Trypsin Action on the Growth of Sendai Virus in Tissue Culture Cells III. Structural Difference of Sendai Viruses Grown in Eggs and Tissue Culture Cells

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J Virol. 1973 December; 12(6): 1457-1465
Copyright © 1973 American Society for Microbiology. All Rights Reserved.

Trypsin Action on the Growth of Sendai Virus in Tissue Culture Cells III. Structural Difference of Sendai Viruses Grown in Eggs and Tissue Culture Cells

Morio Homma¹ and Masanobu Ohuchi²

Department of Bacteriology, Yamagata University School of Medicine, Yamagata, Japan
Department of Bacteriology, Tohoku University School of Medicine, Sendai, Japan

ABSTRACT

Polypeptides of egg-borne Sendai virus (egg Sendai), which isbiologically active on the basis of criteria of the infectivityfor L cells and of hemolytic and cell fusion activities, werecompared by polyacrylamide gel electrophoresis with those ofL cell-borne (L Sendai) and HeLa cell-borne Sendai (HeLa Sendai)viruses, which are judged biologically inactive by the abovecriteria. Densitometer profiles on the stained gels of egg Sendairesolved six polypeptides (virion protein [VP] 1 to VP6), inwhich VP2 and VP4 were identified as glycoproteins by PAS stain.Comparative electropherograms of both L Sendai and HeLa Sendairevealed that there were significantly larger amounts in theVP2 region of these viruses but VP4 was present only in greatlyreduced amounts as compared to egg Sendai. It was also foundthat VP2 of L Sendai and HeLa Sendai consisted of two components,VP2a and VP2b, but the one of egg Sendai consisted of only VP2a.A mild trypsin treatment which converts both L Sendai and HeLaSendai to a biologically active form selectively removed VP2bfrom these viruses and increased concomitantly the amounts ofmaterials in the VP4 region. The same treatment of egg Sendaiaffected neither its biological activities nor its electropherogram.Consequently, gross polypeptide profiles on the stained gelsof L Sendai and HeLa Sendai after trypsin treatment became favorablycomparable to that of egg Sendai. Electrophoresis of labeledL Sendai and HeLa Sendai with a ³H-amino acids mixture and ¹⁴C-glucosamineresolved at least three glycoproteins, GP1, GP2, and GP3, eachcorresponding to VP2a, VP2b, and VP4, respectively. The trypsintreatment of these viruses removed almost all the radioactivityof GP2 and simultaneously increased the radioactive counts ofGP3 and raised small amounts of rapidly moving heterogeneousglycoprotein, GP4. A possible relationship between the biologicalmodification and the above characteristic polypeptide patternsof Sendai virus was discussed.

J Virol. 1973 December; 12(6): 1457-1465
Copyright © 1973 American Society for Microbiology. All Rights Reserved.

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