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213 a.a.
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213 a.a.
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251 a.a.
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* Residue conservation analysis
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PDB id:
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Immune system
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Title:
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Lyme disease antigen ospa in complex with neutralizing antibody fab la-2
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Structure:
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Hybridoma antibody la2 (light chain). Chain: a, c. Fragment: fab fragment. Synonym: la2 fab. Hybridoma antibody la2 (heavy chain). Chain: b, d. Fragment: fab fragment. Synonym: la2 fab. Outer surface protein a.
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Source:
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Mus musculus. House mouse. Organism_taxid: 10090. Other_details: la-2 hybridoma, gift of m.M. Simon, max planck instutut, freiburg. Other_details: la-2 hybridoma. Borrelia burgdorferi. Organism_taxid: 224326. Strain: b31.
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Biol. unit:
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Trimer (from
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Resolution:
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2.68Å
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R-factor:
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0.226
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R-free:
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0.281
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Authors:
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W.Ding,C.L.Lawson
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Key ref:
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W.Ding
et al.
(2000).
Structural identification of a key protective B-cell epitope in Lyme disease antigen OspA.
J Mol Biol,
302,
1153-1164.
PubMed id:
DOI:
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Date:
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07-Aug-00
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Release date:
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11-Oct-00
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Supersedes:
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PROCHECK
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Headers
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References
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P01837
(IGKC_MOUSE) -
Immunoglobulin kappa constant from Mus musculus
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Seq:
Struc:
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107 a.a.
213 a.a.
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DOI no:
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J Mol Biol
302:1153-1164
(2000)
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PubMed id:
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Structural identification of a key protective B-cell epitope in Lyme disease antigen OspA.
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W.Ding,
X.Huang,
X.Yang,
J.J.Dunn,
B.J.Luft,
S.Koide,
C.L.Lawson.
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ABSTRACT
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Outer surface protein A (OspA) is a major lipoprotein of the Borrelia
burgdorferi spirochete, the causative agent of Lyme disease. Vaccination with
OspA generates an immune response that can prevent bacterial transmission to a
mammalian host during the attachment of an infected tick. However, the
protective capacity of immune sera cannot be predicted by measuring total
anti-OspA antibody. The murine monoclonal antibody LA-2 defines an important
protective B-cell epitope of OspA against which protective sera have strong
levels of reactivity. We have now mapped the LA-2 epitope of OspA using both NMR
chemical-shift perturbation measurements in solution and X-ray crystal structure
determination. LA-2 recognizes the three surface-exposed loops of the C-terminal
domain of OspA that are on the tip of the elongated molecule most distant from
the lipid-modified N terminus. The structure suggests that the natural variation
at OspA sequence position 208 in the first loop is a major limiting factor for
antibody cross-reactivity between different Lyme disease-causing Borrelia
strains. The unusual Fab-dominated lattice of the crystal also permits a rare
view of antigen flexibility within an antigen:antibody complex. These results
provide a rationale for improvements in OspA-based vaccines and suggest possible
designs for more direct tests of antibody protective levels in vaccinated
individuals.
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Selected figure(s)
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Figure 3.
Figure 3. Structural comparison of NMR and crystallographic
LA-2 epitope maps. (a) Schematic of OspA. The view is nearly
"end-on", with the C-terminal domain of the molecule in the
foreground. The polypeptide backbone is shown as a worm tube
with labeled N and C-terminal ends. The three contiguous regions
recognized by LA-2 are identified by blue, green, and magenta
shading, respectively, and labeled by loop number as defined in
the main text. The positions of Ala208 and Ala215 are indicated
by red C^a-C^b bonds. Strictly conserved Trp216 on b-strand 17
is shown in cyan for reference. (b) By-residue
NMR-chemical-shift perturbation data mapped onto the OspA
structure, with non-hydrogen atoms shown as spheres (color
scheme as in Figure 2). (c) Crystallographic identification of
the LA-2 epitope. OspA atoms are shaded using a color gradient
by their minimum distance from LA-2 atoms. Red, <3.5 Å;
orange-bright yellow, 3.5-7.0 Å; yellow-faint yellow,
7.0-10 Å; white/gray, >10 Å. In (b) and (c), the C^b
atoms of Ala208 and Ala215 are indicated with asterisks.
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Figure 4.
Figure 4. Schematic of the OspA/LA-2 Fab complex crystal
lattice. The view is perpendicular to the crystallographic
a-axis, and a one unit cell thick slice is shown. The b and c
lattice repeats are indicated. The two LA-2 Fab dimers in the
crystal asymmetric unit are indicated in light and dark gray,
respectively. Two OspA/Fab complexes that define a single
crystal asymmetric unit are shown in a thick trace. These two
OspA molecules are shaded according to refined C^a-atom B-value
(blue, B < 35 Å2; red, B > 65 Å2). This view
highlights the alternating dense and sparsely packed molecular
layers along the c-axis, corresponding to LA-2 Fab (gray) and
OspA (green) layers, respectively. The 80 Å long OspA
molecules are strongly anchored at their C-terminal tips to the
Fab antigen combining sites, but they extend into the sparse
layer where they are nearly entirely surrounded by solvent. Only
one of the two OspAs in the asymmetric unit (lower OspA in this
view) makes a weak bridging lattice contact with its N-terminal
domain to the adjoining Fab layer, consisting of two salt
bridges between flexible side-chains. These weak lattice
contacts and corresponding thin-plate crystal morphology
resulted in poor diffraction along the c*-axis.
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The above figures are
reprinted
by permission from Elsevier:
J Mol Biol
(2000,
302,
1153-1164)
copyright 2000.
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Figures were
selected
by the author.
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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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I.Livey,
M.O'Rourke,
A.Traweger,
H.Savidis-Dacho,
B.A.Crowe,
P.N.Barrett,
X.Yang,
J.J.Dunn,
and
B.J.Luft
(2011).
A new approach to a lyme disease vaccine.
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Clin Infect Dis,
52,
s266-s270.
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A.Walker,
C.Skamel,
J.Vorreiter,
and
M.Nassal
(2008).
Internal core protein cleavage leaves the hepatitis B virus capsid intact and enhances its capacity for surface display of heterologous whole chain proteins.
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J Biol Chem,
283,
33508-33515.
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S.Ghosh,
and
B.T.Huber
(2007).
Clonal diversification in OspA-specific antibodies from peripheral circulation of a chronic Lyme arthritis patient.
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J Immunol Methods,
321,
121-134.
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C.L.Lawson,
B.H.Yung,
A.G.Barbour,
and
W.R.Zückert
(2006).
Crystal structure of neurotropism-associated variable surface protein 1 (Vsp1) of Borrelia turicatae.
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J Bacteriol,
188,
4522-4530.
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PDB codes:
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K.Makabe,
V.Tereshko,
G.Gawlak,
S.Yan,
and
S.Koide
(2006).
Atomic-resolution crystal structure of Borrelia burgdorferi outer surface protein A via surface engineering.
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Protein Sci,
15,
1907-1914.
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PDB code:
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X.Yang,
Y.Li,
J.J.Dunn,
and
B.J.Luft
(2006).
Characterization of a unique borreliacidal epitope on the outer surface protein C of Borrelia burgdorferi.
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FEMS Immunol Med Microbiol,
48,
64-74.
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J.M.Jacobs,
X.Yang,
B.J.Luft,
J.J.Dunn,
D.G.Camp,
and
R.D.Smith
(2005).
Proteomic analysis of Lyme disease: global protein comparison of three strains of Borrelia burgdorferi.
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Proteomics,
5,
1446-1453.
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M.Becker,
J.Bunikis,
B.D.Lade,
J.J.Dunn,
A.G.Barbour,
and
C.L.Lawson
(2005).
Structural investigation of Borrelia burgdorferi OspB, a bactericidal Fab target.
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J Biol Chem,
280,
17363-17370.
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PDB codes:
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M.Jäger,
X.Michalet,
and
S.Weiss
(2005).
Protein-protein interactions as a tool for site-specific labeling of proteins.
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Protein Sci,
14,
2059-2068.
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M.Nassal,
C.Skamel,
P.A.Kratz,
R.Wallich,
T.Stehle,
and
M.M.Simon
(2005).
A fusion product of the complete Borrelia burgdorferi outer surface protein A (OspA) and the hepatitis B virus capsid protein is highly immunogenic and induces protective immunity similar to that seen with an effective lipidated OspA vaccine formula.
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Eur J Immunol,
35,
655-665.
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T.J.Templeton
(2004).
Borrelia outer membrane surface proteins and transmission through the tick.
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J Exp Med,
199,
603-606.
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K.P.Wu,
C.W.Wu,
Y.P.Tsao,
T.W.Kuo,
Y.C.Lou,
C.W.Lin,
S.C.Wu,
and
J.W.Cheng
(2003).
Structural basis of a flavivirus recognized by its neutralizing antibody: solution structure of the domain III of the Japanese encephalitis virus envelope protein.
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J Biol Chem,
278,
46007-46013.
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PDB code:
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S.J.Landry
(2003).
Structure and energetics of an allele-specific genetic interaction between dnaJ and dnaK: correlation of nuclear magnetic resonance chemical shift perturbations in the J-domain of Hsp40/DnaJ with binding affinity for the ATPase domain of Hsp70/DnaK.
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Biochemistry,
42,
4926-4936.
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B.J.Luft,
J.J.Dunn,
and
C.L.Lawson
(2002).
Approaches toward the directed design of a vaccine against Borrelia burgdorferi.
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J Infect Dis,
185,
S46-S51.
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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
