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用于水相聚合物双相体系中细胞分离的聚乙二醇-抗体亲和配体的合成与应用

Synthesis and application of a poly(ethylene glycol)-antibody affinity ligand for cell separations in aqueous polymer two-phase systems.

作者信息

Sharp K A, Yalpani M, Howard S J, Brooks D E

出版信息

Anal Biochem. 1986 Apr;154(1):110-7. doi: 10.1016/0003-2697(86)90503-8.

DOI:10.1016/0003-2697(86)90503-8
PMID:3706718
Abstract

The possibility of producing biospecific affinity ligands for separating cells in two polymer aqueous phase systems on the basis of cell surface antigens was investigated. Rabbit anti-human erythrocyte IgG was reacted with cyanuric chloride-activated monomethyl poly(ethylene glycol) (PEG) fractions (molecular weights approximately 200, 1900, and 5000) at various molar ratios of PEG to protein lysine groups. The partition coefficient of the protein in a Dextran/PEG two-phase system increased with increasing degree of modification and increasing PEG molecular weight. There was a concomitant loss in ability to agglutinate human erythrocytes. The ability of the modified IgG to bind to a DEAE-cellulose column was almost eliminated by reaction with the PEG 5000, and was decreased to a lesser extent by PEG 1900. This PEG 1900-modified IgG substantially increased the partition of fresh or fixed human erythrocytes into the PEG-rich phase of a suitable phase system, while having no effect on rabbit cell partition. The partition increase could be inhibited by unmodified anti-human red cell IgG but not by nonspecific unmodified human IgG, demonstrating that the ligand effects were specific for the cell type against which the antibody was raised. A mixture of rabbit and human erythrocytes, which ordinarily have very similar partitions in the phase systems used, could be separated on a countercurrent distribution apparatus using the modified IgG. These results demonstrate the feasibility of producing immunologically specific affinity partition ligands for cell separation.

摘要

研究了基于细胞表面抗原在两个聚合物水相体系中制备用于分离细胞的生物特异性亲和配体的可能性。兔抗人红细胞IgG与三聚氯氰活化的单甲基聚(乙二醇)(PEG)级分(分子量约为200、1900和5000)以不同的PEG与蛋白质赖氨酸基团摩尔比进行反应。在葡聚糖/PEG双相体系中,蛋白质的分配系数随修饰程度的增加和PEG分子量的增加而增大。同时,其凝集人红细胞的能力有所丧失。与PEG 5000反应后,修饰后的IgG与DEAE-纤维素柱结合的能力几乎完全丧失,与PEG 1900反应后该能力有较小程度的降低。这种PEG 1900修饰的IgG显著增加了新鲜或固定的人红细胞在合适相体系富含PEG相中的分配,而对兔细胞的分配没有影响。未修饰的抗人红细胞IgG可抑制分配增加,但非特异性未修饰的人IgG则不能,这表明配体效应对于产生抗体所针对的细胞类型具有特异性。在逆流分配装置上使用修饰后的IgG,可以分离兔和人红细胞的混合物,在所用的相体系中,它们通常具有非常相似的分配情况。这些结果证明了制备用于细胞分离的免疫特异性亲和分配配体的可行性。

相似文献

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Synthesis and application of a poly(ethylene glycol)-antibody affinity ligand for cell separations in aqueous polymer two-phase systems.用于水相聚合物双相体系中细胞分离的聚乙二醇-抗体亲和配体的合成与应用
Anal Biochem. 1986 Apr;154(1):110-7. doi: 10.1016/0003-2697(86)90503-8.
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Development of a general ligand for immunoaffinity partitioning in two phase aqueous polymer systems.
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Immuno-affinity partition of cells in aqueous polymer two-phase systems.水相聚合物双相体系中细胞的免疫亲和分配
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Cell separation by immunoaffinity partitioning with polyethylene glycol-modified protein A in aqueous polymer two-phase systems.在水性聚合物双相系统中通过用聚乙二醇修饰的蛋白A进行免疫亲和分配来分离细胞。
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Separation of cell mixtures by immunoaffinity cell partitioning: strategies for low abundance cells.通过免疫亲和细胞分配分离细胞混合物:低丰度细胞的策略
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Aging of erythrocytes results in altered red cell surface properties in the rat, but not in the human. Studies by partitioning in two-polymer aqueous phase systems.红细胞衰老会导致大鼠红细胞表面特性发生改变,但人类红细胞不会。通过在双聚合物水相系统中分配进行研究。
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Affinity partitioning. A method for purification of proteins using specific polymer-ligands in aqueous polymer two-phase systems.亲和分配。一种在聚合物双水相系统中使用特定聚合物配体纯化蛋白质的方法。
J Biol Chem. 1975 Feb 25;250(4):1484-9.
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Column chromatographic separation of cells using aqueous polymeric two-phase systems.使用水性聚合物双相系统对细胞进行柱色谱分离。
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Effect of cell exposure to top or bottom phase prior to cell partitioning in dextran-poly(ethylene glycol) aqueous phase systems: erythrocytes as a model.在葡聚糖 - 聚(乙二醇)水相体系中细胞分配前,细胞暴露于上相或下相的影响:以红细胞为模型
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Membrane surface properties other than charge involved in cell separation by partition in polymer, aqueous two-phase systems.聚合物双水相体系中通过分配作用进行细胞分离所涉及的除电荷以外的膜表面性质。
Biochemistry. 1976 Jul 13;15(14):2959-64. doi: 10.1021/bi00659a004.

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