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PDBsum entry 2kfk
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Signaling protein
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PDB id
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2kfk
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References listed in PDB file
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Key reference
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Title
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Nmr structure of the heterodimer of bem1 and cdc24 pb1 domains from saccharomyces cerevisiae.
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Authors
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K.Ogura,
T.Tandai,
S.Yoshinaga,
Y.Kobashigawa,
H.Kumeta,
T.Ito,
H.Sumimoto,
F.Inagaki.
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Ref.
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J Biochem (tokyo), 2009,
146,
317-325.
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PubMed id
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Abstract
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Bem1 and Cdc24 of the budding yeast Saccharomyces cerevisiae interact with each
other through PB1-PB1 heterodimer formation to regulate the establishment of
cell polarity. Here we present the tertiary structure of the heterodimer of Bem1
and Cdc24 PB1 domains determined by NMR spectroscopy. To avoid ambiguity in the
NMR spectral analysis, we first prepared a mutant of the Cdc24 PB1 domain that
had truncated loops. The mutant provided well dispersed spectra without spectral
overlapping, thus allowing unambiguous spectral assignments for structure
determination. We confirmed that the loop deletion-mutant was quite similar to
the wild-type in both 3D structure and binding affinity. The NMR structure of
the heterodimer of the deletion-mutant of Cdc24 PB1 and Bem1 PB1 was determined
using a variety of isotope labelled samples including perdeuteration. The
interface between the Bem1/Cdc24 PB1 heterodimer was analysed at atomic
resolution. Through a comparison with the tertiary structures of other PB1-PB1
heterodimers, we found that conserved electrostatic properties on the molecular
surface were commonly used for PB1-PB1 interaction, but hydrophobic interactions
were important for cognate interaction in Bem1/Cdc24 PB1 heterodimer formation.
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