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变性、表面吸附抗体的飞行时间二次离子质谱及主成分分析研究

ToF-SIMS and Principal Component Analysis Investigation of Denatured, Surface-Adsorbed Antibodies.

作者信息

Welch Nicholas G, Madiona Robert M T, Scoble Judith A, Muir Benjamin W, Pigram Paul J

机构信息

Centre for Materials and Surface Science and Department of Chemistry and Physics, School of Molecular Sciences, La Trobe University , Melbourne, VIC 3086, Australia.

CSIRO Manufacturing , Clayton, VIC 3168, Australia.

出版信息

Langmuir. 2016 Oct 25;32(42):10824-10834. doi: 10.1021/acs.langmuir.6b02754. Epub 2016 Oct 14.

Abstract

Antibody denaturation at solid-liquid interfaces plays an important role in the sensitivity of protein assays such as enzyme-linked immunosorbent assays (ELISAs). Surface immobilized antibodies must maintain their native state, with their antigen binding (Fab) region intact, to capture antigens from biological samples and permit disease detection. In this work, two identical sample sets were prepared with whole antibody IgG, F(ab') and Fc fragments, immobilized to either a silicon wafer or a diethylene glycol dimethyl ether plasma polymer surface. Analysis was conducted on one sample set at day 0, and the second sample set after 14 days in vacuum, with time-of-flight secondary ion mass spectrometry (ToF-SIMS) for molecular species representative of denaturation. A 1003 mass fragment peak list was compiled from ToF-SIMS data and compared to a 35 amino acid mass fragment peak list using principal component analysis. Several ToF-SIMS secondary ions, pertaining to disulfide and thiol species, were identified in the 14 day (presumably denatured) samples. A substrate and primary ion independent marker for denaturation (aging) was then produced using a ratio of mass peak intensities according to denaturation ratio: [I + I + I + I + I]/[I + I + I + I]. The ratio successfully identifies denaturation on both the silicon and plasma polymer substrates and for spectra generated with Mn, Bi, and Bi primary ions. We believe this ratio could be employed to as a marker of denaturation of antibodies on a plethora of substrates.

摘要

抗体在固液界面的变性在诸如酶联免疫吸附测定(ELISA)等蛋白质检测的灵敏度方面起着重要作用。表面固定的抗体必须保持其天然状态,其抗原结合(Fab)区域完整,以便从生物样品中捕获抗原并实现疾病检测。在这项工作中,制备了两组相同的样品,将完整抗体IgG、F(ab')和Fc片段固定在硅片或二甘醇二甲醚等离子体聚合物表面。在第0天对一组样品进行分析,第二组样品在真空中放置14天后,使用飞行时间二次离子质谱(ToF-SIMS)对代表变性的分子种类进行分析。从ToF-SIMS数据编制了一个1003质量碎片峰列表,并使用主成分分析将其与一个35个氨基酸的质量碎片峰列表进行比较。在14天(可能已变性)的样品中鉴定出了几个与二硫键和硫醇种类有关的ToF-SIMS二次离子。然后根据变性比[I + I + I + I + I]/[I + I + I + I],利用质量峰强度比产生了一种与底物和一次离子无关的变性(老化)标记物。该比值成功地识别了硅和等离子体聚合物底物上的变性情况,以及用Mn、Bi和Bi一次离子产生的光谱中的变性情况。我们相信这个比值可以用作多种底物上抗体变性的标记物。

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