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在体外重建的人表皮中,loricrin的表达受视黄酸的负调控。

Expression of loricrin is negatively controlled by retinoic acid in human epidermis reconstructed in vitro.

作者信息

Magnaldo T, Bernerd F, Asselineau D, Darmon M

机构信息

Cell Biology Department, Centre International de Recherches Dermatologiques Galderma (CIRD Galderma), Valbonne, France.

出版信息

Differentiation. 1992 Jan;49(1):39-46. doi: 10.1111/j.1432-0436.1992.tb00767.x.

Abstract

In epidermis, the last steps of keratinocyte differentiation are characterized by the covalent cross-linking of cornified envelope precursors such as involucrin and loricrin, a hydrophobic protein recently described in mouse and human epidermis. In situ hybridization of normal human skin sections with a human loricrin cRNA probe and immunolabeling with an antiserum directed against a synthetic peptide corresponding to the carboxyterminus of human loricrin revealed the presence of loricrin transcripts and protein in the granular layers of epidermis. In human epidermis reconstructed in vitro by growing keratinocytes on dermal equivalents, loricrin and loricrin mRNAs were also restricted to granular cells, but their amounts seemed higher than in epidermis from skin biopsies. The reactivities for both loricrin and loricrin mRNAs were abolished by a treatment of the cultures with a retinoic acid concentration (10(-6) M) provoking a complete inhibition of terminal epidermal differentiation (parakeratosis). Thus, the regulation of loricrin synthesis is different from that of another envelope precursor, involucrin, which does not seem to be significantly modulated by retinoic acid. Together with the well-documented inhibition of epidermal transglutaminase by retinoic acid, our results provide a molecular basis for the inhibition of cornified envelope formation by retinoic acid.

摘要

在表皮中,角质形成细胞分化的最后步骤的特征是角质包膜前体(如内披蛋白和兜甲蛋白,一种最近在小鼠和人类表皮中发现的疏水蛋白)的共价交联。用人兜甲蛋白cRNA探针原位杂交正常人皮肤切片,并用针对对应于人兜甲蛋白羧基末端的合成肽的抗血清进行免疫标记,结果显示在表皮颗粒层中存在兜甲蛋白转录本和蛋白质。在通过在真皮替代物上培养角质形成细胞而体外重建的人表皮中,兜甲蛋白和兜甲蛋白mRNA也局限于颗粒细胞,但它们的含量似乎高于皮肤活检获得的表皮中的含量。用能完全抑制终末表皮分化(角化不全)的视黄酸浓度(10^(-6) M)处理培养物后,兜甲蛋白和兜甲蛋白mRNA的反应性均消失。因此,兜甲蛋白合成的调节不同于另一种包膜前体内披蛋白的调节,内披蛋白似乎不受视黄酸的显著调节。与视黄酸对表皮转谷氨酰胺酶的抑制作用已得到充分证明一样,我们的结果为视黄酸抑制角质包膜形成提供了分子基础。

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