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利用反向疫苗学开发 B 型脑膜炎球菌疫苗。

The Development of a Vaccine Against Meningococcus B Using Reverse Vaccinology.

机构信息

GSK Vaccines, Siena, Italy.

Department of Pediatrics, Oxford University, Oxford, United Kingdom.

出版信息

Front Immunol. 2019 Apr 16;10:751. doi: 10.3389/fimmu.2019.00751. eCollection 2019.

DOI:10.3389/fimmu.2019.00751
PMID:31040844
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6477034/
Abstract

The discovery of vaccine antigens through whole genome sequencing (WGS) contrasts with the classical hypothesis-driven laboratory-based analysis of microbes to identify components to elicit protective immunity. This radical change in scientific direction and action in vaccine research is captured in the term . The complete genome sequence of an isolate of serogroup B (MenB) was systematically analyzed to identify proteins predicted to be secreted or exported to the outer membrane. This identified hundreds of genes coding for potential surface-exposed antigens. These were amplified, cloned in expression vectors and used to immunize mice. Antisera against 350 recombinant antigens were obtained and analyzed in a panel of immunological assays from which 28 were selected as potentially protective based on the -antibody dependent, complement mediated- serum bactericidal activity assay. Testing of these candidate vaccine antigens, using a large globally representative strain collection of Neisseria species isolated from cases of disease and carriage, indicated that no single component would be sufficient to induce broad coverage and that a "universal" vaccine should contain multiple antigens. The final choice of antigens to be included was based on cross-protective ability, assayed by serum bactericidal activity and maximum coverage of the extensive antigenic variability of MenB strains. The resulting multivalent vaccine formulation selected consisted of three recombinant antigens (Neisserial Heparin Binding Antigen or NHBA, Factor H binding protein or fHbp and Neisseria Adhesin A or NadA). To improve immunogenicity and potential strain coverage, an outer membrane vesicle component obtained from the epidemic New Zealand strain (OMVNz) was added to the formulation to create a four component vaccine, called 4CMenB. A series of phase 2 and 3 clinical trials were conducted to evaluate safety and tolerability and to estimate the vaccine effectiveness of human immune responses at different ages and how these were affected by various factors including concomitant vaccine use and lot-to-lot consistency. 4CMenB was approved in Europe in 2013 and introduced in the National Immunization Program in the UK starting from September 2015 when the vaccine was offered to all newborns using a 2, 4, and 12 months schedule., The effectiveness against invasive MenB disease measured at 11 months after the study start and 5 months after the second vaccination was 83% and there have been no safety concerns.

摘要

通过全基因组测序(WGS)发现疫苗抗原,与通过经典的基于实验室的基于微生物的分析来识别引发保护性免疫的成分形成鲜明对比。这种疫苗研究中科学方向和行动的彻底改变体现在术语 中。对 B 群(MenB)血清型分离株的完整基因组序列进行了系统分析,以鉴定预测分泌或输出至外膜的蛋白质。这鉴定了数百个编码潜在表面暴露抗原的基因。这些基因被扩增、克隆在表达载体中,并用于免疫小鼠。针对 350 种重组抗原的抗血清获得,并在一系列免疫测定中进行分析,其中 28 种基于抗体依赖性、补体介导的血清杀菌活性测定被选为潜在保护性抗原。使用从疾病和携带病例中分离的大量具有全球代表性的奈瑟菌种菌株的集合对这些候选疫苗抗原进行测试表明,没有单一成分足以诱导广泛的覆盖范围,并且“通用”疫苗应该包含多种抗原。选择包含的抗原最终基于交叉保护能力,通过血清杀菌活性和 MenB 菌株广泛抗原变异性的最大覆盖范围进行测定。选择的包含三个重组抗原(奈瑟氏菌肝素结合抗原或 NHBA、因子 H 结合蛋白或 fHbp 和奈瑟氏菌粘附素 A 或 NadA)的多价疫苗制剂。为了提高免疫原性和潜在的菌株覆盖率,从流行的新西兰菌株(OMVNz)获得的外膜囊泡成分被添加到制剂中,以创建一种四价疫苗,称为 4CMenB。进行了一系列 2 期和 3 期临床试验,以评估安全性和耐受性,并估计不同年龄组人类免疫反应的疫苗有效性以及这些反应如何受到各种因素的影响,包括同时使用疫苗和批次一致性。4CMenB 于 2013 年在欧洲获得批准,并于 2015 年 9 月在英国国家免疫计划中引入,当时该疫苗以 2、4 和 12 个月的时间表提供给所有新生儿。研究开始后 11 个月和第二次接种后 5 个月测量的针对侵袭性 MenB 疾病的有效性为 83%,并且没有安全性问题。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/4fb1eed621c9/fimmu-10-00751-g0005.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/1ee98ffdaad9/fimmu-10-00751-g0001.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/4fb1eed621c9/fimmu-10-00751-g0005.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/1ee98ffdaad9/fimmu-10-00751-g0001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/9ad9d782224f/fimmu-10-00751-g0002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/3c3ef7bbfa6f/fimmu-10-00751-g0003.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/c6a40c7bc2fc/fimmu-10-00751-g0004.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cf3/6477034/4fb1eed621c9/fimmu-10-00751-g0005.jpg

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