In this study, we investigated the antigenic structures and maturation of some C‐terminal‐deficient derivatives of rabies virus glycoprotein (G). The Gs protein, a soluble form of G protein shed from infected cells, displayed antigenicity to most of our conformational epitope‐specific anti‐G mAbs, but took the 1‐30‐44 epitope‐deficient conformation (termed GC form). (The 1‐30‐44 epitope was acid‐sensitive and dependent on two separate regions, the Lys‐202‐containing and Asn‐336‐containing regions; Kankanamge et al., Microbiol. Immunol., 47: 507–519). Intact G proteins took the 1‐30‐44 epitope‐positive form (referred to as GB form) on the cell surface, but not inside the cell. A deletion mutant G(1–429) (termed GATC), lacking the transmembrane (TM) and cytoplasmic domains, was shown to be accumulated in the rough endoplasmic reticulum (rER) with BiP and did not seem to be shed. Another C‐terminal‐deficient mutant G(1–462) (termed CT1) was deprived of the whole cytoplasmic domain except for a basic amino acid left at the C‐terminus, but was transported to the cell surface, where it showed pH‐dependent cell fusion activity and almost full antigenicity to most of the anti‐G mAbs with the exception of very weak antigenicity to mAb #1‐30‐44. No Gs protein could be detected in the CT1‐producing cultures. Based on these results, we think that the cytoplasmic domain was not necessary for the G protein to be transported to the cell surface, but was necessary to keep its 1‐30‐44 epitope‐positive GB conformation. Gs proteins might have lost the C‐terminal regions during the maturation process after being exported from the rER.
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