Gilmore A P, Wood C, Ohanian V, Jackson P, Patel B, Rees D J, Hynes R O, Critchley D R
Department of Biochemistry, University of Leicester, England.
J Cell Biol. 1993 Jul;122(2):337-47. doi: 10.1083/jcb.122.2.337.
We have mapped the vinculin-binding sites in the cytoskeletal protein talin as well as those sequences which target the talin molecule to focal contacts. Using a series of overlapping talin-fusion proteins expressed in E. coli and 125I-vinculin in both gel-overlay and microtitre well binding assays, we present evidence for three separable binding sites for vinculin. All three are in the tail segment of talin (residues 434-2541) and are recognized by the same fragment of vinculin (residues 1-258). Two sites are adjacent to each other and span residues 498-950, and the third site is more than 700 residues distant in the primary sequence. Scatchard analysis of 125I-vinculin binding to talin also indicates three sites, each with a similar affinity (Kd = 2-6 x 10(-7) M). We also detect a substoichiometric interaction of higher affinity (Kd = 3 x 10(-8) M) which remains unexplained. By expressing regions of the chicken talin molecule in heterologous cells, we have shown that the sequences required to target talin to focal contacts overlap those which bind vinculin.
我们已绘制出细胞骨架蛋白踝蛋白中的纽蛋白结合位点,以及将踝蛋白分子靶向粘着斑的那些序列。通过在凝胶覆盖和微量滴定板结合试验中使用一系列在大肠杆菌中表达的重叠踝蛋白融合蛋白和125I-纽蛋白,我们提供了纽蛋白存在三个可分离结合位点的证据。所有这三个位点都在踝蛋白的尾部片段(残基434 - 2541)中,并且被纽蛋白的同一片段(残基1 - 258)识别。两个位点彼此相邻,跨越残基498 - 950,第三个位点在一级序列中距离超过700个残基。对125I-纽蛋白与踝蛋白结合的Scatchard分析也表明存在三个位点,每个位点具有相似的亲和力(Kd = 2 - 6×10^(-7) M)。我们还检测到一种亲和力更高(Kd = 3×10^(-8) M)的亚化学计量相互作用,其原因尚不清楚。通过在异源细胞中表达鸡踝蛋白分子的区域,我们已经表明将踝蛋白靶向粘着斑所需的序列与那些结合纽蛋白的序列重叠。
