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PDBsum entry 1ltp
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Transcription regulation
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PDB id
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1ltp
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J Biol Chem
268:17602-17612
(1993)
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PubMed id:
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Model of lactose repressor core based on alignment with sugar-binding proteins is concordant with genetic and chemical data.
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J.C.Nichols,
N.K.Vyas,
F.A.Quiocho,
K.S.Matthews.
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ABSTRACT
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Using primary sequence similarity to arabinose-binding protein,
D-glucose/D-galactose-binding protein, and ribose-binding protein (Vyas, N. K.,
Vyas, M. N., and Quiocho, F. A. (1991) J. Biol. Chem. 266, 5226-5237; Mowbray,
S. L., and Cole, L. B. (1992) J. Mol. Biol. 225, 155-175), the core domain
(residues 62-323) of the bacterial regulatory protein lac repressor has been
aligned to these sugar-binding proteins of known structure. Although the
sequence identity is not striking, there is strong overall homology based on two
separate matrix scoring systems (minimum base change per codon (MBC/C) and amino
acid homology per residue (AAH/R)) (mean score: MBC/C < 1.25, AAH/R >
5.50; random sequences: MBC/C = 1.45, AAH/R = 4.46). Similarly, the predicted
secondary structure of the repressor exhibits excellent agreement with the known
secondary structures of the sugar-binding proteins. Using this primary sequence
alignment, the tertiary structure of the core domain of the lac repressor has
been modeled based on the known structures of the sugar-binding proteins as
templates. While the structure deduced for the repressor is hypothetical, the
model generated allows a comparison between the predicted tertiary arrangement
and the wealth of genetic and chemical data elucidated for the repressor.
Important residues involved in operator and sugar binding and in protein
assembly have been identified using genetic methods, and placement of these
residues in the model is consistent with their known function. This approach,
therefore, provides a means to visualize the core domain of the lac repressor
that allows interpretation of genetic and chemical data for specific residues
and rational design of future experiments.
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Literature references that cite this PDB file's key reference
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PubMed id
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Reference
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S.J.Lee,
A.Böhm,
M.Krug,
and
W.Boos
(2007).
The ABC of binding-protein-dependent transport in Archaea.
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Trends Microbiol,
15,
389-397.
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Y.Xu,
S.Rosenkranz,
C.L.Weng,
J.M.Scharer,
M.Moo-Young,
and
C.P.Chou
(2006).
Characterization of the T7 promoter system for expressing penicillin acylase in Escherichia coli.
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Appl Microbiol Biotechnol,
72,
529-536.
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L.Swint-Kruse,
C.R.Elam,
J.W.Lin,
D.R.Wycuff,
and
K.Shive Matthews
(2001).
Plasticity of quaternary structure: twenty-two ways to form a LacI dimer.
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Protein Sci,
10,
262-276.
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B.D.Nelson,
C.Manoil,
and
B.Traxler
(1997).
Insertion mutagenesis of the lac repressor and its implications for structure-function analysis.
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J Bacteriol,
179,
3721-3728.
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D.D.Dalma-Weiszhausz,
and
M.Brenowitz
(1996).
Interactions between RNA polymerase and the positive and negative regulators of transcription at the Escherichia coli gal operon.
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Biochemistry,
35,
3735-3745.
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F.A.Quiocho,
and
P.S.Ledvina
(1996).
Atomic structure and specificity of bacterial periplasmic receptors for active transport and chemotaxis: variation of common themes.
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Mol Microbiol,
20,
17-25.
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T.A.Thanaraj,
and
P.Argos
(1996).
Ribosome-mediated translational pause and protein domain organization.
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Protein Sci,
5,
1594-1612.
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P.Bork,
L.Holm,
E.V.Koonin,
and
C.Sander
(1995).
The cytidylyltransferase superfamily: identification of the nucleotide-binding site and fold prediction.
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Proteins,
22,
259-266.
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M.H.Saier
(1994).
Computer-aided analyses of transport protein sequences: gleaning evidence concerning function, structure, biogenesis, and evolution.
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Microbiol Rev,
58,
71-93.
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The most recent references are shown first.
Citation data come partly from CiteXplore and partly
from an automated harvesting procedure. Note that this is likely to be
only a partial list as not all journals are covered by
either method. However, we are continually building up the citation data
so more and more references will be included with time.
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