从胎鼠脑部分离出的神经生长锥。IV. 膜亚组分的制备以及对出芽神经元上表达的一种膜糖蛋白的鉴定。
Nerve growth cones isolated from fetal rat brain. IV. Preparation of a membrane subfraction and identification of a membrane glycoprotein expressed on sprouting neurons.
作者信息
Ellis L, Wallis I, Abreu E, Pfenninger K H
出版信息
J Cell Biol. 1985 Nov;101(5 Pt 1):1977-89. doi: 10.1083/jcb.101.5.1977.
This study describes the preparation of a membrane subfraction from isolated nerve growth cone particles (GCPs) (see Pfenninger, K. H., L. Ellis, M. P. Johnson, L. B. Friedman, and S. Somlo, 1983, Cell, 35:573-584) and the identification in this fraction of a glycoprotein expressed during neurite growth. While approximately 40 major polypeptides are visible in Coomassie Blue-stained SDS polyacrylamide gels of pelleted (partially disrupted) GCPs, a salt-washed membrane fraction prepared from lysed, detergent-permeabilized GCPs contains only 14% of this protein and has an unusually simple polypeptide pattern of seven major bands. Monoclonal antibodies have been generated to GCP membranes isolated from fetal rat brain. These antibodies have been screened differentially with synaptosomes from adult rat brain in order to identify those which recognize antigens expressed selectively during neurite growth. One such antibody (termed 5B4) recognizes a developmentally regulated membrane glycoprotein that is enriched in GCP membranes and expressed in fetal neurons sprouting in vitro. The 5B4 antigen in fetal brain migrates in SDS polyacrylamide gels as a diffuse band of approximately 185-255 kD, is rich in sialic acid, and consists of a small family of isoelectric variants. Freezing-thawing and neuraminidase digestion result in the cleavage of the native antigen into two new species migrating diffusely around 200 and 160 kD. Prolonged neuraminidase digestion sharpens these bands at about 180 and 135 kD, respectively. In the mature brain, antibody 5B4 recognizes a sparse polypeptide migrating at approximately 140 kD. As shown in the following paper (Wallis, I., L. Ellis, K. Suh, and K. H. Pfenninger, 1985, J. Cell Biol., 101:1990-1998), the fetal antigen is specifically associated with regions of neuronal sprouting and, therefore, can be used as a molecular marker of neurite growth.
本研究描述了从分离的神经生长锥颗粒(GCPs)制备膜亚组分的方法(见Pfenninger, K. H., L. Ellis, M. P. Johnson, L. B. Friedman, and S. Somlo, 1983, Cell, 35:573 - 584),并在该组分中鉴定出一种在神经突生长过程中表达的糖蛋白。在经考马斯亮蓝染色的沉淀(部分破碎)GCPs的SDS聚丙烯酰胺凝胶中可看到约40种主要多肽,而从裂解的、经去污剂通透处理的GCPs制备的盐洗膜组分仅含有该蛋白质的14%,且具有异常简单的多肽图谱,有七条主要条带。已针对从胎鼠脑分离的GCP膜产生了单克隆抗体。这些抗体已用成年大鼠脑的突触体进行了差异筛选,以鉴定那些识别在神经突生长过程中选择性表达的抗原的抗体。其中一种抗体(称为5B4)识别一种受发育调控的膜糖蛋白,该糖蛋白在GCP膜中富集,并在体外发芽的胎神经元中表达。胎脑中的5B4抗原在SDS聚丙烯酰胺凝胶中迁移为一条约185 - 255 kD的弥散条带,富含唾液酸,由一小族等电变体组成。冻融和神经氨酸酶消化导致天然抗原裂解为两个新物种,分别在约200和160 kD处弥散迁移。长时间的神经氨酸酶消化分别使这些条带在约180和135 kD处变清晰。在成熟脑中,抗体5B4识别一条迁移在约140 kD的稀疏多肽。如以下论文(Wallis, I., L. Ellis, K. Suh, and K. H. Pfenninger, 1985, J. Cell Biol., 101:1990 - 1998)所示,胎抗原与神经元发芽区域特异性相关,因此可作为神经突生长的分子标记。
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