par Jacquet, Alain 
;Haumont, M;Massaer, Marc ;Garcia, L;Mazzu, P;Daminet, V;Grégoire, Diane ;Jacobs, Paul ;Bollen, Alex
Référence Vaccine, 20, 11-12, page (1593-1602)
Publication Publié, 2002-02
;Haumont, M;Massaer, Marc ;Garcia, L;Mazzu, P;Daminet, V;Grégoire, Diane ;Jacobs, Paul ;Bollen, Alex Référence Vaccine, 20, 11-12, page (1593-1602)
Publication Publié, 2002-02
Article révisé par les pairs
| Résumé : | The varicella-zoster virus (VZV) envelope glycoprotein E (gE) and immediate early protein 63 (IE63) are well known targets for specific humoral and cell-mediated immune responses during VZV infection and latency, respectively. The present study evaluated the immunogenicity of an engineered chimeric recombinant gE-IE63 (recgE-IE63) protein secreted from CHO cells, wherein a soluble form of gE, deleted of its anchor and cytoplasmic domains was fused to IE63. Guinea pig vaccinations with adjuvanted recgE-IE63 elicited a strong and specific humoral immune response directed to each counterpart. Sera from recgE-IE63-immunized animals neutralized cell-free VZV. This neutralizing capacity was dependent only on the recgE moiety as serum depletions on recgE-immobilized sepharose totally abolished VZV neutralization. The cell-mediated immune response induced by recgE-IE63 was evaluated in lymphoproliferation assays. An antigen-specific proliferative response was demonstrated after lymphocyte stimulation with recIE63 but not with recgE. We conclude that recombinant chimeric recgE-IE63 induced both humoral and cell-mediated immune responses and thus could constitute a putative subunit vaccine candidate against VZV primary infection and zoster reactivation. |
