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PDBsum entry 1j3e
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Replication/DNA
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PDB id
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1j3e
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Contents |
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* Residue conservation analysis
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References listed in PDB file
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Key reference
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Title
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Structural and biochemical analyses of hemimethylated DNA binding by the seqa protein.
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Authors
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N.Fujikawa,
H.Kurumizaka,
O.Nureki,
Y.Tanaka,
M.Yamazoe,
S.Hiraga,
S.Yokoyama.
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Ref.
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Nucleic Acids Res, 2004,
32,
82-92.
[DOI no: ]
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PubMed id
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Abstract
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The Escherichia coli SeqA protein recognizes the 11 hemimethylated G-mA-T-C
sites in the oriC region of the chromosome, and prevents replication
over-initiation within one cell cycle. The crystal structure of the SeqA
C-terminal domain with hemimethylated DNA revealed the N6-methyladenine
recognition mechanism; however, the mechanism of discrimination between the
hemimethylated and fully methylated states has remained elusive. In the present
study, we performed mutational analyses of hemimethylated G-mA-T-C sequences
with the minimal DNA-binding domain of SeqA (SeqA71-181), and found that
SeqA71-181 specifically binds to hemimethylated DNA containing a sequence with a
mismatched mA:G base pair [G-mA(:G)-T-C] as efficiently as the normal
hemimethylated G-mA(:T)-T-C sequence. We determined the crystal structures of
SeqA71-181 complexed with the mismatched and normal hemimethylated DNAs at 2.5
and 3.0 A resolutions, respectively, and found that the mismatched mA:G base
pair and the normal mA:T base pair are recognized by SeqA in a similar manner.
Furthermore, in both crystal structures, an electron density is present near the
unmethylated adenine, which is only methylated in the fully methylated state.
This electron density, which may be due to a water molecule or a metal ion, can
exist in the hemimethylated state, but not in the fully methylated state,
because of steric clash with the additional methyl group.
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