首页> 外文期刊>Mikrochimica Acta: An International Journal for Physical and Chemical Methods of Analysis >Silica microspheres functionalized with the iminodiacetic acid/copper(II) complex as a peroxidase mimic for use in metal affinity chromatography-based colorimetric determination of histidine-tagged proteins
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Silica microspheres functionalized with the iminodiacetic acid/copper(II) complex as a peroxidase mimic for use in metal affinity chromatography-based colorimetric determination of histidine-tagged proteins

机译:用亚单乙酸/铜(II)复合物官能化的二氧化硅微球作为过氧化物酶模拟,用于基于金属亲和力色谱法的比较测定组氨酸标记的蛋白质

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摘要

Monodisperse porous silica microspheres were functionalized with the iminodiacetic acid/copper(II) complex and then evaluated as a group-specific peroxidase-mimicking nanozyme for colorimetric determination of histidine-tagged (His-tagged) proteins. The green fluorescent protein (GFP) was selected as a typical His-tagged protein. The specificity for GFP and the peroxidase-like activity for the selected substrate were obtained by immobilizing the complex on the porous microspheres. The modified microspheres were also evaluated as a group specific immobilized metal affinity chromatography (IMAC) sorbent for the purification of GFP from Escherichia coli extract. The peroxidase-like activity of the microspheres was inhibited by the GFP adsorbed onto the microspheres due to the interaction of His-tagged protein with the immobilized Cu(II) complex. Ortho-phenylenediamine is used as a substrate for the enzyme mimic. The photometric response (measured at 416 nm) is linear in the 9.0-92 mu g center dot mL(-1) GFP concentration range in E. coli lysate. The limit of detection is 6.9 mu g center dot mL(-1).
机译:用亚氨基乙酸/铜(II)络合物官能化的单分散多孔二氧化硅微球,然后评价为特异性过氧化物酶模拟纳米碱基,用于比色测定组氨酸标记(His标记)蛋白的蛋白质。选择绿色荧光蛋白(GFP)作为典型的他标记的蛋白质。通过将复合物固定在多孔微球上,获得所选衬底的GFP和过氧化物酶样活性的特异性。还评估改性的微球作为基团的特异性固定金属亲和层析(IMAC)吸附剂,用于从大肠杆菌提取物中纯化GFP。由于His标记的蛋白质与固定化的Cu(II)复合物,通过吸附到微球上的GFP抑制微球的过氧化物酶样活性。邻苯二胺用作酶模拟的基材。在大肠杆菌裂解物中的9.0-92μg中心点ML(-1)GFP浓度范围内,光度响应(在416nm处测量)是线性的。检测限为6.9μg中心点M1(-1)。

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