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人皮脂腺细胞在体外的渐进性分化表现为细胞大小增加、抗原表达改变,并受培养时间和类视黄醇调节。

Progressive differentiation of human sebocytes in vitro is characterized by increasing cell size and altering antigen expression and is regulated by culture duration and retinoids.

作者信息

Zouboulis C C, Krieter A, Gollnick H, Mischke D, Orfanos C E

机构信息

Department of Dermatology, University Medical Center Steglitz, Free University of Berlin, Germany.

出版信息

Exp Dermatol. 1994 Aug;3(4):151-60. doi: 10.1111/j.1600-0625.1994.tb00271.x.

Abstract

Increasing cell size, lipid accumulation, and altered antigen expression are features of sebaceous differentiation in vivo. Enhanced lipid synthesis with progressive differentiation is also present in cultured human sebocytes. This study was conducted to investigate the evolution of cell size and antigen expression of human sebocytes with progressive differentiation in vitro. Subconfluent human sebocyte cultures were examined for sebocyte differentiation evaluated on cytocentrifuge preparations by light microscopy and classified in stages according to morphological criteria described for sebocytes in vivo. Rates of 5.1 +/- 2.2% undifferentiated sebocytes, 29.2 +/- 4.9% early differentiated, 20.7 +/- 4.1% advanced differentiated, 37.6 +/- 6.4% fully differentiated, and 5.9 +/- 1.9% mature sebocytes were calculated in secondary cultures. The size of cultured sebocytes measured by computer-assisted planimetry significantly increased with progressive differentiation up to 4-5.5 times. The low rates of mature sebocytes and the only moderate increase of their size with progressive differentiation indicate an incomplete terminal differentiation in vitro. Sebocytes were subsequently stained with a series of monoclonal antibodies (mAb) to determine antigen expression using the alkaline phosphatase anti-alkaline phosphatase technique. The number of sebocytes labeled with the anti-keratin mAb CK8.12 and KL1, and the mAb 34D11 (82 kD protein) increased with progressive differentiation; significant differences were found after comparing early and advanced differentiated sebocytes. Sebocytes were positively stained with the anti-keratin mAb 6B10 (K 4), RPN1162 (K 7), CK13 (K 13), RPN1165 (K 19), CK8.60, and the mAb 115F5 (MAM-6c), OM-1 (sebaceous gland antigen), and 24F10 (basic polypeptides) only at late-stage differentiation. The expression of keratins 4, 7, 13, and 19 was confirmed by gel electrophoresis and immunoblotting. The data obtained were used to study the effects of the duration of cultivation and of the retinoids isotretinoin and tretinoin on sebocyte differentiation in vitro. Subcultivation of sebocytes upregulated, and treatment with isotretinoin but not with tretinoin downregulated labeling with mAb which recognize indicating progressive and late-stage differentiation.

摘要

细胞大小增加、脂质蓄积以及抗原表达改变是体内皮脂腺分化的特征。在培养的人皮脂腺细胞中也存在随着分化进程脂质合成增强的现象。本研究旨在探讨体外培养的人皮脂腺细胞随着分化进程细胞大小和抗原表达的演变。对亚汇合的人皮脂腺细胞培养物进行检查,通过光学显微镜在细胞离心涂片上评估皮脂腺细胞分化情况,并根据体内皮脂腺细胞的形态学标准进行分期。在传代培养物中计算出未分化皮脂腺细胞的比例为5.1±2.2%,早期分化的为29.2±4.9%,晚期分化的为20.7±4.1%,完全分化的为37.6±6.4%,成熟皮脂腺细胞的为5.9±1.9%。通过计算机辅助平面测量法测量的培养皮脂腺细胞大小随着分化进程显著增加,可达4 - 5.5倍。成熟皮脂腺细胞比例较低且随着分化进程其大小仅适度增加,表明体外存在不完全的终末分化。随后用一系列单克隆抗体(mAb)对皮脂腺细胞进行染色,采用碱性磷酸酶抗碱性磷酸酶技术确定抗原表达。用抗角蛋白单克隆抗体CK8.12、KL1以及单克隆抗体34D(82kD蛋白)标记的皮脂腺细胞数量随着分化进程增加;在比较早期和晚期分化的皮脂腺细胞后发现显著差异。皮脂腺细胞仅在分化后期被抗角蛋白单克隆抗体6B10(K4)、RPN1162(K7)、CK13(K13)、RPN1165(K19)、CK8.60以及单克隆抗体115F5(MAM - 6c)、OM - 1(皮脂腺抗原)和24F10(碱性多肽)阳性染色。角蛋白4、7、13和19的表达通过凝胶电泳和免疫印迹得到证实。所获得的数据用于研究培养时间以及维甲酸类药物异维甲酸和维甲酸对体外皮脂腺细胞分化的影响。皮脂腺细胞传代培养上调了表达,而异维甲酸处理而非维甲酸处理下调了用识别渐进性和晚期分化的单克隆抗体的标记。

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