Döppler Heike, Storz Peter
Department of Cancer Biology; Mayo Clinic Comprehensive Cancer Center; Mayo Clinic; Jacksonville, FL USA.
Cell Adh Migr. 2013 Nov-Dec;7(6):482-6. doi: 10.4161/cam.27351. Epub 2013 Dec 5.
Phosphorylations control all aspects of vasodilator-stimulated phospho-protein (VASP) function. Mapped phosphorylation sites include Y39, S157, S239, T278, and S322, and multiple kinases have been shown to mediate their phosphorylation. Recently, Protein Kinase D1 (PKD1) as a direct kinase for S157 and S322 joined this group. While S157 phosphorylation generally seems to serve as a signal for membrane localization, phosphorylations at S322 or at S239 and T278 have opposite effects on F-actin accumulation. In migrating cells, S322 phosphorylation increases filopodia numbers and length, while S239/T278 phosphorylations decrease these and also disrupt formation of focal adhesions. Therefore, the kinases mediating these phosphorylations can be seen as switches needed to facilitate cell motility.
磷酸化作用控制着血管舒张刺激磷蛋白(VASP)功能的各个方面。已定位的磷酸化位点包括Y39、S157、S239、T278和S322,并且已证明多种激酶可介导它们的磷酸化。最近,蛋白激酶D1(PKD1)作为S157和S322的直接激酶加入了这一类别。虽然S157磷酸化通常似乎作为膜定位的信号,但S322或S239和T278处的磷酸化对F-肌动蛋白积累具有相反的作用。在迁移细胞中,S322磷酸化增加丝状伪足的数量和长度,而S239/T278磷酸化则减少这些并破坏粘着斑的形成。因此,介导这些磷酸化的激酶可被视为促进细胞运动所需的开关。
