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用于检测癌症患者血清免疫反应的酵母表面重组抗原表达(RAYS)

Recombinant antigen expression on yeast surface (RAYS) for the detection of serological immune responses in cancer patients.

作者信息

Mischo Axel, Wadle Andreas, Wätzig Kristin, Jäger Dirk, Stockert Elisabeth, Santiago Darren, Ritter Gerd, Regitz Evi, Jäger Elke, Knuth Alex, Old Lloyd, Pfreundschuh Michael, Renner Christoph

机构信息

I. Med. Klinik, Saarland University Medical School, Homburg/Saar, Germany.

出版信息

Cancer Immun. 2003 Jun 27;3:5.

Abstract

The serological analysis of antigens by recombinant expression cloning (SEREX) has identified a multitude of new tumor antigens in many different tumor entities. These antigens can be grouped into different classes according to their specificities, with cancer/testis antigens appearing to be the most attractive candidates for vaccine development. The observation that CD8 and CD4 T-cell responses against cancer/testis antigens such as NY-ESO-1 correlate with the presence of specific antibodies demonstrates the importance of serological monitoring patients participating in vaccine trials. However, all serological assays available (Western blot, phage display and ELISA) are hampered by the fact that the protein cannot be analyzed in its natural conformation. We have thus developed a yeast display system where the antigen is expressed on the yeast surface (RAYS), allowing for a more natural folding of the protein. To validate this approach we displayed the A33 colorectal cancer antigen on the yeast cell surface and demonstrated specific binding by an A33 monoclonal antibody recognizing a conformation-dependent epitope on the A33 antigen. We then compared RAYS with the more commonly used ELISA and Western blot serological monitoring methods by analyzing 50 sera from cancer patients with known NY-ESO-1 antibody status and 10 sera from patients with unknown SSX2 antibody status in a blind fashion. RAYS appears at least equivalent to both ELISA and Western blotting for the monitoring of antibodies against NY-ESO-1 as regards specificity and sensitivity, while antibodies against SSX2 were detected more frequently by RAYS than by ELISA or phage display.

摘要

通过重组表达克隆进行抗原的血清学分析(SEREX)已在许多不同肿瘤实体中鉴定出大量新的肿瘤抗原。这些抗原可根据其特异性分为不同类别,其中癌胚抗原似乎是疫苗开发中最具吸引力的候选抗原。针对癌胚抗原(如NY-ESO-1)的CD8和CD4 T细胞反应与特异性抗体的存在相关,这一观察结果证明了对参与疫苗试验的患者进行血清学监测的重要性。然而,现有的所有血清学检测方法(蛋白质印迹法、噬菌体展示法和酶联免疫吸附测定法)都受到无法对天然构象的蛋白质进行分析这一事实的限制。因此,我们开发了一种酵母展示系统,其中抗原在酵母表面表达(RAYS),使蛋白质能够更自然地折叠。为了验证这种方法,我们将A33结直肠癌抗原展示在酵母细胞表面,并通过识别A33抗原上构象依赖性表位的A33单克隆抗体证明了特异性结合。然后,我们以盲法分析了50份已知NY-ESO-1抗体状态的癌症患者血清和10份未知SSX2抗体状态的患者血清,将RAYS与更常用的酶联免疫吸附测定法和蛋白质印迹血清学监测方法进行了比较。就监测针对NY-ESO-1的抗体而言,RAYS在特异性和敏感性方面至少与酶联免疫吸附测定法和蛋白质印迹法相当,而针对SSX2的抗体通过RAYS检测到的频率高于酶联免疫吸附测定法或噬菌体展示法。

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