Recruitment of Thr 319-phosphorylated Ndd1p to the FHA domain of Fkh2p requires Clbkinase activity: a mechanism for CLB cluster gene activation

  1. David Reynolds1,4,
  2. Bu Jun Shi1,4,
  3. Cameron McLean1,3,
  4. Frosa Katsis2,
  5. Bruce Kemp2, and
  6. Stephen Dalton1,3,5
  1. 1 Department of Molecular Biosciences and Center for Molecular Genetics of Development, University of Adelaide, Adelaide, South Australia
  2. 2 St. Vincent's Institute of Medical Research, Melbourne, Victoria, Australia
  3. 3 Rhodes Center, University of Georgia, Athens, Georgia 30602, USA

Abstract

Activation of the CLB gene cluster through the assembly of Mcm1p–Fkh2p complexes at target promoters is essential for mitotic entry and transition through M phase. We show that the activation of this mitotic transcriptional program is dependent on the recruitment of Ndd1p, a coactivator that performs its essential function by acting through Fkh2p. Although an essential gene, NDD1 is dispensable in cells expressing a truncated form of Fkh2p lacking its C terminus. When phosphorylated on T319, Ndd1p is recruited to CLB cluster promoters by association with the forkhead-associated (FHA) domain of Fkh2p. Substitution of T319 for alanine significantly reduces recruitment of Ndd1p, resulting in loss of normal transcriptional regulation, severe impairment of cell growth, and a budding defect reminiscent of cells with a Cdk-Clbkinase deficiency. Finally, we show that phosphorylation of T319 and recruitment of Ndd1p to CLB2 and SWI5 promoters is dependent on Cdc28-Clbkinase activity. These data provide a model describing the activation of G2/M transcription through the phosphorylation of Ndd1p by Cdc28-Clb kinase activity.

Keywords

Footnotes

  • Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.1074103.

  • 4 These authors contributed equally to this work.

  • 5 Corresponding author. E-MAIL sdalton{at}arches.uga.edu; FAX (706) 542-7925.

    • Accepted May 20, 2003.
    • Received January 23, 2003.
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