NMR an introduction

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NMR an introduction

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Title: NMR an introduction

1
NMRan introduction

by
Burcu Kaplan

2
Kurt Wüthrich
3
The Nobel Prize in Chemistry 2002

"for his development of nuclear magnetic
resonance spectroscopy for determining the
three-dimensional structure of biological
macromolecules in solution"

4
NOBEL

Through his work at the beginning of the 1980s
Kurt Wüthrich has made it possible to use NMR on
proteins. He developed a general method of
systematically assigning certain fixed points in
the protein molecule, and also a principle for
determining the distances between these. Using
the distances, he was able to calculate the
three-dimensional structure of the protein. The
advantage of NMR is that proteins can be studied
in solution, i.e. an environment similar to that
in the living cell.

5
NOVEL

1-the nuclear overhauser effect (NOE) as an
experimentally accessible NMR parameter in
proteins that can yield the information needed
for de novo global fold determination of a
polymer chain
2-sequence-specific assignment of the many
hundred to several thousand NMR peaks from a
protein
3-computational tools for the structural
interpretation of the NMR data and the evaluation
of the resulting molecular structures.
4-multidimensional NMR techniques for efficient
data collection.

6
Protein NMR

In the NMR experiments, solution conditions such
as the temperature, pH and salt concentration can
be adjusted so as to closely mimic a given
physiological fluid.
Solutions may also be changed to quite extreme
non-physiological conditions, for example, for
studies of protein denaturation.
investigations of dynamic features of the
molecular structures
structural, thermodynamic and kinetic aspects of
interactions between proteins and other solution
components other macromolecules or low molecular
weight ligands

7
1965 postdoctoral trainingUniversity of
California, Berkeley

used NMR spin relaxation measurements of 17O, 2H
and 1H in addition to EPR for studies of the
hydration of metal ions and metal complexes

8
(No Transcript)
9
1967 Bell Telephone Laboratories

important qualitative NMR features of amino acids
and proteins had already been noted and
tentatively rationalized by 1967
the maintenance of what was one of the first
super conducting high resolution NMR
spectrometers, which operated at a proton
resonance frequency of 220 MHz.
hemoproteinsblood sampled from my arm
with the limited sensitivity and spectral
resolution of the instrumentation available in
1968, the special spectral properties of
hemoproteins were a great asset for successful
NMR applications

10
1976 ETH Zürich

identification of the nuclear Overhauser effect
(NOE) as a NMR parameter that can be related in
an unambiguous way to three-dimensional
macromolecular structures
NOE gives crosspeaks between resonances from
protons close in space inter-atomic distances

11
NOE

NOE had a key role in the approach used for
obtaining sequence-specific assignments of the
many hundred to several thousand NMR lines in a
protein.
NOE are due to dipolar interactions between
different nuclei. The intensity of the NOE is
related to the product of the inverse sixth power
of the internuclear distance
A 1 H1 H NOE is related to the through-space
distance between a pair of atoms that are either
not at all linked by covalent bonds
(intermolecular NOE), or that may be far apart in
the amino acid sequence of a polypeptide chain.

12
2D NMR

In 1977 the first 2D NMR spectrum of a protein
was recorded
Kumar, A., Ernst, R.R., and Wüthrich, K. (1980).
A two-dimensional nuclear Overhauser enhancement
(2D NOE) experiment for the elucidation of
complete proton-proton cross-relaxation networks
in biological macromolecules. Biochem. Biophys.
Res. Commun. 95, 16.

13
Contour Plot of a Proton Two-Dimensional NOESY
Spectrum of Basic Pancreatic Trypsin Inhibitor
Recorded at 360 MHz
14
2D NMR

2D 1 H NMR enables the recording of selective
interactions between pairs of hydrogen atoms, or
groups of chemical shift-equivalent hydrogen
atoms, without selective irradiation of
individual resonance lines.
The dispersion of the resonances in a
two-dimensional frequency plane affords greatly
improved separation of the individual peaks.

15
1980

four 2D NMR experiments were conducted that were
then used for the initial protein structure
determinations
COSY (2D correlated spectroscopy),
SECSY (2D spin-echo correlated spectroscopy),
FOCSY (2D foldover-corrected correlated
spectroscopy)
NOESY (2D nuclear Overhauser enhancement
spectroscopy)

16
1982

complete sequence-specific assignments BPTI(basic
pancreatic trypsin inhibitor)
Wagner,G.and Wüthrich,K.Sequential resonance
assignments in protein 1 H nuclear magnetic
resonance spectrabasic pancreatic trypsin
inhibitor.J.Mol.Biol.155 (1982) 347-366.
the polypeptide hormone glucagon bound to
lipid micelles
Wider,G.,Lee,K.H.and Wüthrich,K.Sequential
resonance assignments in protein 1 H nuclear
magnetic resonance spectraglucagon bound to
perdeuterated dodecylphosphocholine
micelles.J.Mol.Biol.155 (1982)367-388.

17
Complete sequence-specific resonance assignments
for BPTI obtained using 2D NMR experiments.
Assigned residues are identified by coloured
patches covering their amide protons.(The colour
code indicates variable amide proton exchange
rates
18
Kinetics of protein folding

Systematic investigation of hydrogen-exchange
dynamics as a function of pH value, temperature
and concentration of denaturants with atomic
resolution.
K.Wüthrich,G.Wagner, NMR investigations of the
dynamics of the aromatic amino acid residues in
the basic pancreatic trypsin inhibitor FEBS
Lett.1975,50 ,265 -268.
G.Wagner,K.Wüthrich, Correlation between the
amide proton exchange rates and the denaturation
temperatures in globular proteins related to the
basic pancreatic trypsin inhibitor,J.Mol.Biol
.1979 ,130 , 31 -37.
H.Roder,G.Wagner,K.Wüthrich, Amide proton
exchange in proteins by EX1 kineticsstudies of
the basic pancreatic trypsin inhibitor at
variable pH and temperature,Biochemistry 1985
,24 ,7396 7407
H.Roder,G. Wagner,K.Wüthrich, Individual amide
proton exchange rates in thermally unfolded basic
pancreatic trypsin inhibitor,Biochemistry
1985,24,7407 7411
H.Roder,K.Wüthrich Protein folding kinetics by
combined use of rapid mixing techniques and NMR
observation of individual amide protons,
Proteins 1986 ,1 ,34-42.

19
1985 BUSI

first NMR structure determination of a globular
protein, bull seminal protease inhibitor (BUSI)
but.....

20
2D 1H,1H-NOE spectroscopy (1 H,1 H-NOESY). A
stacked plot representation of a spectrum of the
small protein bullseminal proteinase
inhibitorIIA) is shown (500 MHz, 45C,
H2O-solution).
21
two more years of intense work....

Many structural constraints,mainly long-range NOE
observations,were recorded and a mathematical
method based on metric matrix distance geometry
was used to calculate the three-dimensional
structure for the protein based on these
constraints by implementation in efficient
software packages

22
1985 BUSI
Williamson,M.P.,Havel,T.F.,and Wüthrich,K.Solution
conformation of proteinase inhibitor IIA from
bull seminal plasma by 1 H nuclear magnetic
resonance and distance geometry.J.Mol.Biol.182
(1985)295-315.
23
After BUSI

When I presented the structure of BUSI in some
lectures in the spring of 1984, the reaction was
one of disbelief and suggestions that our
structure must have been modeled after the
crystal structure of a homologous protein,PSTI

24
independently solving a new protein structure

amylase inhibitor Tendamistat
Professor Robert Huber (Nobel laureate in
Chemistry, 1988) by X-ray crystallography
Kurt Wüthrich by NMR

25
Suprise...

Almost identical three-dimensional structures in
terms of the global fold of the polypeptide chain
were demonstrated in accompanying publications
Kline,A.D.,Braun,W.and Wüthrich,K.Studies by 1 H
nuclear magnetic resonance and distance geometry
of the solution conformation of the á -amylase
inhibitor Tendamistat. J.Mol.Biol.189
(1986)377-382.
Pflugrath,J.,Wiegand,E.Huber,R.and
Vertesy,L.Crystal structure determination,refineme
nt and the molecular model of the á -amylase
inhibitor Hoe-467A.
J.Mol.Biol.189 (1986)383-386.

26
Tendamistat

in the interior of the protein the two structures
are nearly identical
Local differences on the surface of the protein
The solution structure appeared more disordered
than the crystal structure
Tyrosine 14 was not observed in the X-ray
diffraction.

27
A)Family of structures of tendamistat, an
amylase inhibitor determined by NMR
spectroscopyB)ribbon diagram of the structure
with lowest energy.
28
1985

subsequently solved NMR structure of rabbit
metallothionein was completely different from an
independently solved rat metallothionein crystal
structure
different polypeptide folds
different coordinating ligands to metals
Nature rejected NMR structure article

29
1992

crystal structure of rat metallothionein was
re-determined and the correct crystal structure
was found to be identical with the NMR structure
of the rabbit, rat and human metallothioneins
that Wüthrich solved from 1985 to 1990
it took six years before the crystal structure
was redetermined and found to coincide with the
NMR structure!

30
today

3 D 4 D NMR
Isotope labelling of the molecules with the
NMR-active nuclei 15 N and 13 C led to the
development of heteronuclear three-dimensional
NMR
Heteronuclear relaxation provides the basis for
NMR studies of molecular dynamics in a
macromolecule,showing that the parts of a
molecule that appear disordered in a structure
determination are often associated with high
mobility.
Protein folding

31
Size limitation ?

Recently reported structures represent molecular
weights up to the order of megaDa in extreme
cases.Compared to these large single-crystal
structures,NMR solution structures generally
concern smaller molecules, typically below 30
kDa,and they are often less precise.
With TROSY and CRINEPT techniques it is now
possible to assign resonances and study a protein
assembly as large as 900 kDa,as shown in the
recent study of the molecular chaperone
GroEL-GroES complex
Pervushin,K.,Riek,R.,Wider,G.and
Wüthrich,K.Attenuated T 2 relaxation by mutual
cancellation of dipole-dipole coupling and
chemical shift anisotropy indicates an avenue to
NMR structures of very large biological
macromolecules in solution.Proc.Natl.Acad.
Sci.USA 94 (1997)12366-12371.
Riek,R.,Wider,G.,Pervushin,K.and
Wüthrich,K.Polarization transfer by
cross-correlated relaxation in solution NMR with
very large molecules.Proc.Natl.Acad.Sci.USA 96
(1999)4918-4923.
Fiaux,J.,Bertelsen,E.B.,Horwich,A.L.and
Wüthrich,K.NMR analysis of a 900K GroEL-GroES
complex.Nature 418 (2002)207-211.

32
TROSY

Complete cancellation of transverse relaxation
effects
for amide sites in a very large protein,in which
all hydrogen atoms but the exchangeable ones such
as the amide hydrogen have been replaced with
deuterium,the effect of cross-correlated
relaxation of different relaxation mechanisms
such as NH dipole -dipole relaxation and N
chemical shift anisotropy leads to enhanced
relaxation for the downfield component of the H N
doublet,while for the upfield component,the two
relaxation processes can mutually cancel.Since
the chemical shift anisotropy is field dependent
and the dipole dipole relaxation is field
independent for large molecules,the two effects
will mutually cancel at a magnetic field of
approximately 950 MHz

33
NMR in PDB

20 of the 14 000 structures
Wüthrichs group contributed with more than 50

34
Prion Protein

PrPc benign cellular form
predominantly expressed in neuronal tissue
transmissible spongiform encephalopathies (TSEs)
are a group of fatal neurodegenerative diseases,
which include Creutzfeldt-Jakob disease (CJD) in
humans and bovine spongiform encephalopathy (BSE)
in cattle

35
Prion protein

A structure determination for the C-terminal half
of the mouse prion protein in April 1996, barely
10 days after the BSE-crisis in Great Britain
broke into the open.
In 1997 characterization the structure of the
intact prion protein showing that the N-terminal
half of the molecule forms a highly flexible,
extended "tail". The prion protein thus presented
a striking illustration of the unique power of
NMR to characterize partially structured
polypeptide chains.
the three-dimensional structure of the benign
cellular form (PrP C ) includes a flexibly
disordered 100-residue tail linked to the
N-terminal end of a globular domain .

36
Partially folded polypeptide chains

difficult to crystallize
the chain segments that are disordered in
solution will either be ordered by intermolecular
contacts in the crystal lattice, or they will not
be visible by diffraction methods.

37
NMR structure of the recombinant murine prion
protein
First the well-ordered structure of a fragment
comprising the C-terminal residues 121-231 was
determined.Then the intact protein 23-231 was
studied and it was found that the N-terminal
23-126 segment formed an extended,highly flexible
coil with high mobility.
38
NMR structure of the bovine prion protein. In
the C-terminal globular domain of residues
126230, -helices are green, an antiparallel
sheet is blue, and non-regular secondary
structure is yellow the unstructured
N-terminal tail of residues 23125 is white.
39
NMR

static picture of the unstructured chain
segments
additional NMR experiments can provide
information on the frequencies of the rate
processes that mediate transitions between
discrete states of the molecule within the
conformation space spanned by the static bundle
of NMR-conformers
Wüthrich, K. (1995) Acta Cryst. D 51,
249270. NMRthis other method for protein and
nucleic acid structure determination.

40
Visual impression of the variation of the bovine
prion protein structure during a time period of
about 1 nanosecond. The superposition of 20
snapshots illustrates that the globular domain
maintains its mean geometry, whereas the tail
undergoes large-scale changes with time.
41
PRION

Considering that the mechanism of transformation
of PrP C into the aggregated, disease-related
form, PrPSc, of mammalian prion proteins is
still subject to speculation, the observation of
this flexible tail has been highly intriguing.

42
Prion

Riek, R., Hornemann, S., Wider, G., Billeter, M.,
Glockshuber,R., and Wüthrich, K. (1996). NMR
structure of the mouse prion protein domain
PrP(121231). Nature 382, 180182.
Riek,R.,Hornemann,S.,Wider,G.,Glockshuber,R.and
Wüthrich,K. (1997) NMR characterization of the
full-length recombinant murine prion protein
mPrP(23-231).FEBS Lett.413 282-288.
Zahn, R., Liu, A., Lührs, T., Riek, R., von
Schroetter,C., Lopez Garcia, F. et al. (2000).
NMR solution structure of the human prion
protein. Proc. Natl Acad. Sci. USA, 97, 145150.
Lopez Garcia, F., Zahn, R., Riek, R. and
Wüthrich, K. (2000) NMR structure of the bovine
prion protein Proc. Natl. Acad. Sci. USA 97,
83348399

43
Thorsten Lührs, Roland Riek, Peter Güntert and
Kurt Wüthrich
NMR Structure of the Human Doppel Protein
J. Mol. Biol. (2003) 326, 15491557
44
Prion Protein

PrPc knockout mice is not susceptible to prion
infection
Reintroduction restores susceptibility
Büeler, H., Aguzzi, A., Sailer, A., Greiner, R.
A.,Autenried, P., Aguet, M. et al. (1993). Mice
devoid of PrP are resistant to scrapie. Cell, 73,
13391347.
Fischer, M., Rülicke, T., Raeber, A., Sailer, A.,
Moser, M., Oesch, B. et al. (1996). Prion protein
(PrP) with amino-proximal deletions restoring
susceptibility of PrP knockout mice to scrapie.
EMBO J. 15, 12551264.
Flechsig, E., Shmerling, D., Hegyi, I., Raeber,
A. J., Fischer, M., Cozzio, A. et al. (2000).
Prion protein devoid of the octapeptide repeat
region restores susceptibility to scrapie in PrP
knockout mice. Neuron,27, 399408. USA, 98,
23522357.

45
Doppel Protein

Knockout strains with no resistance
Knockout strains developing signs of ataxia
within 70 weeks after birth
discovery of a novel gene locus (Prnd) 16 kb
downstream of Prnp and its product, the doppel
protein (Dpl).
Moore, R. C., Lee, I. Y., Silverman, G. L.,
Harrison, P. M., Strome, R., Heinrich,C. et al.
(1999). Ataxia in prion protein (PrP)-deficient
mice is associated with upregulation of the novel
PrP-like protein doppel.
J. Mol. Biol. 292, 797817.

46
Dpl disease?

An involvement of Dpl in prion diseases or a role
in neural differentiation is unlikely.
Behrens, A., Brandner, S., Genoud, N.
Aguzzi, A. (2001). Normal neurogenesis and
scrapie pathogenesis in neural grafts lacking the
prion protein homologue Doppel. EMBO Rep. 2,
347352.
Thus two distinct neurological diseases,
simultaneously with overexpression of two
distinct proteins, seem to be cured by benign
cellular form of prion protein.

47
Rationale

sequence identity between Dpl and PrP is only
about 20, so that experimental determination of
Dpl 3D-structure is a significant addition to the
data available as a foundation for functional
studies of these proteins.

48
MM

PCR from Prnd, Dpl coding region
Cloning in E.coli pRSETA
17 residue N-terminal histidine tail
Engineered thrombin cleavage site
DNA sequencing
N-terminal Edman sequencing
MALDI-TOF mass spectrometry

49
MM

Expression
incubation of soluble protein fraction with
Ni-NTA agarose
Refolding of protein using a linear gradient of
0100 (v/v) of buffer B (100 mM NaPi, 10 mM Tris
(pH 8.0), 10 mM imidazole).
The refolded hDpl(24152) was then eluted with
buffer B containing 500 mM imidazole.

50
MM

N-terminal histidine tail cleavage
Separation of cleavage products by
cation-exchange chromatography, CM52-cellulose
Dialysis
Lyophilized/ fresh solution purified protein

51
NMR spectroscopy

1.3 mM solution of uniformly 13 C 15 N-labelled
protein in 95 (v/v) H2O,
5 (v/v) 2H2O
for sequence-specific polypeptide backbone
assignments TOCSY
for the collection of conformational
constraints,three 3D NOESY-experiments
1.9 mM solution of unlabeled protein in 100 2H2O
for 2D NOESY

52
NOESY ( 750 MHz)

3D 15N/13C-resolved 1H,1H-NOESY H2O
3D 13C-resolved 1H,1H-NOESY in D2O
3D 13C-resolved 1H,1H-NOESY in D2O
2D 1H,1H-NOESY in D2O

53
15N,1H-correlated spectroscopy (COSY)

Resonance doubling for some residues
SDS-PAGE MALDI-TOF 95 homogenous
Oxidation states of the 4 Cysteine residues
2 disulfide bridges
Resonance doublings seen for protein fragment
hDpl(52152), globular domain

54
Chemical shift assignments

incomplete assignments
backbone amide protons of Y91, K143, C145 and
F147,
all side-chain protons of R32, K34 and K143
H? of R27,
H? 1 of H31
H? of P86
H? of D87
H? of I89
H? of C145
H? of F147
Proline trans conformation 13 C? 32 ppm

55
CSA

For doubled peaks separated by less than 0.02 ppm
in the 1 H-dimension and/or less than 0.1 ppm in
the 15 N or 13 C dimension of the
heteronuclear-resolved 3D 1H,1H-NOESY spectra
,only one chemical shift in each dimension was
assigned and the sum of the peak intensities was
used.

56
(No Transcript)
57
CSA

2. For doubled resonances separated by more
than these limits, the more intense peak was
arbitrarily added to the input, with an intensity
corresponding to the sum of the intensities of
the two peaks.

58
CSA

Computational...
Peak lists of the four NOESY spectra were
generated by interactive peak picking with the
program XEASY and automatic integration of the
peak volumes with the program SPSCAN
Automated combined NOE cross peak assignment and
three-dimensional protein structure determination
was obtained using the programs CANDID and DYANA

59
Input for the structure calculation of hDpl(24
152) and characterization of the energy-minimized
NMR structure of the globular domain 52152
60
3-D structure human doppel protein,
61
(No Transcript)
62
3-D structure human doppel protein,
63
Beta sheet

anti-parallel ?-sheet comprising residues 5860
(?1) and 8890 (?2)
was identified on the basis of strong H ?
(F59)H?(I89), H? (G88) HN (I89) and H? (A58)
HN(F59) NOEs
with the inter-strand hydrogen bonds HN
(H90)O(A58) and HN (I60) O(G88) implicated
by the atom coordinates of the energy-refined
structure.

64
Bundle of 20 energy-minimized conformers with the
lowest DYANA target functions of the polypeptide
segment 52149 of hDpl(24152) obtained by
super-position of the N, C? and C atoms of the
residues 5290, 101121 and 126141 for best fit.
The backbone (cyan), and the two disulfide
bridges (yellow) are displayed.
65
Packing of amino acid side-chains in the core of
hDpl(24152).The residues shown originate from
loops preceding and following helix a1 (magenta),
helix a1 (green), helix a3 (orange) and backbone
is shown in cyan.
66
Environment of the residue F59, shown in green,
formed by residues in the helices ?2 and ?3
(orange), and in the first ? -strand and the
preceding loop (magenta).
67
C-terminal
68
disulfide bond in C-terminal
69
hDpl(24152) (red) vs mDpl(26155) (white)
Regular secondary structure elements are
indicated next to the ribbons, the chain ends are
indicated by sequence numbers. The disulfide
bridge homologous to that in the prion protein is
shown in yellow ,rmsd 1.8 A
70
Tentative alignment

CirclesN-glycosylation sites
Dots conserverd a.a.
Hyphen deletions
pairwise amino acid identities between hDpl/mDpl,
hDpl/hPrP and mDpl/hPrP are 79, 20 and 20,
respectively

71
hDpl vs mDpl

22 Amino acid substitutions
9 on the surface of the molecule none appear to
be involved in long-range or medium-range
interactions with other segments of the
polypeptide chain, so that they are unlikely to
contribute significantly to structural
differences between the two proteins.

72
helix ?2 b and the loop connecting ?2b with ?3
nine differences G118A, Q121S, K122R, P123E,
D124K, N125Q and K126D, and a dipeptide insertion
following position 126 in the hDpl amino acid
sequence. Interestingly, although four variations
of the amino acid sequence near helix ?2 b
involve charged residues, the net local charge of
the segment 117127 (hDpl numeration) is
invariant between the two proteins.
73
Core substitutions

I109V and V136I strictly preserve the hydrophobic
core packing
F104L and L139A could relate to the structural
differences between the two proteins at the start
of helix ? 2a

74
hDpl (red) vs hPrP (white)
rmsd 2.5 A
75
Conserved residues

I68 (I139 in hPrP), F70 (F141), Y77 (Y149) and
Y78 (Y150)
G71 (G142)
N81 (N153)
P86(P158)
Y91 (Y163)
F104 (F175), V105 (V176) and C108 (C179)

76
H-bond

The side-chain of T112 (T183) in ?2 forms a
long-range hydrogen bond to the ?-sheet
in hDpl this interaction involves the hydroxyl
proton of T112 and O of G57 on strand ?1
in hPrP it involves the hydroxyl oxygen atom of
T183 and HN of Y162 on strand ?2.
This switch in donor/acceptor function is
reflected in largely different ?1 angles of this
Thr residue, which is virtually
solvent-inaccessible in both hDpl and hPrP.
In hPrP, this core hydrogen bond has been shown
to contribute significantly to the thermodynamic
stability of PrP, and it probably has a similar
role in Dpl.

77
A cartoon of glycosylated,GPI-anchored hPrP and
hDpl. ? -helices are red and yellow, ? -strands
are cyan, and the segments with non-regular
secondary structure within the C-terminal domain
are gray. The GPI anchor and the glycan moieties
are black, and the disulfide bridges are green.
conserved glycosylation site
78
significant differences

the ?1-strand and the sequentially adjacent
residues show a displacement of corresponding
C?atom coordinates of approximately 8 A . The
?-sheet is shifted by two residues towards helix
?1, resulting in a significant rearrangement of
the loop connecting ?1 and ?1 with respect to
helix ?3, while leaving the position of the loop
connecting ?1 and ?2 virtually unaffected.
different packing of the side-chains in this
molecular region, where residue F59 of the
?1-strand in hDpl is part of the hydrophobic core
The C-terminal polypeptide segments of hPrP and
hDpl have a low level of sequence conservation
and different 3D structures. While in hPrP the
helix ?3 proceeds almost to the C terminus, the
helix ?3 of Dpl terminates after C140 in the
common disulfide bond.
The peptide segment between the end of ?3 and the
chain end of hDpl has a non-regular secondary
structure and is folded against the loop
connecting ?2 with ?2,giving the hDpl molecule an
overall more contracted appearance when compared
with hPrP.
the additional disulfide bond C94C145 in hDpl
would be sterically incompatible with a regular
a-helix structure beyond about residue 142.

79
hydrophobic cleft
Negative charges are shown in red, positive
charges in blue, and residues belonging to the
hydrophobic core and other hydrophobic
side-chains are shown in yellow.The charged
residues are identified by the one-lettersymbols
and the sequence numbers.
80
TSE

In the pathology of TSEs the refolding of PrPc
to PrPsc appears to be a central event.
Substitutions of the residues D178, V180, T183,
R208, V210, E211 and Q212 in hPrP, which
correspond to G107,I109, T112, R134, V136, Q137
and E138 in hDpl have been identified as genetic
mutations that relate to increased probability to
develop familial forms of TSE.
Three of these residues are conserved in the
sequences of hDpl and hPrP, i.e. T112 (T183),
R134 (R208) and V136 (V210), and are found in
corresponding locations in the 3D structure

81
hPrP
Taken from Kurt Wüthrich, NMR solution
structure of the human prion protein PNAS ,
2000, 97(1), 145150
82
Critique?

A Nobel laureate ?
No critique about the techniques used !
Maybe the fact that there was incomplete
assignments too much simplification of NOESY
spectrum
But results, I believe , will not much
contribute to prion disease research directly
Further functional studies with hDpl,can be a
good feedback to determine the function of hPrP
One should be a genius or crazy to try to deal
with such a complex data generated by NMR!
Still....

83
GOD BLESS Kurt Wüthrich
84
REFERENCES

Harald Schwalbe, Kurt Wüthrich,the ETH
Zürich,and the Development of NMR Spectroscopy
for the Investigation of Structure,Dynamics,and
Folding of Proteins ChemBioChem 2003,4,135 142
Karin Markides, Astrid Gräslund , Mass
spectrometry (MS)and nuclear magnetic resonance
(NMR) applied to biological macromolecules
Advanced information on the Nobel Prize in
Chemistry 2002,9 October 2002
Kurt Wüthrich, NMR studies of structure and
function of biological macromolecules , Nobel
Lecture, December 8, 2002
Arthur G. Palmer and Dinshaw J. Patel , Kurt
Wüthrich and NMR of Biological Macromolecules,
Structure, Vol. 10, 16031604, 2002
Kurt Wüthrich, The way to NMR structures of
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