Hexameric assembly of the proteasomal ATPases is templated through their C termini

Park, Soyeon; Roelofs, Jeroen; Kim, Woong; Robert, J; Schmidt, Marion; Gygi, Steven P.; Finley, Daniel

doi:10.1038/nature08065

Cited by 129 publications

(303 citation statements)

References 31 publications

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“…6c, right panel), suggesting that almost all proteasomes contained stoichiometric amounts of the fusion proteins. These observations support the CP template assembly model of the RP 39 . Furthermore, structural analysis by cryo-electron microscopy revealed that the Pre6-Rpt2-fused proteasome was almost indistinguishable from the wild-type proteasome (Fig.…”

Section: Resultssupporting

confidence: 76%

“…Our FCS analysis did not detect proteasome assembly intermediates in wild-type cells, probably because such intermediates are not abundant [37][38][39][40] . Previous studies using a specific importin-a mutant, srp1-49, suggested that nucleocytoplasmic transport mediated by importin a/b is coupled to proteasome biogenesis [19][20][21]23 .…”

Section: Resultsmentioning

confidence: 92%

“…Rpn4 is a transcription factor that regulates proteasome concentrations; deletion of RPN4 significantly reduces the levels of proteasome subunits 39,41 . Consistent with this, the cytoplasmic concentration of Rpn7-GFP, measured by FCS, decreased to B160 nM in srp1-49 rpn4D double-mutant cells at both the permissive and non-permissive temperatures (Supplementary Fig.…”

Section: Resultsmentioning

confidence: 99%

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Quantitative live-cell imaging reveals spatio-temporal dynamics and cytoplasmic assembly of the 26S proteasome

et al. 2014

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The 26S proteasome is a 2.5-MDa multisubunit protease complex that degrades polyubiquitylated proteins. Although its functions and structure have been extensively characterized, little is known about its dynamics in living cells. Here, we investigate the absolute concentration, spatio-temporal dynamics and complex formation of the proteasome in living cells using fluorescence correlation spectroscopy. We find that the 26S proteasome complex is highly mobile, and that almost all proteasome subunits throughout the cell are stably incorporated into 26S proteasomes. The interaction between 19S and 20S particles is stable even in an importin-a mutant, suggesting that the 26S proteasome is assembled in the cytoplasm. Furthermore, a genetically stabilized 26S proteasome mutant is able to enter the nucleus. These results suggest that the 26S proteasome completes its assembly process in the cytoplasm and translocates into the nucleus through the nuclear pore complex as a holoenzyme.

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Section: Resultssupporting

confidence: 76%

Section: Resultsmentioning

confidence: 92%

Section: Resultsmentioning

confidence: 99%

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Quantitative live-cell imaging reveals spatio-temporal dynamics and cytoplasmic assembly of the 26S proteasome

et al. 2014

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“…Two competing models exist for RP assembly ( Funakoshi et al , 2009; Le Tallec et al , 2009; Park et al , 2009; Roelofs et al , 2009). The first posits that RP assembly occurs in modules independent of the CP with the help of four RP-dedicated chaperones, named Hsm3, Nas2, Nas6 and Rpn14 ( Funakoshi et al , 2009).…”

Section: Discussion/analysis Of the Literaturementioning

confidence: 99%

“…The first posits that RP assembly occurs in modules independent of the CP with the help of four RP-dedicated chaperones, named Hsm3, Nas2, Nas6 and Rpn14 ( Funakoshi et al , 2009). In contrast, the second model proposes that the CP serves as a scaffold for the heterohexameric ATPase ring of the RP base ( Park et al , 2009). The second model, however, appears less likely with regard to X-ray structure analysis showing that the RP-dedicated chaperones hinder the association between the RP base and CP α ring ( Barrault et al , 2012).…”

Section: Discussion/analysis Of the Literaturementioning

confidence: 99%

Intracellular Dynamics of the Ubiquitin-Proteasome-System

Chowdhury

Enenkel

2015

F1000Res

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The ubiquitin-proteasome system is the major degradation pathway for short-lived proteins in eukaryotic cells. Targets of the ubiquitin-proteasome-system are proteins regulating a broad range of cellular processes including cell cycle progression, gene expression, the quality control of proteostasis and the response to geno- and proteotoxic stress. Prior to degradation, the proteasomal substrate is marked with a poly-ubiquitin chain. The key protease of the ubiquitin system is the proteasome. In dividing cells, proteasomes exist as holo-enzymes composed of regulatory and core particles. The regulatory complex confers ubiquitin-recognition and ATP dependence on proteasomal protein degradation. The catalytic sites are located in the proteasome core particle. Proteasome holo-enzymes are predominantly nuclear suggesting a major requirement for proteasomal proteolysis in the nucleus. In cell cycle arrested mammalian or quiescent yeast cells, proteasomes deplete from the nucleus and accumulate in granules at the nuclear envelope (NE) / endoplasmic reticulum (ER) membranes. In prolonged quiescence, proteasome granules drop off the NE / ER membranes and migrate as stable organelles throughout the cytoplasm, as thoroughly investigated in yeast. When quiescence yeast cells are allowed to resume growth, proteasome granules clear and proteasomes are rapidly imported into the nucleus.Here, we summarize our knowledge about the enigmatic structure of proteasome storage granules and the trafficking of proteasomes and their substrates between the cyto- and nucleoplasm.Most of our current knowledge is based on studies in yeast. Their translation to mammalian cells promises to provide keen insight into protein degradation in non-dividing cells which comprise the majority of our body’s cells.

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One Ligand in Dual Roles: Self‐Assembly of a Bis‐Rhomboidal‐Shaped, Three‐Dimensional Molecular Wheel

Guo

et al. 2014

Chemistry A European J

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A facile high yield, self-assembly process that leads to a terpyridine-based, three-dimensional, bis-rhomboidal-shaped, molecular wheel is reported. The desired coordination-driven supramolecular wheel involves eight structurally distorted tristerpyridine (tpy) ligands possessing a 60° angle between the adjacent tpy units and twelve Zn(2+) ions. The tpy ligand plays dual roles in the self-assembly process: two are staggered at 180° to create the internal hub, while six produce the external rim. The wheel can be readily generated by mixing the tpy ligand and Zn(2+) in a stoichiometric ratio of 2:3; full characterization is provided by ESI-MS, NMR spectroscopy, and TEM imaging.

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Hexameric assembly of the proteasomal ATPases is templated through their C termini

Cited by 129 publications

References 31 publications

Quantitative live-cell imaging reveals spatio-temporal dynamics and cytoplasmic assembly of the 26S proteasome

Quantitative live-cell imaging reveals spatio-temporal dynamics and cytoplasmic assembly of the 26S proteasome

Intracellular Dynamics of the Ubiquitin-Proteasome-System

One Ligand in Dual Roles: Self‐Assembly of a Bis‐Rhomboidal‐Shaped, Three‐Dimensional Molecular Wheel

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