Tscherne Alina, Kalodimou Georgia, Kupke Alexandra, Rohde Cornelius, Freudenstein Astrid, Jany Sylvia, Kumar Satendra, Sutter Gerd, Krähling Verena, Becker Stephan, Volz Asisa
Division of Virology, Department of Veterinary Sciences, Ludwig Maximilians University (LMU Munich), 85764 Oberschleißheim, Germany.
German Center for Infection Research, Partner Site Munich, 85764 Oberschleißheim, Germany.
Vaccines (Basel). 2024 Nov 24;12(12):1316. doi: 10.3390/vaccines12121316.
BACKGROUND/OBJECTIVES: Marburg virus (MARV) is the etiological agent of Marburg Virus Disease (MVD), a rare but severe hemorrhagic fever disease with high case fatality rates in humans. Smaller outbreaks have frequently been reported in countries in Africa over the last few years, and confirmed human cases outside Africa are, so far, exclusively imported by returning travelers. Over the previous years, MARV has also spread to non-endemic African countries, demonstrating its potential to cause epidemics. Although MARV-specific vaccines are evaluated in preclinical and clinical research, none have been approved for human use. Modified Vaccinia virus Ankara (MVA), a well-established viral vector used to generate vaccines against emerging pathogens, can deliver multiple antigens and has a remarkable clinical safety and immunogenicity record, further supporting its evaluation as a vaccine against MARV. The rapid availability of safe and effective MVA-MARV vaccine candidates would expand the possibilities of multi-factored intervention strategies in endemic countries.
We have used an optimized methodology to rapidly generate and characterize recombinant MVA candidate vaccines that meet the quality requirements to proceed to human clinical trials. As a proof-of-concept for the optimized methodology, we generated two recombinant MVAs that deliver either the MARV glycoprotein (MVA-MARV-GP) or the MARV nucleoprotein (MVA-MARV-NP).
Infections of human cell cultures with recombinant MVA-MARV-GP and MVA-MARV-NP confirmed the efficient synthesis of MARV-GP and MARV-NP proteins in mammalian cells, which are non-permissive for MVA replication. Prime-boost immunizations in C57BL/6J mice readily induced circulating serum antibodies binding to recombinant MARV-GP and MARV-NP proteins. Moreover, the MVA-MARV-candidate vaccines elicited MARV-specific T-cell responses in C57BL/6J mice.
We confirmed the suitability of our two backbone viruses MVA-mCherry and MVA-GFP in a proof-of-concept study to rapidly generate candidate vaccines against MARV. However, further studies are warranted to characterize the protective efficacy of these recombinant MVA-MARV vaccines in other preclinical models and to evaluate them as vaccine candidates in humans.
背景/目的:马尔堡病毒(MARV)是马尔堡病毒病(MVD)的病原体,MVD是一种罕见但严重的出血热疾病,人类病死率很高。在过去几年中,非洲国家频繁报告小规模疫情,而且到目前为止,非洲以外确诊的人类病例均为由回国旅行者输入。在过去几年里,马尔堡病毒还传播到了非洲非流行国家,显示出其引发疫情的潜力。尽管针对马尔堡病毒的特异性疫苗正在进行临床前和临床研究评估,但尚无疫苗获批用于人类。安卡拉改良痘苗病毒(MVA)是一种成熟的病毒载体,用于生产针对新出现病原体的疫苗,它可以递送多种抗原,并且具有出色的临床安全性和免疫原性记录,这进一步支持将其作为抗马尔堡病毒疫苗进行评估。快速获得安全有效的MVA - MARV候选疫苗将扩大在流行国家采取多因素干预策略的可能性。
我们采用了一种优化方法,快速生成并表征符合进入人体临床试验质量要求的重组MVA候选疫苗。作为优化方法的概念验证,我们生成了两种分别递送马尔堡病毒糖蛋白(MVA - MARV - GP)或马尔堡病毒核蛋白(MVA - MARV - NP)的重组MVA。
用重组MVA - MARV - GP和MVA - MARV - NP感染人类细胞培养物,证实了在对MVA复制不敏感的哺乳动物细胞中高效合成了马尔堡病毒糖蛋白和核蛋白。在C57BL / 6J小鼠中进行的初免 - 加强免疫很容易诱导循环血清抗体与重组马尔堡病毒糖蛋白和核蛋白结合。此外,MVA - MARV候选疫苗在C57BL / 6J小鼠中引发了马尔堡病毒特异性T细胞反应。
我们在一项概念验证研究中证实了我们的两种主干病毒MVA - mCherry和MVA - GFP适用于快速生成抗马尔堡病毒的候选疫苗。然而,有必要进一步开展研究,以表征这些重组MVA - MARV疫苗在其他临床前模型中的保护效果,并评估它们作为人类候选疫苗的潜力。
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