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提高蛋白质固定化效率以制备肿瘤相关抗原微阵列:应用于乳腺癌血清中肿瘤标志物的灵敏和特异性检测。

Improvement of protein immobilization for the elaboration of tumor-associated antigen microarrays: application to the sensitive and specific detection of tumor markers from breast cancer sera.

机构信息

Université de Lyon, Institut des Nanotechnologies de Lyon (INL)-UMR CNRS 5270, Ecole Centrale de Lyon, 36 Avenue Guy de Collongue, 69134 Ecully cedex, France.

出版信息

Biosens Bioelectron. 2013 Feb 15;40(1):385-92. doi: 10.1016/j.bios.2012.08.019. Epub 2012 Sep 1.

DOI:10.1016/j.bios.2012.08.019
PMID:23017679
Abstract

There is an urgent need to identify relevant tumor markers showing high sensitivity and specificity for early diagnosis and prognosis of breast cancer. Protein microarrays have demonstrated to be cost-effective, high through-put and powerful tools for screening and identifying tumor markers with only minute samples. Autoantibodies directed against tumor-associated antigens (TAAs) were shown to be relevant tumor markers. However, due to the variability of immune response from one individual to another and depending on the type of cancer, detection of only one type of anti-TAA autoantibody is not sufficient to give a reliable and precise diagnosis. It is necessary to use a set of several TAAs for determining specific autoimmune profiles. Therefore, combining various TAAs on different surfaces could improve sensitivity and specificity for anti-TAA autoantibody detection. Herein a panel of 10 proteins, including well-known tumor-associated antigens (TAAs) and potential new biomarkers of breast cancer, were immobilized onto microstructured microarray under optimized conditions (spotting pH buffer, surface chemistry, blocking procedure), in order to determine an autoimmune signature of breast cancer. Sera from 29 breast cancer patients and 28 healthy donors were screened in sandwich immunoassays on the miniaturized system to detect the eventual presence of anti-TAAs autoantibodies. Results indicated that the detection level of each anti-TAA autoantibody in a given serum sample was strongly dependant on the surface chemistry. Combining five TAAs (p53, Hsp60, Hsp70, Her2-Fc, NY-ESO-1) on two different surface chemistries (NHS and APDMES) allowed the significant detection of more than 82% breast cancer sera.

摘要

迫切需要确定具有高灵敏度和特异性的相关肿瘤标志物,用于乳腺癌的早期诊断和预后。蛋白质微阵列已被证明是一种具有成本效益、高通量和强大的工具,可用于筛选和识别仅微量样本中的肿瘤标志物。针对肿瘤相关抗原 (TAA) 的自身抗体已被证明是相关的肿瘤标志物。然而,由于个体之间免疫反应的可变性以及癌症的类型,仅检测一种类型的抗 TAA 自身抗体不足以提供可靠和精确的诊断。有必要使用一组几种 TAA 来确定特定的自身免疫谱。因此,在不同的表面上结合各种 TAA 可以提高抗 TAA 自身抗体检测的灵敏度和特异性。在此,将 10 种蛋白质(包括众所周知的肿瘤相关抗原 (TAA) 和潜在的新乳腺癌生物标志物)组合在微结构微阵列上,在优化的条件下(点样 pH 缓冲液、表面化学、封闭程序),以确定乳腺癌的自身免疫特征。在微型化系统上的夹心免疫测定中筛选了 29 名乳腺癌患者和 28 名健康供体的血清,以检测抗 TAA 自身抗体的存在。结果表明,给定血清样本中每种抗 TAA 自身抗体的检测水平强烈依赖于表面化学。在两种不同的表面化学(NHS 和 APDMES)上结合五种 TAA(p53、Hsp60、Hsp70、Her2-Fc、NY-ESO-1)可以显著检测到超过 82%的乳腺癌血清。

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