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人红细胞膜的阴离子位点。I. 胰蛋白酶、磷脂酶C和pH对结合的带正电荷胶体颗粒拓扑结构的影响。

Anionic sites of human erythrocyte membranes. I. Effects of trypsin, phospholipase C, and pH on the topography of bound positively charged colloidal particles.

作者信息

Nicolson G L

出版信息

J Cell Biol. 1973 May;57(2):373-87. doi: 10.1083/jcb.57.2.373.

Abstract

The effects of pH, trypsin, and phospholipase C on the topographic distribution of acidic anionic residues on human erythrocytes was investigated using colloidal iron hydroxide labeling of mounted, fixed ghost membranes. After glutaraldehyde fixation at pH 6.5-7.5, the positively charged colloidal particles were bound to the membranes in small randomly distributed clusters. The clusters of anionic sites were reversibly aggregated by incubation at pH 5.5 before fixation at the same pH. These results correlate with the distribution of intramembranous particles found by Pinto da Silva (J. Cell Biol.53:777), with the exception that the distribution of anionic sites on a majority of the fixed ghosts at pH 4.5 was aggregated instead of dispersed. The randomly distributed clusters could be nonreversibly aggregated by trypsin or phospholipase C treatment of intact ghosts before glutaraldehyde fixation. Previous glutaraldehyde fixation prevented trypsin and pH induced aggregation of the colloidal iron sites. Evidence that N-acetylneuraminic acid groups are the principal acidic residues binding colloidal iron was the elimination of greater than 85% of the colloidal iron labeling to neuraminidase-treated cell membranes. Colloidal iron binding N-acetylneuraminic acid residues may reside on membrane molecules such as glycophorin, a sialoglycoprotein which contains the majority of the N-acetylneuraminic acid found on the human erythrocyte membrane.

摘要

利用胶体氢氧化铁对固定的红细胞空影膜进行标记,研究了pH值、胰蛋白酶和磷脂酶C对人红细胞酸性阴离子残基拓扑分布的影响。在pH 6.5 - 7.5下用戊二醛固定后,带正电荷的胶体颗粒以随机分布的小簇形式结合在膜上。在相同pH值下固定前,通过在pH 5.5下孵育,阴离子位点的簇可逆聚集。这些结果与平托·达席尔瓦(《细胞生物学杂志》53:777)发现的膜内颗粒分布相关,不同之处在于,在pH 4.5时,大多数固定空影上的阴离子位点分布是聚集的而非分散的。在戊二醛固定前,用胰蛋白酶或磷脂酶C处理完整的空影,可使随机分布的簇不可逆聚集。先前的戊二醛固定可防止胰蛋白酶和pH诱导的胶体铁位点聚集。N - 乙酰神经氨酸基团是结合胶体铁的主要酸性残基的证据是,用神经氨酸酶处理细胞膜后,超过85%的胶体铁标记被消除。结合N - 乙酰神经氨酸残基的胶体铁可能存在于膜分子上,如血型糖蛋白,一种唾液糖蛋白,它含有在人红细胞膜上发现的大部分N - 乙酰神经氨酸。

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