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鱼类细胞系SSN-1对鱼类诺达病毒的高敏感性。

High permissivity of the fish cell line SSN-1 for piscine nodaviruses.

作者信息

Iwamoto T, Mori K, Arimoto M, Nakai T

机构信息

Fish Pathology Laboratory, Faculty of Applied Biological Science, Hiroshima University, Higashihiroshima, Japan.

出版信息

Dis Aquat Organ. 1999 Dec 22;39(1):37-47. doi: 10.3354/dao039037.

Abstract

Seventeen isolates of piscine nodavirus from larvae or juveniles of 13 marine fish species affected with viral nervous necrosis (VNN) were examined for their infectivity to a fish cell line SSN-1. Based on cytopathic effects (CPE) and virus antigen detection by fluorescent antibody technique (FAT) after incubation at 25 degrees C, the infectivity of these virus isolates was divided into 4 groups. Group 1, including 9 virus isolates from 4 species of grouper, 2 species of sea bass, barramundi, rock porgy, and Japanese flounder showed CPE characterized by rounded, granular cells with heavy cytoplasmic vacuoles within 3 d post-incubation (p.i.), and the monolayer partially or completely disintegrated over 3 to 6 d p.i. Scattered FAT-positive cells appeared at 3 h p.i. and spread through the cell sheet with an increasing fluorescence signal over 24 h p.i. Group 2, consisting of 3 virus isolates from striped jack, induced CPE with thin or rounded, granular, refractile cells without conspicuous vacuole formation, and extensive FAT-positive reaction was observed in a time course similar to that of Group 1. Cells inoculated with Group 3 (1 isolate from tiger puffer) developed no distinct CPE but viral infection was evidenced by localized FAT-positive cells. There were no FAT-positive cells in Group 4, which included 4 isolates from Japanese flounder, Pacific cod and Atlantic halibut. However, when incubation was performed at 20 degrees C, the SSN-1 cells inoculated with the Group 3 isolate showed CPE similar to that of Group 1 and extensive FAT-positive reaction. Evidence of virus proliferation at 20 degrees C was also obtained in Group 4 isolates. The virus titers in the infected fish varied from 10(11) to 10(16) tissue culture infectious dose (TCID50) g(-1) of fish. There is a good correlation between these infectivities to the SSN-1 cells and the coat protein gene genotypes of the isolates. The present results indicate that SSN-1 cells are useful for propagating and differentiating genotypic variants of piscine nodavirus.

摘要

对从13种患有病毒性神经坏死病(VNN)的海水鱼类幼体或幼鱼中分离出的17株鱼类诺达病毒,检测其对鱼类细胞系SSN-1的感染性。根据在25℃孵育后的细胞病变效应(CPE)以及通过荧光抗体技术(FAT)进行的病毒抗原检测,将这些病毒分离株的感染性分为4组。第1组包括来自4种石斑鱼、2种海鲈、尖吻鲈、条石鲷和牙鲆的9株病毒分离株,在孵育后3天内(p.i.)表现出CPE,特征为细胞变圆、颗粒状,胞质内有大量空泡,在孵育后3至6天内单层细胞部分或完全解体。在孵育后3小时出现散在的FAT阳性细胞,并在孵育后24小时内荧光信号增强,遍布整个细胞片层。第2组由来自条蛳的3株病毒分离株组成,诱导出CPE,细胞呈细长或圆形、颗粒状、折光性,无明显空泡形成,并且在与第1组相似的时间进程中观察到广泛的FAT阳性反应。接种第3组(来自虎河豚的1株分离株)的细胞未出现明显的CPE,但局部FAT阳性细胞证明了病毒感染。第4组包括来自牙鲆、太平洋鳕和大西洋庸鲽的4株分离株,未出现FAT阳性细胞。然而,当在20℃进行孵育时,接种第3组分离株的SSN-1细胞表现出与第1组相似的CPE以及广泛的FAT阳性反应。在第4组分离株中也获得了病毒在20℃增殖的证据。感染鱼体内的病毒滴度在10(11)至10(16)组织培养感染剂量(TCID50)/克鱼之间。这些对SSN-1细胞的感染性与分离株的衣壳蛋白基因基因型之间存在良好的相关性。目前的结果表明,SSN-1细胞可用于繁殖和区分鱼类诺达病毒的基因型变体。

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