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经典猪瘟亚临床感染野猪中的非洲猪瘟病毒感染

African swine fever virus infection in Classical swine fever subclinically infected wild boars.

作者信息

Cabezón Oscar, Muñoz-González Sara, Colom-Cadena Andreu, Pérez-Simó Marta, Rosell Rosa, Lavín Santiago, Marco Ignasi, Fraile Lorenzo, de la Riva Paloma Martínez, Rodríguez Fernando, Domínguez Javier, Ganges Llilianne

机构信息

IRTA, Centre de Recerca en Sanitat Animal (CReSA, IRTA-UAB), Campus de la Universitat Autònoma de Barcelona, 08193, Bellaterra, Spain.

Servei d'Ecopatologia de Fauna Salvatge, Departament de Medicina i Cirurgia Animals, Universitat Autònoma de Barcelona, 08193, Bellaterra, Spain.

出版信息

BMC Vet Res. 2017 Aug 1;13(1):227. doi: 10.1186/s12917-017-1150-0.

Abstract

BACKGROUND

Recently moderate-virulence classical swine fever virus (CSFV) strains have been proven capable of generating postnatal persistent infection (PI), defined by the maintenance of viremia and the inability to generate CSFV-specific immune responses in animals. These animals also showed a type I interferon blockade in the absence of clinical signs. In this study, we assessed the infection generated in 7-week-old CSFV PI wild boars after infection with the African swine fever virus (ASFV). The wild boars were divided in two groups and were infected with ASFV. Group A comprised boars who were CSFV PI in a subclinical form and Group B comprised pestivirus-free wild boars. Some relevant parameters related to CSFV replication and the immune response of CSFV PI animals were studied. Additionally, serum soluble factors such as IFN-α, TNF-α, IL-6, IL-10, IFN-γ and sCD163 were analysed before and after ASFV infection to assess their role in disease progression.

RESULTS

After ASFV infection, only the CSFV PI wild boars showed progressive acute haemorrhagic disease; however, the survival rates following ASFV infection was similar in both experimental groups. Notwithstanding, the CSFV RNA load of CSFV PI animals remained unaltered over the study; likewise, the ASFV DNA load detected after infection was similar between groups. Interestingly, systemic type I FN-α and IL-10 levels in sera were almost undetectable in CSFV PI animals, yet detectable in Group B, while detectable levels of IFN-γ were found in both groups. Finally, the flow cytometry analysis showed an increase in myelomonocytic cells (CD172a) and a decrease in CD4 T cells in the PBMCs from CSFV PI animals after ASFV infection.

CONCLUSIONS

Our results showed that the immune response plays a role in the progression of disease in CSFV subclinically infected wild boars after ASFV infection, and the immune response comprised the systemic type I interferon blockade. ASFV does not produce any interference with CSFV replication, or vice versa. ASFV infection could be a trigger factor for the disease progression in CSFV PI animals, as their survival after ASFV was similar to that of the pestivirus-free ASFV-infected group. This fact suggests a high resistance in CSFV PI animals even against a virus like ASFV; this may mean that there are relevant implications for CSF control in endemic countries. The diagnosis of ASFV and CSFV co-infection in endemic countries cannot be ruled out and need to be studied in greater depth.

摘要

背景

最近已证实,中等毒力的经典猪瘟病毒(CSFV)毒株能够引发出生后持续性感染(PI),其定义为动物体内病毒血症持续存在且无法产生CSFV特异性免疫反应。这些动物在没有临床症状的情况下还表现出I型干扰素阻断。在本研究中,我们评估了7周龄的CSFV PI野猪感染非洲猪瘟病毒(ASFV)后产生的感染情况。将野猪分为两组并感染ASFV。A组包括亚临床形式的CSFV PI野猪,B组包括无瘟病毒的野猪。研究了一些与CSFV复制和CSFV PI动物免疫反应相关的参数。此外,在ASFV感染前后分析了血清可溶性因子,如IFN-α、TNF-α、IL-6、IL-10、IFN-γ和sCD163,以评估它们在疾病进展中的作用。

结果

ASFV感染后,只有CSFV PI野猪出现进行性急性出血性疾病;然而,两个实验组ASFV感染后的存活率相似。尽管如此,在整个研究过程中,CSFV PI动物的CSFV RNA载量保持不变;同样,感染后检测到的ASFV DNA载量在两组之间相似。有趣的是,CSFV PI动物血清中的全身性I型FN-α和IL-10水平几乎检测不到,但在B组中可检测到,而两组中均发现了可检测水平的IFN-γ。最后,流式细胞术分析显示,ASFV感染后,CSFV PI动物外周血单核细胞中的骨髓单核细胞(CD172a)增加,CD4 T细胞减少。

结论

我们的结果表明,免疫反应在ASFV感染后CSFV亚临床感染野猪的疾病进展中起作用,且免疫反应包括全身性I型干扰素阻断。ASFV不会对CSFV复制产生任何干扰,反之亦然。ASFV感染可能是CSFV PI动物疾病进展的触发因素,因为它们感染ASFV后的存活率与无瘟病毒的ASFV感染组相似。这一事实表明CSFV PI动物即使对ASFV这样的病毒也具有高度抵抗力;这可能意味着对流行国家的猪瘟控制具有相关意义。在流行国家不能排除ASFV和CSFV合并感染的诊断,需要更深入地研究。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9320/5540480/a298ff6fb989/12917_2017_1150_Fig1_HTML.jpg

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