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PDBsum entry 2pvx
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Electron transport
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PDB id
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2pvx
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Contents |
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* Residue conservation analysis
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PDB id:
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| Name: |
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Electron transport
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Title:
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Nmr and x-ray analysis of structural additivity in metal binding site- swapped hybrids of rubredoxin
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Structure:
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Rubredoxin. Chain: a, b, c, d, e, f, g, h. Synonym: rd. Engineered: yes. Mutation: yes
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Source:
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Pyrococcus furiosus. Organism_taxid: 2261. Gene: rub. Expressed in: escherichia coli. Expression_system_taxid: 562
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Resolution:
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1.04Å
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R-factor:
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0.139
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R-free:
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0.180
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Authors:
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L.Wang,D.M.Lemaster,G.Hernandez,H.Li
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Key ref:
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D.M.LeMaster
et al.
(2007).
NMR and X-ray analysis of structural additivity in metal binding site-swapped hybrids of rubredoxin.
Bmc Struct Biol,
7,
81-81.
PubMed id:
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Date:
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10-May-07
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Release date:
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18-Dec-07
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PROCHECK
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Headers
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References
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P24297
(RUBR_PYRFU) -
Rubredoxin from Pyrococcus furiosus (strain ATCC 43587 / DSM 3638 / JCM 8422 / Vc1)
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Seq:
Struc:
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54 a.a.
53 a.a.*
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Key: |
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PfamA domain |
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Secondary structure |
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CATH domain |
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*
PDB and UniProt seqs differ
at 8 residue positions (black
crosses)
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Bmc Struct Biol
7:81-81
(2007)
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PubMed id:
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NMR and X-ray analysis of structural additivity in metal binding site-swapped hybrids of rubredoxin.
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D.M.LeMaster,
J.S.Anderson,
L.Wang,
Y.Guo,
H.Li,
G.Hernández.
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ABSTRACT
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BACKGROUND: Chimeric hybrids derived from the rubredoxins of Pyrococcus furiosus
(Pf) and Clostridium pasteurianum (Cp) provide a robust system for the
characterization of protein conformational stability and dynamics in a
differential mode. Interchange of the seven nonconserved residues of the metal
binding site between the Pf and Cp rubredoxins yields a complementary pair of
hybrids, for which the sum of the thermodynamic stabilities is equal to the sum
for the parental proteins. Furthermore, the increase in amide hydrogen exchange
rates for the hyperthermophile-derived metal binding site hybrid is faithfully
mirrored by a corresponding decrease for the complementary hybrid that is
derived from the less thermostable rubredoxin, indicating a degree of additivity
in the conformational fluctuations that underlie these exchange reactions.
RESULTS: Initial NMR studies indicated that the structures of the two
complementary hybrids closely resemble "cut-and-paste" models derived from the
parental Pf and Cp rubredoxins. This protein system offers a robust opportunity
to characterize differences in solution structure, permitting the quantitative
NMR chemical shift and NOE peak intensity data to be analyzed without recourse
to the conventional conversion of experimental NOE peak intensities into
distance restraints. The intensities for 1573 of the 1652 well-resolved NOE
crosspeaks from the hybrid rubredoxins were statistically indistinguishable from
the intensities of the corresponding parental crosspeaks, to within the
baseplane noise level of these high sensitivity data sets. The differences in
intensity for the remaining 79 NOE crosspeaks were directly ascribable to
localized dynamical processes. Subsequent X-ray analysis of the metal binding
site-swapped hybrids, to resolution limits of 0.79 A and 1.04 A, demonstrated
that the backbone and sidechain heavy atoms in the NMR-derived structures lie
within the range of structural variability exhibited among the individual
molecules in the crystallographic asymmetric unit (approximately 0.3 A),
indicating consistency with the "cut-and-paste" structuring of the hybrid
rubredoxins in both crystal and solution. CONCLUSION: Each of the significant
energetic interactions in the metal binding site-swapped hybrids appears to
exhibit a 1-to-1 correspondence with the interactions present in the
corresponding parental rubredoxin structure, thus providing a structural basis
for the observed additivity in conformational stability and dynamics. The
congruence of these X-ray and NMR experimental data offers additional support
for the interpretation that the conventional treatment of NOE distance
restraints contributes substantially to the systematic differences that are
commonly reported between NMR- and X-ray-derived protein structures.
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Links
