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利用电泳迁移技术,结合紫外和荧光检测,快速分离和鉴定猪和马流感 A 病毒的亚型。

Rapid separation and identification of the subtypes of swine and equine influenza A viruses by electromigration techniques with UV and fluorometric detection.

机构信息

Institute of Analytical Chemistry of the ASCR, v. v. i., Veveří 97, 602 00 Brno, Czech Republic.

出版信息

Analyst. 2011 Jul 21;136(14):3010-5. doi: 10.1039/c0an00896f. Epub 2011 Jun 8.

DOI:10.1039/c0an00896f
PMID:21655602
Abstract

Influenza A is viral disease, which is a cause of yearly epidemics and, potentially, pandemics. The conventional techniques used today are equipment-demanding, time-consuming and laborious. Recently, we have confirmed that the capillary isoelectric focusing is a suitable fast alternative for the verifying of virus purity. In the wide pH gradient of pH range 2.0-7.5 the isoelectric points for subtypes of equine (H3N8) and swine (H1N2) influenza A viruses were determined approximately as 6.6 and 6.5, respectively. In this contribution we have verified these findings using different isolates of different viral subtypes of swine influenza, H1N1, H1N2, and of equine influenza, H3N8, H7N7, which were separated by capillary zone electrophoresis (CZE) and capillary isoelectric focusing (CIEF) in the narrow pH gradient pH range from 6.0 to 7.0. It was found that the isoelectric points of different isolates and subtypes of equine and swine influenza are almost independent of their origin. The electromigration velocities of subtypes of equine or swine influenza viruses were dependent on the antigenic subtypes of their surface glycoproteins. The detection sensitivity of the influenza viruses labeled by the fluorescent non-ionogenic tenside based on poly(ethylene glycol)pyrenebutanoate for fluorometric detection was increased and down to ten labeled viruses were detected. The isoelectric points of the native and labeled equine and swine influenza A viruses and their subtypes do not differ. According to our experiments these methods appear to be useful for the fast preliminary differentiation of influenza viruses in future.

摘要

甲型流感是一种病毒性疾病,是每年流行疫情的原因,并可能导致大流行。目前使用的常规技术设备要求高、耗时且费力。最近,我们已经证实,毛细管等电聚焦是验证病毒纯度的合适快速替代方法。在 pH 值范围 2.0-7.5 的宽 pH 梯度下,马(H3N8)和猪(H1N2)流感 A 病毒的亚型等电点分别约为 6.6 和 6.5。在本研究中,我们使用不同的病毒亚型的不同分离株(猪流感 H1N1、H1N2 和马流感 H3N8、H7N7)验证了这些发现,这些分离株通过毛细管区带电泳(CZE)和毛细管等电聚焦(CIEF)在 pH 值范围为 6.0 至 7.0 的窄 pH 梯度下进行分离。结果发现,不同的马和猪流感分离株和亚型的等电点几乎与其起源无关。马和猪流感病毒的亚型的电泳迁移速度取决于其表面糖蛋白的抗原亚型。用基于聚乙二醇基 pyrenebutanoate 的荧光非离子表面活性剂标记流感病毒的荧光检测灵敏度提高,可检测到低至 10 个标记的病毒。天然和标记的马和猪流感 A 病毒及其亚型的等电点没有差异。根据我们的实验,这些方法似乎可用于将来快速初步区分流感病毒。

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