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Conformational structure of the central nervous system proteolipid apoprotein. A Raman and infrared spectroscopic study
43
JoumalofA4olecular Structure,175 (1988) 43-48 Elsevier
Science
Publishers
CONFORMATIONAL
B.V., Amsterdam
STRUCTURE
APOPROTEIN.
A RAMAN
P. CARMONA' 1 Instituto
, J.M.
OF
AND
-Printed
THE
CENTRAL
INFRARED
RAMOS,
M.
de
Optica
(CSIC),
Instituto de 28006 Madrid
Neurob (Spain
ologia
in The Netherlands
NERVOUS
SYSTEM
SPECTROSCOPIC
COZAR
and
Serrano S.R.
STUDY.
J.
MONREAL
121,
28006
Cajal
PROTEOLIPID
Madrid
(CSIC),
(Spain).
Velazquez
144,
ABSTRACT Raman and infrared spectroscopy have been applied to investigate the structure of proteolipid apoprotein, PLA, in the solid state. These techniques reveal the presence of a-helical, B-sheet and unordered structures through the amide A, I, II, III and V bands. A fitting program for resolution of infrared amide I band provided an estimate of the protein secondary structure including 39% a-helix, 36% B-sheet and 25% coil and turns. PLA displays higher content of B and unordered structures than non-delipidated proteolipid PLP which, however, is more rich in a-helical segments. The Raman spectra also reveal the hydrogen-bonding environments of tyrosine residues in this protein. These residues are known from these Raman spectra to be exposed on the protein surface.
INTRODUCTION The of
conformational
prime
importance
architecture
and
membrane
that
proteins
on
cidated.
The
study the
the of
main
intrinsic
proteolipid
core
of
the
cant
interest,
functional
only
reconstituted
membranes
and
of
get
is
(refs. (refs. PLP
0022-2860/88/$03.50 0 1988 Elsevier
3-4)
of has
is
be
60% a
in
of
the
This
protein
into
the
but
also
interactions
is
membrane to
the
model PLP,
is
the in
be
total for that
of
reported
Publishers
on
some
B.V.
the
the is,
study
natural
signifiand of and
l-2). we
elu-
hydrophobic
structural
to
the a
so-called
of
good
form
embedded
insight
the
is
on
Myelin
myelin
about
to
l-2).
emphasizing
Science
influence
influence
myelin up
proteins
of
delipidated
membrane,
protein-protein
papers
myelin
to
myelin
their
The
makes
(PLA)
of
of
function
The
membrane
membranes.
revealed
(refs.
and
of
been
bilayer
lipid-protein
spectra
which
has
apoprotein
not
role
In earlier
fibres. and
proteins.
lipid
point
component
(PLP)
and
intrinsic
biological
nerve
protein
protein
of view
architecture
fraction of
from function
surrounds the
proteolipid protein
structure
vibrational
environment-depend-
44
ent
conformational
information
on
the
high
hydrophobicity
cult
to
ondary are
break
and
in
(refs.
most
of 4-5),
have
not
work
these
is
two
previously
have of
compare
used
which
scarce
to
are
its
diffi-
protein
sec-
spectroscopy vibrational
the
PLA
in
the
solid
state.
the
secondary
characterize
either the
of
is
due
vibrational
infrared
for
PLA
studied
to
techniques,
been
forms
pure
procedure to
There
of
estimates
using we
state
reliable
proteins.
aggregation
protein
this
proteins
and
structure
quantitative
this
In
lipids
strong on
conformational
the
structure
secondary
Data
structure
spectra
of
protein and
up.
non-existent.
Although
aspects
and
Raman
separately
structural
spectra or
study
together, of
PLA.
METHODS Proteolipid matter Lees
protein
according method
to
(ref.
(PLP)
was
a modification
6).
The
concentration
of
n-butanol.
This
was
apoprotein
(PLA)
solution by
Aguilar
ratio
found
was
Infrared
et to
lyophilized
PLA
samples
and
was
drying
9)
for
mine
in
arrangements. shape
for
Raman
and
algorithm
were
using as
the
and
the
are
reported
ferred
to
RESULTS The shows
AND
5145
to
on
i
cm-l.
internal
turns)
a Jobin-Yvon
with
to
(ref. deterof
a Lorentzian
the
amide
Ramanor
spectral
Lyophilized
diameter
used
164
slit
plasma samples
I band.
U-1000
a Spectra-Physics
The
water
polypeptide
of
calibrated
tl
heavy program
percentages
assumes
of
Deuteration
with
was
of
5998
of
fitting
program
line
molar
model
components
source.
frequencies,
mm
the
terms
as
respectively.
Samples
them
and
proteolipid
PLP,
I band
in
at
width
lines were
argon was
from
the
trans-
capillaries.
DISCUSSION
infrared some
recorded
excitation
laser,
amide
(coil of
the
techniques.
A
and
ultrafiltration
and
station.
bands.
PLA
unresolved
the
2 cm-l
0.9-l
of
Folch-Pi
lipid/protein
PLA
white
water-saturated
by
pellet
amide
brain
solubilized
a Perkin-Elmer
KBr
infrared
the
obtain
equilibrating
unordered
original
spectra
laser
by
assign
the
on
bovine
was of
The
for
a data by
structure
The the
spectrometer ion
of
B-sheet
a-helix,
studied out
to
7-8).
by
to
protein/ml
25.0
scanned
carried
secondary
and
were
order
of
a delipidation
(refs.
0.5
5)
protein
employed
assisted were
resolution
the
1 mg
of
al.
be
spectra
spectrophotometer
of
means
from
(ref.
lyophilized
a constant
described
extracted
spectrum
spectral
of
features
proteolipid indicative
apoprotein of
(see
a predominant
Fig.
1)
helical
45
t4000
3500
3000
2500
2000
BOO
1400
1600
1200
1000
600
600
400
200
cm-'
Fig.
1.
Infrared but
structure, tures
are
with
an
cm-l)
dered
and
of
the
a splitting (ref.
be
of
Raman
romporent
range
amide
at
structures,
It
and
PLA. unordered
infrared amide -1 , which cm
either
In
known
and
the and
the
wavenum,bers
and
for
and/or of
the
infrared
a-helix
with -1
be
the
con-
Raman
that
uncr-
distingbished
Raman hand
as
this
) and
spectra.
other
is
consistent
10)
can
Rarran
infrared on
cm
(ref.
arrangements
infrared
five
(1654
struc-
A band is
a-helical
agreement
infrared
is well
backbone
1668
usually
in
appear
PLA at
Other are
1625
and
cated
in
modes
caused
the
can
be
is
these
!n
the
amide there
u-helical
1685
B-structure side
due
2)
case
! fremust
be
ccnfcrmation
of
for
the 1520
usually (ref. the
also
the
of
v(~,o)
11).
and
695
assigned
cm to
Moreover,
infrared
and
amide
another unordered
Raman
polypeptide
infrared
and
shows
B-sheet
in
indicaticns
the
cf
to
located
Typical
cm-I
range
Fig.
types
following.
spectral by
tc
whereas
high-frequency
(see
qualitative
the
respectively,
PLA
frequency
assigned
modes
the
I band of I cmwhich
as this
ccnformations.
on
the
coincident,
about
of
10).
The
ture
of
their
protein
must
3290
arrangement.
polypeptide
account
unordered
near
I modes.
a-helical
b-sheet
the
fact,
powder
the position and intensity -1 cm) suppcrt the existence of
splitting
amide
into
quencies
1654
of
structure,
polypeptide
is
:1659
However, at
predocir,ant clusion
In
located
secondary
forms.
1 band
taking
and
lyophilized
amounts
present.
sharp ordered
B-sheet amide
of
significant
also
relatively
spectrum
spectral chain
secor,dary bands
of
V(O,IT)
-1
amide
I
are
lo-
bands
the
strucB-sheet
amide
II
and
a weak
shoulder
I band
near
1665
V
6
600
800
1000
I
I
1200
I
1400
1600
2800
3000
cm-’ 2.
Y
-1
Raman
indicates
agreement
Raman
to
band
with
the
I band
the
random appears
assigned
resolution
36%
b-sheet
obtained
from
amide
bands
12),
Raman
areas area
protein.
The
the
chains.
larly
infcrmative
concerning
involving
the
gation
Siamwiza
of
is
due
out-of-plane zenes.
If
donor;
the
phenolic et
to
al.
tyrosine
ratio
of
(ref.
13)
850/830
buried, cm-'
III
Raman
of it bands
known
on
is
the of
sum
of
the
f-ccnient
the
spectra
interac-
are
particu-
interactions
and
to
the
doublet the
a strong
about
C.5,
investi-
at
850
overtone
parasubstituted as
unknown
helices.
tyrosine
acts
of
that
total
According
the
were
proteins
that
the
bonding
the
a-helix,
different
a fraction
to the
program
the
the
eleven
basis
vibration
vibration is
of
as
tyrosine.
ring-breathing
ring-bending the
of
that
is well
information The
39%
of
study
with
hydrogen
group
it
fitting
components
question
as
occurs
side
protein
band
amide
percentages
resolved
related
some
of
the
B-strands
provides
in
II!
the
provided
empirical
closely
same
the
These
The
an
also
amide of
absorptivities)
spectroscopy
tions
cm-'
of
equal. on
of is
of
I band
a problem,
suggests
the
is
to a-helix and is consistent -1 component of the amide
amide
area
not
of
result
cm
therefore,
(the
This
application
area
PLA.
component
structures.
could,
I band
due
1654
infrared
are
integrated
a given
-1
The
integrated
however,
amide
cm
of
shoulder
The
unordered
represent
(ref.
830
the
One
absorptivities
of
1269
a-helix.
the
these
the
main
intensities
component
total
forms.
25%
I band.
integrated
all
1241 coil
infrared
of
powder
structure.
at
to
and
lyophilized
secondary -1 cm Raman
predominant
for
of
unordered
with
assigned
the
sprctrum
and
of
an
ben-
hydrogen-bond resulting
from
41 the
higher
most
intensity
tyrosine
The can
S-S
residues
to
that
the
configurations (ref.
infrared
the
the
chain
present
consists
of
unordered
510
to
Fig.
2,
surface.
the
and
disulfide bonds in PLA -1 (see Fig. 2). This 542 cm
and
moiety
must
trans-gauche-trans coexist
from
the
unordered
sitions
from
a-helix
Besides
the
Raman
spectra
the
of
to
in
the
protein
The
the
reported obtained revealed residues
rest
to
3-4). cause
expense
other
about some
the
in
polypeptide
in
increase
coat
about
of
a-helix.
of
Tran-
protein
(refs.
secondary
this
(36%).
an
of
of
content
loss
authors
details
which
the
B-sheet
conformations by
structure
of
and
seems
Raman
u-helical
(refs.
the
application
of
15-16).
structure, the
case
molecular
were
found
to
surface.
This The
secondary
(25%)
at
first
classical
the
reference
B-sheet
been
have
ACKNOWLEDGEMENTS. (CAICYT).
regions as
the
with
state.
and
environment
tyrosine
protein
solid
structures
information
environments on
also
determine
percent,
protein
and
have
39
represents
combination
the
protein
B-sheet
virus
to in
be
lipids
sora
According
protein of
study in
to
proteolipid
fully
at
C-S-S-C
apoprotein
Taking
be
the
band.
gauche-gauche-gauche
the
determined
the
bands
spectroscopy
proteolipid
pf3
on
cm-l
frequencies
spectroscopy
scattering
was
830
14). summary,
In of
of
the are
stretching
correspond
suggests
of
work
technical
has
been
assistance
supported of
Mrs.
by E.
the
Comision
Rubio
is
Ase-
grate-
acknowledged.
REFERENCES 1 A. Watts and J.H.M. De Pont, Progress in Protein-Lipid interactions, vol. 1, Elsevier, Amsterdam, 1985, pp. l-56. 2 L.M. Garcia-Segura, M. de CGzar, M.C. Moreno and J. Monreal, Brain Res., 380 (1986) 261-266. 3 G. Ayala, P. Carmona, M. de C6zar and J. Monreal, Eur. Biophys. J 14 (1987) 219-225. 4 P:'Carmona, J.M. Ramos, M. de C6zar and J. Monreal, J. Raman Spectrosc., in press. 5 J. Monreal J. Neurochem., 25 (1975) 539-541. 6 J. Folch-Pi and M. Lees J. Biol. Chem., 191 (1951) 807-817. 7 J.S. Aguilar, M. de C6zir, M. Criado and J. Monreal, J. Neurochem., 39 (1982) 1733-1736. 8 J.S. Aguilar, M. de C6zar, M. Criado and J. Monreal, J. Neurochem., 40 (1983) 585-588. 9 M.A. Raso, J. Tortajada, D. Escolar and F..Accidn, Comput. Chem., 11 (1987) 125-135. 10 C. .de Lizi, M.H. Baron and F. Fillaux, J..Chim. Phys., 75 (1978) 631-649.
48 11
12 13
14 15 16
G. Zundel, U. Bb;hner, J. Fritsch, H. Merz and B. Vogt, in D.W Gruenwedel and J.R. Whitaker (Editors), Food Analysis, Marcel Dekker, In., New York, 1984, pp. 435-509. M. Levitt and J. Greer, J. Mol. Biol., 114 (1977) 181-239. R.C. Lord, M.C. Chen, T. Takamatsu, I. Harada, M.N. Siamwiza, H. Matsuura and T. Shimanouchi, Biochemistry, 14 (1975) 48704876. H.E. van Wart, A. Lewis, H.A. Scheraga and F.D. Saeva, Proc. Natl. Acad., Sci. USA., 70 (1973) 2619-2623. G.J. Thomas, Jr., and L. A. Day, Proc. Natl. Acad. Sci. USA., 78 (1981) 2962-2966. G.J. Thomas, Jr., Biophys. J., 46 (1984) 763-768.
JoumalofA4olecular Structure,175 (1988) 43-48 Elsevier
Science
Publishers
CONFORMATIONAL
B.V., Amsterdam
STRUCTURE
APOPROTEIN.
A RAMAN
P. CARMONA' 1 Instituto
, J.M.
OF
AND
-Printed
THE
CENTRAL
INFRARED
RAMOS,
M.
de
Optica
(CSIC),
Instituto de 28006 Madrid
Neurob (Spain
ologia
in The Netherlands
NERVOUS
SYSTEM
SPECTROSCOPIC
COZAR
and
Serrano S.R.
STUDY.
J.
MONREAL
121,
28006
Cajal
PROTEOLIPID
Madrid
(CSIC),
(Spain).
Velazquez
144,
ABSTRACT Raman and infrared spectroscopy have been applied to investigate the structure of proteolipid apoprotein, PLA, in the solid state. These techniques reveal the presence of a-helical, B-sheet and unordered structures through the amide A, I, II, III and V bands. A fitting program for resolution of infrared amide I band provided an estimate of the protein secondary structure including 39% a-helix, 36% B-sheet and 25% coil and turns. PLA displays higher content of B and unordered structures than non-delipidated proteolipid PLP which, however, is more rich in a-helical segments. The Raman spectra also reveal the hydrogen-bonding environments of tyrosine residues in this protein. These residues are known from these Raman spectra to be exposed on the protein surface.
INTRODUCTION The of
conformational
prime
importance
architecture
and
membrane
that
proteins
on
cidated.
The
study the
the of
main
intrinsic
proteolipid
core
of
the
cant
interest,
functional
only
reconstituted
membranes
and
of
get
is
(refs. (refs. PLP
0022-2860/88/$03.50 0 1988 Elsevier
3-4)
of has
is
be
60% a
in
of
the
This
protein
into
the
but
also
interactions
is
membrane to
the
model PLP,
is
the in
be
total for that
of
reported
Publishers
on
some
B.V.
the
the is,
study
natural
signifiand of and
l-2). we
elu-
hydrophobic
structural
to
the a
so-called
of
good
form
embedded
insight
the
is
on
Myelin
myelin
about
to
l-2).
emphasizing
Science
influence
influence
myelin up
proteins
of
delipidated
membrane,
protein-protein
papers
myelin
to
myelin
their
The
makes
(PLA)
of
of
function
The
membrane
membranes.
revealed
(refs.
and
of
been
bilayer
lipid-protein
spectra
which
has
apoprotein
not
role
In earlier
fibres. and
proteins.
lipid
point
component
(PLP)
and
intrinsic
biological
nerve
protein
protein
of view
architecture
fraction of
from function
surrounds the
proteolipid protein
structure
vibrational
environment-depend-
44
ent
conformational
information
on
the
high
hydrophobicity
cult
to
ondary are
break
and
in
(refs.
most
of 4-5),
have
not
work
these
is
two
previously
have of
compare
used
which
scarce
to
are
its
diffi-
protein
sec-
spectroscopy vibrational
the
PLA
in
the
solid
state.
the
secondary
characterize
either the
of
is
due
vibrational
infrared
for
PLA
studied
to
techniques,
been
forms
pure
procedure to
There
of
estimates
using we
state
reliable
proteins.
aggregation
protein
this
proteins
and
structure
quantitative
this
In
lipids
strong on
conformational
the
structure
secondary
Data
structure
spectra
of
protein and
up.
non-existent.
Although
aspects
and
Raman
separately
structural
spectra or
study
together, of
PLA.
METHODS Proteolipid matter Lees
protein
according method
to
(ref.
(PLP)
was
a modification
6).
The
concentration
of
n-butanol.
This
was
apoprotein
(PLA)
solution by
Aguilar
ratio
found
was
Infrared
et to
lyophilized
PLA
samples
and
was
drying
9)
for
mine
in
arrangements. shape
for
Raman
and
algorithm
were
using as
the
and
the
are
reported
ferred
to
RESULTS The shows
AND
5145
to
on
i
cm-l.
internal
turns)
a Jobin-Yvon
with
to
(ref. deterof
a Lorentzian
the
amide
Ramanor
spectral
Lyophilized
diameter
used
164
slit
plasma samples
I band.
U-1000
a Spectra-Physics
The
water
polypeptide
of
calibrated
tl
heavy program
percentages
assumes
of
Deuteration
with
was
of
5998
of
fitting
program
line
molar
model
components
source.
frequencies,
mm
the
terms
as
respectively.
Samples
them
and
proteolipid
PLP,
I band
in
at
width
lines were
argon was
from
the
trans-
capillaries.
DISCUSSION
infrared some
recorded
excitation
laser,
amide
(coil of
the
techniques.
A
and
ultrafiltration
and
station.
bands.
PLA
unresolved
the
2 cm-l
0.9-l
of
Folch-Pi
lipid/protein
PLA
white
water-saturated
by
pellet
amide
brain
solubilized
a Perkin-Elmer
KBr
infrared
the
obtain
equilibrating
unordered
original
spectra
laser
by
assign
the
on
bovine
was of
The
for
a data by
structure
The the
spectrometer ion
of
B-sheet
a-helix,
studied out
to
7-8).
by
to
protein/ml
25.0
scanned
carried
secondary
and
were
order
of
a delipidation
(refs.
0.5
5)
protein
employed
assisted were
resolution
the
1 mg
of
al.
be
spectra
spectrophotometer
of
means
from
(ref.
lyophilized
a constant
described
extracted
spectrum
spectral
of
features
proteolipid indicative
apoprotein of
(see
a predominant
Fig.
1)
helical
45
t4000
3500
3000
2500
2000
BOO
1400
1600
1200
1000
600
600
400
200
cm-'
Fig.
1.
Infrared but
structure, tures
are
with
an
cm-l)
dered
and
of
the
a splitting (ref.
be
of
Raman
romporent
range
amide
at
structures,
It
and
PLA. unordered
infrared amide -1 , which cm
either
In
known
and
the and
the
wavenum,bers
and
for
and/or of
the
infrared
a-helix
with -1
be
the
con-
Raman
that
uncr-
distingbished
Raman hand
as
this
) and
spectra.
other
is
consistent
10)
can
Rarran
infrared on
cm
(ref.
arrangements
infrared
five
(1654
struc-
A band is
a-helical
agreement
infrared
is well
backbone
1668
usually
in
appear
PLA at
Other are
1625
and
cated
in
modes
caused
the
can
be
is
these
!n
the
amide there
u-helical
1685
B-structure side
due
2)
case
! fremust
be
ccnfcrmation
of
for
the 1520
usually (ref. the
also
the
of
v(~,o)
11).
and
695
assigned
cm to
Moreover,
infrared
and
amide
another unordered
Raman
polypeptide
infrared
and
shows
B-sheet
in
indicaticns
the
cf
to
located
Typical
cm-I
range
Fig.
types
following.
spectral by
tc
whereas
high-frequency
(see
qualitative
the
respectively,
PLA
frequency
assigned
modes
the
I band of I cmwhich
as this
ccnformations.
on
the
coincident,
about
of
10).
The
ture
of
their
protein
must
3290
arrangement.
polypeptide
account
unordered
near
I modes.
a-helical
b-sheet
the
fact,
powder
the position and intensity -1 cm) suppcrt the existence of
splitting
amide
into
quencies
1654
of
structure,
polypeptide
is
:1659
However, at
predocir,ant clusion
In
located
secondary
forms.
1 band
taking
and
lyophilized
amounts
present.
sharp ordered
B-sheet amide
of
significant
also
relatively
spectrum
spectral chain
secor,dary bands
of
V(O,IT)
-1
amide
I
are
lo-
bands
the
strucB-sheet
amide
II
and
a weak
shoulder
I band
near
1665
V
6
600
800
1000
I
I
1200
I
1400
1600
2800
3000
cm-’ 2.
Y
-1
Raman
indicates
agreement
Raman
to
band
with
the
I band
the
random appears
assigned
resolution
36%
b-sheet
obtained
from
amide
bands
12),
Raman
areas area
protein.
The
the
chains.
larly
infcrmative
concerning
involving
the
gation
Siamwiza
of
is
due
out-of-plane zenes.
If
donor;
the
phenolic et
to
al.
tyrosine
ratio
of
(ref.
13)
850/830
buried, cm-'
III
Raman
of it bands
known
on
is
the of
sum
of
the
f-ccnient
the
spectra
interac-
are
particu-
interactions
and
to
the
doublet the
a strong
about
C.5,
investi-
at
850
overtone
parasubstituted as
unknown
helices.
tyrosine
acts
of
that
total
According
the
were
proteins
that
the
bonding
the
a-helix,
different
a fraction
to the
program
the
the
eleven
basis
vibration
vibration is
of
as
tyrosine.
ring-breathing
ring-bending the
of
that
is well
information The
39%
of
study
with
hydrogen
group
it
fitting
components
question
as
occurs
side
protein
band
amide
percentages
resolved
related
some
of
the
B-strands
provides
in
II!
the
provided
empirical
closely
same
the
These
The
an
also
amide of
absorptivities)
spectroscopy
tions
cm-'
of
equal. on
of is
of
I band
a problem,
suggests
the
is
to a-helix and is consistent -1 component of the amide
amide
area
not
of
result
cm
therefore,
(the
This
application
area
PLA.
component
structures.
could,
I band
due
1654
infrared
are
integrated
a given
-1
The
integrated
however,
amide
cm
of
shoulder
The
unordered
represent
(ref.
830
the
One
absorptivities
of
1269
a-helix.
the
these
the
main
intensities
component
total
forms.
25%
I band.
integrated
all
1241 coil
infrared
of
powder
structure.
at
to
and
lyophilized
secondary -1 cm Raman
predominant
for
of
unordered
with
assigned
the
sprctrum
and
of
an
ben-
hydrogen-bond resulting
from
41 the
higher
most
intensity
tyrosine
The can
S-S
residues
to
that
the
configurations (ref.
infrared
the
the
chain
present
consists
of
unordered
510
to
Fig.
2,
surface.
the
and
disulfide bonds in PLA -1 (see Fig. 2). This 542 cm
and
moiety
must
trans-gauche-trans coexist
from
the
unordered
sitions
from
a-helix
Besides
the
Raman
spectra
the
of
to
in
the
protein
The
the
reported obtained revealed residues
rest
to
3-4). cause
expense
other
about some
the
in
polypeptide
in
increase
coat
about
of
a-helix.
of
Tran-
protein
(refs.
secondary
this
(36%).
an
of
of
content
loss
authors
details
which
the
B-sheet
conformations by
structure
of
and
seems
Raman
u-helical
(refs.
the
application
of
15-16).
structure, the
case
molecular
were
found
to
surface.
This The
secondary
(25%)
at
first
classical
the
reference
B-sheet
been
have
ACKNOWLEDGEMENTS. (CAICYT).
regions as
the
with
state.
and
environment
tyrosine
protein
solid
structures
information
environments on
also
determine
percent,
protein
and
have
39
represents
combination
the
protein
B-sheet
virus
to in
be
lipids
sora
According
protein of
study in
to
proteolipid
fully
at
C-S-S-C
apoprotein
Taking
be
the
band.
gauche-gauche-gauche
the
determined
the
bands
spectroscopy
proteolipid
pf3
on
cm-l
frequencies
spectroscopy
scattering
was
830
14). summary,
In of
of
the are
stretching
correspond
suggests
of
work
technical
has
been
assistance
supported of
Mrs.
by E.
the
Comision
Rubio
is
Ase-
grate-
acknowledged.
REFERENCES 1 A. Watts and J.H.M. De Pont, Progress in Protein-Lipid interactions, vol. 1, Elsevier, Amsterdam, 1985, pp. l-56. 2 L.M. Garcia-Segura, M. de CGzar, M.C. Moreno and J. Monreal, Brain Res., 380 (1986) 261-266. 3 G. Ayala, P. Carmona, M. de C6zar and J. Monreal, Eur. Biophys. J 14 (1987) 219-225. 4 P:'Carmona, J.M. Ramos, M. de C6zar and J. Monreal, J. Raman Spectrosc., in press. 5 J. Monreal J. Neurochem., 25 (1975) 539-541. 6 J. Folch-Pi and M. Lees J. Biol. Chem., 191 (1951) 807-817. 7 J.S. Aguilar, M. de C6zir, M. Criado and J. Monreal, J. Neurochem., 39 (1982) 1733-1736. 8 J.S. Aguilar, M. de C6zar, M. Criado and J. Monreal, J. Neurochem., 40 (1983) 585-588. 9 M.A. Raso, J. Tortajada, D. Escolar and F..Accidn, Comput. Chem., 11 (1987) 125-135. 10 C. .de Lizi, M.H. Baron and F. Fillaux, J..Chim. Phys., 75 (1978) 631-649.
48 11
12 13
14 15 16
G. Zundel, U. Bb;hner, J. Fritsch, H. Merz and B. Vogt, in D.W Gruenwedel and J.R. Whitaker (Editors), Food Analysis, Marcel Dekker, In., New York, 1984, pp. 435-509. M. Levitt and J. Greer, J. Mol. Biol., 114 (1977) 181-239. R.C. Lord, M.C. Chen, T. Takamatsu, I. Harada, M.N. Siamwiza, H. Matsuura and T. Shimanouchi, Biochemistry, 14 (1975) 48704876. H.E. van Wart, A. Lewis, H.A. Scheraga and F.D. Saeva, Proc. Natl. Acad., Sci. USA., 70 (1973) 2619-2623. G.J. Thomas, Jr., and L. A. Day, Proc. Natl. Acad. Sci. USA., 78 (1981) 2962-2966. G.J. Thomas, Jr., Biophys. J., 46 (1984) 763-768.