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Literature DB >> 6383823

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

J M Pages, J Anba, A Bernadac, H Shinagawa, A Nakata, C Lazdunski.

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 electron-microscopy 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. Electron microscope studies demonstrated that the cytoplasmic pre-PhoS cannot be exported post-translationally.

Entities: Chemical Species

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Year: 1984 PMID： 6383823 DOI： 10.1111/j.1432-1033.1984.tb08398.x

Source DB: PubMed Journal: Eur J Biochem ISSN： 0014-2956

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Cited

16 in total

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4. High-level expression of the colicin A lysis protein.

Authors: D Cavard; S P Howard; R Lloubes; C Lazdunski
Journal: Mol Gen Genet Date: 1989-06

5. Secretion of the overproduced periplasmic PhoA protein into the medium and accumulation of its precursor in phoA-transformed Escherichia coli strains: involvement of outer membrane vesicles.

Authors: M A Nesmeyanova; I M Tsfasman; A L Karamyshev; N E Suzina
Journal: World J Microbiol Biotechnol Date: 1991-05 Impact factor: 3.312

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10. Immediate entrance to the export pathway after synthesis as a requirement for export of the sak gene product in Escherichia coli.

Authors: T Sako
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