four subpopulations that differed in their stages of terminal differentiation. 7-EC and 7-ER activities varied among these subpopulations and correlated with the degree of MEK differentiation. Specifically, the lowest and highest per cell activities (greater than 7-fold difference) were in the basal and most differentiated spinous cell populations, respectively. Collectively, the current studies demonstrate that in vivo P-450 activities are markedly different in proliferating and differentiating MEKs and suggest that constitutive P-450 expression may be modulated as a function of changes in Ca2+ concentration that occur during keratinocyte terminal differentiation.

摘要

已开发出一种程序,用于对小鼠表皮角质形成细胞(MEK)培养物和全细胞悬液中细胞色素P-450依赖性单加氧酶活性进行单细胞水平的评估。在含有小于或等于0.04 mM Ca2+的培养基中培养的小鼠角质形成细胞,可通过将培养基Ca2+浓度提高到1.2 mM诱导分化。在Ca2+浓度改变后的13至24小时内,单加氧酶7-乙氧基异吩恶唑酮O-脱乙基酶(7-ER)和7-乙氧基香豆素O-脱乙基酶(7-EC)的单细胞活性分别提高了大于或等于2090%和约460%。在Ca2+浓度改变之前立即向培养基中添加放线菌素D或环己酰亚胺,可完全抑制这些增加。在低Ca2+培养基中长时间培养后,一些MEK从单层中脱离。这些脱离的细胞具有分化中MEK的特征,但7-EC或7-ER活性并未升高。使用Percoll梯度离心法对新鲜分离的背部皮肤MEK进行处理,以制备四个终末分化阶段不同的亚群。7-EC和7-ER活性在这些亚群中有所不同,且与MEK的分化程度相关。具体而言,单细胞活性最低和最高的(相差7倍以上)分别是基底细胞群和分化程度最高的棘细胞群。总体而言,当前研究表明,在增殖和分化的MEK中,体内P-450活性存在显著差异,并提示组成型P-450表达可能作为角质形成细胞终末分化过程中Ca2+浓度变化的函数而受到调节。

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本文引用的文献

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Induction of mouse epidermal ornithine decarboxylase activity and skin tumors by 7,12-dimethylben.7,12-二甲基苯诱导小鼠表皮鸟氨酸脱羧酶活性及皮肤肿瘤
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Benzo(a)pyrene metabolism in primary cultures of mouse epidermal cells and untransformed and transformed epidermal cell lines.苯并(a)芘在小鼠表皮细胞原代培养物以及未转化和转化的表皮细胞系中的代谢。
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