Literature DB >> 11145456

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

T Iwamoto1, T Nakai, K Mori, M Arimoto, I Furusawa.   

Abstract

Six cell clones were derived from the SSN-1 cell line, which is composed of a mixed cell population and persistently infected with a C-type retrovirus (SnRV). These clones were susceptible to 4 piscine nodavirus strains belonging to different genotypes (SJNNV, RGNNV, TPNNV and *BFNNV [striped jack, redspotted grouper, tiger puffer and barfin flounder nervous necrosis viruses]). Three clones, designated A-6, E-9, and E-11, were highly permissive to nodavirus infection and production. The virus-induced cytopathic effects appeared as cytoplasmic vacuoles and intensive disintegration at 3 to 5 d post-incubation. These observations were highly reproducible and formed the basis for a successful virus titration system. Quantitative analysis using the cloned E-11 cell line clearly revealed differences in the optimal growth temperatures among the 4 genotypic variants: 25 to 30 degrees C for strain SGWak97 (RGNNV), 20 to 25 degrees C for strain SJNag93 (SJNNV), 20 degrees C for strain TPKag93 (TPNNV), and 15 to 20 degrees C for strain JFIwa98 (BFNNV). Electron microscopy demonstrated SnRV retrovirus particles only in A-6 and E-9 cells, but PCR amplification for the pol gene and LTR region of the proviral DNA indicated the presence of the retrovirus in the other clones, including E-11. The cell clones obtained in the present study will be more useful for qualitative and quantitative analyses of piscine nodaviruses than the SSN-1 cell line.

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Year:  2000        PMID: 11145456     DOI: 10.3354/dao043081

Source DB:  PubMed          Journal:  Dis Aquat Organ        ISSN: 0177-5103            Impact factor:   1.802


  40 in total

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7.  Cell Culture Isolation of Piscine Nodavirus (Betanodavirus) in Fish-Rearing Seawater.

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Authors:  Dennis K Gomez; Gun Wook Baeck; Ji Hyung Kim; Casiano H Choresca; Se Chang Park
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9.  Identification of host-specificity determinants in betanodaviruses by using reassortants between striped jack nervous necrosis virus and sevenband grouper nervous necrosis virus.

Authors:  Tokinori Iwamoto; Yasushi Okinaka; Kazuyuki Mise; Koh-Ichiro Mori; Misao Arimoto; Tetsuro Okuno; Toshihiro Nakai
Journal:  J Virol       Date:  2004-02       Impact factor: 5.103

10.  Development of a Novel Allele-Specific PCR Method for Rapid Assessment of Nervous Necrosis Virus Genotypes.

Authors:  Dimitra K Toubanaki; Maritsa Margaroni; Evdokia Karagouni
Journal:  Curr Microbiol       Date:  2015-07-26       Impact factor: 2.188

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