Article
- The EMBO Journal (2008) 27, 1491 - 1501
- doi:10.1038/emboj.2008.83
Published online: 17 April 2008
Subject Categories:
Oxygen-regulated degradation of fission yeast SREBP by Ofd1, a prolyl hydroxylase family member
Bridget T Hughes1 and Peter J Espenshade1
- Department of Cell Biology, Johns Hopkins University School of Medicine, Baltimore, MD, USA
Correspondence to:
Peter J Espenshade, Department of Cell Biology, Johns Hopkins University School of Medicine, 725 N Wolfe Street, Physiology 107B, Baltimore, MD 21205, USA. Tel: +1 443 287 5026; Fax: +1 410 502 7826; E-mail: peter.espenshade@jhmi.edu
Received 14 February 2008; Accepted 28 March 2008
Abstract
Sre1, the fission yeast sterol regulatory element binding protein, is an endoplasmic reticulum membrane-bound transcription factor that responds to changes in oxygen-dependent sterol synthesis as an indirect measure of oxygen availability. Under low oxygen, Sre1 is proteolytically cleaved and the released N-terminal transcription factor (Sre1N) activates gene expression essential for hypoxic growth. Here, we describe an oxygen-dependent mechanism for regulation of Sre1 that is independent of sterol-regulated proteolysis. Using yeast expressing only Sre1N, we show that Sre1N turnover is regulated by oxygen. Ofd1, an uncharacterized prolyl 4-hydroxylase-like 2-oxoglutarate-Fe(II) dioxygenase, accelerates Sre1N degradation in the presence of oxygen. However, unlike the prolyl 4-hydroxylases that regulate mammalian hypoxia-inducible factor, Ofd1 uses multiple domains to regulate Sre1N degradation by oxygen; the Ofd1 N-terminal dioxygenase domain is required for oxygen sensing and the Ofd1 C-terminal domain accelerates Sre1N degradation. Our data support a model whereby the Ofd1 N-terminal dioxygenase domain is an oxygen sensor that regulates the activity of the C-terminal degradation domain.
Keywords:
- degradation,
- hydroxylase,
- oxygen,
- SREBP,
- yeast
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