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PDBsum entry 1tt2
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* Residue conservation analysis
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Enzyme class:
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E.C.3.1.31.1
- micrococcal nuclease.
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Reaction:
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Endonucleolytic cleavage to nucleoside 3'-phosphates and 3'-phosphooligonucleotide end-products.
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DOI no:
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J Mol Biol
341:565-574
(2004)
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PubMed id:
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X-ray and thermodynamic studies of staphylococcal nuclease variants I92E and I92K: insights into polarity of the protein interior.
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D.M.Nguyen,
R.Leila Reynald,
A.G.Gittis,
E.E.Lattman.
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ABSTRACT
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We have used crystallography and thermodynamic analysis to study nuclease
variants I92E and I92K, in which an ionizable side-chain is placed in the
hydrophobic core of nuclease. We find that the energetic cost of burying
ionizable groups is rather modest. The X-ray determinations show water molecules
solvating the buried glutamic acid under cryo conditions, but not at room
temperature. The lysine side-chain does not appear solvated in either case.
Guanidine hydrochloride (GnHCl) denaturation of I92E and I92K, done as a
function of pH and monitored by tryptophan fluorescence, showed that I92E and
I92K are folded in the pH range pH 3.5-9.0 and pH 5.5-9.5, respectively. The
stability of the parental protein is independent of pH over a broad range. In
contrast, the stabilities of I92E and I92K exhibit a pH dependence, which is
quantitatively explained by thermodynamic analysis: the PK(a) value of the
buried K92 is 5.6, while that of the buried E92 is 8.65. The free energy
difference between burying the uncharged and charged forms of the groups is
modest, about 6 kcal/mol. We also found that epsilon(app) for I92K and I92E is
in the range approximately 10-12, instead of 2-4 commonly used to represent the
protein interior. Side-chains 92E and 92K were uncharged under the conditions of
the X-ray experiment. Both are buried completely inside the well-defined
hydrophobic core of the variant proteins without forming salt-bridges or
hydrogen bonds to other functional groups of the proteins. Under cryo conditions
92E shows a chain of four water molecules, which hydrate one oxygen atom of the
carboxyl group of the glutamic acid. Two other water molecules, which are
present in the wild-type at all temperatures, are also connected to the water
ring observed inside the hydrophobic core. The ready burial of water with an
uncharged E92 raises the possibility that solvent excursions into the interior
also take place in the wild-type protein, but in a random, dynamic way not
detectable by crystallography. Such transient excursions could increase the
average polarity, and thus epsilon(app), of the protein interior.
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Selected figure(s)
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Figure 3.
Figure 3. Ribbon representation of the superposition of
the I92E cryo (cyan) and (a) I92E room temperature (red)
structures and (b) the I92K cryo structure. (a) The side-
chain of 92E in both cryo (blue) and room temperature
(orange) adopts an identical conformation. The blue
spheres represent the four completely buried and the
two bridging water molecules seen in the I92E cryo
structure. (b) The two conformations of 92K as observed
in the I92K cryo structure with hydrophobic residues
that surround conformers 1 (magenta) and conformer 2
(green) within 4 Å .
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Figure 5.
Figure 5. The two conformations of 92K built into the
2Fo 2 Fc (blue) and Fo 2 Fc (magenta) electron density
maps, contoured at 1s and 3.5s respectively, calculated
from a model that had alanine at position 92. The sub-
sequent refinement of the model with the alternate 92K
conformations showed no electron density for the C
d
and N
z
atoms for conformer 1 or for the N
z
for conformer
2, which is indicative of increased mobility of the 92K
side-chain. The electron density maps displayed might
suggest the native isoleucine at this position. The lysine
mutation was confirmed by DNA sequencing and mass
spectrometry (data not shown). Moreover, none of the
four most frequent isoleucine conformers could be built
into these electron density maps (see Supplementary
Material).
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The above figures are
reprinted
by permission from Elsevier:
J Mol Biol
(2004,
341,
565-574)
copyright 2004.
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Figures were
selected
by an automated process.
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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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D.G.Isom,
C.A.Castañeda,
B.R.Cannon,
P.D.Velu,
and
B.García-Moreno E
(2010).
Charges in the hydrophobic interior of proteins.
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Proc Natl Acad Sci U S A,
107,
16096-16100.
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A.Damjanović,
X.Wu,
B.García-Moreno E,
and
B.R.Brooks
(2008).
Backbone relaxation coupled to the ionization of internal groups in proteins: a self-guided Langevin dynamics study.
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Biophys J,
95,
4091-4101.
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D.G.Isom,
B.R.Cannon,
C.A.Castañeda,
A.Robinson,
and
B.García-Moreno
(2008).
High tolerance for ionizable residues in the hydrophobic interior of proteins.
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Proc Natl Acad Sci U S A,
105,
17784-17788.
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J.L.Schlessman,
C.Abe,
A.Gittis,
D.A.Karp,
M.A.Dolan,
and
B.García-Moreno E
(2008).
Crystallographic study of hydration of an internal cavity in engineered proteins with buried polar or ionizable groups.
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Biophys J,
94,
3208-3216.
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PDB codes:
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M.J.Harms,
J.L.Schlessman,
M.S.Chimenti,
G.R.Sue,
A.Damjanović,
and
B.García-Moreno
(2008).
A buried lysine that titrates with a normal pKa: role of conformational flexibility at the protein-water interface as a determinant of pKa values.
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Protein Sci,
17,
833-845.
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PDB code:
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A.Damjanović,
J.L.Schlessman,
C.A.Fitch,
A.E.García,
and
B.García-Moreno E
(2007).
Role of flexibility and polarity as determinants of the hydration of internal cavities and pockets in proteins.
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Biophys J,
93,
2791-2804.
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D.A.Karp,
A.G.Gittis,
M.R.Stahley,
C.A.Fitch,
W.E.Stites,
and
B.García-Moreno E
(2007).
High apparent dielectric constant inside a protein reflects structural reorganization coupled to the ionization of an internal Asp.
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Biophys J,
92,
2041-2053.
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PDB code:
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D.A.Kraut,
P.A.Sigala,
B.Pybus,
C.W.Liu,
D.Ringe,
G.A.Petsko,
and
D.Herschlag
(2006).
Testing electrostatic complementarity in enzyme catalysis: hydrogen bonding in the ketosteroid isomerase oxyanion hole.
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PLoS Biol,
4,
e99.
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PDB codes:
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S.L.Flaugh,
I.A.Mills,
and
J.King
(2006).
Glutamine deamidation destabilizes human gammaD-crystallin and lowers the kinetic barrier to unfolding.
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J Biol Chem,
281,
30782-30793.
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A.Damjanović,
B.García-Moreno,
E.E.Lattman,
and
A.E.García
(2005).
Molecular dynamics study of water penetration in staphylococcal nuclease.
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Proteins,
60,
433-449.
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L.Cruzeiro
(2005).
Influence of the nonlinearity and dipole strength on the amide I band of protein alpha-helices.
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J Chem Phys,
123,
234909.
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V.P.Denisov,
J.L.Schlessman,
B.García-Moreno E,
and
B.Halle
(2004).
Stabilization of internal charges in a protein: water penetration or conformational change?
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Biophys J,
87,
3982-3994.
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PDB code:
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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.
Where a reference describes a PDB structure, the PDB
codes are
shown on the right.
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Links
