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Heparinization of gas plasma-modified polystyrene surfaces and the interactions of these surfaces with proteins studied with surface plasmon resonance

机译:气体等离子体改性聚苯乙烯表面的肝素化和这些表面与表面等离子体共振研究的蛋白质的相互作用

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摘要

Polystyrene surfaces obtained by spin-coating a solution of polystyrene in toluene on a gold layer were functionalized with carboxylic acid groups by preadsorption of the sodium salt of undecylenic acid, followed by an argon plasma treatment. A conjugate of albumin and heparin (alb-hep) was covalently immobilized onto the functionalized surface via preactivation of carboxylic acid groups with a water-soluble carbodiimide. The immobilization of alb-hep conjugate and the subsequent interactions of the heparinized surface with antithrombin III (ATIII, a heparin cofactor) and thrombin were monitored with surface plasmon resonance (SPR). The surface concentration of conjugate as determined with SPR deviated quantitatively from the results obtained with radiolabelled conjugate. The difference in surface concentrations of conjugate obtained with the two methods probably originates from the uncertainty of the refractive index of the alb-hep conjugate in the SPR technique. ATIII could be bound to the surface modified with alb-hep conjugate but not to a polystyrene surface modified with albumin. Rabbit anti-human ATIII did bind to the alb-hep surface previously exposed to ATIII, confirming the presence of surface bound ATIII. The alb-hep immobilized surface was able to bind much more thrombin than ATIII, which is probably due to the less specific heparin-thrombin interaction as compared to the heparin-ATIII interaction. This study shows that SPR is a technique that can be used to study, in real time, both the modification of polymer surfaces and the subsequent interactions of the modified surfaces with proteins.
机译:聚苯乙烯的表面,通过旋涂聚苯乙烯的甲苯金层上的溶液与由十一碳烯酸的钠盐的预吸附的羧酸基团,接着在氩气等离子处理进行了官能化得到。白蛋白和肝素(ALB-HEP)的缀合物经由与水溶性碳化二亚胺羧酸基团的预活化共价固定到所述官能化的表面。 ALB-HEP偶联物的固定,并用抗凝血酶III(ATIII,一个肝素辅因子)和凝血酶用表面等离子共振(SPR)监测肝素化表面的后续交互。与SPR测定偶联物的表面浓度从与放射标记的缀合物获得的结果定量地偏离。在与这两种方法得到的缀合物的表面浓度差可能是由在SPR技术的ALB-HEP缀合物的折射率的不确定性源于。 ATIII可以绑定到ALB-HEP缀合物,但不与白蛋白改性聚苯乙烯表面改性的表面。兔抗人ATIII并结合先前暴露于ATIII的ALB-HEP表面,确认表面的存在下的结合ATIII。相比于肝素ATIII相互作用ALB-HEP固定表面能够更凝血酶比ATIII,这可能是结合由于不太具体肝素凝血酶相互作用。这项研究表明,SPR是可用于研究,在实时的技术中,两个聚合物表面的改性,与蛋白质的改性表面的后续交互。

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