Basis for a ubiquitin-like protein thioester switch toggling E1–E2 affinity

Huang, Danny T.; Hunt, Harold W.; Zhuang, Min; Ohi, Melanie D.; Holton, James M.; Schulman, Brenda A.

doi:10.1038/nature05490

Cited by 194 publications

(304 citation statements)

References 35 publications

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“…6B and data not shown). It has been found that an E1-E2 transthiolation event requires significant conformational rearrangements of the E1 enzyme (31,34,35). Crystallography studies with the NAE ternary complex and Ubc12 show that the core domain of Ubc12 associates with the UFD of NAE and a peptide-like extension on Ubc12 docks into a groove in the adenylation domain, adjacent to the ATP-binding site on NAE (35).…”

Section: Discussionmentioning

confidence: 99%

“…Crystallography studies with the NAE ternary complex and Ubc12 show that the core domain of Ubc12 associates with the UFD of NAE and a peptide-like extension on Ubc12 docks into a groove in the adenylation domain, adjacent to the ATP-binding site on NAE (35). It is hypothesized that formation of NEDD8-adenylate on the NAEϳNEDD8 thioester induces a rotation in the UFD domain of almost 120°, which enables NAE to bind Ubc12 and align it in prime position for transthiolation (35). After the NEDD8 thioester is transferred to Ubc12, the loss of the covalent bond with NEDD8 induces the UFD of NAE to rotate back (35).…”

Section: Discussionmentioning

confidence: 99%

“…It has been found that an E1-E2 transthiolation event requires significant conformational rearrangements of the E1 enzyme (31,34,35). Crystallography studies with the NAE ternary complex and Ubc12 show that the core domain of Ubc12 associates with the UFD of NAE and a peptide-like extension on Ubc12 docks into a groove in the adenylation domain, adjacent to the ATP-binding site on NAE (35). It is hypothesized that formation of NEDD8-adenylate on the NAEϳNEDD8 thioester induces a rotation in the UFD domain of almost 120°, which enables NAE to bind Ubc12 and align it in prime position for transthiolation (35).…”

Section: Discussionmentioning

confidence: 99%

“…It is hypothesized that formation of NEDD8-adenylate on the NAEϳNEDD8 thioester induces a rotation in the UFD domain of almost 120°, which enables NAE to bind Ubc12 and align it in prime position for transthiolation (35). After the NEDD8 thioester is transferred to Ubc12, the loss of the covalent bond with NEDD8 induces the UFD of NAE to rotate back (35). Considering the mechanism proposed for NAE, we hypothesize that high concentrations of ATP could trap the UFD domain of Uba6 in a confirmation that is unfavorable for UBL charging.…”

Section: Discussionmentioning

confidence: 99%

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Mechanistic Studies on Activation of Ubiquitin and Di-ubiquitin-like Protein, FAT10, by Ubiquitin-like Modifier Activating Enzyme 6, Uba6

Gavin

Chen

Liao

et al. 2012

Journal of Biological Chemistry

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Background:The Uba6 pathway and its components play an important role in a variety of biological processes. Results: The mechanism of how Uba6 activates two distinct substrates, ubiquitin and FAT10, was characterized. Conclusion: Uba6 was shown to use a similar mechanism for activating both substrates with a greater affinity for FAT10. Significance: Relative levels of ubiquitin and FAT10 could regulate the Uba6 pathway in cells.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

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Mechanistic Studies on Activation of Ubiquitin and Di-ubiquitin-like Protein, FAT10, by Ubiquitin-like Modifier Activating Enzyme 6, Uba6

Gavin

Chen

Liao

et al. 2012

Journal of Biological Chemistry

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“…During the transfer of Ublp from E1 to E2, the E2 enzyme is recruited to the E1-SUMO thioester conjugate by binding to multiple sites on E1, including the Cys domain (the domain containing the active Cys residue) and the ubiquitin-like (Ubl) domain (10,11). Among these multiple binding sites, the Ubl domain has the highest binding affinity, and thus it is the key E2-binding site.…”

mentioning

confidence: 99%

Conformational Transition Associated with E1-E2 Interaction in Small Ubiquitin-like Modifications

Wang¹,

Lee²,

Cai³

et al. 2009

Journal of Biological Chemistry

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Ubiquitin-like modifications regulate nearly every aspect of cellular functions. A key step in these modifications is the recognition of the carrier enzyme (E2) by the activating enzyme (E1). In this study, we have found that a critical E2-binding surface on the E1 of the small ubiquitin-like modifier has unusually high populations in both ordered and disordered states. Upon binding the E2, the disordered state is converted to the ordered state, which resembles the structure of the bound conformation, providing a mechanism to resolve the "Levinthal Paradox" search problem in a folding-upon-binding process. The significance of the folding-unfolding equilibrium is shown by the loss of functions of the mutations that shift the equilibrium to the folded state. This study highlights the importance of conformational flexibility in the molecular recognition event.The conjugation of ubiquitin or ubiquitin-like proteins to other cellular proteins is one of the most important mechanisms in regulating cellular functions in eukaryotic systems and is broadly involved in controlling the life spans, trafficking, and functions of a wide range of proteins (1-4). Among the ubiquitin-like modifiers, the small ubiquitin-like modifier (SUMO) 5 is the most studied, and its modification regulates many essential functions, such as gene transcription, hormone response, DNA repair, and nuclear import (5-7). Multiple enzymes are required for post-translational modifications by ubiquitin or ubiquitin-like proteins (1,8). A ubiquitin-like protein (Ublp) is first activated by E1. The E1 required for SUMO modification is a tight heterodimer of two proteins, known as SUMO activation enzymes 1 and 2 (SAE1 and SAE2), which are homologous to the N-terminal and C-terminal portions of the ubiquitin E1, respectively (9). E1 catalyzes the adenylation of the C-terminal carboxyl group of the Ublp, and it then forms a thioester bond between the -SH group of the active site Cys residue and the C-terminal carboxyl group of the Ublp. The Ublp is then transferred to E2 (known as Ubc9 in the SUMO pathway), forming a thioester bond with the -SH group of the active site Cys residue. In the final step, the Ublp is attached to target proteins by forming an isopeptide bond between its C-terminal carboxyl group and the ⑀-amino group of a Lys residue on the target protein. This step generally requires another enzyme, isopeptide ligase.During the transfer of Ublp from E1 to E2, the E2 enzyme is recruited to the E1-SUMO thioester conjugate by binding to multiple sites on E1, including the Cys domain (the domain containing the active Cys residue) and the ubiquitin-like (Ubl) domain (10, 11). Among these multiple binding sites, the Ubl domain has the highest binding affinity, and thus it is the key E2-binding site. The multivalent interaction produces high affinity binding between E1 and E2, which accounts for the efficiency of E1 at low concentrations. At the same time, the low to medium affinity of each of the individual interactions allows fast turnover of the enzym...

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How ubiquitination regulates the TGF‐β signalling pathway: New insights and new players

Soond

Chantry

2011

BioEssays

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Subtitle:TGF-β regulation by NEDD4 E3s are discussed, while emphasising the potential role of isoform-derivatives of E1-E3 proteins in ubiquitination.Key Words: TGF beta, Smad, Ubiquitination, Uniquitinome, EMT, cancer Abstract Ubiquitination of protein species in regulating signal transduction pathways is universally accepted as fundamental during normal development and has been implicated in the progression of many human diseases, such as cancer. One particular pathway that has received much attention in this context is TGF-β signalling, particularly during the regulation of EMT and tumour progression. While E3-ubiquitin ligases offer themselves as potential therapeutic targets (based on their ability to confer substrate specificity), much remains to be unveiled regarding mechanisms that culminate in their regulation. With this in mind, the focus of this review highlights the significance of a recently described group of E3-ubiquitin ligase isoforms in the context of the TGF-β pathway regulation. Moreover, we now broaden these observations to incorporate a growing number of protein-isoforms within the ubiquitin ligase superfamily as a whole, and discuss what relevance they may have in defining a new 'iso-ubiquitinome'.

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Basis for a ubiquitin-like protein thioester switch toggling E1–E2 affinity

Cited by 194 publications

References 35 publications

Mechanistic Studies on Activation of Ubiquitin and Di-ubiquitin-like Protein, FAT10, by Ubiquitin-like Modifier Activating Enzyme 6, Uba6

Mechanistic Studies on Activation of Ubiquitin and Di-ubiquitin-like Protein, FAT10, by Ubiquitin-like Modifier Activating Enzyme 6, Uba6

Conformational Transition Associated with E1-E2 Interaction in Small Ubiquitin-like Modifications

How ubiquitination regulates the TGF‐β signalling pathway: New insights and new players

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