Hoffman S, Friedlander D R, Chuong C M, Grumet M, Edelman G M
J Cell Biol. 1986 Jul;103(1):145-58. doi: 10.1083/jcb.103.1.145.
Individual neurons can express both the neural cell adhesion molecule (N-CAM) and the neuron-glia cell adhesion molecule (Ng-CAM) at their cell surfaces. To determine how the functions of the two molecules may be differentially controlled, we have used specific antibodies to each cell adhesion molecule (CAM) to perturb its function, first in brain membrane vesicle aggregation and then in tissue culture assays testing the fasciculation of neurite outgrowths from cultured dorsal root ganglia, the migration of granule cells in cerebellar explants, and the formation of histological layers in the developing retina. Our strategy was initially to delineate further the binding mechanisms for each CAM. Antibodies to Ng-CAM and N-CAM each inhibited brain membrane vesicle aggregation but the binding mechanisms of the two CAMs differed. As expected from the known homophilic binding mechanism of N-CAM, anti-N-CAM-coated vesicles did not co-aggregate with uncoated vesicles. Anti-Ng-CAM-coated vesicles readily co-aggregated with uncoated vesicles in accord with a postulated heterophilic binding mechanism. It was also shown that N-CAM was not a ligand for Ng-CAM. In contrast to assays with brain membrane vesicles, cellular systems can reveal functional differences for each CAM reflecting its relative amount (prevalence modulation) and location (polarity modulation). Consistent with this, each of the three cellular processes examined in vitro was preferentially inhibited only by anti-N-CAM or by anti-Ng-CAM antibodies. Both neurite fasciculation and the migration of cerebellar granule cells were preferentially inhibited by anti-Ng-CAM antibodies. Anti-N-CAM antibodies inhibited the formation of histological layers in the retina. The data on perturbation by antibodies were correlated with the relative levels of expression of Ng-CAM and N-CAM in each of these different neural regions. Quantitative immunoblotting experiments indicated that the relative Ng-CAM/N-CAM ratios in comparable extracts of brain, dorsal root ganglia, and retina were respectively 0.32, 0.81, and 0.04. During culture of dorsal root ganglia in the presence of nerve growth factor, the Ng-CAM/N-CAM ratio rose to 4.95 in neurite outgrowths and 1.99 in the ganglion proper, reflecting both polarity and prevalence modulation. These results suggest that the relative ability of anti-Ng-CAM and anti-N-CAM antibodies to inhibit cell-cell interactions in different neural tissues is strongly correlated with the local Ng-CAM/N-CAM ratio.(ABSTRACT TRUNCATED AT 400 WORDS)
单个神经元能够在其细胞表面同时表达神经细胞黏附分子(N-CAM)和神经元-神经胶质细胞黏附分子(Ng-CAM)。为了确定这两种分子的功能如何受到不同的调控,我们使用了针对每种细胞黏附分子(CAM)的特异性抗体来干扰其功能,首先是在脑膜囊泡聚集实验中,然后是在组织培养实验中,检测培养的背根神经节神经突生长的成束、小脑外植体中颗粒细胞的迁移以及发育中的视网膜中组织学层的形成。我们的策略最初是进一步阐明每种CAM的结合机制。针对Ng-CAM和N-CAM的抗体均抑制脑膜囊泡聚集,但两种CAM的结合机制不同。正如从已知的N-CAM同嗜性结合机制所预期的那样,抗N-CAM包被的囊泡不会与未包被的囊泡共同聚集。抗Ng-CAM包被的囊泡根据假定的异嗜性结合机制很容易与未包被的囊泡共同聚集。还表明N-CAM不是Ng-CAM的配体。与脑膜囊泡实验不同,细胞系统可以揭示每种CAM反映其相对量(丰度调节)和位置(极性调节)的功能差异。与此一致的是,体外检测的三个细胞过程中,每一个都仅优先被抗N-CAM或抗Ng-CAM抗体抑制。神经突成束和小脑颗粒细胞的迁移优先被抗Ng-CAM抗体抑制。抗N-CAM抗体抑制视网膜中组织学层的形成。抗体干扰的数据与这些不同神经区域中Ng-CAM和N-CAM的相对表达水平相关。定量免疫印迹实验表明,脑、背根神经节和视网膜的可比提取物中相对的Ng-CAM/N-CAM比值分别为0.32、0.81和0.04。在神经生长因子存在的情况下培养背根神经节时,神经突生长中Ng-CAM/N-CAM比值升至4.95,神经节本身中升至1.99,反映了极性和丰度调节。这些结果表明,抗Ng-CAM和抗N-CAM抗体在不同神经组织中抑制细胞间相互作用的相对能力与局部Ng-CAM/N-CAM比值密切相关。(摘要截断于400字)
