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Chimeric Influenza Virus Hemagglutinin Proteins Containing Large Domains of the Bacillus anthracis Protective Antigen: Protein Characterization, Incorporation into Infectious Influenza Viruses, and Antigenicity

机译:包含大域炭疽芽孢杆菌保护性抗原的嵌合流感病毒血凝素蛋白:蛋白质表征,并入传染性流感病毒和抗原性

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摘要

Large polypeptides of the Bacillus anthracis protective antigen (PA) were inserted into an influenza A virus hemagglutinin glycoprotein (HA), and the chimeric proteins were functionally characterized and incorporated into infectious influenza viruses. PA domain 1′, the region responsible for binding to the other toxin components, the lethal factor and edema factor, and domain 4, the receptor binding domain (RBD), were inserted at the C-terminal flank of the HA signal peptide and incorporated into the HA1 subunit of HA. The chimeric proteins, designated as LEF/HA (90 amino acid insertion) and RBD/HA (140 amino acid insertion), were initially analyzed following expression using recombinant vaccinia viruses. Both chimeric proteins were shown to display functional phenotypes similar to that of the wild-type HA. They transport to the cell surface, can be cleaved into the HA1 and HA2 subunits by trypsin to activate membrane fusion potential, are able to undergo the low-pH-induced conformational changes required for fusion, and are capable of inducing the fusion process. We were also able to generate recombinant influenza viruses containing the chimeric RBD/HA and LEF/HA genes, and the inserted PA domains were maintained in the HA gene segments following several passages in MDCK cells or embryonated chicken eggs. Furthermore, DNA immunization of mice with plasmids that express the chimeric RBD/HA and LEF/HA proteins, and the recombinant viruses containing them, induced antibody responses against both the HA and PA components of the protein. These approaches may provide useful tools for vaccines against anthrax and other diseases.
机译:将炭疽芽孢杆菌保护性抗原(PA)的大多肽插入A型流感病毒血凝素糖蛋白(HA)中,并对嵌合蛋白进行功能鉴定,并掺入传染性流感病毒中。 PA结构域1'(负责与其他毒素成分,致死因子和浮肿因子结合的区域)和结构域4(受体结合结构域(RBD))插入HA信号肽的C末端侧面并整合进入HA的HA1亚基。使用重组牛痘病毒表达后,首先分析了称为LEF / HA(插入90个氨基酸)和RBD / HA(插入140个氨基酸)的嵌合蛋白。两种嵌合蛋白均显示出与野生型HA相似的功能表型。它们转运到细胞表面,可以被胰蛋白酶裂解为HA1和HA2亚基以激活膜融合潜能,能够经历融合所需要的低pH诱导的构象变化,并能够诱导融合过程。我们还能够产生包含嵌合RBD / HA和LEF / HA基因的重组流感病毒,并且在MDCK细胞或胚胎鸡卵中传代数次后,插入的PA结构域仍保持在HA基因片段中。此外,用表达嵌合的RBD / HA和LEF / HA蛋白的质粒以及含有它们的重组病毒对小鼠进行DNA免疫,可诱导针对该蛋白的HA和PA成分的抗体反应。这些方法可能为抗炭疽和其他疾病的疫苗提供有用的工具。

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