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Vol. 13, Issue 5, 1709-1721, May 2002

and
*Department of Genetics, The Hebrew University, Jerusalem 91904, Israel; and Rme1p, a repressor of meiosis in the yeast Saccharomyces
cerevisiae, acts as both a transcriptional repressor and
activator. Rme1p is a zinc-finger protein with no other homology to any
protein of known function. The C-terminal DNA binding domain of Rme1p is essential for function. We find that mutations and progressive deletions in all three zinc fingers can be rescued by fusion of RME1 to the DNA binding domain of another protein. Thus,
structural integrity of the zinc fingers is not required for the
Rme1p-mediated effects on transcription. Using a series of mutant Rme1
proteins, we have characterized domains responsible for repression and
activation. We find that the minimal transcriptional repression and
activation domains completely overlap and lie in an 88-amino-acid
N-terminal segment (aa 61-148). An additional transcriptional effector
determinant lies in the first 31 amino acids of the protein.
Notwithstanding the complete overlap between repression and activation
domains of Rme1p, we demonstrated a functional difference between
repression and activation: Rgr1p and Sin4p are absolutely required for
repression but dispensable for activation.
Institute of Cancer Research and Department
of Microbiology, Columbia University, New York, NY 10032
Corresponding author. E-mail address:
simchen{at}vms.huji.ac.il.
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