Recruitment of CREB Binding Protein Is Sufficient for CREB-Mediated Gene Activation

Author:

Cardinaux Jean-Rene1,Notis John C.1,Zhang Qinghong1,Vo Ngan1,Craig Johanna C.1,Fass Daniel M.1,Brennan Richard G.2,Goodman Richard H.1

Affiliation:

1. Vollum Institute 1 and

2. Department of Biochemistry, 2 Oregon Health Sciences University, Portland, Oregon 97201

Abstract

ABSTRACT Phosphorylation of the transcription factor CREB leads to the recruitment of the coactivator, CREB binding protein (CBP). Recent studies have suggested that CBP recruitment is not sufficient for CREB function, however. We have identified a conserved protein-protein interaction motif within the CBP-binding domains of CREB and another transcription factor, SREBP (sterol-responsive element binding protein). In contrast to CREB, SREBP interacts with CBP in the absence of phosphorylation. We have exploited the conservation of this interaction motif to test whether CBP recruitment to CREB is sufficient for transcriptional activation. Substitution of six nonconserved amino acids from SREBP into the activation domain of CREB confers high-affinity, phosphorylation-independent CBP binding. The mutated CREB molecule, CREB DIEDML , activates transcription in F9 teratocarcinoma and PC12 cells even in the absence of protein kinase A (PKA). Addition of exogenous CBP augments the level of transcription mediated by CREB DIEDML , and adenovirus 12S E1A blocks transcription, implicating CBP in the activation process. Thus, recruitment of CBP to CREB is sufficient for transcriptional activation. Addition of PKA stimulates transcription induced by CREB DIEDML further, suggesting that a phosphorylation event downstream from CBP recruitment augments CREB signaling.

Publisher

American Society for Microbiology

Subject

Cell Biology,Molecular Biology

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