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Advantages of aptamers as ligands upon protein detection by AFM-based fishing

机译:APTamers作为配体的蛋白质检测的优点,基于AFM的钓鱼

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摘要

A combined AFM/MS method was employed for protein registration in solution. This method is based on reversible specific capturing of a target protein from a large volume of analyzed solution onto a small sensor area of a chip with immobilized aptamer ligands. Fishing of the core antigen of hepatitis C virus (HCVcoreAg) from 10(-12) M solution of this protein in buffer was carried out. It has been shown that the AFM/MS method allows the detection of HCVcoreAg in the form of a protein conjugate as well as in the presence of protein matrix (components of human serum). At the first stage, aptamer/antigen complexes were AFM-registered on the chip surface after its incubation in 10(-12) M solution of antigen in buffer. A technique for the analysis was developed, and criteria for the evaluation of AFM analysis data based on the counting of the aptamer/antigen complexes were proposed. At the second stage, the mass spectrometric identification of protein objects on the chip surface was accomplished; this allowed the reliable identification of the target protein (the core antigen of hepatitis C virus, HCVcoreAg) and confirmed the AFM analysis data.
机译:在溶液中使用组合的AFM / MS方法进行蛋白质配准。该方法基于从大量分析的溶液到具有固定的适体配体的芯片的小传感器区域上的靶蛋白的可逆特异性捕获。进行捕获丙型肝炎病毒(HCVCOREAG)的核心抗原从10(-12)米在缓冲液中的该蛋白质溶液中进行。已经表明,AFM / MS方法允许以蛋白质缀合物的形式检测HCVCOREAG以及在蛋白质基质的存在(人血清的组分)。在第一阶段,在缓冲液中的10(-12)米抗原溶液的培养后,Aptamer /抗原复合物在芯片表面上注册在芯片表面上。提出了一种用于分析的技术,提出了基于适体/抗原复合物的计数评估AFM分析数据的标准。在第二阶段,完成了芯片表面上的蛋白质物体的质谱鉴定;这允许靶蛋白的可靠鉴定(丙型肝炎病毒的核心抗原,HCVCOREAG)并确认AFM分析数据。

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