角质形成细胞中α6β4整合素的动态变化
Dynamics of the alpha6beta4 integrin in keratinocytes.
作者信息
Geuijen Cecile A W, Sonnenberg Arnoud
机构信息
Division of Cell Biology, The Netherlands Cancer Institute, 1066 CX Amsterdam, The Netherlands.
出版信息
Mol Biol Cell. 2002 Nov;13(11):3845-58. doi: 10.1091/mbc.02-01-0601.
The integrin alpha6beta4 has been implicated in two apparently contrasting processes, i.e., the formation of stable adhesions, and cell migration and invasion. To study the dynamic properties of alpha6beta4 in live cells two different beta4-chimeras were stably expressed in beta4-deficient PA-JEB keratinocytes. One chimera consisted of full-length beta4 fused to EGFP at its carboxy terminus (beta4-EGFP). In a second chimera the extracellular part of beta4 was replaced by EGFP (EGFP-beta4), thereby rendering it incapable of associating with alpha6 and thus of binding to laminin-5. Both chimeras induce the formation of hemidesmosome-like structures, which contain plectin and often also BP180 and BP230. During cell migration and division, the beta4-EGFP and EGFP-beta4 hemidesmosomes disappear, and a proportion of the beta4-EGFP, but not of the EGFP-beta4 molecules, become part of retraction fibers, which are occasionally ripped from the cell membrane, thereby leaving "footprints" of the migrating cell. PA-JEB cells expressing beta4-EGFP migrate considerably more slowly than those that express EGFP-beta4. Studies with a beta4-EGFP mutant that is unable to interact with plectin and thus with the cytoskeleton (beta4(R1281W)-EGFP) suggest that the stabilization of the interaction between alpha6beta4 and LN-5, rather than the increased adhesion to LN-5, is responsible for the inhibition of migration. Consistent with this, photobleaching and recovery experiments revealed that the interaction of beta4 with plectin renders the bond between alpha6beta4 and laminin-5 more stable, i.e., beta4-EGFP is less dynamic than beta4(R1281W)-EGFP. On the other hand, when alpha6beta4 is bound to laminin-5, the binding dynamics of beta4 to plectin are increased, i.e., beta4-EGFP is more dynamic than EGFP-beta4. We suggest that the stability of the interaction between alpha6beta4 and laminin-5 is influenced by the clustering of alpha6beta4 through the deposition of laminin-5 underneath the cells. This clustering ultimately determines whether alpha6beta4 will inhibit cell migration or not.
整合素α6β4与两个明显相反的过程有关,即形成稳定黏附以及细胞迁移和侵袭。为了研究活细胞中α6β4的动态特性,两种不同的β4嵌合体在β4缺陷的PA-JEB角质形成细胞中稳定表达。一种嵌合体由全长β4在其羧基末端与EGFP融合组成(β4-EGFP)。在第二种嵌合体中,β4的细胞外部分被EGFP取代(EGFP-β4),从而使其无法与α6结合,进而不能与层粘连蛋白-5结合。两种嵌合体均诱导形成半桥粒样结构,其中含有网蛋白,且通常还含有BP180和BP230。在细胞迁移和分裂过程中,β4-EGFP和EGFP-β4半桥粒消失,一部分β4-EGFP分子(而非EGFP-β4分子)成为收缩纤维的一部分,收缩纤维偶尔会从细胞膜上撕裂,从而留下迁移细胞的“足迹”。表达β4-EGFP的PA-JEB细胞迁移速度明显慢于表达EGFP-β4的细胞。对一种无法与网蛋白相互作用从而无法与细胞骨架相互作用的β4-EGFP突变体(β4(R1281W)-EGFP)的研究表明,α6β4与LN-5之间相互作用的稳定,而非与LN-5黏附的增加,是迁移受到抑制的原因。与此一致的是,光漂白和恢复实验表明,β4与网蛋白的相互作用使α6β4与层粘连蛋白-5之间的结合更稳定,即β4-EGFP的动态性低于β4(R1281W)-EGFP。另一方面,当α6β4与层粘连蛋白-5结合时,β4与网蛋白的结合动态性增加,即β4-EGFP的动态性高于EGFP-β4。我们认为,α6β4与层粘连蛋白-5之间相互作用的稳定性受层粘连蛋白-5在细胞下方沉积导致的α6β4聚集的影响。这种聚集最终决定α6β4是否会抑制细胞迁移。
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