Normal precursors of periplasmic proteins accumulated in the cytoplasm are not exported post‐translationally in Escherichia coli

Abstract

Hyperproduction of phosphate-binding protein, PhoS, in strains carrying a multicopy plasmic containing the phoS gene, resulted in saturation of export sites. As a consequence, pre-PhoS was accumulated both in the inner membrane and in the cytoplasm. This was evidenced both in EM and after cell fractionation. Only the membrane-associated precursor could be matured and exported. The signal sequence of the cytoplasmic pre-PhoS was slowly degraded. It was first cleaved about in its middle and then completely removed. EM studies demonstrated that the cytoplasmic pre-PhoS cannot be exported post-translationally.