Sakai N, Sasaki K, Ikegaki N, Shirai Y, Ono Y, Saito N
Laboratory of Molecular Pharmacology, Biosignal Research Center, Faculty of Science, Kobe University, Kobe 657, Japan.
J Cell Biol. 1997 Dec 15;139(6):1465-76. doi: 10.1083/jcb.139.6.1465.
We expressed the gamma-subspecies of protein kinase C (gamma-PKC) fused with green fluorescent protein (GFP) in various cell lines and observed the movement of this fusion protein in living cells under a confocal laser scanning fluorescent microscope. gamma-PKC-GFP fusion protein had enzymological properties very similar to that of native gamma-PKC. The fluorescence of gamma-PKC- GFP was observed throughout the cytoplasm in transiently transfected COS-7 cells. Stimulation by an active phorbol ester (12-O-tetradecanoylphorbol 13-acetate [TPA]) but not by an inactive phorbol ester (4alpha-phorbol 12, 13-didecanoate) induced a significant translocation of gamma-PKC-GFP from cytoplasm to the plasma membrane. A23187, a Ca2+ ionophore, induced a more rapid translocation of gamma-PKC-GFP than TPA. The A23187-induced translocation was abolished by elimination of extracellular and intracellular Ca2+. TPA- induced translocation of gamma-PKC-GFP was unidirected, while Ca2+ ionophore-induced translocation was reversible; that is, gamma-PKC-GFP translocated to the membrane returned to the cytosol and finally accumulated as patchy dots on the plasma membrane. To investigate the significance of C1 and C2 domains of gamma-PKC in translocation, we expressed mutant gamma-PKC-GFP fusion protein in which the two cysteine rich regions in the C1 region were disrupted (designated as BS 238) or the C2 region was deleted (BS 239). BS 238 mutant was translocated by Ca2+ ionophore but not by TPA. In contrast, BS 239 mutant was translocated by TPA but not by Ca2+ ionophore. To examine the translocation of gamma-PKC-GFP under physiological conditions, we expressed it in NG-108 cells, N-methyl-D-aspartate (NMDA) receptor-transfected COS-7 cells, or CHO cells expressing metabotropic glutamate receptor 1 (CHO/mGluR1 cells). In NG-108 cells , K+ depolarization induced rapid translocation of gamma-PKC-GFP. In NMDA receptor-transfected COS-7 cells, application of NMDA plus glycine also translocated gamma-PKC-GFP. Furthermore, rapid translocation and sequential retranslocation of gamma-PKC-GFP were observed in CHO/ mGluR1 cells on stimulation with the receptor. Neither cytochalasin D nor colchicine affected the translocation of gamma-PKC-GFP, indicating that translocation of gamma-PKC was independent of actin and microtubule. gamma-PKC-GFP fusion protein is a useful tool for investigating the molecular mechanism of gamma-PKC translocation and the role of gamma-PKC in the central nervous system.
我们在多种细胞系中表达了与绿色荧光蛋白(GFP)融合的蛋白激酶C的γ亚基(γ-PKC),并在共聚焦激光扫描荧光显微镜下观察了这种融合蛋白在活细胞中的移动情况。γ-PKC-GFP融合蛋白具有与天然γ-PKC非常相似的酶学特性。在瞬时转染的COS-7细胞中,γ-PKC-GFP的荧光在整个细胞质中都能观察到。活性佛波酯(12-O-十四酰佛波醇13-乙酸酯[TPA])刺激可诱导γ-PKC-GFP从细胞质向质膜的显著转位,而非活性佛波酯(4α-佛波醇12,13-十二烷酸酯)则无此作用。钙离子载体A23187诱导γ-PKC-GFP的转位比TPA更快。消除细胞外和细胞内的钙离子可消除A23187诱导的转位。TPA诱导的γ-PKC-GFP转位是单向的,而钙离子载体诱导的转位是可逆的;也就是说,转位到膜上后的γ-PKC-GFP会回到细胞质中,最终在质膜上聚集成斑状小点。为了研究γ-PKC的C1和C2结构域在转位中的意义,我们表达了突变型γ-PKC-GFP融合蛋白,其中C1区域的两个富含半胱氨酸的区域被破坏(命名为BS 238)或C2区域被缺失(BS 239)。BS 238突变体可被钙离子载体转位,但不能被TPA转位。相反,BS 239突变体可被TPA转位,但不能被钙离子载体转位。为了检测γ-PKC-GFP在生理条件下的转位,我们在NG-108细胞、转染了N-甲基-D-天冬氨酸(NMDA)受体的COS-7细胞或表达代谢型谷氨酸受体1的CHO细胞(CHO/mGluR1细胞)中表达了它。在NG-108细胞中,钾离子去极化诱导γ-PKC-GFP快速转位。在转染了NMDA受体的COS-7细胞中,应用NMDA加甘氨酸也可使γ-PKC-GFP转位。此外,在CHO/mGluR1细胞中,用受体刺激时可观察到γ-PKC-GFP的快速转位和随后的再转位。细胞松弛素D和秋水仙素均不影响γ-PKC-GFP的转位,这表明γ-PKC的转位与肌动蛋白和微管无关。γ-PKC-GFP融合蛋白是研究γ-PKC转位的分子机制以及γ-PKC在中枢神经系统中作用的有用工具。
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