Baas P W, Ahmad F J
Department of Anatomy, University of Wisconsin Medical School, Madison 53706.
J Cell Biol. 1993 Mar;120(6):1427-37. doi: 10.1083/jcb.120.6.1427.
It is well established that axonal microtubules (MTs) are uniformly oriented with their plus ends distal to the neuronal cell body (Heidemann, S. R., J. M. Landers, and M. A. Hamborg. 1981. J. Cell Biol. 91:661-665). However, the mechanisms by which these MTs achieve their uniform polarity orientation are unknown. Current models for axon growth differ with regard to the contributions of MT assembly and transport to the organization and elaboration of the axonal MT array. Do the transport properties or assembly properties of axonal MTs determine their polarity orientation? To distinguish between these possibilities, we wished to study the initiation and outgrowth of axons under conditions that would arrest MT assembly while maintaining substantial levels of preexisting polymer in the cell body that could still be transported into the axon. We found that we could accomplish this by culturing rat sympathetic neurons in the presence of nanomolar levels of vinblastine. In concentrations of the drug up to and including 100 nM, the neurons actively extend axons. The vinblastine-axons are shorter than control axons, but clearly contain MTs. To quantify the effects of the drug on MT mass, we compared the levels of polymer throughout the cell bodies and axons of neurons cultured overnight in the presence of 0, 16, and 50 nM vinblastine with the levels of MT polymer in freshly plated neurons before axon outgrowth. Without drug, the total levels of polymer increase by roughly twofold. At 16 nM vinblastine, the levels of polymer are roughly equal to the levels in freshly plated neurons, while at 50 nM, the levels of polymer are reduced by about half this amount. Thus, 16 nM vinblastine acts as a "kinetic stabilizer" of MTs, while 50 nM results in some net MT disassembly. At both drug concentrations, there is a progressive increase in the levels of MT polymer in the axons as they grow, and a corresponding depletion of polymer from the cell body. These results indicate that highly efficient mechanisms exist in the neuron to transport preassembled MTs from the cell body into the axon. These mechanisms are active even at the expense of the cell body, and even under conditions that promote some MT disassembly in the neuron. MT polarity analyses indicate that the MTs within the vinblastine-axons, like those in control axons, are uniformly plus-end-distal.(ABSTRACT TRUNCATED AT 400 WORDS)
轴突微管(MTs)以其正端远离神经元细胞体的方式均匀排列,这一点已得到充分证实(海德曼,S.R.,J.M.兰德斯和M.A.汉伯格。1981年。《细胞生物学杂志》91:661 - 665)。然而,这些微管实现其均匀极性排列的机制尚不清楚。目前关于轴突生长的模型在微管组装和运输对轴突微管阵列的组织和细化的贡献方面存在差异。轴突微管的运输特性还是组装特性决定了它们的极性方向?为了区分这些可能性,我们希望在能阻止微管组装同时在细胞体中维持大量仍可运输到轴突中的预先存在的聚合物水平的条件下研究轴突的起始和生长。我们发现通过在纳摩尔水平的长春花碱存在下培养大鼠交感神经元可以实现这一点。在高达并包括100 nM的药物浓度下,神经元能积极延伸轴突。长春花碱处理的轴突比对照轴突短,但明显含有微管。为了量化药物对微管质量的影响,我们比较了在0、16和50 nM长春花碱存在下过夜培养的神经元的整个细胞体和轴突中的聚合物水平与轴突生长前新鲜接种的神经元中的微管聚合物水平。无药物时,聚合物总水平大约增加两倍。在16 nM长春花碱时,聚合物水平大致等于新鲜接种神经元中的水平,而在50 nM时,聚合物水平降低约一半。因此,16 nM长春花碱作为微管的“动力学稳定剂”,而50 nM导致一些微管净拆解。在这两种药物浓度下,随着轴突生长,轴突中微管聚合物水平逐渐增加,而细胞体中的聚合物相应减少。这些结果表明神经元中存在高效机制将预先组装的微管从细胞体运输到轴突中。这些机制即使以细胞体为代价且即使在促进神经元中一些微管拆解的条件下仍很活跃。微管极性分析表明,长春花碱处理的轴突内的微管如同对照轴突内的微管一样,正端均匀地远离细胞体。(摘要截于400字)
