首页> 外文期刊>In Vitro Cellular and Developmental Biology. Animal: Journal of the Tissues Culture Association >Topography of amphiregulin expression in cultured human keratinocytes: colocalization with the epidermal growth factor receptor and CD44.
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Topography of amphiregulin expression in cultured human keratinocytes: colocalization with the epidermal growth factor receptor and CD44.

机译:培养的人角质形成细胞中双调蛋白表达的地形:与表皮生长因子受体和CD44的共定位。

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Much of the autonomous growth of cultured keratinocytes is attributable to the signaling of amphiregulin, a heparin-binding autocrine growth factor, through the epidermal growth factor receptor. Emerging evidence suggests, moreover, that the membrane proteoglycan, CD44, is a cofactor for the interaction of heparin-binding ligands with their receptors. This model was evaluated by characterizing the patterns of the immunolabeled molecules in cultured human neonatal keratinocytes, to test the hypothesis that involvement in a common function results in coordinate segregation within or on the cell. The molecules were localized by double immunofluorescence labeling to detect amphiregulin and either the epidermal growth factor receptor or CD44, and the immunostained products were imaged by scanning laser confocal microscopy. Both amphiregulin and the epidermal growth factor receptor segregated to a perinuclear distribution and to intercellular contacts. In addition, amphiregulin localized to the outer leading edge of colonies and focally to intranuclear sites. Metabolic blockade of proteoglycan sulfation with sodium chlorate inhibited growth of the cells and concurrently enhanced the nuclear, but decreased the outer leading edge, labeling for amphiregulin. There was no nuclear or perimeter labeling for the epidermal growth factor receptor. Cultures co-immunolabeled for CD44 and amphiregulin exhibited variable perinuclear staining for both, but otherwise CD44 was distributed to intercellular contacts. The intercellular localizations of CD44 with amphiregulin and of amphiregulin with the epidermal growth factor receptor were strongly concordant. These data are consistent with a concerted function at intercellular contacts, where cytokine signaling is mediated via receptor binding and possibly regulated by the CD44 proteoglycan as cofactor. The intranuclear and perimeter labeling of amphiregulin, however, suggests that this cytokine has additional functions, both in the nucleus and as a matrix receptor.
机译:培养的角质形成细胞的大部分自主生长可归因于通过表皮生长因子受体的双调蛋白(肝素结合自分泌生长因子)的信号传导。此外,新兴证据表明,膜蛋白聚糖CD44是肝素结合配体与其受体相互作用的辅助因子。通过表征培养的人类新生儿角质形成细胞中免疫标记分子的模式来评估该模型,以检验以下假设:参与共同功能会导致细胞内或细胞上的坐标分离。通过双重免疫荧光标记对分子进行定位,以检测双调蛋白和表皮生长因子受体或CD44,并通过扫描激光共聚焦显微镜对免疫染色的产物成像。两性调节蛋白和表皮生长因子受体都分离成核周分布和细胞间接触。此外,双调蛋白定位于菌落的外部前缘,并集中于核内部位。用氯酸钠对蛋白聚糖硫酸盐进行的代谢阻断可抑制细胞生长并同时增强细胞核,但降低了外部前沿,标记为双调蛋白。表皮生长因子受体没有核或周边标记。共免疫标记的CD44和双调蛋白的培养物均显示可变的核周染色,但CD44分布在细胞间接触中。 CD44与两性调节蛋白和两性调节蛋白与表皮生长因子受体的细胞间定位是高度一致的。这些数据与细胞间接触的协调功能相一致,其中细胞因子信号传导是通过受体结合介导的,并可能由CD44蛋白聚糖作为辅因子调节。但是,两性调节蛋白的核内和周边标记表明该细胞因子在细胞核中和作为基质受体均具有其他功能。

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