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首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >The cytoplasmic domain of L-selectin interacts with cytoskeletal proteins via alpha-actinin: receptor positioning in microvilli does not require interaction with alpha-actinin
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The cytoplasmic domain of L-selectin interacts with cytoskeletal proteins via alpha-actinin: receptor positioning in microvilli does not require interaction with alpha-actinin

机译:L-选择蛋白的胞质结构域通过α-肌动蛋白与细胞骨架蛋白相互作用:微绒毛中的受体定位不需要与α-肌动蛋白相互作用

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The leukocyte adhesion molecule L-selectin mediates binding to lymph node high endothelial venules (HEV) and contributes to leukocyte rolling on endothelium at sites of inflammation. Previously, it was shown that truncation of the L-selectin cytoplasmic tail by 11 amino acids abolished binding to lymph node HEV and leukocyte rolling in vivo, but the molecular basis for that observation was not determined. This study examined potential interactions between L-selectin and cytoskeletal proteins. We found that the cytoplasmic domain of L- selectin interacts directly with the cytoplasmic actin-binding protein alpha-actinin and forms a complex with vinculin and possibly talin. Solid phase binding assays using the full-length L-selectin cytoplasmic domain bound to microtiter wells demonstrated direct, specific, and saturable binding of purified alpha-actinin to L-selectin (Kd = 550 nM), but no direct binding of purified talin or vinculin. Interestingly, talin potentiated binding of alpha-actinin to the L- selectin cytoplasmic domain peptide despite the fact that direct binding of talin to L-selectin could not be measured. Vinculin binding to the L-selectin cytoplasmic domain peptide was detectable only in the presence of alpha-actinin. L-selectin coprecipitated with a complex of cytoskeletal proteins including alpha-actinin and vinculin from cells transfected with L-selectin, consistent with the possibility that alpha- actinin binds directly to L-selectin and that vinculin associates by binding to alpha-actinin in vivo to link actin filaments to the L- selectin cytoplasmic domain. In contrast, a deletion mutant of L- selectin lacking the COOH-terminal 11 amino acids of the cytoplasmic domain failed to coprecipitate with alpha-actinin or vinculin. Surprisingly, this mutant L-selectin localized normally to the microvillar projections on the cell surface. These data suggest that the COOH-terminal 11 amino acids of the L-selectin cytoplasmic domain are required for mediating interactions with the actin cytoskeleton via a complex of alpha-actinin and vinculin, but that this portion of the cytoplasmic domain is not necessary for proper localization of L- selectin on the cell surface. Correct L-selectin receptor positioning is therefore insufficient for leukocyte adhesion mediated by L- selectin, suggesting that this adhesion may also require direct interactions with the cytoskeleton.
机译:白细胞粘附分子L-选择蛋白介导与淋巴结高内皮小静脉(HEV)的结合,并有助于白细胞在炎症部位在内皮上滚动。先前已显示,L-选择蛋白胞质尾部被11个氨基酸截短可消除与淋巴结HEV的结合以及体内白细胞的滚动,但尚未确定该观察的分子基础。这项研究检查了L-选择蛋白和细胞骨架蛋白之间的潜在相互作用。我们发现,L-选择蛋白的胞质结构域与胞质肌动蛋白结合蛋白α-肌动蛋白直接相互作用,并与纽蛋白和塔林蛋白形成复合物。使用与微量滴定孔结合的全长L-选择蛋白胞质域的固相结合测定法证明了纯化的α-辅肌动蛋白与L-选择素的直接,特异性和饱和结合(Kd = 550 nM),但没有纯化的talin或talin的直接结合新蛋白。有趣的是,尽管无法测量出塔林蛋白与L-选择蛋白的直接结合,但塔林增强了α-肌动蛋白与L-选择蛋白胞质域肽的结合。仅在存在α-肌动蛋白的情况下,才能检测到结合于L-选择蛋白胞质域肽的长春花蛋白。 L-选择素与被L-选择素转染的细胞中的包括α-肌动蛋白和纽蛋白的细胞骨架蛋白共沉淀,这与α-肌动蛋白直接结合到L-选择素上以及纽蛋白在体内通过与α-肌动蛋白结合而缔合的可能性一致将肌动蛋白丝连接到L-选择蛋白胞质结构域。相反,缺少细胞质结构域的COOH-末端11个氨基酸的L-选择蛋白的缺失突变体不能与α-肌动蛋白或纽蛋白共沉淀。令人惊讶的是,该突变体L-选择蛋白通常定位于细胞表面上的微绒毛突起。这些数据表明,L-选择蛋白胞质结构域的COOH末端11个氨基酸是介导α-肌动蛋白和纽蛋白的复合体与肌动蛋白细胞骨架相互作用的必需物质,但是胞质结构域的这一部分对于适当的调节不是必需的。 L-选择蛋白在细胞表面的定位。因此,正确的L-选择蛋白受体定位不足以由L-选择蛋白介导的白细胞粘附,提示这种粘附可能还需要与细胞骨架的直接相互作用。

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