Conformation- and Fusion-Defective Mutations in the Hypothetical Phospholipid-Binding and Fusion Peptides of Viral Hemorrhagic Septicemia Salmonid Rhabdovirus Protein G

doi:10.1128/JVI.78.17.9115-9122.2004

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Journal of Virology, September 2004, p. 9115-9122, Vol. 78, No. 17
0022-538X/04/$08.00+0 DOI: 10.1128/JVI.78.17.9115-9122.2004
Copyright © 2004, American Society for Microbiology. All Rights Reserved.

Conformation- and Fusion-Defective Mutations in the Hypothetical Phospholipid-Binding and Fusion Peptides of Viral Hemorrhagic Septicemia Salmonid Rhabdovirus Protein G

A. Rocha,¹ S. Ruiz,¹ C. Tafalla,² and J. M. Coll¹^*

Departamento di Biotecnología, SGIT,¹ CISA Valdeolmos, INIA, Madrid, Spain²

Received 23 October 2003/ Accepted 20 May 2004

Fourteen single and two double point mutants in the highly conservedregion (positions 56 to 159) of the G gene of viral hemorrhagicsepticaemia virus (VHSV), a salmonid rhabdovirus, were selectedand obtained in plasmids by site-directed mutagenesis. Fishcell monolayers transfected with the mutant plasmids were thenassayed for protein G (pG) expression, conformation-dependentmonoclonal antibody (MAb) reactivity, and cell-cell fusion.Some mutations located in the phospholipid-binding p2 peptide(positions 82 to 110; mutants P86A, A96E, G98A, and R107A) abolishedboth MAb recognition and fusion activity, while others (P79A,L85S, and R103A) abolished MAb recognition but retained fusionat similar or lower pHs compared to those for the wild type.Phospholipid-binding assays of p2-derived synthetic peptidessuggested that phosphatidylserine binding was not affected bythe mutations studied. On the other hand, three (P79A, L85S,and T135E) of the four mutants retaining fusion activity mappedaround two locations showing amino acid variation in 22 VHSVisolates and in neutralizing MAb-resistant mutants describedpreviously. Mutations located in the hypothetical fusion peptide(positions 142 to 159; mutants F147K, P148K, and W154K) abolishedboth MAb recognition and fusion activity. The existence of mutantswith altered conformation and defective fusion in both p2 andfusion peptides provides further evidence in favor of the participationof these and adjacent regions in some of the steps of the VHSVfusion processes, as suggested by previous studies. In addition,because the studied region induced strong immunological responsesin trout, some of the mutants described here might be used todesign attenuated VHSV vaccines.

* Corresponding author. Mailing address: INIA, Biotechnology, Crt Coruna Km7, Madrid, 28130, Spain. Phone: 34-1-3476850. Fax: 34-1-3572293. E-mail: juliocoll{at}inia.es.