工程β-半乳糖苷酶传感器对抗体结合的增强反应

Jordi X Feliu , Neus Ferrer-Miralles , Esther Blanco , Daniel Cazorla , Francisco Sobrino , Antonio Villaverde
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引用次数: 23

摘要

肽显示在工程酶的溶剂暴露表面上,使它们能够通过可检测的酶活性变化对抗肽抗体作出反应,为生物传感器的开发提供了新的原理。在这项工作中,我们发现在大肠杆菌β-半乳糖苷酶活性位点附近插入多个肽可以显著提高酶对特定抗肽抗体的反应性。修饰酶HD7872A和HT7278CA,每个酶分子分别携带8个和12个口蹄疫肽拷贝,显示出抗体介导的激活因子高于先前在第一代酶传感器中观察到的,其中HT7278CA接近400%。对多个插入蛋白的信号转导过程的分析强烈提示了一种新的、非排他的酶调节机制,在这种机制中,结合的抗体可能会稳定靶蛋白,延长酶的半衰期,从而提高信号背景比。此外,测试的传感器对来自免疫农场动物的血清的反应不同,这取决于免疫病毒中的b细胞表位与酶表面用作传感元件的肽中的b细胞表位之间的抗原相似性。总之,这些结果指出了这些酶生物传感器在一个极快的同质分析中对口蹄疫的简单诊断的效用。
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Enhanced response to antibody binding in engineered β-galactosidase enzymatic sensors

Peptide display on solvent-exposed surfaces of engineered enzymes allows them to respond to anti-peptide antibodies by detectable changes in their enzymatic activity, offering a new principle for biosensor development. In this work, we show that multiple peptide insertion in the vicinity of the Escherichia coli β-galactosidase active site dramatically increases the enzyme responsiveness to specific anti-peptide antibodies. The modified enzymes HD7872A and HT7278CA, carrying eight and 12 copies respectively of a foot-and-mouth disease peptide per enzyme molecule, show antibody-mediated activation factors higher than those previously observed in the first generation enzymatic sensors, for HT7278CA being close to 400%. The analysis of the signal transduction process with multiple inserted proteins strongly suggests a new, non-exclusive mechanism of enzymatic regulation in which the target proteins might be stabilised by the bound antibody, extending the enzyme half-life and consequently enhancing the signal–background ratio. In addition, the tested sensors are differently responsive to sera from immune farm animals, depending on the antigenic similarity between the B-cell epitopes in the immunising virus and those in the peptide used as sensing element on the enzyme surface. Altogether, these results point out the utility of these enzymatic biosensors for a simple diagnosis of foot-and-mouth disease in an extremely fast homogeneous assay.

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