4.8 Article

Allosteric control of Ubp6 and the proteasome via a bidirectional switch

NATURE COMMUNICATIONS (2022)

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Journal

NATURE COMMUNICATIONS
Volume 13, Issue 1, Pages -

Publisher

NATURE PORTFOLIO
DOI: 10.1038/s41467-022-28186-y

Keywords

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Categories

Multidisciplinary Sciences

Funding

  1. National Institutes of Health [R01 GM043601, R01-GM101135, R01-GM134064-01]
  2. Dean's initiative grant
  3. Waters Corporation
  4. Deutsche Forschungsgemeinschaft (DFG) through Germany's Excellence Strategy [EXC 2067/1-390729940, CRC889]
  5. Marie Curie Career Integration grant [PCIG14-GA-2013-631577]
  6. National Research Foundation of Korea (NRF) grants
  7. DGIST R&D program of the Ministry of Science and ICT of Korea [2019R1A4A1024278, 2019R1A2C1089413, 21-CoE-BT-04]
  8. Gauss Center for Supercomputing e.V [pn56ri]
  9. National Research Foundation of Korea [21-COE-BT-04, 2019R1A4A1024278, 2019R1A2C1089413] Funding Source: Korea Institute of Science & Technology Information (KISTI), National Science & Technology Information Service (NTIS)

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The interplay between the proteasome and deubiquitinase Ubp6 is essential for the degradation of ubiquitylated substrates. This study provides structural insights into the mechanism by which Ubp6 and the proteasome are regulated. The researchers found that the proteasome recognizes ubiquitinated proteins and can edit ubiquitin marks, while Ubp6 inhibits the proteasome through deubiquitination and a noncatalytic effect. Cryo-EM structures of the proteasome bound to Ubp6 revealed the interaction between Ubp6 mutations and the proteasome subunit Rpt1, which abrogate Ubp6 activation. The findings suggest that a multicomponent allosteric switch controls both Ubp6 and the proteasome.
The interplay of the proteasome and deubiquitinase Ubp6 is crucial for the degradation of ubiquitylated substrates. Here, the authors provide structural insights into the allosteric mechanism by which the activities of both Ubp6 and the proteasome are regulated. The proteasome recognizes ubiquitinated proteins and can also edit ubiquitin marks, allowing substrates to be rejected based on ubiquitin chain topology. In yeast, editing is mediated by deubiquitinating enzyme Ubp6. The proteasome activates Ubp6, whereas Ubp6 inhibits the proteasome through deubiquitination and a noncatalytic effect. Here, we report cryo-EM structures of the proteasome bound to Ubp6, based on which we identify mutants in Ubp6 and proteasome subunit Rpt1 that abrogate Ubp6 activation. The Ubp6 mutations define a conserved region that we term the ILR element. The ILR is found within the BL1 loop, which obstructs the catalytic groove in free Ubp6. Rpt1-ILR interaction opens the groove by rearranging not only BL1 but also a previously undescribed network of three interconnected active-site-blocking loops. Ubp6 activation and noncatalytic proteasome inhibition are linked in that they are eliminated by the same mutations. Ubp6 and ubiquitin together drive proteasomes into a unique conformation associated with proteasome inhibition. Thus, a multicomponent allosteric switch exerts simultaneous control over both Ubp6 and the proteasome.

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