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Role for Slimb in the degradation of Drosophila Period protein phosphorylated by Doubletime

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  • Hyuk Wan Ko

    (Graduate Program in Physiology and Neurobiology, Rutgers University, Center for Advanced Biotechnology and Medicine)

  • Jin Jiang

    (University of Texas Southwestern Medical Center)

  • Isaac Edery

    (Department of Molecular Biology and Biochemistry, Rutgers University, Center for Advanced Biotechnology and Medicine)

Abstract

Protein phosphorylation has a key role in modulating the stabilities of circadian clock proteins in a manner specific to the time of day1. A conserved feature of animal clocks is that Period (Per) proteins undergo daily rhythms in phosphorylation and levels2,3, events that are crucial for normal clock progression4,5,6,7. Casein kinase Iε (CKIε) has a prominent role in regulating the phosphorylation and abundance of Per proteins in animals8. This was first shown in Drosophila with the characterization of Doubletime (Dbt), a homologue of vertebrate casein kinase Iε4,6. However, it is not clear how Dbt regulates the levels of Per. Here we show, using a cell culture system, that Dbt promotes the progressive phosphorylation of Per, leading to the rapid degradation of hyperphosphorylated isoforms by the ubiquitin–proteasome pathway. Slimb, an F-box/WD40-repeat protein functioning in the ubiquitin–proteasome pathway9,10 interacts preferentially with phosphorylated Per and stimulates its degradation. Overexpression of slimb or expression in clock cells of a dominant-negative version of slimb disrupts normal rhythmic activity in flies. Our findings suggest that hyperphosphorylated Per is targeted to the proteasome by interactions with Slimb.

Suggested Citation

  • Hyuk Wan Ko & Jin Jiang & Isaac Edery, 2002. "Role for Slimb in the degradation of Drosophila Period protein phosphorylated by Doubletime," Nature, Nature, vol. 420(6916), pages 673-678, December.
  • Handle: RePEc:nat:nature:v:420:y:2002:i:6916:d:10.1038_nature01272
    DOI: 10.1038/nature01272
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