Ingoglia N A, Sharma S C, Pilchman J, Baranowski K, Sturman J A
J Neurosci. 1982 Oct;2(10):1412-23. doi: 10.1523/JNEUROSCI.02-10-01412.1982.
The axonal transport, metabolism, and transcellular transfer of uridine, adenosine, putrescine, and spermidine have been examined in intact and regenerating optic nerves of goldfish. Following intraocular injection of labeled nucleosides, axonal transport was determined by comparing left-right differences in tectal radioactivity, and transcellular transfer was indicated by light autoradiographic analysis. The results demonstrated axonal transport, transcellular transfer, and periaxonal cell utilization of both nucleosides in intact axons and severalfold increases of all of these processes in regenerating axons. Experiments in which the metabolism of the nucleosides was studied resulted in data which suggested that uridine and adenosine, when delivered to the tectum by axonal transport, are protected from degradation and thus are relatively more available for periaxonal cell utilization than nucleosides reaching these cells via the blood. In intact axons, the majority of the nonmetabolized radioactivity was present as UMP, UDP, and UTP following [3H]uridine injections, whereas the majority of the radioactivity following [3H]adenosine injections was present as adenosine, with the phosphorylated derivatives constituting a smaller proportion. During nerve regeneration, the relative proportion of nucleosides to nucleotides was reversed, with uridine being the principal labeled compound in the first case, and AMP, ADP, and ATP being the major labeled compounds in the latter case. The nucleosides also were found to be different from each other in that adenosine, but not uridine, can be taken up by optic axons and transported retrogradely from the tectum to retinal ganglion cell bodies in the eye. Following intraocular injection of [3H]spermidine, radioactivity was transported to the optic tectum and transferred to tectal cells in the vicinity of the regenerating axons. Following [3H]putrescine injections, silver grains were found over periaxonal glia, but preliminary findings suggest that they are not present over tectal neurons nor over radial glial cells in the periependymal layers. Analysis of tectal radioactivity showed in each case that it was composed primarily of the injected compounds. These studies indicate that, following axonal transport, the polyamines do not remain within regenerating axons but are transferred to cells surrounding the axon. On the basis of these and previous findings, we speculate that the axonal transport and transcellular transfer of uridine, adenosine, polyamines, and perhaps other small molecules are means of communication between axons and periaxonal cells; that the axon can affect RNA and protein synthesis in periaxonal cells by regulating the availability of these small molecules; and that, during nerve regeneration, the increased metabolic needs of periaxonal cells are met by an increased axonal supply of precursors (adenosine and uridine) and other molecules (polyamines) critical for protein synthesis.
在金鱼完整的和再生的视神经中,对尿苷、腺苷、腐胺和亚精胺的轴突运输、代谢及跨细胞转运进行了研究。眼内注射标记核苷后,通过比较视叶放射性的左右差异来确定轴突运输,并通过光镜放射自显影分析来显示跨细胞转运。结果表明,在完整轴突中两种核苷均存在轴突运输、跨细胞转运及轴周细胞利用,而在再生轴突中所有这些过程均增加了数倍。研究核苷代谢的实验所得到的数据表明,当尿苷和腺苷通过轴突运输到达视叶时,它们受到保护而不被降解,因此与通过血液到达这些细胞的核苷相比,相对更易于被轴周细胞利用。在完整轴突中,注射[³H]尿苷后,大部分未代谢的放射性以UMP、UDP和UTP的形式存在,而注射[³H]腺苷后,大部分放射性以腺苷的形式存在,磷酸化衍生物所占比例较小。在神经再生过程中,核苷与核苷酸的相对比例发生了逆转,在第一种情况下尿苷是主要的标记化合物,而在第二种情况下AMP、ADP和ATP是主要的标记化合物。还发现这两种核苷彼此不同,因为腺苷能被视神经轴突摄取并从视叶逆向运输到眼内的视网膜神经节细胞体,而尿苷则不能。眼内注射[³H]亚精胺后,放射性被运输到视叶并转移到再生轴突附近的视叶细胞。注射[³H]腐胺后,在轴周神经胶质细胞上发现了银粒,但初步研究结果表明,在视叶神经元上以及室管膜周层的放射状神经胶质细胞上没有银粒。对视叶放射性的分析表明,在每种情况下其主要由注射的化合物组成。这些研究表明,轴突运输后,多胺并不保留在再生轴突内,而是转移到轴突周围的细胞中。基于这些及先前的研究结果,我们推测尿苷、腺苷、多胺以及可能的其他小分子的轴突运输和跨细胞转运是轴突与轴周细胞之间的通讯方式;轴突可通过调节这些小分子的可利用性来影响轴周细胞中的RNA和蛋白质合成;并且在神经再生过程中,轴突对蛋白质合成至关重要的前体(腺苷和尿苷)及其他分子(多胺)供应增加,从而满足轴周细胞增加的代谢需求。
