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通过表面等离子体共振对维生素B12结合蛋白与钴胺素之间相互作用的平衡和动力学分析。

Equilibrium and kinetic analyses of the interactions between vitamin B(12) binding proteins and cobalamins by surface plasmon resonance.

作者信息

Cannon Michelle J, Myszka David G, Bagnato Joshua D, Alpers David H, West Frederick G, Grissom Charles B

机构信息

Department of Chemistry, University of Utah, 315 S. 1400 E., Salt Lake City, UT 84112-0850, USA.

出版信息

Anal Biochem. 2002 Jun 1;305(1):1-9. doi: 10.1006/abio.2002.5647.

DOI:10.1006/abio.2002.5647
PMID:12018940
Abstract

Surface plasmon resonance biosensor analysis was used to evaluate the thermodynamics and binding kinetics of naturally occurring and synthetic cobalamins interacting with vitamin B(12) binding proteins. Cyanocobalamin-b-(5-aminopentylamide) was immobilized on a biosensor chip surface to determine the affinity of different cobalamins for transcobalamin, intrinsic factor, and nonintrinsic factor. A solution competition binding assay, in which a surface immobilized cobalamin analog competes with analyte cobalamin for B(12) protein binding, shows that only recombinant human transcobalamin is sensitive to modification of the corrin ring b-propionamide of cyanocobalamin. A direct binding assay, where recombinant human transcobalamin is conjugated to a biosensor chip, allows kinetic analysis of cobalamin binding. Response data for cyanocobalamin binding to the transcobalamin protein surface were globally fitted to a bimolecular interaction model that includes a term for mass transport. This model yields association and dissociation rate constants of k(a) = 3 x 10(7) M(-1) s(-1) and k(d) = 6 x 10(-4) s(-1), respectively, with an overall dissociation constant of K(D) = 20 pM at 30 degrees C. Transcobalamin binds cyanocobalamin-b-(5-aminopentylamide) with association and dissociation rates that are twofold slower and threefold faster, respectively, than transcobalamin binding to cyanocobalamin. The affinities determined for protein-ligand interaction, using the solution competition and direct binding assays, are comparable, demonstrating that surface plasmon resonance provides a versatile way to study the molecular recognition properties of vitamin B(12) binding proteins.

摘要

表面等离子体共振生物传感器分析用于评估天然存在的和合成的钴胺素与维生素B12结合蛋白相互作用的热力学和结合动力学。将氰钴胺素-b-(5-氨基戊酰胺)固定在生物传感器芯片表面,以确定不同钴胺素对转钴胺素、内因子和非内因子的亲和力。一种溶液竞争结合测定法,其中表面固定的钴胺素类似物与分析物钴胺素竞争B12蛋白结合,结果表明只有重组人转钴胺素对氰钴胺素的钴胺环b-丙酰胺修饰敏感。一种直接结合测定法,将重组人转钴胺素与生物传感器芯片偶联,可对钴胺素结合进行动力学分析。氰钴胺素与转钴胺素蛋白表面结合的响应数据整体拟合到一个包含传质项的双分子相互作用模型中。该模型在30℃时分别得到结合和解离速率常数ka = 3×107 M-1 s-1和kd = 6×10-4 s-1,总解离常数KD = 20 pM。转钴胺素与氰钴胺素-b-(5-氨基戊酰胺)结合的结合和解离速率分别比转钴胺素与氰钴胺素结合慢两倍和快三倍。使用溶液竞争和直接结合测定法确定的蛋白质-配体相互作用亲和力具有可比性,表明表面等离子体共振为研究维生素B12结合蛋白的分子识别特性提供了一种通用方法。

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