肌动蛋白结合域通过与特定肌动蛋白丝亚群的不同亲和力,介导了两个 Dictyostelium Talin 在定向细胞迁移过程中的不同分布。
Actin-binding domains mediate the distinct distribution of two Dictyostelium Talins through different affinities to specific subsets of actin filaments during directed cell migration.
机构信息
Electron Microscope Laboratory, RIKEN, Center for Developmental Biology, 2-2-3 Minatojima-minamimachi, Chuo-ku, Kobe, Japan.
Department of Physics, Faculty of Science and Technology, Waseda University, Tokyo, Japan.
出版信息
PLoS One. 2019 Apr 4;14(4):e0214736. doi: 10.1371/journal.pone.0214736. eCollection 2019.
Although the distinct distribution of certain molecules along the anterior or posterior edge is essential for directed cell migration, the mechanisms to maintain asymmetric protein localization have not yet been fully elucidated. Here, we studied a mechanism for the distinct localizations of two Dictyostelium talin homologues, talin A and talin B, both of which play important roles in cell migration and adhesion. Using GFP fusion, we found that talin B, as well as its C-terminal actin-binding region, which consists of an I/LWEQ domain and a villin headpiece domain, was restricted to the leading edge of migrating cells. This is in sharp contrast to talin A and its C-terminal actin-binding domain, which co-localized with myosin II along the cell posterior cortex, as reported previously. Intriguingly, even in myosin II-null cells, talin A and its actin-binding domain displayed a specific distribution, co-localizing with stretched actin filaments. In contrast, talin B was excluded from regions rich in stretched actin filaments, although a certain amount of its actin-binding region alone was present in those areas. When cells were sucked by a micro-pipette, talin B was not detected in the retracting aspirated lobe where acto-myosin, talin A, and the actin-binding regions of talin A and talin B accumulated. Based on these results, we suggest that talin A predominantly interacts with actin filaments stretched by myosin II through its C-terminal actin-binding region, while the actin-binding region of talin B does not make such distinctions. Furthermore, talin B appears to have an additional, unidentified mechanism that excludes it from the region rich in stretched actin filaments. We propose that these actin-binding properties play important roles in the anterior and posterior enrichment of talin B and talin A, respectively, during directed cell migration.
虽然某些分子沿着前后边缘的独特分布对定向细胞迁移至关重要,但维持不对称蛋白定位的机制尚未完全阐明。在这里,我们研究了两种 Dictyostelium talin 同源物(talin A 和 talin B)的独特定位机制,它们在细胞迁移和黏附中都发挥着重要作用。使用 GFP 融合,我们发现 talin B 及其包含 I/LWEQ 结构域和 villin 头部结构域的 C 端肌动蛋白结合结构域仅限于迁移细胞的前缘。这与 talin A 及其 C 端肌动蛋白结合结构域形成鲜明对比,此前报道称该结构域与肌球蛋白 II 一起沿细胞后皮质共定位。有趣的是,即使在肌球蛋白 II 缺失的细胞中,talin A 及其肌动蛋白结合结构域也表现出特定的分布,与伸展的肌动蛋白丝共定位。相反,talin B 被排除在富含伸展的肌动蛋白丝的区域之外,尽管在这些区域中存在一定量的其肌动蛋白结合结构域。当细胞被微吸管抽吸时,talin B 不会在回缩的抽吸叶中被检测到,该区域积聚了肌球蛋白 II、talin A 和 talin A 和 talin B 的肌动蛋白结合区域。基于这些结果,我们认为 talin A 主要通过其 C 端肌动蛋白结合结构域与肌球蛋白 II 伸展的肌动蛋白丝相互作用,而 talin B 的肌动蛋白结合结构域则不做这样的区分。此外,talin B 似乎具有一种额外的、未知的机制,将其排除在富含伸展的肌动蛋白丝的区域之外。我们提出,这些肌动蛋白结合特性分别在定向细胞迁移中对 talin B 和 talin A 的前后富集起着重要作用。
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