Groswald D E, Kelly P T
J Neurochem. 1984 Feb;42(2):534-46. doi: 10.1111/j.1471-4159.1984.tb02711.x.
Subcellular fractions from rat cerebellum and other tissues were examined for the presence of a 240K glycoprotein, designated GP-A. Previous results have shown that GP-A is enriched in cerebellum synaptic junction (SJ) fractions when compared to parent synaptic plasma membrane (SPM) fractions and is not detected in forebrain SPM or SJ fractions. In the present studies, GP-A was not detected in myelin, mitochondria, purified nuclei, or cytosolic fractions from cerebellum, but was present in microsomal fractions. GP-A is partially soluble in the non-ionic detergent Triton X-100 and is completely soluble when cerebellum SPMs are treated with the ionic detergent N-lauryl sarcosinate. The solubilization of GP-A from cerebellum membranes was shown to be a function of bound calcium ions, e.g., pretreating SPMs with 100 microM-1mM Ca2+ decreased the solubility of GP-A in Triton by approximately threefold. GP-A is a major concanavalin A (Con A)-binding glycoprotein in cerebellum SJ fractions and migrates on sodium dodecyl sulfate (SDS) gels with a slower relative mobility than the 235K/230K fodrin doublet. Comparisons between purified fodrin and the 235K/230K doublet in cerebellum and forebrain synaptic fractions by two-dimensional peptide mapping indicated that they were identical. The Con A-binding property of GP-A was exploited to purify it by affinity chromatography with agarose-Con A. Peptide mapping comparisons between affinity-purified GP-A and GP-A in SPM and SJ fractions indicated that GP-A in synaptic fractions is apparently homogeneous. Peptide map comparisons between GP-A and 235K fodrin poly-peptide indicated that these two synaptic components are highly related (50% of their respective peptides are shared). The 235K fodrin polypeptide in SJs reacted with anti-fodrin antisera on Western blots; however, GP-A failed to cross-react. These observations, together with results from previous studies, indicate that GP-A is highly enriched in cerebellum compared to other neuronal and nonneural tissues. Moreover, GP-A is enriched in SJs relative to SPM fractions, is related to fodrin, and is most likely a cell-surface glycoprotein at asymmetric synapses in cerebellum. GP-A may be involved in neuronal recognition or synaptic transmission in the cerebellum. The important role of calcium in synaptic transmission, together with the decreased solubility of GP-A in Triton that results from micromolar concentrations of calcium, suggest that GP-A may play a role in stabilizing cerebellar synaptic junctions.
检测大鼠小脑及其他组织的亚细胞组分中是否存在一种名为GP-A的240K糖蛋白。先前的研究结果表明,与亲代突触质膜(SPM)组分相比,GP-A在小脑突触连接(SJ)组分中含量丰富,而在前脑SPM或SJ组分中未检测到。在本研究中,在小脑的髓磷脂、线粒体、纯化的细胞核或胞质组分中未检测到GP-A,但在微粒体组分中存在。GP-A部分可溶于非离子去污剂Triton X-100,当小脑SPM用离子去污剂N-十二烷基肌氨酸钠处理时则完全可溶。从小脑细胞膜中溶解GP-A显示是结合钙离子的一种功能,例如,用100微摩尔/升 - 1毫摩尔/升的Ca2+预处理SPM会使GP-A在Triton中的溶解度降低约三倍。GP-A是小脑SJ组分中主要的伴刀豆球蛋白A(Con A)结合糖蛋白,在十二烷基硫酸钠(SDS)凝胶上迁移时相对迁移率比235K/230K血影蛋白双峰慢。通过二维肽图分析比较小脑和前脑突触组分中纯化的血影蛋白与235K/230K双峰,表明它们是相同的。利用GP-A的Con A结合特性通过琼脂糖-Con A亲和层析对其进行纯化。亲和纯化的GP-A与SPM和SJ组分中的GP-A之间的肽图比较表明,突触组分中的GP-A显然是均一的。GP-A与235K血影蛋白多肽之间的肽图比较表明,这两种突触成分高度相关(它们各自50%的肽是相同的)。SJ中的235K血影蛋白多肽在Western印迹上与抗血影蛋白抗血清反应;然而,GP-A未能发生交叉反应。这些观察结果与先前的研究结果一起表明,与其他神经元和非神经组织相比,GP-A在小脑中高度富集。此外,相对于SPM组分,GP-A在SJ中富集,与血影蛋白相关,并且很可能是小脑不对称突触处的一种细胞表面糖蛋白。GP-A可能参与小脑中的神经元识别或突触传递。钙在突触传递中的重要作用,以及微摩尔浓度的钙导致GP-A在Triton中的溶解度降低,表明GP-A可能在稳定小脑突触连接中起作用。
