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Literature DB >> 16601692

Glycine-alanine repeats impair proper substrate unfolding by the proteasome.

Martin A Hoyt¹, Judith Zich, Junko Takeuchi, Mingsheng Zhang, Cedric Govaerts, Philip Coffino.

Abstract

Proteasome ATPases unravel folded proteins. Introducing a sequence containing only glycine and alanine residues (GAr) into substrates can impair their digestion. We previously proposed that a GAr interferes with the unfolding capacity of the proteasome, leading to partial degradation of products. Here we tested that idea in several ways. Stabilizing or destabilizing a folded domain within substrate proteins changed GAr-mediated intermediate production in the way predicted by the model. A downstream folded domain determined the sites of terminal proteolysis. The spacing between a GAr and a folded domain was critical for intermediate production. Intermediates containing a GAr did not remain associated with proteasomes, excluding models whereby retained GAr-containing proteins halt further processing. The following model is supported: a GAr positioned within the ATPase ring reduces the efficiency of coupling between nucleotide hydrolysis and work performed on the substrate. If this impairment takes place when unfolding must be initiated, insertion pauses and proteolysis is limited to the portion of the substrate that has already entered the catalytic chamber of the proteasome.

Entities: Chemical

Mesh：

Substances：

Year: 2006 PMID： 16601692 PMCID： PMC1440830 DOI： 10.1038/sj.emboj.7601058

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

44 in total

1. Repeat sequence of Epstein-Barr virus-encoded nuclear antigen 1 protein interrupts proteasome substrate processing.

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3. An unstructured initiation site is required for efficient proteasome-mediated degradation.

Authors: Sumit Prakash; Lin Tian; Kevin S Ratliff; Rebecca E Lehotzky; Andreas Matouschek
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4. Linkage between ATP consumption and mechanical unfolding during the protein processing reactions of an AAA+ degradation machine.

Authors: Jon A Kenniston; Tania A Baker; Julio M Fernandez; Robert T Sauer
Journal: Cell Date: 2003-08-22 Impact factor: 41.582

5. Binding of a specific ligand inhibits import of a purified precursor protein into mitochondria.

Authors: M Eilers; G Schatz
Journal: Nature Date: 1986 Jul 17-23 Impact factor: 49.962

6. Expression and site-directed mutagenesis of human dihydrofolate reductase.

Authors: N J Prendergast; T J Delcamp; P L Smith; J H Freisheim
Journal: Biochemistry Date: 1988-05-17 Impact factor: 3.162

7. Trypanosome ornithine decarboxylase is stable because it lacks sequences found in the carboxyl terminus of the mouse enzyme which target the latter for intracellular degradation.

Authors: L Ghoda; M A Phillips; K E Bass; C C Wang; P Coffino
Journal: J Biol Chem Date: 1990-07-15 Impact factor: 5.157

Glycine-alanine repeats impair proper substrate unfolding by the proteasome.

1. Repeat sequence of Epstein-Barr virus-encoded nuclear antigen 1 protein interrupts proteasome substrate processing.

2. Substrate recognition by the AAA+ chaperone ClpB.

3. An unstructured initiation site is required for efficient proteasome-mediated degradation.

4. Linkage between ATP consumption and mechanical unfolding during the protein processing reactions of an AAA+ degradation machine.

5. Binding of a specific ligand inhibits import of a purified precursor protein into mitochondria.

6. Expression and site-directed mutagenesis of human dihydrofolate reductase.

7. Trypanosome ornithine decarboxylase is stable because it lacks sequences found in the carboxyl terminus of the mouse enzyme which target the latter for intracellular degradation.

8. Sem1p is a novel subunit of the 26 S proteasome from Saccharomyces cerevisiae.

9. Prevention of rapid intracellular degradation of ODC by a carboxyl-terminal truncation.

10. Proteasomes begin ornithine decarboxylase digestion at the C terminus.

1. m-AAA protease-driven membrane dislocation allows intramembrane cleavage by rhomboid in mitochondria.

2. Slippery substrates impair ATP-dependent protease function by slowing unfolding.

3. The ubiquitin ligase Hul5 promotes proteasomal processivity.

4. Gly-Ala repeats induce position- and substrate-specific regulation of 26 S proteasome-dependent partial processing.

5. Paddling mechanism for the substrate translocation by AAA+ motor revealed by multiscale molecular simulations.

Review 6. Multitasking with ubiquitin through multivalent interactions.

7. Dependence of proteasome processing rate on substrate unfolding.

Review 8. Substrate selection by the proteasome through initiation regions.

9. Slippery substrates impair ATP-dependent protease function by slowing unfolding.

10. Slippery substrates impair function of a bacterial protease ATPase by unbalancing translocation versus exit.