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基于水凝胶的分子印迹聚合物(HydroMIPs)内蛋白质结合亲和力的测定。

Determination of protein binding affinities within hydrogel-based molecularly imprinted polymers (HydroMIPs).

作者信息

EL-Sharif Hazim F, Hawkins Daniel M, Stevenson Derek, Reddy Subrayal M

机构信息

Department of Chemistry, Faculty of Engineering and Physical Sciences, University of Surrey, Guildford, Surrey, GU2 7XH, UK.

出版信息

Phys Chem Chem Phys. 2014 Aug 7;16(29):15483-9. doi: 10.1039/c4cp01798f. Epub 2014 Jun 20.

DOI:10.1039/c4cp01798f
PMID:24950144
Abstract

Hydrogel-based molecularly imprinted polymers (HydroMIPs) were prepared for several proteins (haemoglobin, myoglobin and catalase) using a family of acrylamide-based monomers. Protein affinity towards the HydroMIPs was investigated under equilibrium conditions and over a range of concentrations using specific binding with Hill slope saturation profiles. We report HydroMIP binding affinities, in terms of equilibrium dissociation constants (Kd) within the micro-molar range (25 ± 4 μM, 44 ± 3 μM, 17 ± 2 μM for haemoglobin, myoglobin and catalase respectively within a polyacrylamide-based MIP). The extent of non-specific binding or cross-selectivity for non-target proteins has also been assessed. It is concluded that both selectivity and affinity for both cognate and non-cognate proteins towards the MIPs were dependent on the concentration and the complementarity of their structures and size. This is tentatively attributed to the formation of protein complexes during both the polymerisation and rebinding stages at high protein concentrations. We have used atomic force spectroscopy to characterize molecular interactions in the MIP cavities using protein-modified AFM tips. Attractive and repulsive force curves were obtained for the MIP and NIP (non-imprinted polymer) surfaces (under protein loaded or unloaded states). Our force data suggest that we have produced selective cavities for the template protein in the MIPs and we have been able to quantify the extent of non-specific protein binding on, for example, a non-imprinted polymer (NIP) control surface.

摘要

使用一系列基于丙烯酰胺的单体,制备了用于几种蛋白质(血红蛋白、肌红蛋白和过氧化氢酶)的水凝胶基分子印迹聚合物(HydroMIPs)。在平衡条件下,使用具有希尔斜率饱和曲线的特异性结合,研究了蛋白质对HydroMIPs的亲和力,并考察了一系列浓度范围。我们报道了HydroMIPs的结合亲和力,以基于聚丙烯酰胺的分子印迹聚合物中血红蛋白、肌红蛋白和过氧化氢酶的平衡解离常数(Kd)表示,分别在微摩尔范围内(分别为25±4μM、44±3μM、17±2μM)。还评估了非靶标蛋白质的非特异性结合或交叉选择性程度。得出的结论是,同源和非同源蛋白质对分子印迹聚合物的选择性和亲和力均取决于其浓度以及结构和大小的互补性。这初步归因于在高蛋白质浓度下聚合和再结合阶段蛋白质复合物的形成。我们使用原子力光谱法,通过蛋白质修饰的原子力显微镜探针来表征分子印迹聚合物腔体内的分子相互作用。获得了分子印迹聚合物和非印迹聚合物(NIP)表面(在加载或未加载蛋白质状态下)的吸引力和排斥力曲线。我们的力数据表明,我们在分子印迹聚合物中为模板蛋白产生了选择性腔体,并且能够量化例如非印迹聚合物(NIP)对照表面上非特异性蛋白质结合的程度。

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