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Antibody Binding Site Mapping of SARS-CoV Spike Protein Receptor-Binding Domain by a Combination of Yeast Surface Display and Phage Peptide Library Screening

机译:酵母表面展示和噬菌体肽库筛选相结合的SARS冠状病毒穗蛋白受体结合域的抗体结合位点图

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摘要

The receptor-binding domain (RBD) of severe acute respiratory syndrome coronavirus (SARS-CoV) spike (S) protein plays an important role in viral infection, and is a potential major neutralizing determinant. In this study, three hybridoma cell lines secreting specific monoclonal antibodies against the RBD of the S protein were generated and their exact binding sites were identified. Using yeast surface display, the binding sites of these antibodies were defined to two linear regions on the RBD: S337–360 and S380–399. Using these monoclonal antibodies in phage peptide library screening identified 10 distinct mimotopes 12 amino acids in length. Sequence comparison between native epitopes and these mimotopes further confirmed the binding sites, and revealed key amino acid residues involved in antibody binding. None of these antibodies could neutralize the murine leukemia virus pseudotyped expressing the SARS-CoV spike protein (MLV/SARS-CoV). However, these mAbs could be useful in the diagnosis of SARS-CoV due to their exclusive reactivity with SARS-CoV. Furthermore, this study established a feasible platform for epitope mapping. Yeast surface display combined with phage peptide library screening provides a convenient strategy for the identification of epitope peptides from certain antigenic proteins.
机译:严重急性呼吸系统综合症冠状病毒(SARS-CoV)刺突(S)蛋白的受体结合域(RBD)在病毒感染中起重要作用,并且是潜在的主要中和决定因素。在这项研究中,生成了分泌针对S蛋白RBD的特异性单克隆抗体的三种杂交瘤细胞系,并确定了它们的确切结合位点。通过酵母表面展示,将这些抗体的结合位点定义为RBD上的两个线性区域:S 337–360 和S 380-399 。在噬菌体肽库筛选中使用这些单克隆抗体,鉴定出10个不同的拟表位,长度为12个氨基酸。天然表位与这些模拟表位之间的序列比较进一步证实了结合位点,并揭示了参与抗体结合的关键氨基酸残基。这些抗体都不能中和假表达SARS-CoV峰值蛋白(MLV / SARS-CoV)的鼠白血病病毒。但是,由于这些单克隆抗体与SARS-CoV有独家反应性,因此可用于诊断SARS-CoV。此外,该研究建立了可行的表位作图平台。酵母表面展示结合噬菌体肽库筛选为从某些抗原蛋白鉴定表位肽提供了一种方便的策略。

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  • 来源
    《Viral Immunology》 |2009年第6期|407-415|共9页
  • 作者单位

    Institute of Immunology, the People's Liberation Army, Third Military Medical University, St. 30 Gaotanyan, District Shapingba, Chongqing 400038, China.;

    Institute of Immunology, the People's Liberation Army, Third Military Medical University, St. 30 Gaotanyan, District Shapingba, Chongqing 400038, China.;

    Central Laboratory, Zhujiang Hospital, First Military Medical University, Guangzhou, China.;

    Institute of Immunology, the People's Liberation Army, Third Military Medical University, St. 30 Gaotanyan, District Shapingba, Chongqing 400038, China.;

    Institute of Immunology, the People's Liberation Army, Third Military Medical University, St. 30 Gaotanyan, District Shapingba, Chongqing 400038, China.;

    Central Laboratory, Zhujiang Hospital, First Military Medical University, Guangzhou, China.;

    Institute of Immunology, the People's Liberation Army, Third Military Medical University, St. 30 Gaotanyan, District Shapingba, Chongqing 400038, China.;

    Institute of Immunology, the People's Liberation Army, Third Military Medical University, St. 30 Gaotanyan, District Shapingba, Chongqing 400038, China.;

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