中国高致病性猪繁殖与呼吸病毒复制酶蛋白nsp2通过促进病毒清除参与保护性免疫

Can Kong, Dan Li, Yanxin Hu, Peng Gao, Yongning Zhang, Lei Zhou, Xinna Ge, Xin Guo, Jun Han, Hanchun Yang
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摘要

复制酶蛋白nsp2基因组片段是猪繁殖与呼吸综合征病毒(PRRSV)进化最快的区域,我们的前期研究表明,PRRSV nsp2基因变异导致交叉中和不良。通过体外抗体吸收实验,我们发现nsp2的木瓜蛋白酶2 (PLP2)结构域是中和抗体的靶点。用中国高致病性PRRSV (HP-PRRSV)毒株JXwn06和低毒力nadc30样毒株CHsx1401(毒株1)的一系列系间嵌合突变体进行交叉中和实验,进一步验证了这一点。随后,用携带JXwn06结构蛋白区(SP)的CHsx1401或其衍生物单独(CHsx1401-SP JX)或与PLP2区联合免疫的方法,在一个月大的SPF仔猪模型中检测了nsp2在保护性免疫中的作用(CHsx1401-SPplp2 JX)或整个nsp2区域(CHsx1401-SPnsp2 JX),然后在免疫后42天(病毒血症检测不到的时间点)用JXwn06攻毒。所有嵌合体组均能免受JXwn06的攻击,而CHsx1401组未能提供有益的保护。有趣的是,CHsx1401-SPnsp2 JX组,而不是CHsx1401-SPplp2 JX组,肺显微病变和病毒组织载量最低。值得注意的是,疫苗病毒CHsx1401-SPnsp2 JX在检查的组织中检测不到,除了一只仔猪外,攻毒病毒也检测不到,这突出了HP-PRRSV nsp2在促进病毒清除方面的重要作用。这些发现提供了对PRRSV保护性免疫机制的深入了解,并对PRRSV疫苗的开发具有重要意义。
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The replicase protein nsp2 of Chinese highly pathogenic porcine reproductive and respiratory virus is involved in protective immunity by promoting viral clearance
Abstract The genome segment for replicase protein nsp2 represents the fastest evolving region of porcine reproductive and respiratory syndrome virus (PRRSV), and our previous studies have shown that the PRRSV nsp2 genetic variation contributes to poor cross-neutralization. By using in vitro antibody absorption assay, here we show that the papain-like protease 2 (PLP2) domain of nsp2 is a target of neutralizing antibodies. This was further verified by cross-neutralization assay with a series of inter-lineage chimeric mutants between the Chinese highly pathogenic PRRSV (HP-PRRSV) strain JXwn06 and the low virulent NADC30-like strain CHsx1401 (lineage 1). The role of nsp2 in protective immunity was subsequently tested in a one-month SPF piglet model by immunizing the piglets with CHsx1401 or its derivatives carrying JXwn06 structural protein region (SP) alone (CHsx1401-SP JX ) or in combination with PLP2 region (CHsx1401-SPplp2 JX ), or the whole nsp2 region (CHsx1401-SPnsp2 JX ), followed by challenge with JXwn06 at 42 days post immunization, a time point when the viremia was undetectable. All chimera groups were protected from the challenge by JXwn06, whereas the group CHsx1401 failed to provide beneficial protection. Interestingly, the group CHsx1401-SPnsp2 JX , but not CHsx1401-SPplp2 JX , showed the lowest lung microscopic lesions and viral tissue load. Significantly, the vaccine virus CHsx1401-SPnsp2 JX was undetectable in the examined tissues, and so was for the challenge virus except for one piglet, highlighting an important role of HP-PRRSV nsp2 in promoting viral clearance. The findings provide insight into the mechanisms underlying the protective immunity against PRRSV and have important implications in PRRSV vaccine development.
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