- Email: [email protected]
Normal glycosaminoglycan production in a galactosylation-defective lectin-resistant CHO cell variant
Vol. 103, No. 1,198l November
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS Pages 38-45
16, 1981
NORMAL GLYCOSAMINOGLYCAN PRODUCTION IN A GALACTOSYLATION-DEFECTIVE
LECTIN-RESISTANT
Eve Barak
CHO CELL VARIANT
Briles
Department of Anatomy University of Alabama in Birmingham Birmingham, Alabama 35294 Received
September
14,
1981
Abstract CHO cell variant clone 13 fails to incorporate galactose into either glycolipids or asn-linked oligosaccharides, even though intracellular UDPgalactose pools, galactosyltransferases, and galactose-acceptor macromolecules are normal. Clone 13 is now shown to produce normal amounts of chondroitin sulfate and heparan sulfate, the biosynthesis of which necessarily involves synthesis of a galactose-containing tetrasaccharide sequence. This is the first evidence of galactosyltransfer reactions which proceed normally in clone 13. Based on the known subcellular sites of glycosyltransfer reactions, it is proposed that a Golgi-specific defect involving compartmentalization may be responsible for the clone 13 trait.
Introduction A variety
of lectin-resistant
have well-defined lectins
surface
to the cell.
major
contributions
are
synthesized
from
CHO cells
defective complex
acceptor Since classes
carbohydrate
Characterization
(1,2,3,4). for
asn-linked
the defect
The defect
in clone
other
levels,
of these 13 is
glycoconjugates
are
already
known
glycoconjugates, are
0 1981 by Academic Press, Inc. of reproduction in any form reserved.
also
38
into
affected.
of
to
oligosaccharides was selected Clone
either
glycolipids
13 is
be attributed pools,
in --in vitro to affect
led
(5,6).
cannot
it
the binding
13, which
UDP-galactose normal
OQO6-291X/81/210038-08$01.00/~ Copyright All rights
affect
surface
clone
galactose
oligosaccharides.
as all
is
many of which
has already
germ agglutinin
to incorporate
of galactose-containing
mine whether
of how cell
to wheat
in galactosyltransferase molecules,
which
of such variants
One such variant
resistance ability
have been isolated,
alterations
to our understanding
in its
terations
variants
assays at least
was of interest
or to al-
or galactose(5,6). two distinct to deter-
Glycosaminoglycans
Vol. 103, No. 1,198l
BIOCHEMICAL
CLONE
3
I
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
qluc N- 'H
13
qluc N- 'H VI
CHO
II 6 III
0
1
Figure
L ti IO
20
30
40
FRACTION
50
02
60
NO
25
35 45 FRACTION
55 NO
65
1
Bio-Gel P-10 elution profiles of ["HI-glycopeptides prepared by Pronase digestion of [3H]glucosamine-labeled cells. Upper panel, clone 13; lower panel, wild-type CHO cell glycopeptides. Figure
2
Bio-Gel P-10 elution profiles digestion of [3H]galactose-labeled wild-type CHO cell glycopeptides.
were
(GAGs)~
dues
of particular
of proteoglycan
sequence, biosynthetic
prerequisite
the GAGS (7).
In this
normal
of the
the
amounts
first
normally the clone
indication in clone
interest
core
glucuronosyl
of [%I]-glycopeptides cells. Upper panel,
proteins
since
they
through
are
prepared by Pronase clone 13; lower panel,
connected
a specific
to serine
tetrasaccharide
linkage
B1,3-galactosylB1,3-galactosylf3l,4-xyloside, for series
assembly
of the repeating
of experiments,
GAGS, chondroitin of a class
13, and provides
clone
sulfate
a possible
which disaccharide
13 is
and heparan
of galactosyltransfer clue
resi-
shown
units
which
to the metabolic
This
39
HMW, high
is
proceed basis
13 trait.
1 Abbreviations used: GAGS, glycosaminoglycans; Adi-4S, 2-acetamido-2-deoxy-3-0-(B-D-gluco-4-enepyranosyluronic sulfo-D-galactose; HONO, nitrous acid.
of
to produce
sulfate.
reactions
is a
molecular weight; acid)-4-0-
for
BIOCHEMICAL
Vol. 103, No. 1,198l
Materials
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
and Methods
Cell culture conditions and the isolation of clone 13 from CHO cells have been described previously (5). Monolayer cultures in 150 mm Falcon dishes were labeled for 48 hr in 25 ml of complete growth medium plus 100 YC of [3H] glucosamine or [3H]galactose (New England Nuclear). The cells were rinsed three times with phosphate-buffered saline, then scraped into 4 ml of 50 mM Tris Cl, pH 8, containing 1 mg/ml Pronase (Calbiochem) and 2.5 mM CaC12. Pronase digestion proceeded at 37" in the presence of a few drops of toluene for 3 to 8 days, with fresh Pronase added daily. The digests were boiled and clarified by centrifugation prior to analysis by gel filtration through a 0.9 cm diameter x 100 cm high column of Bio-Gel P-10, 200-400 mesh (BioRad Laboratories), equilibrated with 0.15 M ammonium acetate, pH 6 or 0.1 M pyridine acetate, pH 5. Column fraction samplings were counted in Scintiverse (Fisher Scientific). Chondroitinase digestion was performed in 800 ul of 12.5 mM Tris Cl pH 8 containing 0.1 U chondroitinase ABC (Miles Laboratories), at room temperature for 24 hr. HONO degradation was performed as described by Shively and Conrad (8). Acid hydrolysis of presumed linkage sequence oligosaccharides was performed in 2 N H2S0,+ for 4 hr at 100". Descending paper chromatography was performed on Whatman 3MM paper in glacial acetic acid : nbutanol : 1 N NH4OH (3:2:1), for analysis of chondroitinase digestion products, or pyridine : ethyl acetate : Hz0 (1:3.6:1.15) (upper phase) for analysis of monosaccharides (5). Samples were mixed with nonradioactive authentic standards before application to the paper. Authentic 4,5-unsaturated disaccharides (Miles Laboratories) were visualized under UV light. Chromatograms were cut into l-cm segments, soaked in 3 ml of water, mixed with 4 ml Scintiverse, and counted in a liquid scintillation counter. Results
and Discussion
Cells
were
and subjected tides rial
were eluting
metabolically to extensive
analyzed
Peak II, 2),
Vi,
(HMW) material
probably
labeled
label
represents
[3H]
to represent
panels,
with
the void from (Fig.
glycopeptides,
either
Figs.
Labeled
mate-
unincorporated 1 and 2),
volume
(V,)
glucosamine
1) and galactose while
glucosamine3
13H] glycopep-
1 and 2).
(lower
glucosamine
complex
(Figs.
was assumed
derived
or
The resulting
column
eluting
by both
[3H]galactose2
digestion. P-10
volume,
+33% of the incorporated
tose. Fig.
on a Bio-Gel
with
In the case of wild-type
molecular-weight for
Pronase
at the salt
metabolites.
labeled
Peak III,
high-
accounted or galac(arrow, labeled
2 UDP-[3H]galactose derived from [3H]galactose is in equilibrium with UDP[3H]-glucose via UDP-glucose-4'-epimerase. In wild-type cells, most of the [3H]galactose supplied in complete medium is incorporated as galactose, but some is incorporated as glucose (e.g., glycolipids), or as other sugars metabolically derived from UDP-glucose (e.g., glucuronic acid, inositol, xylose). In clone 13, supplied [3H]galactose is incorporated mainly as glucose and its derivatives (unpublished data). 3 [3H]glucosamine N-acetylgalactosamine,
is
metabolically and sialic
incorporated acid.
40
as N-acetylglucosamine,
Vol. 103, No. 1,1981
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
VO
3
CLONE
COMMUNICATIONS
13 gal- ‘H
CLONE 13 glcN-‘H
2 8 2 x
’
,I
22-
z u2
I I
0
3
15
25
35
45
55
FRACTION
Figure
00
65
Ii
4 4
NO
I5
25
35 45 FRACTION
55 NO
65
3
~io-~el P-10 elution profiles of [3H]glucosamine-labeled HMWPronase digest products (V, from Figure l), after treatment with chondroitinase ABC. Upper panel, clone 13; lower panel, wild-type. Figure
4
Blo-Gel P-10 elution profiles of [3H]galactose-labeled HMW Pronase digest products (V, from Figure 2), after treatment with chondroitinase ABC. Upper panel, clone 13; lower panel, wild-type.
only
with
glucosamine,
case of clone
probably
13 (upper
panels,
~22% of the incorporated the
remaining
position rich gal
glycopeptides sequences
further.
Peak III,
In the present
mannose-rich
1 and 2), and most
glucosamine
and truncated (5).
Figs.
glucosamine,
incorporated
as wild-type
represents
(arrow,
and probably complex studies,
HMW material of the Fig.
represents
glycopeptides only
In the
glycopeptides. accounted
incorporated
1) eluted
galactose;
in
a mixture lacking
the HMW material
for
the same of mannose-
terminal
sia-
was analyzed
Vol. 103, No. 1,198l
BIOCHEMICAL
0
4
8
AND
12
BIOPHYSICAL
16 20
24
28
RESEARCH
32
36
COMMUNICATIONS
40
44
SEGMENT NUMBER Figure
5 Paper chromatography
"minor peaks" HMW material
by acid hydrolysis
from the
digestion of [3H]galactose-labeled 4). A, clone 13 peak a; B, clone indicate origin peak a; D, wild-type peak a. Arrows sample lanes were cut into l-cm segments for deterPositions of authentic standard monosaccharides,
peak 2; C, wild-type Radioactive positions. mining
of sugars released
obtained after chondroitinase (peaks 5 and a from Figure
radioactivity.
13
chromatographed on the same sheet in separate lanes between the radioactive samples, are indicated: U, glucuronic acid; gal, D(+)galactose; glc, D(+)glucose;
xyl,
D(+)xylose.
The HMW material with
each Pronase
ABC, and the products
chondroitinase
(Figs.
from
Chondroitinase
3 and 4).
and %33% of the wild
type
HMW material,
In the case of galactose-labeled products
was reproducibly
prior
to the major
minor
peaks
represent
were
Paper
sumed linkage tose
sulfate
never
sequences
disaccharides, (Fig.
resolved
observed sequences
chromatographic
and Z3H]-xylose
of A-di-4s
material, into
small-molecular-weight
GAG linkage
peptides.
degraded
by acid (Fig.
5).
digest were
(V,,
Figs.
analyzed
on the P-10
~50% of the
13 HMW material,
to small-molecular-weight
products.
%9% of the two minor
label
peaks,
at Vi
to serine
analysis
of sugars
hydrolysis
revealed
characteristic
peaks digest
6).
42
in
the digest
a and b-, eluting
(arrows,
in glucosamine-labeled
The major
column
clone
peak
attached
1 and 2) was treated
Fig.
material, or small released
products
These
4).
and probably
serine-containing from
the presence
eluting
just
these
pre-
of
[3H]galac-
at Vi mainly
consisted
of chondroitin-4-
Vol. 103, No. 1,198l
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
CHO
CLONE
SEGMENT Figure
13
NUMBER
6
Paper chromatography of chondroitinase digestion products (Vi from Figure 4). The chromatogram was cut into l-cm segments, and the radioactivity in each segment was determined. The positions of co-chromatographed authentic 4,5-unsaturated disaccharide standards are indicated: 6S, Adi-6s; 4s. Adi-4s; OS, Adi-OS. Upper panel, wild-type; lower panel, clone 13.
A
CLONE
13 glcN-
B
3H
CLONE
13
gal-
3H
I
500
1,000
500
20
30
40
50
60
20
FRACTION NO Figure
30
40
FRACTION
50
60
NO
7
Bio-Gel P-10 elution profiles of chondroitinase-resistant (Vo from Figures 3 and 4). after treatment with HONO. labeled material; B. [3H]galactose-labeled material. lower panels, wild-type.
43
HMW material A, [3H]glucosamineUpper panels, clone
13;
Vol. 103, No. 1,1981
BIOCHEMICAL
AND
The chondroitinase-resistant treated
with
column
(Fig.
free
HONO cleaves
or N-sulfated
N-acetylated
amino
residues
substituted
charides
residues
a broad
chondroitinase-resistant ly all
type
CHO cells,
of the
total
clude
that
sulfate
incorporated
label
the biosynthesis
droitinase
digestion
amount
of this
fected
by the clone
contains
less
smaller
molecular
solves
the material
is
than
size
by mild
into
it
for
CHO cells
These
asn-linked
reactions
galactosyltransfer of GAGS, which plasmic
reticulum
are
is
likely
that
is
essential-
susceptible. 13 and wildfor
in clone
con-
13 cells.
even after
chon-
Since
no appreciable
biosynthesis
is probably
indicate
little
that
at least
to
on DEAE-Sephacel
Although
af-
the material
can be converted
(9)
~11%
re-
the material(s)
a portion which
consists
has recently
have of the been
(10). reactions
involved
oligosaccharides
occur
to be defective
reactions
involved
(X,13).
its
peaks.
~~50% of the
We therefore
Chromatography
three
only
each account
7).
results
and very
known
proceed
13,
along
of oligosac-
clone
persists
Fig.
polysaccharide
The galactosyltransfer and complex
(V,,
alkali.
at least
both
sulfate
HMW material
acid,
type,
GAGS is unimpaired
Preliminary
10% sialic
distributed
from glucosamine.
in clone
13 defect.
"erythroglycan"-like
described
derived
contains
to HONO, while
for
bearing
the variously-
HMW material
and chondroitin
found
residues
mixture
susceptible
that,
and HONO treatment
been identified,
asn-linked
is
of wild-type
material
on the P-10
also
randomly
In the case of wild
of these
amounts
sulfate
a heterogeneous
can be calculated
heparan
Substantial
not yet
it
analyzed
heparan
13 chondroitinase-resistant
data,
3 and 4) was next
to HONO, and since
HMW material
of the clone From this
Since
are
range.
Figs.
COMMUNICATIONS
at glucosamine
are more-or-less
products
size
(V,,
sulfate
(8).
RESEARCH
was again
are resistant
the degradation with
mixture
heparan
groups
which
,glucosamine
the chain,
HMW material
MONO, and the reaction 7).
BIOPHYSICAL
normally
in the assembly in
in clone
the Golgi
in clone
We therefore
13,
take place
propose
44
apparatus
13 (5).
in the assembly
that
of
of glycolipids (11).
In contrast, the linkage
in the rough there
exists
the sequence endo-
a Golgi-
Vol. 103, No. 1,198l
specific clone
BIOCHEMICAL
compartmentalization
BIOPHYSICAL
problem
RESEARCH
of some kind
which
COMMUNICATIONS
accounts
for
the
13 trait. For example,
UDP-galactose
a specific from
In addition,
(15). removing the
AND
action
subsequent mechanisms
mechanism
the cytosol a further
the inhibitory
could
product
for
into
is
synthesized)
mechanism
of the
has been
galactosyltransfer
nucleotide
of UMP out account
for
it
specific
of a luminally-oriented transport
has been described
(where
of the
the clone
apparatus.
may be due to improper
insertion
of the
the Golgi
membrane,
or there
may be a defect
transports
nascent
glycoproteins
through
reaction,
UDP, by
(16,17), A defect
and in these
the clone
galactosyltranferases
in the mechanism
the Golgi
lumen
for
Alternatively,
13 trait.
13 defect
the Golgi
described
diphosphatase
Golgi
transporting
in
which
apparatus.
Acknowledgements I gratefully acknowledge the generous support, both moral and a portion of this work was of Lennart Roden, in whose laboratory The work was supported by USPHS Grants # 5 T32 AMO7069, DE 02670, AM25822. Some of the results in this report were presented as a the 1980 Annual Meeting of the American Society for Cell Biology
material, performed. and ROl poster at (14).
References 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17.
Briles, E.B., and Kornfeld, S. (1978) Trends in Biochem. Sci. 1, 223227. Wright, J.A. (1979) Int. J. Biochem. lo, 951-956. Stanley, P. (1980) in The Biochemistry of Glycoproteins and Proteoglycans (W.J. Lennarz, ed.), pp. 161-189, Plenum Publishing Co., New York. Briles, E.B. (1982) Int. Rev. Cytol., in the press. Briles, E.B., Li, E., and Kornfeld, S. (1977) J. Biol. Chem. 252, 1107-1116. Briles, E.B., Li, E., and Kornfeld, S. (1976) Fed. Proc. 35, 1642. Rod&, L. (1980) in The Biochemistry of Glycoproteins and Proteoglycans (W.J. Lennarz, ed.), pp. 267-371, Plenum Publishing Co., New York. (1976) Biochemistry 15, 3932-3942. Shively, J.E. and Conrad, H.E. (1978) J. Biol. JIrnefelt, .I., Rush, J., Li, Y-T., and Laine, R.A. Chem. 253, 8006-8009. Li, E., Gibson, R., and Kornfeld, S. (1980) Arch. Biochem. Biophys. 199, 393-399. in The Glycoconjugates (M.I. Horowitz and Schachter, H. (1978) W. Pigman, eds.), Vol. II, pp. 87-185, Academic Press, New York. (1968) J. Cell. Biol. 38, 358-368. Horwitz, A.L., and Dorfman, A. Sugahara, K., Cifonelli, J.A., and Dorfman, A. (1981) Fed. Proc. 40, 1705. (1980) J. Cell Biol. 87, 3UOa. Briles, E.B. Kuhn, N., and White, A. (1975) Biochem. .I. 148, 77-84. Kuhn, N., and White, A. (1977) Biochem. J. 168, 423-433. Brandan, E. and Fleischer, B. (1980) J. Cell Biol. 87, 200a.
45
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS Pages 38-45
16, 1981
NORMAL GLYCOSAMINOGLYCAN PRODUCTION IN A GALACTOSYLATION-DEFECTIVE
LECTIN-RESISTANT
Eve Barak
CHO CELL VARIANT
Briles
Department of Anatomy University of Alabama in Birmingham Birmingham, Alabama 35294 Received
September
14,
1981
Abstract CHO cell variant clone 13 fails to incorporate galactose into either glycolipids or asn-linked oligosaccharides, even though intracellular UDPgalactose pools, galactosyltransferases, and galactose-acceptor macromolecules are normal. Clone 13 is now shown to produce normal amounts of chondroitin sulfate and heparan sulfate, the biosynthesis of which necessarily involves synthesis of a galactose-containing tetrasaccharide sequence. This is the first evidence of galactosyltransfer reactions which proceed normally in clone 13. Based on the known subcellular sites of glycosyltransfer reactions, it is proposed that a Golgi-specific defect involving compartmentalization may be responsible for the clone 13 trait.
Introduction A variety
of lectin-resistant
have well-defined lectins
surface
to the cell.
major
contributions
are
synthesized
from
CHO cells
defective complex
acceptor Since classes
carbohydrate
Characterization
(1,2,3,4). for
asn-linked
the defect
The defect
in clone
other
levels,
of these 13 is
glycoconjugates
are
already
known
glycoconjugates, are
0 1981 by Academic Press, Inc. of reproduction in any form reserved.
also
38
into
affected.
of
to
oligosaccharides was selected Clone
either
glycolipids
13 is
be attributed pools,
in --in vitro to affect
led
(5,6).
cannot
it
the binding
13, which
UDP-galactose normal
OQO6-291X/81/210038-08$01.00/~ Copyright All rights
affect
surface
clone
galactose
oligosaccharides.
as all
is
many of which
has already
germ agglutinin
to incorporate
of galactose-containing
mine whether
of how cell
to wheat
in galactosyltransferase molecules,
which
of such variants
One such variant
resistance ability
have been isolated,
alterations
to our understanding
in its
terations
variants
assays at least
was of interest
or to al-
or galactose(5,6). two distinct to deter-
Glycosaminoglycans
Vol. 103, No. 1,198l
BIOCHEMICAL
CLONE
3
I
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
qluc N- 'H
13
qluc N- 'H VI
CHO
II 6 III
0
1
Figure
L ti IO
20
30
40
FRACTION
50
02
60
NO
25
35 45 FRACTION
55 NO
65
1
Bio-Gel P-10 elution profiles of ["HI-glycopeptides prepared by Pronase digestion of [3H]glucosamine-labeled cells. Upper panel, clone 13; lower panel, wild-type CHO cell glycopeptides. Figure
2
Bio-Gel P-10 elution profiles digestion of [3H]galactose-labeled wild-type CHO cell glycopeptides.
were
(GAGs)~
dues
of particular
of proteoglycan
sequence, biosynthetic
prerequisite
the GAGS (7).
In this
normal
of the
the
amounts
first
normally the clone
indication in clone
interest
core
glucuronosyl
of [%I]-glycopeptides cells. Upper panel,
proteins
since
they
through
are
prepared by Pronase clone 13; lower panel,
connected
a specific
to serine
tetrasaccharide
linkage
B1,3-galactosylB1,3-galactosylf3l,4-xyloside, for series
assembly
of the repeating
of experiments,
GAGS, chondroitin of a class
13, and provides
clone
sulfate
a possible
which disaccharide
13 is
and heparan
of galactosyltransfer clue
resi-
shown
units
which
to the metabolic
This
39
HMW, high
is
proceed basis
13 trait.
1 Abbreviations used: GAGS, glycosaminoglycans; Adi-4S, 2-acetamido-2-deoxy-3-0-(B-D-gluco-4-enepyranosyluronic sulfo-D-galactose; HONO, nitrous acid.
of
to produce
sulfate.
reactions
is a
molecular weight; acid)-4-0-
for
BIOCHEMICAL
Vol. 103, No. 1,198l
Materials
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
and Methods
Cell culture conditions and the isolation of clone 13 from CHO cells have been described previously (5). Monolayer cultures in 150 mm Falcon dishes were labeled for 48 hr in 25 ml of complete growth medium plus 100 YC of [3H] glucosamine or [3H]galactose (New England Nuclear). The cells were rinsed three times with phosphate-buffered saline, then scraped into 4 ml of 50 mM Tris Cl, pH 8, containing 1 mg/ml Pronase (Calbiochem) and 2.5 mM CaC12. Pronase digestion proceeded at 37" in the presence of a few drops of toluene for 3 to 8 days, with fresh Pronase added daily. The digests were boiled and clarified by centrifugation prior to analysis by gel filtration through a 0.9 cm diameter x 100 cm high column of Bio-Gel P-10, 200-400 mesh (BioRad Laboratories), equilibrated with 0.15 M ammonium acetate, pH 6 or 0.1 M pyridine acetate, pH 5. Column fraction samplings were counted in Scintiverse (Fisher Scientific). Chondroitinase digestion was performed in 800 ul of 12.5 mM Tris Cl pH 8 containing 0.1 U chondroitinase ABC (Miles Laboratories), at room temperature for 24 hr. HONO degradation was performed as described by Shively and Conrad (8). Acid hydrolysis of presumed linkage sequence oligosaccharides was performed in 2 N H2S0,+ for 4 hr at 100". Descending paper chromatography was performed on Whatman 3MM paper in glacial acetic acid : nbutanol : 1 N NH4OH (3:2:1), for analysis of chondroitinase digestion products, or pyridine : ethyl acetate : Hz0 (1:3.6:1.15) (upper phase) for analysis of monosaccharides (5). Samples were mixed with nonradioactive authentic standards before application to the paper. Authentic 4,5-unsaturated disaccharides (Miles Laboratories) were visualized under UV light. Chromatograms were cut into l-cm segments, soaked in 3 ml of water, mixed with 4 ml Scintiverse, and counted in a liquid scintillation counter. Results
and Discussion
Cells
were
and subjected tides rial
were eluting
metabolically to extensive
analyzed
Peak II, 2),
Vi,
(HMW) material
probably
labeled
label
represents
[3H]
to represent
panels,
with
the void from (Fig.
glycopeptides,
either
Figs.
Labeled
mate-
unincorporated 1 and 2),
volume
(V,)
glucosamine
1) and galactose while
glucosamine3
13H] glycopep-
1 and 2).
(lower
glucosamine
complex
(Figs.
was assumed
derived
or
The resulting
column
eluting
by both
[3H]galactose2
digestion. P-10
volume,
+33% of the incorporated
tose. Fig.
on a Bio-Gel
with
In the case of wild-type
molecular-weight for
Pronase
at the salt
metabolites.
labeled
Peak III,
high-
accounted or galac(arrow, labeled
2 UDP-[3H]galactose derived from [3H]galactose is in equilibrium with UDP[3H]-glucose via UDP-glucose-4'-epimerase. In wild-type cells, most of the [3H]galactose supplied in complete medium is incorporated as galactose, but some is incorporated as glucose (e.g., glycolipids), or as other sugars metabolically derived from UDP-glucose (e.g., glucuronic acid, inositol, xylose). In clone 13, supplied [3H]galactose is incorporated mainly as glucose and its derivatives (unpublished data). 3 [3H]glucosamine N-acetylgalactosamine,
is
metabolically and sialic
incorporated acid.
40
as N-acetylglucosamine,
Vol. 103, No. 1,1981
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
VO
3
CLONE
COMMUNICATIONS
13 gal- ‘H
CLONE 13 glcN-‘H
2 8 2 x
’
,I
22-
z u2
I I
0
3
15
25
35
45
55
FRACTION
Figure
00
65
Ii
4 4
NO
I5
25
35 45 FRACTION
55 NO
65
3
~io-~el P-10 elution profiles of [3H]glucosamine-labeled HMWPronase digest products (V, from Figure l), after treatment with chondroitinase ABC. Upper panel, clone 13; lower panel, wild-type. Figure
4
Blo-Gel P-10 elution profiles of [3H]galactose-labeled HMW Pronase digest products (V, from Figure 2), after treatment with chondroitinase ABC. Upper panel, clone 13; lower panel, wild-type.
only
with
glucosamine,
case of clone
probably
13 (upper
panels,
~22% of the incorporated the
remaining
position rich gal
glycopeptides sequences
further.
Peak III,
In the present
mannose-rich
1 and 2), and most
glucosamine
and truncated (5).
Figs.
glucosamine,
incorporated
as wild-type
represents
(arrow,
and probably complex studies,
HMW material of the Fig.
represents
glycopeptides only
In the
glycopeptides. accounted
incorporated
1) eluted
galactose;
in
a mixture lacking
the HMW material
for
the same of mannose-
terminal
sia-
was analyzed
Vol. 103, No. 1,198l
BIOCHEMICAL
0
4
8
AND
12
BIOPHYSICAL
16 20
24
28
RESEARCH
32
36
COMMUNICATIONS
40
44
SEGMENT NUMBER Figure
5 Paper chromatography
"minor peaks" HMW material
by acid hydrolysis
from the
digestion of [3H]galactose-labeled 4). A, clone 13 peak a; B, clone indicate origin peak a; D, wild-type peak a. Arrows sample lanes were cut into l-cm segments for deterPositions of authentic standard monosaccharides,
peak 2; C, wild-type Radioactive positions. mining
of sugars released
obtained after chondroitinase (peaks 5 and a from Figure
radioactivity.
13
chromatographed on the same sheet in separate lanes between the radioactive samples, are indicated: U, glucuronic acid; gal, D(+)galactose; glc, D(+)glucose;
xyl,
D(+)xylose.
The HMW material with
each Pronase
ABC, and the products
chondroitinase
(Figs.
from
Chondroitinase
3 and 4).
and %33% of the wild
type
HMW material,
In the case of galactose-labeled products
was reproducibly
prior
to the major
minor
peaks
represent
were
Paper
sumed linkage tose
sulfate
never
sequences
disaccharides, (Fig.
resolved
observed sequences
chromatographic
and Z3H]-xylose
of A-di-4s
material, into
small-molecular-weight
GAG linkage
peptides.
degraded
by acid (Fig.
5).
digest were
(V,,
Figs.
analyzed
on the P-10
~50% of the
13 HMW material,
to small-molecular-weight
products.
%9% of the two minor
label
peaks,
at Vi
to serine
analysis
of sugars
hydrolysis
revealed
characteristic
peaks digest
6).
42
in
the digest
a and b-, eluting
(arrows,
in glucosamine-labeled
The major
column
clone
peak
attached
1 and 2) was treated
Fig.
material, or small released
products
These
4).
and probably
serine-containing from
the presence
eluting
just
these
pre-
of
[3H]galac-
at Vi mainly
consisted
of chondroitin-4-
Vol. 103, No. 1,198l
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
CHO
CLONE
SEGMENT Figure
13
NUMBER
6
Paper chromatography of chondroitinase digestion products (Vi from Figure 4). The chromatogram was cut into l-cm segments, and the radioactivity in each segment was determined. The positions of co-chromatographed authentic 4,5-unsaturated disaccharide standards are indicated: 6S, Adi-6s; 4s. Adi-4s; OS, Adi-OS. Upper panel, wild-type; lower panel, clone 13.
A
CLONE
13 glcN-
B
3H
CLONE
13
gal-
3H
I
500
1,000
500
20
30
40
50
60
20
FRACTION NO Figure
30
40
FRACTION
50
60
NO
7
Bio-Gel P-10 elution profiles of chondroitinase-resistant (Vo from Figures 3 and 4). after treatment with HONO. labeled material; B. [3H]galactose-labeled material. lower panels, wild-type.
43
HMW material A, [3H]glucosamineUpper panels, clone
13;
Vol. 103, No. 1,1981
BIOCHEMICAL
AND
The chondroitinase-resistant treated
with
column
(Fig.
free
HONO cleaves
or N-sulfated
N-acetylated
amino
residues
substituted
charides
residues
a broad
chondroitinase-resistant ly all
type
CHO cells,
of the
total
clude
that
sulfate
incorporated
label
the biosynthesis
droitinase
digestion
amount
of this
fected
by the clone
contains
less
smaller
molecular
solves
the material
is
than
size
by mild
into
it
for
CHO cells
These
asn-linked
reactions
galactosyltransfer of GAGS, which plasmic
reticulum
are
is
likely
that
is
essential-
susceptible. 13 and wildfor
in clone
con-
13 cells.
even after
chon-
Since
no appreciable
biosynthesis
is probably
indicate
little
that
at least
to
on DEAE-Sephacel
Although
af-
the material
can be converted
(9)
~11%
re-
the material(s)
a portion which
consists
has recently
have of the been
(10). reactions
involved
oligosaccharides
occur
to be defective
reactions
involved
(X,13).
its
peaks.
~~50% of the
We therefore
Chromatography
three
only
each account
7).
results
and very
known
proceed
13,
along
of oligosac-
clone
persists
Fig.
polysaccharide
The galactosyltransfer and complex
(V,,
alkali.
at least
both
sulfate
HMW material
acid,
type,
GAGS is unimpaired
Preliminary
10% sialic
distributed
from glucosamine.
in clone
13 defect.
"erythroglycan"-like
described
derived
contains
to HONO, while
for
bearing
the variously-
HMW material
and chondroitin
found
residues
mixture
susceptible
that,
and HONO treatment
been identified,
asn-linked
is
of wild-type
material
on the P-10
also
randomly
In the case of wild
of these
amounts
sulfate
a heterogeneous
can be calculated
heparan
Substantial
not yet
it
analyzed
heparan
13 chondroitinase-resistant
data,
3 and 4) was next
to HONO, and since
HMW material
of the clone From this
Since
are
range.
Figs.
COMMUNICATIONS
at glucosamine
are more-or-less
products
size
(V,,
sulfate
(8).
RESEARCH
was again
are resistant
the degradation with
mixture
heparan
groups
which
,glucosamine
the chain,
HMW material
MONO, and the reaction 7).
BIOPHYSICAL
normally
in the assembly in
in clone
the Golgi
in clone
We therefore
13,
take place
propose
44
apparatus
13 (5).
in the assembly
that
of
of glycolipids (11).
In contrast, the linkage
in the rough there
exists
the sequence endo-
a Golgi-
Vol. 103, No. 1,198l
specific clone
BIOCHEMICAL
compartmentalization
BIOPHYSICAL
problem
RESEARCH
of some kind
which
COMMUNICATIONS
accounts
for
the
13 trait. For example,
UDP-galactose
a specific from
In addition,
(15). removing the
AND
action
subsequent mechanisms
mechanism
the cytosol a further
the inhibitory
could
product
for
into
is
synthesized)
mechanism
of the
has been
galactosyltransfer
nucleotide
of UMP out account
for
it
specific
of a luminally-oriented transport
has been described
(where
of the
the clone
apparatus.
may be due to improper
insertion
of the
the Golgi
membrane,
or there
may be a defect
transports
nascent
glycoproteins
through
reaction,
UDP, by
(16,17), A defect
and in these
the clone
galactosyltranferases
in the mechanism
the Golgi
lumen
for
Alternatively,
13 trait.
13 defect
the Golgi
described
diphosphatase
Golgi
transporting
in
which
apparatus.
Acknowledgements I gratefully acknowledge the generous support, both moral and a portion of this work was of Lennart Roden, in whose laboratory The work was supported by USPHS Grants # 5 T32 AMO7069, DE 02670, AM25822. Some of the results in this report were presented as a the 1980 Annual Meeting of the American Society for Cell Biology
material, performed. and ROl poster at (14).
References 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17.
Briles, E.B., and Kornfeld, S. (1978) Trends in Biochem. Sci. 1, 223227. Wright, J.A. (1979) Int. J. Biochem. lo, 951-956. Stanley, P. (1980) in The Biochemistry of Glycoproteins and Proteoglycans (W.J. Lennarz, ed.), pp. 161-189, Plenum Publishing Co., New York. Briles, E.B. (1982) Int. Rev. Cytol., in the press. Briles, E.B., Li, E., and Kornfeld, S. (1977) J. Biol. Chem. 252, 1107-1116. Briles, E.B., Li, E., and Kornfeld, S. (1976) Fed. Proc. 35, 1642. Rod&, L. (1980) in The Biochemistry of Glycoproteins and Proteoglycans (W.J. Lennarz, ed.), pp. 267-371, Plenum Publishing Co., New York. (1976) Biochemistry 15, 3932-3942. Shively, J.E. and Conrad, H.E. (1978) J. Biol. JIrnefelt, .I., Rush, J., Li, Y-T., and Laine, R.A. Chem. 253, 8006-8009. Li, E., Gibson, R., and Kornfeld, S. (1980) Arch. Biochem. Biophys. 199, 393-399. in The Glycoconjugates (M.I. Horowitz and Schachter, H. (1978) W. Pigman, eds.), Vol. II, pp. 87-185, Academic Press, New York. (1968) J. Cell. Biol. 38, 358-368. Horwitz, A.L., and Dorfman, A. Sugahara, K., Cifonelli, J.A., and Dorfman, A. (1981) Fed. Proc. 40, 1705. (1980) J. Cell Biol. 87, 3UOa. Briles, E.B. Kuhn, N., and White, A. (1975) Biochem. .I. 148, 77-84. Kuhn, N., and White, A. (1977) Biochem. J. 168, 423-433. Brandan, E. and Fleischer, B. (1980) J. Cell Biol. 87, 200a.
45