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建立酶联免疫吸附试验(ELISA)快速、灵敏、特异识别画作中蛋白质的分析方案。

Development of an analytical protocol for a fast, sensitive and specific protein recognition in paintings by enzyme-linked immunosorbent assay (ELISA).

机构信息

Centro SMAArt, Dipartimento di Chimica, Università di Perugia, Via Elce di Sotto 8, 06123 Perugia, Italy.

出版信息

Anal Bioanal Chem. 2011 Mar;399(9):3011-23. doi: 10.1007/s00216-010-4308-1. Epub 2010 Dec 19.

DOI:10.1007/s00216-010-4308-1
PMID:21170522
Abstract

Enzyme-linked immunosorbent assay (ELISA) analysis of proteins offers a particularly promising approach for investigations in cultural heritage on account of its appreciated properties of being highly specific, sensitive, relatively fast, and cost-affordable with respect to other conventional techniques. In spite of that, it has never been fully exploited for routine analyses of painting materials in consideration of several analytical issues that inhibited its diffusion in conservation science: limited sample dimensions, decrease of binder solubility and reduced availability of antibody bonding sites occurring with protein degradation. In this study, an ELISA analytical protocol suited for the identification of aged denatured proteins in ancient painting micro-samples has been developed. We focused on the detection of bovine β-casein and chicken ovalbumin as markers of bovine milk (or casein) and chicken albumen, respectively. A systematic experimentation of the ELISA protocol has been carried out on mock-ups of mural and easel painting prepared with 13 different pigments to assess limits and strengths of the method when applied for the identification of proteins in presence of a predominant inorganic matrix. The analytical procedure has been optimized with respect to protein extraction, antibodies' concentrations, incubation time and temperature; it allows the detection of the investigated proteins with sensitivity down to nanograms. The optimized protocol was then tested on artificially aged painting models. Analytical results were very encouraging and demonstrated that ELISA allows for protein analysis also in degraded painting samples. To address the feasibility of the developed ELISA methodology, we positively investigated real painting samples and results have been cross-validated by gas chromatography-mass spectrometry.

摘要

酶联免疫吸附测定(ELISA)分析蛋白质为文化遗产领域的研究提供了一种特别有前景的方法,因为它具有高度特异性、敏感性、相对快速以及相对于其他传统技术而言价格合理等优点。尽管如此,由于存在一些分析问题,如蛋白质降解导致的结合位点减少、结合物溶解度降低和有限的样品尺寸等,该方法从未被充分应用于绘画材料的常规分析中,从而阻碍了它在保护科学中的普及。在这项研究中,我们开发了一种适合于鉴定古代绘画微样本中老化变性蛋白质的 ELISA 分析方案。我们专注于检测牛β-酪蛋白和鸡卵清蛋白,分别作为牛乳制品(或酪蛋白)和鸡白蛋白的标志物。通过对用 13 种不同颜料制备的壁画和架上绘画模拟物进行 ELISA 方案的系统实验,评估了该方法在存在主要无机基质的情况下用于鉴定蛋白质的局限性和优势。该分析程序针对蛋白质提取、抗体浓度、孵育时间和温度进行了优化;它允许以纳克为单位检测到所研究的蛋白质。优化后的方案随后在人工老化的绘画模型上进行了测试。分析结果非常令人鼓舞,证明了 ELISA 允许在降解的绘画样品中进行蛋白质分析。为了评估所开发的 ELISA 方法的可行性,我们积极研究了真实的绘画样本,并通过气相色谱-质谱法对结果进行了交叉验证。

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