Abstract
The Yeast MATa1 and MATα2 are homeodomain proteins that bind DNA cooperatively to repress transcription of cell type specific genes. The DNA affinity and specificity of MATa1 in the absence of MATα2, however, is very low. MATa1 is converted to a higher affinity DNA-binding protein by its interaction with the C-terminal tail of MATα2. To understand why MATa1 binds DNA weakly by itself, and how the MATα2 tail affects the affinity of MATa1 for DNA, we determined the crystal structure of a maltose- binding protein (MBP)-a1 chimera whose DNA binding behavior is similar to MATa1. The overall MATa1 conformation in the MBP-a1 structure, which was determined in the absence of α2 and DNA, is similar to that in the a1/α2/DNA structure. The sole difference is in the C-terminal portion of the DNA recognition helix of MATa1, which is flexible in the present structure. However, these residues are not in a location likely to be affected by binding of the MATα2 tail. The results argue against conformational changes in al induced by the tail of MATα2, suggesting instead that the MATα2 tail energetically couples the DNA binding of MATα2 and MATa1.
Original language | English (US) |
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Pages (from-to) | 306-312 |
Number of pages | 7 |
Journal | Protein Science |
Volume | 12 |
Issue number | 2 |
DOIs | |
State | Published - Feb 1 2003 |
Keywords
- Crystal structure
- Homeodomain
- MATa1
- Maltose binding protein
- Protein chimera
- Protein-DNA interactions
- Transcription
ASJC Scopus subject areas
- Biochemistry
- Molecular Biology