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胆固醇硫酸酯激活多种蛋白激酶C同工酶,并诱导培养的小鼠角质形成细胞中的颗粒细胞分化。

Cholesterol sulfate activates multiple protein kinase C isoenzymes and induces granular cell differentiation in cultured murine keratinocytes.

作者信息

Denning M F, Kazanietz M G, Blumberg P M, Yuspa S H

机构信息

Laboratory of Cellular Carcinogenesis and Tumor Promotion, National Cancer Institute, Bethesda, Maryland 20892, USA.

出版信息

Cell Growth Differ. 1995 Dec;6(12):1619-26.

PMID:9019167
Abstract

The accumulation of cholesterol sulfate (CS) in differentiating keratinocytes coincides with the expression of protein kinase C (PKC)-regulated granular layer differentiation markers both in vitro and in vivo. In this study, we examined the ability of Cs to induce differentiation marker expression in primary mouse keratinocytes and to modulate keratinocyte PKC isozymes (alpha, delta, epsilon, eta, and sigma). Treatment of basal keratinocytes with CS induced the expression of the granular layer proteins filaggrin and loricrin and decreased the level of the spinous keratin K1. CS stimulated cornification and blocked the induction of K10 in keratinocytes induced to differentiate by calcium. The induction of filaggrin and loricrin by CS corresponds to a granular layer differentiation program, where PKC activation occurs and was blocked by the PKC inhibitor GF 109203X. Treatment of keratinocytes with CS caused PKC epsilon, eta, and sigma to be selectively lost from the cytosol fraction and increased in the cytoskeletal fraction. The loss of soluble PKC epsilon, eta, and sigma was rapid (1 h) and sustained (44 h). PKC alpha and delta were not redistributed. In vitro, CS induced kinase activity of PKC epsilon, eta, and sigma to a greater extent than did the phorbol ester 12-O-tetradecanoylphorbol-13-acetate for these isoforms. PKC alpha and delta were activated to a lesser extent by CS than by 12-O-tetradecanoylphorbol-13-acetate. The translocation of PKC epsilon, eta, and sigma in intact cells treated with CS, together with the in vitro activation of recombinant PKC epsilon, eta, and sigma preferentially by CS, suggests a role for these isoforms in the induction of keratinocyte differentiation by CS.

摘要

硫酸胆固醇(CS)在分化的角质形成细胞中的积累与蛋白激酶C(PKC)调节的颗粒层分化标志物在体外和体内的表达相一致。在本研究中,我们检测了CS诱导原代小鼠角质形成细胞中分化标志物表达以及调节角质形成细胞PKC同工酶(α、δ、ε、η和σ)的能力。用CS处理基底角质形成细胞可诱导颗粒层蛋白聚丝蛋白和兜甲蛋白的表达,并降低棘层角蛋白K1的水平。CS刺激角质化,并阻断钙诱导分化的角质形成细胞中K10的诱导。CS诱导聚丝蛋白和兜甲蛋白的表达对应于颗粒层分化程序,其中PKC激活发生,并被PKC抑制剂GF 109203X阻断。用CS处理角质形成细胞导致PKCε、η和σ从胞质部分选择性丢失,并在细胞骨架部分增加。可溶性PKCε、η和σ的丢失迅速(1小时)且持续(44小时)。PKCα和δ没有重新分布。在体外,对于这些同工型,CS比佛波酯12-O-十四酰佛波醇-13-乙酸酯更能诱导PKCε、η和σ的激酶活性。与12-O-十四酰佛波醇-13-乙酸酯相比,CS对PKCα和δ的激活程度较低。CS处理的完整细胞中PKCε、η和σ的易位,以及CS优先对重组PKCε、η和σ的体外激活,表明这些同工型在CS诱导角质形成细胞分化中起作用。

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