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A comparative study of capillary electrophoresis and isothermal titration calorimetry for the determination of binding constant of human serum albumin to monoclonal antibody

机译:毛细管电泳与等温滴定热法测定人血清白蛋白与单克隆抗体结合常数的比较研究

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This paper focuses on the investigation of the interactions between the anti-HSA-mAb and its protein antigen using CZE, ACE, and isothermal titration calorimetry. The CZE revealed the formation of the anti-HSA-mAb center dot HSA and anti-HSA-mAb center dot(HSA)(2) complexes and the binding constants determined by plotting the amount of the bound anti-HSA-mAb as a function of the concentration of HSA. The ACE provided information on the binding strength from the change in effective electrophoretic mobility of the anti-HSA-mAb. These two separation techniques estimated the presence of two binding sites. The equilibrium dissociation constant values obtained by CZE and ACE were found to be 2.26 x 10(-6) M for anti-HSA-mAb center dot HSA, 1.22 x 10(-6) M for anti-HSA-mAb center dot(HSA)(2) and 4.45 x 10(-8) M for anti-HSA-mAb center dot HSA, 1.08 x 10(-7) M for anti-HSA-mAb center dot(HSA)(2), respectively. The dissociation constant data obtained by ACE were in congruence with the values obtained by isothermal titration calorimetry (2.74 x 10(-8) M, 1.04 x 10(-7) M).
机译:本文重点研究了使用CZE,ACE和等温滴定量热法研究抗HSA-mAb及其蛋白抗原之间的相互作用。 CZE揭示了抗HSA-mAb中心点HSA和抗HSA-mAb中心点(HSA)(2)配合物的形成以及通过将结合的抗HSA-mAb量绘制为函数确定的结合常数HSA的浓度。 ACE通过抗HSA-mAb的有效电泳迁移率变化提供了结合强度的信息。这两种分离技术估计存在两个结合位点。通过CZE和ACE获得的平衡解离常数值对于抗HSA-mAb中心点HSA为2.26 x 10(-6)M,对于抗HSA-mAb中心点(HSA)为1.22 x 10(-6)M )(2)和抗HSA-mAb中心点HSA为4.45 x 10(-8)M,抗HSA-mAb中心点(HSA)(2)为1.08 x 10(-7)M.通过ACE获得的解离常数数据与通过等温滴定量热法(2.74 x 10(-8)M,1.04 x 10(-7)M)获得的值一致。

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