Warning: Undefined array key "mm" in /www/wwwroot/www.ai-bt.com/si.php on line 10 Deprecated: trim(): Passing null to parameter #1 ($string) of type string is deprecated in /www/wwwroot/www.ai-bt.com/si.php on line 10 Targeting of signal sequenceless proteins for export in Escherichia coli with altered protein translocase.

Literature DB >> 8895566

Targeting of signal sequenceless proteins for export in Escherichia coli with altered protein translocase.

W A Prinz¹, C Spiess, M Ehrmann, C Schierle, J Beckwith.

Abstract

Most extracytoplasmic proteins are synthesized with an N-terminal signal sequence that targets them to the export apparatus. Escherichia coli prlA mutants (altered in the secY gene) are able to export cell envelope proteins lacking any signal sequence. In order to understand how such proteins are targeted for export, we isolated mutations in a signal sequenceless version of alkaline phosphatase that block its export in a prlA mutant. The mutations introduce basic amino acyl residues near the N-terminus of alkaline phosphatase. These changes do not disrupt an N-terminal export signal in this protein since the first 25 amino acids can be removed without affecting its export competence. These findings suggest that signal sequenceless alkaline phosphatase does not contain a discrete domain that targets it for export and may be targeted simply because it remains unfolded in the cytoplasm. We propose that basic amino acids near the N-terminus of a signal sequenceless protein affect its insertion into the translocation apparatus after it has been targeted for export. These findings allow the formulation of a model for the entry of proteins into the membrane-embedded export machinery.

Entities: Chemical Gene Species

Mesh：

Substances：

Year: 1996 PMID： 8895566 PMCID： PMC452265

Source DB: PubMed Journal: EMBO J ISSN： 0261-4189 Impact factor: 11.598

45 in total

1. Signal-sequence recognition by an Escherichia coli ribonucleoprotein complex.

Authors: J Luirink; S High; H Wood; A Giner; D Tollervey; B Dobberstein
Journal: Nature Date: 1992-10-22 Impact factor: 49.962

2. Modulation of folding pathways of exported proteins by the leader sequence.

Authors: S Park; G Liu; T B Topping; W H Cover; L L Randall
Journal: Science Date: 1988-02-26 Impact factor: 47.728

3. Effects of signal sequence mutations on the kinetics of alkaline phosphatase export to the periplasm in Escherichia coli.

Authors: S Michaelis; J F Hunt; J Beckwith
Journal: J Bacteriol Date: 1986-07 Impact factor: 3.490

Review 4. Export of protein: a biochemical view.

Authors: L L Randall; S J Hardy; J R Thom
Journal: Annu Rev Microbiol Date: 1987 Impact factor: 15.500

5. The antifolding activity of SecB promotes the export of the E. coli maltose-binding protein.

Authors: D N Collier; V A Bankaitis; J B Weiss; P J Bassford
Journal: Cell Date: 1988-04-22 Impact factor: 41.582

6. Localization and processing of outer membrane and periplasmic proteins in Escherichia coli strains harboring export-specific suppressor mutations.

Authors: S D Emr; P J Bassford
Journal: J Biol Chem Date: 1982-05-25 Impact factor: 5.157

10. PrlA4 prevents the rejection of signal sequence defective preproteins by stabilizing the SecA-SecY interaction during the initiation of translocation.

Authors: J P van der Wolk; P Fekkes; A Boorsma; J L Huie; T J Silhavy; A J Driessen
Journal: EMBO J Date: 1998-07-01 Impact factor: 11.598

Targeting of signal sequenceless proteins for export in Escherichia coli with altered protein translocase.

1. Signal-sequence recognition by an Escherichia coli ribonucleoprotein complex.

2. Modulation of folding pathways of exported proteins by the leader sequence.

3. Effects of signal sequence mutations on the kinetics of alkaline phosphatase export to the periplasm in Escherichia coli.

Review 4. Export of protein: a biochemical view.

5. The antifolding activity of SecB promotes the export of the E. coli maltose-binding protein.

6. Localization and processing of outer membrane and periplasmic proteins in Escherichia coli strains harboring export-specific suppressor mutations.

7. Suppressor mutations that restore export of a protein with a defective signal sequence.

8. Signal sequences. The limits of variation.

9. Molecular characterization of the MalT-dependent periplasmic alpha-amylase of Escherichia coli encoded by malS.

10. A two-step recognition of signal sequences determines the translocation efficiency of proteins.

1. The PrlA and PrlG phenotypes are caused by a loosened association among the translocase SecYEG subunits.

Review 2. Protein targeting to the bacterial cytoplasmic membrane.

3. Projection structure and oligomeric properties of a bacterial core protein translocase.

4. SecA-dependent quality control of intracellular protein localization.

Review 5. Interactions that drive Sec-dependent bacterial protein transport.

Review 6. A little help from my friends: quality control of presecretory proteins in bacteria.

7. Modeling the effects of prl mutations on the Escherichia coli SecY complex.

8. Investigating the SecY plug movement at the SecYEG translocation channel.

9. Signal peptides are allosteric activators of the protein translocase.

10. PrlA4 prevents the rejection of signal sequence defective preproteins by stabilizing the SecA-SecY interaction during the initiation of translocation.