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DNA杂交体、IgG抗体以及与碳水化合物结合模块融合的IgG结合ZZ结构域的嵌合蛋白络合作用的荧光相关光谱研究

Fluorescence correlation spectroscopy study of the complexation of DNA hybrids, IgG antibody, and a chimeric protein of IgG-binding ZZ domains fused with a carbohydrate binding module.

作者信息

Rosa A M M, Prazeres D M F, Paulo P M R

机构信息

iBB - Institute for Bioengineering and Biosciences, Department of Bioengineering, Instituto Superior Técnico, Universidade de Lisboa, Av. Rovisco Pais 1, 1049-001 Lisbon, Portugal.

出版信息

Phys Chem Chem Phys. 2017 Jun 28;19(25):16606-16614. doi: 10.1039/c7cp00662d.

Abstract

Fluorescence correlation spectroscopy (FCS) was used to characterize the molecular interactions between the four components of a DNA recognition system. A fluorescent DNA probe was used to assess: (i) the hybridization with a complementary biotin-labeled target, (ii) the complexation of the resulting hybrid and an anti-biotin antibody, and (iii) the binding of the latter complex to a ZZ-CBM fusion protein that combines small synthetic IgG Fc-binding Z domains with a carbohydrate binding module (CBM). These binding interactions were monitored by exposing the fluorescent DNA probe to different amounts and combinations of the other molecules in solution. Through the analysis of FCS autocorrelation curves, an association constant (K) of 2.9 × 10 M was estimated for DNA·DNA hybridization, and the presence of (non-) complementary target DNA in solution could be discriminated. The specific capture of biotinylated DNA hybrids by anti-biotin IgG was verified, with an apparent K of 2.5 × 10 M. The increment in the diffusion time measured when the DNA·DNA:antibody complexes were in contact with the ZZ-CBM fusion protein suggested that the binding occurs at a stoichiometric ratio of DNA/antibody complex to fusion larger than 1 : 1. The FCS-derived information obtained is useful to gain insight into molecular interactions involved in diagnostic assays.

摘要

荧光相关光谱法(FCS)用于表征DNA识别系统中四种组分之间的分子相互作用。使用荧光DNA探针来评估:(i)与互补生物素标记靶标的杂交,(ii)所得杂交体与抗生物素抗体的络合,以及(iii)后一种络合物与ZZ-CBM融合蛋白的结合,该融合蛋白将小的合成IgG Fc结合Z结构域与碳水化合物结合模块(CBM)结合在一起。通过将荧光DNA探针暴露于溶液中不同量和组合的其他分子来监测这些结合相互作用。通过对FCS自相关曲线的分析,估计DNA·DNA杂交的缔合常数(K)为2.9×10 M,并且可以区分溶液中(非)互补靶DNA的存在。验证了抗生物素IgG对生物素化DNA杂交体的特异性捕获,表观K为2.5×10 M。当DNA·DNA:抗体复合物与ZZ-CBM融合蛋白接触时测量的扩散时间增加表明,结合以DNA/抗体复合物与融合蛋白的化学计量比大于1:1发生。获得的FCS衍生信息有助于深入了解诊断分析中涉及的分子相互作用。

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