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D2细胞粘附分子的生物合成:培养的胎鼠神经元细胞中的脉冲追踪研究

Biosynthesis of the D2 cell adhesion molecule: pulse-chase studies in cultured fetal rat neuronal cells.

作者信息

Lyles J M, Norrild B, Bock E

出版信息

J Cell Biol. 1984 Jun;98(6):2077-81. doi: 10.1083/jcb.98.6.2077.

Abstract

D2 is a membrane glycoprotein that is believed to function as a cell adhesion molecule (CAM) in neural cells. We have examined its biosynthesis in cultured fetal rat brain neurones. We found D2-CAM to be synthesized initially as two polypeptides: Mr 186,000 (A) and Mr 136,000 (B). With increasing chase times the Mr of both molecules increased to 187,000-201,000 (A) and 137,000-158,000 (B). These were similar to the sizes of D2-CAM labeled with [14C]glucosamine, [3H]fucose and [14C]mannosamine, indicating that the higher Mr species are glycoproteins. In the presence of tunicamycin, which specifically blocks the synthesis of high mannose cores, Mr were reduced to 175,000 (A) and 124,000 (B). Newly synthesized A and B are susceptible to degradation by endo-beta-N-acetyl-glucosaminidase H, which specifically degrades high mannose cores, but they are resistant to such degradation after 150 min of posttranslational processing. Hence, we deduce that A and B are initially synthesized with four to five high mannose cores which are later converted into N-linked complex oligosaccharides attached to asparagine residues. However, no shift of [35S]methionine radioactivity between A and B was detected with different pulse or chase times, showing that these molecules are not interconverted. Thus, our data indicate that the neuronal D2-CAM glycoproteins are derived from two mRNAs.

摘要

D2是一种膜糖蛋白,被认为在神经细胞中作为细胞粘附分子(CAM)发挥作用。我们研究了其在培养的胎鼠脑神经元中的生物合成。我们发现D2-CAM最初以两种多肽形式合成:分子量为186,000(A)和136,000(B)。随着追踪时间的增加,两种分子的分子量增加到187,000 - 201,000(A)和137,000 - 158,000(B)。这些与用[14C]葡糖胺、[3H]岩藻糖和[14C]甘露糖胺标记的D2-CAM的大小相似,表明分子量较高的物种是糖蛋白。在衣霉素存在下,衣霉素特异性地阻断高甘露糖核心的合成,分子量降低到175,000(A)和124,000(B)。新合成的A和B易受内切β-N-乙酰葡糖胺糖苷酶H的降解,该酶特异性地降解高甘露糖核心,但在翻译后加工150分钟后它们对这种降解具有抗性。因此,我们推断A和B最初合成时带有四到五个高甘露糖核心,这些核心后来转化为连接到天冬酰胺残基上的N-连接复合寡糖。然而,在不同的脉冲或追踪时间下,未检测到[35S]甲硫氨酸放射性在A和B之间的转移,表明这些分子不会相互转化。因此,我们的数据表明神经元D2-CAM糖蛋白来自两种mRNA。

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