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Differential replication properties among H9N2 avian influenza viruses of Eurasian origin

机译:欧亚起源的H9N2禽流感病毒之间的差异复制特性

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Avian influenza H9N2 viruses have become panzootic in Eurasia causing respiratory manifestations, great economic losses and occasionally being transmitted to humans. To evaluate the replication properties and compare the different virus quantification methods, four Eurasian H9N2 viruses from different geographical origins were propagated in embryonated chicken egg (ECE) and Madin-Darby canine kidney epithelial cell systems. The ECE-grown and cell culture-grown viruses were monitored for replication kinetics based on tissue culture infectious dose (TCID 50 ), Hemagglutination (HA) test and quantitative real time RT-PCR (qRT-PCR). The cellular morphology was analyzed using immunofluorescence (IF) and cellular ELISA was used to screen the sensitivity of the viruses to amantadine. The Eurasian wild type-H9N2 virus produced lower titers compared to the three G1-H9N2 viruses at respective time points. Detectable titers were observed earliest at 16?h post inoculation (hpi), significant morphological changes on cells were first observed at 32 hpi. Few nucleotide and amino acid substitutions were noticed in the HA, NA and NS gene sequences but none of them are related to the known conserved region that can alter pathogenesis or virulence following a single passage in cell culture. All studied H9N2 viruses were sensitive to amantadine. The G1-H9N2 viruses have higher replication capabilities compared to the European wild bird-H9N2 probably due to their specific genetic constitutions which is prerequisite for a successful vaccine candidate. Both the ECE and MDCK cell system allowed efficient replication but the ECE system is considered as the better cultivation system for H9N2 viruses in order to get maximum amounts of virus within a short time period.
机译:禽流感H9N2病毒已在欧亚大陆流行,引起呼吸道疾病,巨大的经济损失,并偶尔传播给人类。为了评估复制特性并比较不同的病毒定量方法,将四种来自不同地理区域的欧亚H9N2病毒在胚胎鸡蛋(ECE)和Madin-Darby犬肾上皮细胞系统中繁殖。根据组织培养物的感染剂量(TCID 50 ),血细胞凝集(HA)试验和实时定量RT-PCR(qRT-PCR),监测ECE生长和细胞培养生长的病毒的复制动力学。 。使用免疫荧光(IF)分析细胞形态,并使用细胞ELISA筛选病毒对金刚烷胺的敏感性。与三种G1-H9N2病毒在各个时间点相比,欧亚野生型H9N2病毒产生的滴度更低。最早在接种后16小时(hpi)观察到可检测的滴度,首先在32 hpi观察到细胞的明显形态学变化。 HA,NA和NS基因序列中几乎没有核苷酸和氨基酸取代,但是它们都与已知的保守区无关,该保守区在细胞培养中单次传代后可以改变发病机理或毒力。所有研究的H9N2病毒均对金刚烷胺敏感。与欧洲野生鸟类H9N2相比,G1-H9N2病毒具有更高的复制能力,这可能是由于其特定的遗传构成,这是成功候选疫苗的前提。 ECE和MDCK细胞系统都允许有效复制,但是ECE系统被认为是H9N2病毒的更好的培养系统,以便在短时间内获得最大数量的病毒。

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