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神经细胞黏附分子N-CAM的跨膜分布研究。利用脂质体插入放射性碘化N-CAM研究其跨双层取向。

Studies on the transmembrane disposition of the neural cell adhesion molecule N-CAM. The use of liposome-inserted radioiodinated N-CAM to study its transbilayer orientation.

作者信息

Gennarini G, Hirn M, Deagostini-Bazin H, Goridis C

出版信息

Eur J Biochem. 1984 Jul 2;142(1):65-73. doi: 10.1111/j.1432-1033.1984.tb08251.x.

Abstract

The transmembrane orientation of the polypeptide chains present in preparations of adult and neonatal mouse N-CAM was studied using, as a model system, liposome-inserted purified N-CAM preparations. N-CAM purified from adult or neonatal mouse brain was 125I-labeled and reconstituted into artificial lipid vesicles. After trypsin digestion, the peptides that remained associated with the liposomes were isolated by floatation of the vesicles on sucrose gradients. In control experiments the liposomes were lysed before trypsin treatment. Large, overlapping peptides were obtained after this treatment, several of which were protected by the liposome membrane. Sialic-acid-bearing peptides were revealed by their sensitivity to neuraminidase. To distinguish between peptides corresponding to intracellular or extracellular domains use was made of the P61 and H28.123 monoclonal antibodies, which recognize determinants located on the cytoplasmic and the extracellular part of the molecules respectively. There was no indication that the N-CAM chains were inserted in an inside-out configuration. Peptides protected from trypsin attack by the liposomes and recognized only by P61 had Mr values of 92 000, 42 000 and 35 000. The H28.123 determinant could be mapped to a 32 000-Mr peptide located close to the membrane at the vesicle's exterior. The bulk of the sialic acid seemed to be carried by a rather short sequence distal to the H28.123-reactive peptide but at some distance from the N terminus. Fragments of very similar Mr were generated from young and adult material. However, a 45 000-Mr peptide from neonatal N-CAM appeared to migrate in the higher-Mr region of sodium dodecyl sulfate/polyacrylamide gels in its fully sialylated form. It is concluded that (a) identical polypeptide chains are present in young and adult preparation, (b) the 180 000-Mr, 140 000-Mr and 120 000-Mr chains differ by the length of their cytoplasmic extensions and (c) the largest cytoplasmic sequences have a Mr close to 90 000. A tentative linear model of the transmembrane topography of the N-CAM polypeptides is presented.

摘要

利用插入脂质体的纯化N-CAM制剂作为模型系统,研究了成年和新生小鼠N-CAM制剂中存在的多肽链的跨膜方向。从成年或新生小鼠脑中纯化的N-CAM用125I标记,然后重构成人工脂质囊泡。胰蛋白酶消化后,通过在蔗糖梯度上漂浮囊泡来分离与脂质体相关的肽。在对照实验中,脂质体在胰蛋白酶处理前被裂解。处理后获得了大的、重叠的肽,其中一些受到脂质体膜的保护。含唾液酸的肽因其对神经氨酸酶的敏感性而被揭示。为了区分对应于细胞内或细胞外结构域的肽,使用了P61和H28.123单克隆抗体,它们分别识别位于分子细胞质和细胞外部分的决定簇。没有迹象表明N-CAM链以由内向外的构型插入。受脂质体保护免受胰蛋白酶攻击且仅被P61识别的肽的Mr值为92000、42000和35000。H28.123决定簇可定位到位于囊泡外部靠近膜的一个32000-Mr肽上。大部分唾液酸似乎由H28.123反应性肽远端相当短的序列携带,但与N末端有一定距离。来自幼年和成年材料的Mr非常相似的片段被产生。然而,新生N-CAM的一个45000-Mr肽以其完全唾液酸化的形式似乎在十二烷基硫酸钠/聚丙烯酰胺凝胶的较高Mr区域迁移。得出以下结论:(a)幼年和成年制剂中存在相同的多肽链,(b)180000-Mr、140000-Mr和120000-Mr链的细胞质延伸长度不同,(c)最大的细胞质序列的Mr接近90000。提出了N-CAM多肽跨膜拓扑结构的初步线性模型。

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