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人血清高密度脂蛋白蛋白质的形式。

Forms of human serum high density lipoprotein protein.

作者信息

Scanu A

出版信息

J Lipid Res. 1966 Mar;7(2):295-306.

PMID:4957797
Abstract

Delipidation by ethanol-diethyl ether at -10 degrees C of human serum high-density lipoprotein (HDL, d 1.063-1.21) or of its subclasses HDL(2) (d 1.063-1.120) and HDL(3) (d 1.120-1.21), yielded proteins-alphaP, alphaP(2), and alphaP(3)-containing 3% phospholipid (largely lecithin) and 3.3% carbohydrate (glucosamine:L-fucose:D-galactose, D-mannose:sialic acid, 1.00:41 : 0.56:0.31). Solubility data and analytical ultracentrifugal analyses indicated that, upon lipid removal, HDL protein aggregates readily; the aggregation is dependent upon pH and ionic strength of the solvent medium. Subunits of 21,000 mol wt were obtained by acetylation or addition of sodium dodecyl sulfate (SDS). HDL and alphaP elicited in the rabbit a similar immunological response. By agar gel immunoelectrophoresis both anti-HDL and anti-alphaP sera detected a major and two minor antigenic determinants in HDL, HDL(3), alphaP, alphaP(2), and alphaP(3). HDL(2), antigenically homogeneous, gave an immunoelectrophoretic pattern of HDL(3) upon mixing with alphaP. alphaP, alphaP(2), and alphaP(3) exhibited a single antigenic determinant after treatment with SDS (0.5 M) or upon acetylation. Native or delipidated forms of HDL, HDL(2), and HDL(3) were separated by vertical starch gel electrophoresis into several components, which showed identical reactions against anti-HDL or anti-alphaP sera. The data suggest that (a) the proteins of HDL, HDL(2), and HDL(3) are made of subunits, probably identical, of an average molecular weight of 21,000; (b) the difference in antigenic behavior between HDL(2) and HDL(3) is due to the presence in the latter of a lipid-poor protein; (c) antigenic polymorphism of alphaP is probably related to the presence in solution of monomeric and polymeric forms having different reactivity against anti-HDL and anti-alphaP sera.

摘要

在-10℃下,用人血清高密度脂蛋白(HDL,密度1.063 - 1.21)或其亚类HDL(2)(密度1.063 - 1.120)和HDL(3)(密度1.120 - 1.21)进行乙醇 - 乙醚脱脂处理,得到含蛋白质 - αP、αP(2)和αP(3)的产物,其含有3%的磷脂(主要是卵磷脂)和3.3%的碳水化合物(葡糖胺:L - 岩藻糖:D - 半乳糖、D - 甘露糖:唾液酸,比例为1.00:41 : 0.56:0.31)。溶解度数据和分析超速离心分析表明,去除脂质后,HDL蛋白质容易聚集;聚集取决于溶剂介质的pH值和离子强度。通过乙酰化或添加十二烷基硫酸钠(SDS)可得到分子量为21,000 mol wt的亚基。HDL和αP在兔体内引发相似的免疫反应。通过琼脂凝胶免疫电泳,抗HDL血清和抗αP血清在HDL、HDL(3)、αP、αP(2)和αP(3)中均检测到一个主要抗原决定簇和两个次要抗原决定簇。抗原性均一的HDL(2)与αP混合后呈现出HDL(3)的免疫电泳图谱。αP、αP(2)和αP(3)在用SDS(0.5 M)处理或乙酰化后呈现单一抗原决定簇。HDL、HDL(2)和HDL(3)的天然或脱脂形式通过垂直淀粉凝胶电泳分离成几个组分,它们对抗HDL或抗αP血清显示相同反应。数据表明:(a) HDL、HDL(2)和HDL(3)的蛋白质由平均分子量为21,000的亚基组成,可能相同;(b) HDL(2)和HDL(3)之间抗原行为的差异是由于后者存在一种低脂质蛋白质;(c) αP的抗原多态性可能与溶液中对抗HDL和抗αP血清具有不同反应性的单体和聚合物形式的存在有关。

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