Structural studies of the yeast DNA damage-inducible protein Ddi1 reveal domain architecture of this eukaryotic protein family

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作者
Jean-François Trempe
Klára Grantz Šašková
Monika Sivá
Colin D. H. Ratcliffe
Václav Veverka
Annabelle Hoegl
Marie Ménade
Xin Feng
Solomon Shenker
Michal Svoboda
Milan Kožíšek
Jan Konvalinka
Kalle Gehring
机构
[1] Groupe de Recherche Axé sur la Structure des Protéines,Department of Biochemistry
[2] McGill University,Department of Biochemistry
[3] 3649 Promenade Sir William Osler,Department of Physical and Macromolecular Chemistry
[4] Gilead Sciences and IOCB Research Center,undefined
[5] Institute of Organic Chemistry and Biochemistry of the Academy of Sciences of the Czech Republic,undefined
[6] Faculty of Science,undefined
[7] Charles University,undefined
[8] First Faculty of Medicine,undefined
[9] Charles University in Prague,undefined
[10] Faculty of Science,undefined
[11] Charles University,undefined
[12] Present address: Department of Pharmacology & Therapeutics,undefined
[13] McGill University,undefined
[14] 3655 Promenade Sir William Osler,undefined
[15] Montreal,undefined
[16] QC,undefined
[17] H3G 1Y6,undefined
[18] Canada.,undefined
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摘要
The eukaryotic Ddi1 family is defined by a conserved retroviral aspartyl protease-like (RVP) domain found in association with a ubiquitin-like (UBL) domain. Ddi1 from Saccharomyces cerevisiae additionally contains a ubiquitin-associated (UBA) domain. The substrate specificity and role of the protease domain in the biological functions of the Ddi family remain unclear. Yeast Ddi1 has been implicated in the regulation of cell cycle progression, DNA-damage repair, and exocytosis. Here, we investigated the multi-domain structure of yeast Ddi1 using X-ray crystallography, nuclear magnetic resonance, and small-angle X-ray scattering. The crystal structure of the RVP domain sheds light on a putative substrate recognition site involving a conserved loop. Isothermal titration calorimetry confirms that both UBL and UBA domains bind ubiquitin, and that Ddi1 binds K48-linked diubiquitin with enhanced affinity. The solution NMR structure of a helical domain that precedes the protease displays tertiary structure similarity to DNA-binding domains from transcription regulators. Our structural studies suggest that the helical domain could serve as a landing platform for substrates in conjunction with attached ubiquitin chains binding to the UBL and UBA domains.
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