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Production of highly and broad-range specific monoclonal antibodies against hemagglutinin of H5-subtype avian influenza viruses and their differentiation by mass spectrometry

机译:抗H5亚型禽流感病毒血凝素的高范围广泛特异性单克隆抗体的生产及其质谱鉴定

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The highly pathogenic avian influenza viruses of the H5 subtype, such as the H5N1 viral strains or the novel H5N8 and H5N2 reassortants, are of both veterinary and public health concern worldwide. To combat these viruses, monoclonal antibodies (mAbs) against H5 hemagglutinin (HA) play a significant role. These mAbs are effective diagnostic and therapeutic agents and powerful tools in vaccine development and basic scientific research. The aim of this study was to obtain diagnostically valuable mAbs with broad strain specificity against H5-subtype AIVs. We applied the hybridoma method to produce anti-HA mAbs. The cloning and screening procedures resulted in the selection of 7 mouse hybridoma cell lines and their respective antibody clones. Preliminary immunoreactivity studies showed that these newly established mAbs, all of the IgG1 isotype, had high specificity and broad-range activities against the H5 HAs. However, these studies did not allow for a clear distinction among the selected antibodies and mAb-secreting hybridoma clones. To differentiate the analyzed mAbs and determine the exact number of hybridoma clones, peptide mapping of the Fc and Fab fragments was performed using a Matrix-Assisted Laser Desorption Ionization Time of Flight (MALDI-TOF/TOF) mass spectrometer. Detailed analyses of the acquired MS and MS/MS spectra confirmed that the Fc fragments constituted highly conserved species- and isotype-immunoglobulin components, whereas the Fab fragments exhibited considerable variation in the sequences that determine antibody specificity. This approach enabled unambiguous characterization of the selected mAbs according to their peptide composition. As a result, 6 different clones were distinguished. Our work provided a unique panel of anti-H5 HA mAbs, which meets the demand for novel, high-specificity analytical tools for use in serologic surveillance. Applications of these mAbs in areas other than diagnostics are also possible. Moreover, we demonstrated for the first time that peptide mapping of antibody fragments with mass spectrometry is an efficient method for the differentiation of antibody clones and relevant antibody-producing cell lines. The method may be successfully used to characterize mAbs at the protein level.
机译:H5亚型的高致病性禽流感病毒,例如H5N1病毒株或新型H5N8和H5N2重配株,在全世界范围内都受到兽医和公共卫生的关注。为了对抗这些病毒,针对H5血凝素(HA)的单克隆抗体(mAb)发挥了重要作用。这些mAb是疫苗开发和基础科学研究中的有效诊断和治疗剂以及强大的工具。这项研究的目的是获得对H5亚型AIV具有广泛毒株特异性的具有诊断价值的单克隆抗体。我们将杂交瘤方法应用于生产抗HA mAb。克隆和筛选程序导致选择了7种小鼠杂交瘤细胞系及其各自的抗体克隆。初步的免疫反应性研究表明,这些新近建立的mAb,即所有IgG1同种型,均具有针对H5 HA的高特异性和广泛活性。但是,这些研究并未明确区分所选抗体和分泌mAb的杂交瘤细胞克隆。为了区分分析的mAb并确定杂交瘤克隆的确切数量,使用基质辅助激光解吸电离飞行时间(MALDI-TOF / TOF)质谱仪对Fc和Fab片段进行肽图分析。对获得的MS和MS / MS谱图的详细分析证实,Fc片段构成高度保守的物种和同种型免疫球蛋白成分,而Fab片段在决定抗体特异性的序列中表现出相当大的变异。这种方法能够根据所选mAb的肽组成对其进行明确表征。结果,区分出6个不同的克隆。我们的工作提供了独特的抗H5 HA mAb面板,可满足对用于血清学监测的新型高特异性分析工具的需求。这些mAb还可用于诊断以外的领域。此外,我们首次证明用质谱对抗体片段进行肽图分析是区分抗体克隆和相关抗体生产细胞系的有效方法。该方法可成功用于在蛋白质水平上表征mAb。

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