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The isolation and the structure of new glycopeptide from blood group substances
Vol. 56, No. 2, 1974
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
THE ISOLATION AND THE STRUCTUREOF NEWGLYCOPEPTIDE FROM BLOOD GROUPSUBSTANCES N.K,Kochetkov,
V.A.Derevitskaga,
L.M.Likhosherstov
and
S.A.Medvedev N.D.Zelinsky Received
Institute of Crganic Chemistry, of Sciences, Moscow, USSR
October
USSR Academy
15.1973
Summary: Three new glgcopeptides with 0-glycosidic and one glycopeptide with N-glycosylaminic carbohydrate-peptide linkages have been isolated after degradation of blood group substances (BGS). Their structure have been determined as 0-(d.-GalNAc)-Ser(I), 0-(GalNAc)-(Pro)-Ser(I1) 0-(GelNAcl-3 GalNAc)-(Thr-Ala)-Ser(III),N-(j3-GlcNAc)-Asn(IV~. The isolation of glyco,peptide I confirmed aC-configuration of 0-glycosidic carbohydrate-peptide bonds. The structure of glycopeptide III with two galactosamine residues is in accordance with the data on the presence of hexosamine core of BGS carbowdrate chains.
Recently
we reported
/1/
on the
isolation
of glycopeptide
0-(N-acetylgalactosaminyl)-threonyl-alanine, products
of blood group
succeeded in isolation
substances of other
die and N-glycosylaminic cidation
of their
Degradation been carried tide
fraction
jected
elution revealed
(A+H)
with
carbohydrate-peptide
C-glycosi-
linkages
and elu-
structure.
out according isolated
to chromatography
from pig stomach lining
to the procedure after
/3/.
gel-filtration
19 peaks (fig,2),
on Aminex AG SOW-X2 resin The fractions
peak were combined and the ratio after
hydrolysis
has
The glycopep(fig.1)
curve was mode up by means of ninhydrin
nes was determined
Now me have
(B&S),
glycopeptides
of BGS isolated II
from degradation
/'l/0
reaction
corresponding
was subThe and to each
of amino acids and hexosami(4N HCl, IOO',
24 h) using
BIOCHEMICAL
Vol. 56, No. 2, 1974
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
glycopeptides
% N
0" 2.0.
,amino aci I peptides
/G/--II---i
8 1
Fig.l.Fractionation of BGS degradation P-2 (column 3 x 200 cm, elution
products on Bio-Gel with O.lM acetic acid).
0.5 13
100
Fig.2.
ChromatograpfUI
200 Fraction
15
17
300
400
number
of glycopeptide
fraction
II
(see
fig.1)
on Aminex AG .5OW-X2 column (1.8 x 80 cm), elution with gradient of pyridine-formate buffer, fraction volume 5 ml. Fractions were assayed by absorbance at 570 nm after reaction with ninhydrin.
the amino acid analyzer and 18-19 contained
amino acids,
amount of glucosamine; and galactosamine simplest
(Biotronic
only,
fractions Fraction
amino acid composition 312
LC 4010).
Fractions
galactosamine IO-17
I-9
and small
contained
2,5 and 'I$ (fig.21 and were used for
amino acids had the the isola-
Vol.
56, No.
tion
2, 1974
BIOCHEMICAL
of glycopeptides.
subjected
AND
BIOPHYSICAL
For this
purpose
to preparative
high-voltage
and paper chromatography phoretic
separations
obtaining
/I/.
cation
the fractions
were
paper electrophoresis
In several
cases two electro-
and paper chromatography of glycopeptides
of Xdman degradation
oxidation
(0,015M NaI04,
treated
with
hydrol;yzed
were used Sor
according 20°,
(4N HCl, IOO', The following
gradation
products
2 h);
to /2/
by appli-
and poriodate
oxidation
products
were
or NaBH4 , 20°, 2 h) then
20 h) and analyzed glycopeptides
using
amino acid
were isolated
from de-
of BGS:
(5.3)
Ser
was determined
NaBH,+ (1.5% solution
analyzer.
II.
Pro-Ser
(5.1.2.1)
I
lioC-GalNAc III.
COMMUNICATIONS
homogeneous glycopeptides.
The structure
I.
RESEARCH
0-d-GalNAc
Thr-Ala-Ser
IV. fsn (2.3)
(14.4.2)
I C-d-GalNAcj-I
GalNAc
N-J3-GlcNAc 5.3 3-f)
C-(A-N-acetylgalactosaminyl)-serine
(I).
with
was isolated
by electro-
oxidation
of I results
GalN:Ser
phoresis
= 1.0:0.98
at pH 1.9 (zone 3). Periodate
in destruction of this
molar ratio
of N-acetylgalactosamine
glycopeptide
which completely of serine
was confirmed
excluded
Glycopeptide
only.
The structure
by Edman degradation
the structure
with
two residues
and N-acstylgalactosamine.&-Configuration
O-glycosidic
carbohydratepeptide
the high positive H20;calculated
optical
linkage
rotation
from the determination
of
was deduced from
value@]? of serine
+
117'
using
(c 0.015;
amino
*) iilhen numbe ring glycopeptides the first figure is the number and of a fraction after ion-exchange chromate raphy (fig.2) next figures are the numbers of the zone 7from the less mobile) after successive paper electrophoresis and chromatogrwhy
l
313
BIOCHEMICAL
Vol. 56, No. 2, 1974
acid analyzer).
This result
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
is in accordance
obtained
by Donald et al.
guration
of carbohydrate-peptide
with
the data
who have established
/3/
linkages
d-confi-
in EGS from the ot-
her source. 0-(d-N-acetglgalactosaminyl)-(prolyl)-serine copeptide
5.1.2.l
with
ed by electrophoresis
at pH
2) and subsequently figuration
GalN:Ser:Pro
(zone
bond for
has been accepted
Gly-
was isolat-
1.0:0.85:1.0
and at pH 3.6 (zone
I>,
by paper chromatography
of 0-glycosidic
des described
1.9
=
(II).
this
(zone and othor
by analogy
with
A-Con-
I).
glycopepti-
glycopeptide
I.
O-/~-O-(hr-acetylgalactosamingl)-d-N-acetglgalactoseming1/threonyl-alanyl :Thr:Ser:Ala at pH te
-serine =
(III
) . Glycopeptide was isolated
2.0:1.08:1,0:1.2
when
III
was subjected
(N HCl, 4 h, IOO'),
NaBH4 treatment
ed by GLC analysis
using Fye series
graph (3% OV-17 on GasChrom &, 0.4 x 150 cm, 215'), tose in III.
by electrophoresis
oxidation
threonine
to serine. galactosamine on alkaline
the absence of galacresults
in the comple-
and only 5O% of galactosamine. residues
bonds in a disaccharide,
The presence residues
follow-
mesh, column size
of III
two N-acetylgalactosamine or 1 --t4
/4/
model 64 gas cbromato-
104
100-120
aceta-
to hydrolysis
and acetylation
thus demonstrating
Periodate
te destruction I-3
with GalN:
(zone 4) and at pH 3.6 (zone 2). No galactitol
1.9
could be detected
quently
14.4.2
of l-3
degradation
of methylamide
with
which is attached
linkage
was established
are linked
Conse-
between N-acetyl-
by comparison
of data
of glycopeptide
III
and of model compound 0-/4-O-(J3-acetglglucosaminyl)-~-N-acetylglucosaminyl/-N-benzyloxycarbonyl-Lserine /5/.
while
In the former in the latter
case 70% of galactosamine case
(1
-4
linkage)
314
methylamide was destroyed, glucosamine
was
not
Vol. 56, No. 2, 1974
affected.
BIOCHEMICAL
Glycopeptide
methylamide
since free
j3-elimination pyridine
/6/.
mixture
diazomethane (36 h,, 0') III
III
had to be first
carboxyl 20 min,
and treated
with
methylamine
isolation
converted
group of serine
It was acetylated (l:l,
/5/;
wi.thout
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
with
acetic
into
inhibits anhydride
and then esterified
100')
8% methylamine
by
in abs. methanol
was removed and methylamide
was treated
with
-
of
0.05M aqueous Na2C03
(4 h, 70’). 0+3-N -acetglglpcosaminyl)-I-serine a model compound for selection of amidation
was used as and degradation
conditions. _N'-( -N*-ace jtylglacosaminyl)-asparagine de 2.3 with
GlcN:Asp = 1.0:0.93
sis at pH 1.9 (zone 3)* Its chromatography A-6 resin, buffer,
Glycopeptiwas isolated
elution
by electrophore-
time upon ion-exchange
(47 min, column 0.9 x 5.5 cm packed with
elution
with
0.2M sodium citrate-hydrochloric
pH 2.2 at 60°, SOml/h) and electrophoretic
at pH 3*6 and 1.9 were identical
hydrolase
/7/
determination
with
subsequent
of aspartic
some preliminary
structure
of peptide
regions direct peptide
of serine
evidence
here and in the previous
conclusions
of glycopeptide
chains
linkages. and threonine acids.
O(-configuration 315
the
of BGS near the The isolation
1)
/I/
of 0-glycosidic
both hydroxyamino
I confirmed
paper
can be made concerning
and carbohydrate (I-III)
and quantitative
acid.
of the presence
bonds with
of
bond were confirmed
identification
of carbohydrate-peptide
glycosides
sample
with ~-aspartyl-glycosylamine-amido-
From the data presented /'l/
mobilities
The structure
of N-glycosaminic
by enz:ymatic hydrolysis
acid
to those of synthetic
of N-(P-Nf-acetylglucosaminyl)-L-asparagine. IV and configuration
Aminex
is the first carbohydrate-
2) The isolation of these bonds.
of
Vol.
56, No.
2, 1974
BIOCHEMICAL
3)
The structure
of glycopeptida
data on the presence substances adjacent lated
AND
built
BIOPHYSICAL
III
hydrophobic
acids - alanine
recent
suggestion
rate-peptide isolated
The isolation /9/
that
bonds alongside
residues
and proline
with
from pig stomach lining
which is
acid linked
with
car-
IV supports
our
are N-glgcosylaminic O-glycosidic according
iso-
are bound either
of glycopeptide there
the
4) In the glycopeptides
with NH*- or COOH-group of hydroxyamino 5)
with
core in blood group
up of N-acetylhexosamine chain /8/.
COMMUNICATIONS
is in accordance
of the carbohydrate
to the peptide
bohydrates.
RESEARCH
to
carbohyd-
bonds in BGS /IO/.
REFERENCES
1, Kochetkov,N.K.,
and Medvedev,S.A.,
(1973).
Derevitskaya,V.A., Likhosher&tov,L.M., Biochem.Biopbys.Res,Commun, 52, 74&
Gray,W.R., in "Methods in Enzymology" (&l. by Hirs,C.H.W.), vol,ll, Acadwmic Press, New York, 1967, p.469. Creeth,J,W., Morgan,W,T,J., and Watkins,W.M,, 3. Donald,A.S,R. 125 (1969). I, Sloneker,J.H,,acd Jeans,A., Anal,Chem.z, 4. 2.
5. Likhosherstov,L.M., Izv,Akad.Nauk
Novikova,ii.S.,and Derevitskaga,V.A., SSSR, Ser.Khim. 2, 652 (1971).
6, 7.
Kaverzneva,E.D,,
and Tiutrine,G.V,,
Biokhi-
8.
Martinova,M,D.,and Dokl,Akad.Nauk SSSR 203, 700 (1972). Kochetkov,N.K., Derevitskaya,V,A., and Fedorova,V.I., IO. Likhosherstov,L.M. Biokhimiya 34, 45 (1969).
9.
316
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
THE ISOLATION AND THE STRUCTUREOF NEWGLYCOPEPTIDE FROM BLOOD GROUPSUBSTANCES N.K,Kochetkov,
V.A.Derevitskaga,
L.M.Likhosherstov
and
S.A.Medvedev N.D.Zelinsky Received
Institute of Crganic Chemistry, of Sciences, Moscow, USSR
October
USSR Academy
15.1973
Summary: Three new glgcopeptides with 0-glycosidic and one glycopeptide with N-glycosylaminic carbohydrate-peptide linkages have been isolated after degradation of blood group substances (BGS). Their structure have been determined as 0-(d.-GalNAc)-Ser(I), 0-(GalNAc)-(Pro)-Ser(I1) 0-(GelNAcl-3 GalNAc)-(Thr-Ala)-Ser(III),N-(j3-GlcNAc)-Asn(IV~. The isolation of glyco,peptide I confirmed aC-configuration of 0-glycosidic carbohydrate-peptide bonds. The structure of glycopeptide III with two galactosamine residues is in accordance with the data on the presence of hexosamine core of BGS carbowdrate chains.
Recently
we reported
/1/
on the
isolation
of glycopeptide
0-(N-acetylgalactosaminyl)-threonyl-alanine, products
of blood group
succeeded in isolation
substances of other
die and N-glycosylaminic cidation
of their
Degradation been carried tide
fraction
jected
elution revealed
(A+H)
with
carbohydrate-peptide
C-glycosi-
linkages
and elu-
structure.
out according isolated
to chromatography
from pig stomach lining
to the procedure after
/3/.
gel-filtration
19 peaks (fig,2),
on Aminex AG SOW-X2 resin The fractions
peak were combined and the ratio after
hydrolysis
has
The glycopep(fig.1)
curve was mode up by means of ninhydrin
nes was determined
Now me have
(B&S),
glycopeptides
of BGS isolated II
from degradation
/'l/0
reaction
corresponding
was subThe and to each
of amino acids and hexosami(4N HCl, IOO',
24 h) using
BIOCHEMICAL
Vol. 56, No. 2, 1974
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
glycopeptides
% N
0" 2.0.
,amino aci I peptides
/G/--II---i
8 1
Fig.l.Fractionation of BGS degradation P-2 (column 3 x 200 cm, elution
products on Bio-Gel with O.lM acetic acid).
0.5 13
100
Fig.2.
ChromatograpfUI
200 Fraction
15
17
300
400
number
of glycopeptide
fraction
II
(see
fig.1)
on Aminex AG .5OW-X2 column (1.8 x 80 cm), elution with gradient of pyridine-formate buffer, fraction volume 5 ml. Fractions were assayed by absorbance at 570 nm after reaction with ninhydrin.
the amino acid analyzer and 18-19 contained
amino acids,
amount of glucosamine; and galactosamine simplest
(Biotronic
only,
fractions Fraction
amino acid composition 312
LC 4010).
Fractions
galactosamine IO-17
I-9
and small
contained
2,5 and 'I$ (fig.21 and were used for
amino acids had the the isola-
Vol.
56, No.
tion
2, 1974
BIOCHEMICAL
of glycopeptides.
subjected
AND
BIOPHYSICAL
For this
purpose
to preparative
high-voltage
and paper chromatography phoretic
separations
obtaining
/I/.
cation
the fractions
were
paper electrophoresis
In several
cases two electro-
and paper chromatography of glycopeptides
of Xdman degradation
oxidation
(0,015M NaI04,
treated
with
hydrol;yzed
were used Sor
according 20°,
(4N HCl, IOO', The following
gradation
products
2 h);
to /2/
by appli-
and poriodate
oxidation
products
were
or NaBH4 , 20°, 2 h) then
20 h) and analyzed glycopeptides
using
amino acid
were isolated
from de-
of BGS:
(5.3)
Ser
was determined
NaBH,+ (1.5% solution
analyzer.
II.
Pro-Ser
(5.1.2.1)
I
lioC-GalNAc III.
COMMUNICATIONS
homogeneous glycopeptides.
The structure
I.
RESEARCH
0-d-GalNAc
Thr-Ala-Ser
IV. fsn (2.3)
(14.4.2)
I C-d-GalNAcj-I
GalNAc
N-J3-GlcNAc 5.3 3-f)
C-(A-N-acetylgalactosaminyl)-serine
(I).
with
was isolated
by electro-
oxidation
of I results
GalN:Ser
phoresis
= 1.0:0.98
at pH 1.9 (zone 3). Periodate
in destruction of this
molar ratio
of N-acetylgalactosamine
glycopeptide
which completely of serine
was confirmed
excluded
Glycopeptide
only.
The structure
by Edman degradation
the structure
with
two residues
and N-acstylgalactosamine.&-Configuration
O-glycosidic
carbohydratepeptide
the high positive H20;calculated
optical
linkage
rotation
from the determination
of
was deduced from
value@]? of serine
+
117'
using
(c 0.015;
amino
*) iilhen numbe ring glycopeptides the first figure is the number and of a fraction after ion-exchange chromate raphy (fig.2) next figures are the numbers of the zone 7from the less mobile) after successive paper electrophoresis and chromatogrwhy
l
313
BIOCHEMICAL
Vol. 56, No. 2, 1974
acid analyzer).
This result
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
is in accordance
obtained
by Donald et al.
guration
of carbohydrate-peptide
with
the data
who have established
/3/
linkages
d-confi-
in EGS from the ot-
her source. 0-(d-N-acetglgalactosaminyl)-(prolyl)-serine copeptide
5.1.2.l
with
ed by electrophoresis
at pH
2) and subsequently figuration
GalN:Ser:Pro
(zone
bond for
has been accepted
Gly-
was isolat-
1.0:0.85:1.0
and at pH 3.6 (zone
I>,
by paper chromatography
of 0-glycosidic
des described
1.9
=
(II).
this
(zone and othor
by analogy
with
A-Con-
I).
glycopepti-
glycopeptide
I.
O-/~-O-(hr-acetylgalactosamingl)-d-N-acetglgalactoseming1/threonyl-alanyl :Thr:Ser:Ala at pH te
-serine =
(III
) . Glycopeptide was isolated
2.0:1.08:1,0:1.2
when
III
was subjected
(N HCl, 4 h, IOO'),
NaBH4 treatment
ed by GLC analysis
using Fye series
graph (3% OV-17 on GasChrom &, 0.4 x 150 cm, 215'), tose in III.
by electrophoresis
oxidation
threonine
to serine. galactosamine on alkaline
the absence of galacresults
in the comple-
and only 5O% of galactosamine. residues
bonds in a disaccharide,
The presence residues
follow-
mesh, column size
of III
two N-acetylgalactosamine or 1 --t4
/4/
model 64 gas cbromato-
104
100-120
aceta-
to hydrolysis
and acetylation
thus demonstrating
Periodate
te destruction I-3
with GalN:
(zone 4) and at pH 3.6 (zone 2). No galactitol
1.9
could be detected
quently
14.4.2
of l-3
degradation
of methylamide
with
which is attached
linkage
was established
are linked
Conse-
between N-acetyl-
by comparison
of data
of glycopeptide
III
and of model compound 0-/4-O-(J3-acetglglucosaminyl)-~-N-acetylglucosaminyl/-N-benzyloxycarbonyl-Lserine /5/.
while
In the former in the latter
case 70% of galactosamine case
(1
-4
linkage)
314
methylamide was destroyed, glucosamine
was
not
Vol. 56, No. 2, 1974
affected.
BIOCHEMICAL
Glycopeptide
methylamide
since free
j3-elimination pyridine
/6/.
mixture
diazomethane (36 h,, 0') III
III
had to be first
carboxyl 20 min,
and treated
with
methylamine
isolation
converted
group of serine
It was acetylated (l:l,
/5/;
wi.thout
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
with
acetic
into
inhibits anhydride
and then esterified
100')
8% methylamine
by
in abs. methanol
was removed and methylamide
was treated
with
-
of
0.05M aqueous Na2C03
(4 h, 70’). 0+3-N -acetglglpcosaminyl)-I-serine a model compound for selection of amidation
was used as and degradation
conditions. _N'-( -N*-ace jtylglacosaminyl)-asparagine de 2.3 with
GlcN:Asp = 1.0:0.93
sis at pH 1.9 (zone 3)* Its chromatography A-6 resin, buffer,
Glycopeptiwas isolated
elution
by electrophore-
time upon ion-exchange
(47 min, column 0.9 x 5.5 cm packed with
elution
with
0.2M sodium citrate-hydrochloric
pH 2.2 at 60°, SOml/h) and electrophoretic
at pH 3*6 and 1.9 were identical
hydrolase
/7/
determination
with
subsequent
of aspartic
some preliminary
structure
of peptide
regions direct peptide
of serine
evidence
here and in the previous
conclusions
of glycopeptide
chains
linkages. and threonine acids.
O(-configuration 315
the
of BGS near the The isolation
1)
/I/
of 0-glycosidic
both hydroxyamino
I confirmed
paper
can be made concerning
and carbohydrate (I-III)
and quantitative
acid.
of the presence
bonds with
of
bond were confirmed
identification
of carbohydrate-peptide
glycosides
sample
with ~-aspartyl-glycosylamine-amido-
From the data presented /'l/
mobilities
The structure
of N-glycosaminic
by enz:ymatic hydrolysis
acid
to those of synthetic
of N-(P-Nf-acetylglucosaminyl)-L-asparagine. IV and configuration
Aminex
is the first carbohydrate-
2) The isolation of these bonds.
of
Vol.
56, No.
2, 1974
BIOCHEMICAL
3)
The structure
of glycopeptida
data on the presence substances adjacent lated
AND
built
BIOPHYSICAL
III
hydrophobic
acids - alanine
recent
suggestion
rate-peptide isolated
The isolation /9/
that
bonds alongside
residues
and proline
with
from pig stomach lining
which is
acid linked
with
car-
IV supports
our
are N-glgcosylaminic O-glycosidic according
iso-
are bound either
of glycopeptide there
the
4) In the glycopeptides
with NH*- or COOH-group of hydroxyamino 5)
with
core in blood group
up of N-acetylhexosamine chain /8/.
COMMUNICATIONS
is in accordance
of the carbohydrate
to the peptide
bohydrates.
RESEARCH
to
carbohyd-
bonds in BGS /IO/.
REFERENCES
1, Kochetkov,N.K.,
and Medvedev,S.A.,
(1973).
Derevitskaya,V.A., Likhosher&tov,L.M., Biochem.Biopbys.Res,Commun, 52, 74&
Gray,W.R., in "Methods in Enzymology" (&l. by Hirs,C.H.W.), vol,ll, Acadwmic Press, New York, 1967, p.469. Creeth,J,W., Morgan,W,T,J., and Watkins,W.M,, 3. Donald,A.S,R. 125 (1969). I, Sloneker,J.H,,acd Jeans,A., Anal,Chem.z, 4. 2.
5. Likhosherstov,L.M., Izv,Akad.Nauk
Novikova,ii.S.,and Derevitskaga,V.A., SSSR, Ser.Khim. 2, 652 (1971).
6, 7.
Kaverzneva,E.D,,
and Tiutrine,G.V,,
Biokhi-
8.
Martinova,M,D.,and Dokl,Akad.Nauk SSSR 203, 700 (1972). Kochetkov,N.K., Derevitskaya,V,A., and Fedorova,V.I., IO. Likhosherstov,L.M. Biokhimiya 34, 45 (1969).
9.
316