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免疫亲和捕获和同位素稀释液相色谱-串联质谱法定量检测免疫反应性病毒流感蛋白。

Quantification of immunoreactive viral influenza proteins by immunoaffinity capture and isotope-dilution liquid chromatography-tandem mass spectrometry.

机构信息

Division of Laboratory Sciences, National Center for Environmental Health, Centers for Disease Control and Prevention, 4770 Buford Highway, MS F-50, Atlanta, Georgia 30341, USA.

出版信息

Anal Chem. 2011 Jun 15;83(12):4729-37. doi: 10.1021/ac2006526. Epub 2011 May 26.

DOI:10.1021/ac2006526
PMID:21591780
Abstract

An immunocapture isotope dilution mass spectrometry (IC-IDMS) method was developed to quantify antibody-bound influenza hemagglutinins (HA) in trivalent influenza vaccines (TIV). Currently, regulatory potency requirements for TIV require HA quantification based on the single radial immunodiffusion (SRID) assay, which is time-consuming, laborious, and requires production of large quantities of reagents globally. In IC-IDMS, antiserum to the HA of interest captured viral proteins that were in the correct conformation to be recognized by the antibodies. The captured proteins were digested, and evolutionarily conserved tryptic peptides were quantified using isotope-dilution liquid chromatography-tandem mass spectrometry. IC-IDMS relies on antibody-antigen binding similar to SRID but incorporates the accuracy and precision of IDMS. Polyclonal antibodies (pAb-H3) prepared by injection of sheep with purified H3 HA captured 82.9% (55.26 fmol/μL) of the total H3 HA (66.69 fmol/μL) from the commercial TIV and 93.6% (57.23 fmol/μL) of the total H3 HA (61.14 fmol/μL) in purified virus. While other HA (H1, B), neuraminidase (N1, N2, NB), viral matrix proteins, and nucleoproteins were also captured by this antiserum, our results were not affected due to the specificity of the mass spectrometer. IC-IDMS is an accurate, precise, sensitive, and selective method to measure antibody-bound HA in purified virus and commercial vaccines.

摘要

建立了一种免疫捕获同位素稀释质谱(IC-IDMS)方法,用于定量三价流感疫苗(TIV)中结合的抗体的流感血凝素(HA)。目前,TIV 的监管效力要求基于单放射免疫扩散(SRID)测定法进行 HA 定量,该方法既耗时又费力,并且需要在全球范围内生产大量试剂。在 IC-IDMS 中,针对感兴趣的 HA 的抗血清捕获了具有正确构象以被抗体识别的病毒蛋白。捕获的蛋白被消化,并用同位素稀释的液相色谱-串联质谱法定量分析进化保守的胰蛋白酶肽。IC-IDMS 依赖于类似于 SRID 的抗体-抗原结合,但结合了 IDMS 的准确性和精密度。用纯化的 H3 HA 免疫绵羊制备的多克隆抗体(pAb-H3)可从商业 TIV 中捕获 82.9%(55.26 fmol/μL)的总 H3 HA(66.69 fmol/μL)和从纯化病毒中捕获 93.6%(57.23 fmol/μL)的总 H3 HA(61.14 fmol/μL)。虽然该抗血清还捕获了其他 HA(H1、B)、神经氨酸酶(N1、N2、NB)、病毒基质蛋白和核蛋白,但由于质谱仪的特异性,我们的结果不受影响。IC-IDMS 是一种准确、精密、灵敏和选择性的方法,可用于测量纯化病毒和商业疫苗中结合的抗体的 HA。

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