Fisher S J, Leitch M S, Laine R A
Biochem J. 1984 Aug 1;221(3):821-8. doi: 10.1042/bj2210821.
The brush-border glycoproteins of first-trimester human placentas were investigated by using two external labelling techniques: (1) sequential digestion with neuraminidase and galactose oxidase, followed by reduction with NaB3H4, which 3H-labels terminal galactose and galactosamine residues; and (2) sequential treatment with periodate and NaB3H4, which 3H-labels terminal sialic acid residues. The labelling procedures were performed on intact tissue so that the results would more closely approximate the topography of the brush border in vivo. The microvilli were isolated, subjected to sodium dodecyl sulphate/polyacrylamide-gel electrophoresis, and the [3H]glycoproteins detected by fluorography. Densitometer scans of the fluorograms of the [3H]galactoproteins showed that, under reducing conditions, 90% of the protein-associated radioactivity was incorporated into two glycoproteins. The major [3H]galactoprotein of early placental microvilli had an estimated molecular mass of 92 kDa (desialylated) and migrated as a diffuse band. A minor 180 kDa glycoprotein was less consistently labelled. No change in the apparent molecular mass of either component was detected in the absence of beta-mercaptoethanol, suggesting that the 180 kDa component was not a dimer of the 92 kDa glycoprotein. The remaining 10% the radioactivity was equally distributed among several minor membrane components. Densitometer scans of the fluorograms of the [3H]sialoproteins showed that, under either reducing or non-reducing conditions, 90% of the 3H was preferentially incorporated into the 92-110 kDa region of the gel. Although no distinct bands were visible, the higher-molecular-mass region of this area was always most heavily labelled. A minor 180 kDa glycoprotein was also 3H-labelled. The pattern of brushborder [3H]glycoproteins from first-trimester placentas differed markedly from that of term placental microvilli and from placental fibroblast plasma membranes that were 3H-labelled by identical external labelling techniques. These results indicate that: (1) the glycoprotein determinants of brush-border topography change during pregnancy; (2) within the placenta, the major 92 kDa (desialylated) determinant, which has not been previously described, is unique to the trophoblastic cells.
(1)先用神经氨酸酶和半乳糖氧化酶顺序消化,然后用NaB3H4还原,该方法用3H标记末端半乳糖和半乳糖胺残基;(2)先用高碘酸盐和NaB3H4顺序处理,该方法用3H标记末端唾液酸残基。标记程序在完整组织上进行,以便结果更接近体内刷状缘的拓扑结构。分离微绒毛,进行十二烷基硫酸钠/聚丙烯酰胺凝胶电泳,通过荧光自显影检测[3H]糖蛋白。对[3H]半乳糖蛋白荧光图谱的光密度扫描显示,在还原条件下,90%的与蛋白质相关的放射性掺入到两种糖蛋白中。早期胎盘微绒毛的主要[3H]半乳糖蛋白估计分子量为92 kDa(去唾液酸化),迁移为弥散带。一种较小的180 kDa糖蛋白标记不太一致。在没有β-巯基乙醇的情况下,未检测到任何一种成分的表观分子量发生变化,这表明180 kDa成分不是92 kDa糖蛋白的二聚体。其余10%的放射性均匀分布在几个较小的膜成分中。对[3H]唾液酸蛋白荧光图谱的光密度扫描显示,在还原或非还原条件下,90%的3H优先掺入凝胶的92 - 110 kDa区域。尽管没有可见的明显条带,但该区域较高分子量部分总是标记最重。一种较小的180 kDa糖蛋白也被3H标记。孕早期胎盘刷状缘[3H]糖蛋白的模式与足月胎盘微绒毛以及用相同外部标记技术进行3H标记的胎盘成纤维细胞质膜的模式明显不同。这些结果表明:(1)刷状缘拓扑结构的糖蛋白决定簇在妊娠期间发生变化;(2)在胎盘中,主要的92 kDa(去唾液酸化)决定簇是滋养层细胞特有的,此前未被描述过。
