Bloom G S, Richards B W, Leopold P L, Ritchey D M, Brady S T
Department of Cell Biology and Neuroscience, University of Texas Southwestern Medical Center, Dallas 75235-9039.
J Cell Biol. 1993 Jan;120(2):467-76. doi: 10.1083/jcb.120.2.467.
Movements of membrane-bounded organelles through cytoplasm frequently occur along microtubules, as in the neuron-specific case of fast axonal transport. To shed light on how microtubule-based organelle motility is regulated, pharmacological probes for GTP-binding proteins, or protein kinases or phosphatases were perfused into axoplasm extruded from squid (Loligo pealei) giant axons, and effects on fast axonal transport were monitored by quantitative video-enhanced light microscopy. GTP gamma S caused concentration-dependent and time-dependent declines in organelle transport velocities. GDP beta S was a less potent inhibitor. Excess GTP, but not GDP, masked the effects of coperfused GTP gamma S. The effects of GTP gamma S on transport were not mimicked by broad spectrum inhibitors of protein kinases (K-252a) or phosphatases (microcystin LR and okadaic acid), or as shown earlier, by ATP gamma S. Therefore, suppression of organelle motility by GTP gamma S was guanine nucleotide-specific and evidently did not involve irreversible transfer of thiophosphate groups to protein. Instead, the data imply that organelle transport in the axon is modulated by cycles of GTP hydrolysis and nucleotide exchange by one or more GTP-binding proteins. Fast axonal transport was not perturbed by AlF4-, indicating that the GTP gamma S-sensitive factors do not include heterotrimeric G-proteins. Potential axoplasmic targets of GTP gamma S include dynamin and multiple small GTP-binding proteins, which were shown to be present in squid axoplasm. These collective findings suggest a novel strategy for regulating microtubule-based organelle transport and a new role for GTP-binding proteins.
膜结合细胞器在细胞质中的移动常常沿着微管发生,就像在快速轴突运输这种神经元特有的情况中一样。为了阐明基于微管的细胞器运动是如何被调控的,将针对GTP结合蛋白、蛋白激酶或磷酸酶的药理探针灌注到从鱿鱼(枪乌贼)巨大轴突中挤出的轴浆中,并通过定量视频增强光学显微镜监测对快速轴突运输的影响。GTPγS导致细胞器运输速度呈浓度依赖性和时间依赖性下降。GDPβS是一种效力较弱的抑制剂。过量的GTP而非GDP掩盖了共灌注的GTPγS的作用。GTPγS对运输的影响不能被蛋白激酶(K-252a)或磷酸酶(微囊藻毒素LR和冈田酸)的广谱抑制剂模拟,或者如之前所示,也不能被ATPγS模拟。因此,GTPγS对细胞器运动的抑制是鸟嘌呤核苷酸特异性的,显然不涉及硫代磷酸基团向蛋白质的不可逆转移。相反,数据表明轴突中的细胞器运输是由一个或多个GTP结合蛋白的GTP水解和核苷酸交换循环调节的。快速轴突运输不受AlF4-的干扰,表明对GTPγS敏感的因子不包括异源三聚体G蛋白。GTPγS潜在的轴浆靶点包括发动蛋白和多种小GTP结合蛋白,已证实在鱿鱼轴浆中存在这些蛋白。这些共同发现提示了一种调控基于微管的细胞器运输的新策略以及GTP结合蛋白的新作用。