Herrera Jenifer, Gómez-Núñez Luis, Lara-Romero Rocío, Diosdado Fernando, Martínez-Lara Atalo, Jasso Miguel, Ramírez-Mendoza Humberto, Pérez-Torres Armando, Rivera-Benítez José Francisco
Centro Nacional de Investigación Disciplinaria en Microbiología Animal, Instituto Nacional de Investigaciones Forestales, Agrícolas y Pecuarias, Mexico City, Mexico.
Departamento de Microbiología e Inmunología, Facultad de Medicina Veterinaria y Zootecnia, UNAM, Mexico City, Mexico.
Virus Res. 2017 Feb 15;230:50-58. doi: 10.1016/j.virusres.2017.01.010. Epub 2017 Jan 16.
The objective of this study was to evaluate the clinical disease, humoral response and viral distribution of recent Porcine rubulavirus (PorPV) isolates in experimentally infected pigs. Four, 6-piglet (5-days old) groups were employed (G1-84, G2-93, G3-147, and G4-T). Three viral strains were used for the experimental infection: the reference strain LPMV-1984 (Michoacán 1984) and two other strains isolated in 2013, one in Queretaro (Qro/93/2013) and the other in Michoacán (Mich/147/2013). Each strain was genetically characterized by amplification and sequencing of the gene encoding hemagglutinin-neuroamidase (HN). The inoculation was performed through the oronasal and ocular routes, at a dose of 1×10TCID/ml. Subsequently, the signs were evaluated daily and necropsies were performed on 3 different days post infection (dpi). We recorded all micro- and macroscopic lesions. Organs from the nervous, lymphatic, and respiratory system were analyzed by quantifying the viral RNA load and the presence of the infectious virus. The presence of the viral antigen in organs was evidenced through immunohistochemistry. Seroconversion was evaluated through the use of a hemagglutination inhibition test. In the characterization of gene HN, only three substitutions were identified in strain Mich/147/2013, two in strain LPMV/1984 (fourth passage) and one in strain Qro/93/2013, with respect to reference strain LPMV-84, these changes had not been identified as virulence factors in previously reported strains. Neurological alterations associated with the infection were found in all three experimental groups starting from 3dpi. Groups G1-84 and G3-147 presented the most exacerbated nervous signs. Group G2-93 only presented milder signs including slight motor incoordination, and an increased rectal temperature starting from day 5 post infection (PI). The main histopathological findings were the presence of a mononuclear inflammatory infiltrate (lymphocytic/monocytic) surrounding the ventricles in the brain and focal interstitial pneumonitis with distention of the alveolar sacs in the lungs. PorPV and RNA distribution were identified in the organs of the nervous, lymphatic, and respiratory systems of the piglets analyzed at different times (days 5, 10, and 15 PI). The viral antigen was detected in the brain and lungs in most of the assessed groups. Seroconversion was evident in groups G1-84 and G2-93. Groups G1-84 and G3-147 were the most clinically affected by the experimental infection. Both strains were isolated in the state of Michoacán. The virulence of the new isolates maintains similar characteristics to those reported more than 30 years ago.
本研究的目的是评估近期猪腮腺炎病毒(PorPV)分离株在实验感染猪中的临床疾病、体液反应和病毒分布情况。采用了4个6头仔猪(5日龄)的组(G1 - 84、G2 - 93、G3 - 147和G4 - T)。使用三种病毒株进行实验感染:参考株LPMV - 1984(米却肯1984)和2013年分离的另外两种毒株,一种在克雷塔罗(Qro/93/2013),另一种在米却肯(Mich/147/2013)。通过对编码血凝素 - 神经氨酸酶(HN)的基因进行扩增和测序,对每个毒株进行基因特征分析。通过口鼻和眼途径接种,剂量为1×10TCID/ml。随后,每天评估症状,并在感染后3个不同时间点(dpi)进行剖检。记录所有微观和宏观病变。通过定量病毒RNA载量和传染性病毒的存在,对神经、淋巴和呼吸系统的器官进行分析。通过免疫组织化学证明器官中病毒抗原的存在。通过血凝抑制试验评估血清转化。在基因HN的特征分析中,相对于参考株LPMV - 84而言,在菌株Mich/147/2013中仅鉴定出3个替换,在菌株LPMV/1984(第4代)中鉴定出2个,在菌株Qro/93/2013中鉴定出1个,这些变化在先前报道的菌株中未被鉴定为毒力因子。从3dpi开始,在所有三个实验组中均发现与感染相关的神经学改变。G1 - 84组和G3 - 147组表现出最严重的神经症状。G2 - 93组仅表现出较轻的症状,包括轻微运动不协调,并且从感染后第5天(PI)开始直肠温度升高。主要组织病理学发现是脑室内有单核炎性浸润(淋巴细胞/单核细胞)以及肺部有局灶性间质性肺炎伴肺泡囊扩张。在不同时间(感染后第5、10和15天)分析的仔猪的神经、淋巴和呼吸系统器官中鉴定出PorPV和RNA分布。在大多数评估组的脑和肺中检测到病毒抗原。G1 - 84组和G2 - 93组出现血清转化。G1 - 84组和G3 - 147组在实验感染中受临床影响最大。两种毒株均在米却肯州分离得到。新分离株的毒力保持与30多年前报道的相似特征。
