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Role of alpha 3 beta 1 integrin in tubulogenesis of Madin-Darby canine kidney cells

机译:Role of alpha 3 beta 1 integrin in tubulogenesis of madin-Darby canine kidney cells

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摘要

Background. We isolated several Madin-Darby canine kidney: (MDCK) subclones that exhibit different degrees of branching tubulogenesis in lower concentrations of collagen gel. The M634 clone formed cell aggregates in 0.3% collagen gel, but developed branching tubules vigorously in 0.1% collagen gel. In contrast, the Y224 clone formed cysts in 0.3% collagen gel and displayed fewer branching structures in 0.1% collagen eel. Morphologically, M634 cells exhibited higher levels of cell scattering as well as collagen-induced cell migration than Y224. We conducted this study to delineate the underlying mechanism of branching tubulogenesis in M634 cells. Methods. Components of the focal contact machinery were analyzed in both cell lines, including the extracellular matrix glycoproteins fibronectin, laminin, and vitronectin; cytoskeleton-associated elements a-actinin. talin, and vinculin: and receptors for extracellular matrix and alpha (2), alpha (3), alpha (5), alpha (8), beta (1), and beta (3) integrins. Furthermore, we established several stable transfectants of alpha (3) integrin antisense RNA in M634 cells to examine the role of alpha (3)beta (1), integrin in branching morphogenesis directly;. Results. There were no obvious differences in levels of the focal adhesion complex proteins between M634 and Y224 cells, except that the content of the alpha (3) and beta (1) integrins were 1.2- and 0.6-fold higher in M634 cells, respectively. The expression of alpha (3) integrin antisense RNA significantly lowered the levels of alpha (3) integrin mRNA and protein. The potential of cell scattering, migration, and branching tubulogenesis in M634 cells was inhibited according to the decrease in alpha (3) integrin expression. Conclusion. Our data indicate that expression of alpha (3)beta (1) integrin regulates cell scattering. migration, and branching tubulogenesis of RIDGE; cells. possibly via adhesion to or serving as a signaling molecule for type I collagen.
机译:背景。我们分离了几个Madin-Darby犬肾:(MDCK)亚克隆,在较低浓度的胶原蛋白凝胶中表现出不同程度的分支微管生成。 M634克隆在0.3%的胶原蛋白凝胶中形成细胞聚集体,但在0.1%的胶原蛋白凝胶中剧烈发育出分支小管。相反,Y224克隆在0.3%的胶原蛋白凝胶中形成囊肿,而在0.1%的胶原鳗鱼中显示较少的分支结构。形态上,与Y224相比,M634细胞表现出更高水平的细胞分散以及胶原蛋白诱导的细胞迁移。我们进行了这项研究来描述M634细胞中分支微管生成的潜在机制。方法。在两种细胞系中均分析了焦点接触机制的成分,包括细胞外基质糖蛋白纤连蛋白,层粘连蛋白和玻连蛋白。细胞骨架相关元素α-肌动蛋白。 talin和vinculin:以及胞外基质和alpha(2),alpha(3),alpha(5),alpha(8),beta(1)和beta(3)整合素的受体。此外,我们在M634细胞中建立了几种稳定的α(3)整合素反义RNA转染子,以直接检测α(3)β(1),整合素在分支形态发生中的作用。结果。在M634和Y224细胞之间,粘着斑复合蛋白的水平没有明显差异,只是在M634细胞中,α(3)和β(1)整合素的含量分别高出1.2倍和0.6倍。 α(3)整合素反义RNA的表达大大降低了α(3)整合素mRNA和蛋白质的水平。根据α(3)整合素表达的减少,抑制了M634细胞中细胞散布,迁移和分支微管生成的潜力。结论。我们的数据表明,α(3)β(1)整合素的表达调节细胞散射。 RIDGE的迁移和分支微管发生;细胞。可能通过粘附或充当I型胶原的信号分子。

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