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Screening of HIV-1 Env glycoproteins for the ability to raise neutralizing antibody using DNA immunization and recombinant vaccinia virus boosting

机译:使用DNa免疫和重组痘苗病毒加强筛选HIV-1 Env糖蛋白提高中和抗体的能力

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摘要

HIV-1 envelopes from two series of primary isolates (from Swedish patients 5 and 6), from JR-FL and BaL (prototypic monocyte/macrophage tropic viruses) and from HXB-2 (a prototypic T-cell-line-adapted virus), have been screened for their ability to elicit neutralizing antibody to HIV-1. Rabbits were primed by gene gun inoculation with plasmids expressing secreted monomeric (gp120) and oligomeric (gp140) forms of each Env. After four to six DNA immunizations administered over a 1-year period, rabbits were boosted with 10(8) plaque-forming units of a mixture of seven recombinant vaccinia viruses which express chimeric gp140 Envs (primary clade B sequences in a IIIb-related BH10 backbone). Neutralizing antibodies were assayed against two T-cell-line-adapted viruses (MN and IIIb), two non-syncytium-inducing (NSI) and two syncytium-inducing (SI) primary isolates, and two HIV-1-NL4-3-recombinants with patients 5 or 6 Envs (NL4-3/5A, NL4-3/6C). The DNA priming and recombinant vaccinia virus boosting raised low titers of neutralizing antibody in 10 of 19 rabbits. The highest titers of neutralizing activity (approximately 1:150 for MN) were raised in rabbits DNA primed with Envs from Swedish patients 5. These sera cross neutralized IIIb and MN but did not neutralize the primary isolates or the NL4-3 recombinant with the homologous 5A Env. Sera from rabbits primed with the HXB-2 Env DNA were, for the most part, type-specific for neutralization of IIIb. In one of three assays, sera from rabbits primed with plasmids expressing the JR-FL and BaL had possible low titer neutralizing activity for two NSI, but not two SI, primary isolates. Our results highlight the low immunogenic potential of the HIV-1 Env and demonstrate that different Envs have different potentials to raise low titer neutralizing antibody.
机译:来自两个系列主要分离株(来自瑞典患者5和6),JR-FL和BaL(原型单核细胞/巨噬细胞嗜性病毒)和HXB-2(原型T细胞系适应性病毒)的HIV-1包膜已经筛选了它们引起HIV-1中和抗体的能力。用表达每种Env的分泌的单体(gp120)和寡聚体(gp140)形式的质粒通过基因枪接种来引发兔。在1年内进行了4到6次DNA免疫接种后,用表达嵌合gp140 Envs(IIIb相关BH10中的主要进化枝B序列的七种重组痘苗病毒)的混合物的10(8)噬菌斑形成单位加强了兔子的免疫骨干)。测定了针对两种适应T细胞系的病毒(MN和IIIb),两种非合胞体诱导(NSI)和两种合胞体诱导(SI)主要分离株以及两种HIV-1-NL4-3-的中和抗体具有5个或6个Envs患者的重组体(NL4-3 / 5A,NL4-3 / 6C)。 DNA引发和重组牛痘病毒的加强在19只兔子中的10只中产生了较低的中和抗体效价。用瑞典患者5的Envs引发的兔DNA产生了最高的中和活性滴度(对于MN约为1:150)。这些血清交叉中和了IIIb和MN,但没有用同源物中和主要分离株或NL4-3重组体。 5A环境用HXB-2 Env DNA引发的兔血清在很大程度上对IIIb的中和具有类型特异性。在三种测定之一中,用表达JR-FL和BaL的质粒引发的兔血清对两种NSI(而非两种SI)主要分离物可能具有较低的滴度中和活性。我们的结果突出了HIV-1 Env的低免疫原性潜力,并证明了不同的Envs具有提高低滴度中和抗体的潜力。

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