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使用互补的 LC-MS 方法对一种重组流感疫苗候选物进行表征。

Characterization of a recombinant influenza vaccine candidate using complementary LC-MS methods.

机构信息

Department of Biopharmaceutical Sciences, Waters Corporation, Milford, MA 01757, USA.

出版信息

Curr Pharm Biotechnol. 2011 Oct;12(10):1568-79. doi: 10.2174/138920111798357447.

DOI:10.2174/138920111798357447
PMID:21542793
Abstract

Influenza vaccination is recognized as the most effective method for reducing morbidity and mortality due to seasonal influenza. To improve vaccine supply and to increase flexibility in vaccine manufacturing, cell culture-based vaccine production has emerged to overcome limitations of egg-based production. The switch of production system and the need for annual re-evaluation of vaccines for the effectiveness due to frequent viral antigenic changes call for methods for complete characterization of the hemagglutinin (HA) antigens and the final vaccine products. This study describes advanced liquid chromatography-mass spectrometry (LC-MS) methods for simultaneous identification of HA proteins and process-related impurities in a trivalent influenza candidate vaccine, comprised of purified recombinant HA (rHA) antigens produced in an insect cell-baculovirus expression vector system (BEVS). N-linked glycosylation sites and glycoforms of the three rHA proteins (corresponding to influenza A subtypes H1N1 and H3N2 and B virus, respectively) were profiled by peptide mapping using reversed-phase (RP) LC-MS(E) (data independent acquisition LC-MS using an alternating low and elevated collision energy scan mode). The detected site-specific glycoforms were further confirmed and quantified by hydrophilic interaction LC (HILIC)-multiple reaction monitoring (MRM) assays. LC-MS(E) was used to characterize the vaccine candidate, providing both protein identities and site-specific information of glycosylation and degradations on each rHA protein. HILIC-MRM methodology was used for rapid confirming and quantifying site-specific glycoforms and potential degradations on each rHA protein. These methods can contribute to the monitoring of vaccine quality especially as it pertains to product comparability studies to evaluate the impact of production process changes.

摘要

流感疫苗接种被认为是降低季节性流感发病率和死亡率的最有效方法。为了提高疫苗供应的灵活性,克服基于鸡蛋的生产的局限性,细胞培养疫苗生产已经出现。生产系统的转变以及由于频繁的病毒抗原变化需要每年重新评估疫苗的有效性,这就需要对血凝素(HA)抗原和最终疫苗产品进行全面的特性描述。本研究描述了用于同时鉴定三价流感候选疫苗中 HA 蛋白和与过程相关杂质的先进液相色谱-质谱(LC-MS)方法,该候选疫苗由在昆虫细胞-杆状病毒表达载体系统(BEVS)中生产的纯化重组 HA(rHA)抗原组成。通过使用反相(RP)LC-MS(E)(使用交替低和升高碰撞能扫描模式的数据非依赖性采集 LC-MS)进行肽图分析,对三种 rHA 蛋白(分别对应于流感 A 亚型 H1N1 和 H3N2 以及 B 病毒)的 N-连接糖基化位点和糖型进行了分析。通过亲水作用 LC(HILIC)-多重反应监测(MRM)测定进一步确认和定量检测到的特定位点糖型。LC-MS(E)用于分析候选疫苗,提供每个 rHA 蛋白的蛋白身份以及糖基化和降解的特定位点信息。HILIC-MRM 方法用于快速鉴定和定量每个 rHA 蛋白的特定位点糖型和潜在降解产物。这些方法可以有助于监测疫苗质量,特别是在产品可比性研究中,以评估生产工艺变化的影响。

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