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Dextranase activity and auxin-induced cell elongation in coleoptiles of Avena
Vol. 38, No. 5, 1970
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
DExTRANAsEAC~ITyAlpDAuxM-INDUCEDCELI,ELoncATIoB IlVCOLMlP!PILgSOFAVlU?A Anton IV. J. Eeyn Department of Biological Sciences Louisiana State University in Iiew Orleans, La.
Received December 8, 1969 Dextranase activity, so far only found in microorganisms and animals, is found to be associated with coleoptiles of Avena. Dextranase breaks down&glucans in which the glucose residues are mainly linked byi$1,6linkages. This enzyme is found to be sensitive to the plant moreover, are growth hormone, auxin. The cell walls of the coleoptiles, found to contain dextran-lib o(Tglucans which can be brolotn down by dextranase . This enzyme, therefore, seemsto meet two main requirements of an intermediate in the plasticieation of the cell wall in auxin-regulated cell elongation in coleoptiles. A knowledge of enzymes which occur in elongating plant cells and which can act on cell wall substances is of interest cell wall and its plasticity
in connection with the role of the
(1, 2, 3) in auxin-regulated
cell elongation.
A
systematic study has therefore been undertaken of such enzymes in coleoptlles Avena, the traditional a previous article
of
material for studies on auxin-induced cell elongation.
(4) four different/-glucanases
enzymes, however , probably do not participate tion because they are not sensitive
have been studied.
In
These
in hormone regulated cell elonga-
to the presence of the hormone in the
tissue. The present coxnunlcation material of an#-glucanaee,
deals with the occurrence and behavior in this
Itdextranase."
the glucose residues are linked by&1,6dextrana .
This enzyme act6 on glucans in which aad c(-1,3- bonds, so-called
It is also shownthat in the cell walls of coleoptiles,
occur which can be broken down by pure dextranaee. lngs for a further
polysacchariden
The importance of these flnd-
analysis of the meahanlemof cell elongation Is discussed.
831
BIOCHEMICAL
Vol. 38, No. 5, 1970
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
MATi-imALs
Am MEYmms
Coleoptiles of Avena sativa were grown in the dark. --
When the coleoptiles
measured about 2$ cm long, sections of 1 cm long were taken 4 zznbelow the tip. 'Ihe sections were ground or homogenized under standard conditions, fuged at 2290 x g with intermittent
washing in water.
twice eentri-
The pellets
so obtained
mainly consist of cell wall materials and were found to contain the enzyme activity,
just as in the case of the/?-glucanases studied before (4).
The specific
substrate used for demonstrating dextranase
natural dextran produced by Leuconostoc mesenteroides sample was received courtesy of Dr. A. Jeanes.
constitute
was a
NRRLB512(F), 50B. This
It had a high purity
and a
This dextran is reported to contain about
molecular weight of 20-30 million. 95s of&l,%
activity
bonds, the remaining bonds areq-1,3-
linkages, which mainly
One percent of the branches would be very long,
the branch points.
the remaining branches are believed to be as short as 1 glucose residue (5, 6). In addition,
a commercial dextran (Worthington Biochemical Corporation)
molecular weight of 2 million
of a
was used.
Two percent solutions of these dextrans were incubated with the pellet derived from 20 or 30 coleoptile
sections at 45OC and p3 5.0.
An incubation
time of 4 hours was found to be the most suitable. !l!he depolymerization
of the dextran molecule was studied viscometrically
in the usual way (6, 7) by the decrease in flowtime.
A semi-micro viscomater
of the Cannon-Manning type for volw~~a of 1 ml was used at 25.0:
Duplicate
determinations did not vary more than 2 seconds. The flowtime of the solvent (water) was 68 seconds. The products of the enzymatic degradation were studied by descending paper chromatography.
The hydrolyzates
streaked across the paper. isopropanol-acetic The locations
were concentrated from 3 ml to 0.2 ml ana
The ChmmatOgramSwere developedwith
acid-water
(54:8:18)
in the conventional manner
of the Products of hydrolysis
samples of isomaltose, isomaltotriose,
used for sugars.
were compared with those of pure
and glucose, which are the final 832
products
Vol. 38, No. 5, 1970
8lOCHEMlCAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Table
1
EFFECT OF BEATING AND OXYGEN ON THE STABILITY AND NITROGENASE ACTIVITY Treatment
of bacteroid
Electron carrier Dithionite-dependent activity1 nitrogenase activity (Ethylene produced (mumoles/min))
extract
None lOO$ 0, for Heating
34.1
92.5
4.6
0.5
34.8
2.0
2 hours
at 60'
for
OF ELECTRON CARRIER
OF RHIZOBIUM BACTEROID EXTRACTS
10 min (under
IThe electron carrier activity ability to support acetylene nitrogenase system described
argon)
of the treated extract was measured reduction in the coupled chloroplastby Yoch and Arnon (1969).
by its
The reaction mixture used to measure dithionite-dependent nitrogenase activity of the Rhizobium bacteroid extract contained, in addition to bacteroid extract (3.75 mg protein), treated as indicated, the following in urnoles: HEPES buffer, pH 7.4, 50; Mg", 5; creatine phosphate, 40; ATP, phosphokinase, 0.05 mg; and sodium dithionite, 20. To measure 4; creatine electron carrier activity, the above reaction mixture was modified by adding a washed A. vinelandii nitrogenase (4.6 mg protein) and replacing the sodium dithionite by spinach chloroplasts (300 ug chlorophyll); ascorbate, 10 umoles; and 2,6-dichlorophenol indophenol, 0.05 umoles. Final volume, 1.5 ml. Light intensity, 9,000 foot-candles. Gas phase, 7;t$ argon and 27s acetylene. The reaction was carried out at JO0 for 30 min.
The supernatant effectiveness
cant
which activity
the crude a rate
bacteroid
parallel
2.
for
contained
of
added
the washed
extract
gave a marked
column
ethylpiperazine-N'-2-ethanesulfonic
increase nitrogenase
of the bacteroid solution previously
(after
the heat
equilibrated acid)
840
buffer,
with
had an
The crude
bacteroid
showed
signifi-
the addition
of carrier
to
in nitrogenase
activity,
at
activity
electron
nitrogenase
nitrogenase
carrier
Its spinach
bacteroid
carrier.
Nevertheless,
carrier.
by illuminated
Azotobacter
and electron
to the carrier-dependent purification
generated
electron
nitrogenase carrier.
of the electron
and to the native
the bacteroid both
The supernatant
a DEAE-cellulose
power
nitrogenase
Activity
without
A further Table
1.
requirement
extract
the reducing
to Azotobacter
shown in Fig.
absolute
was used as the source
in coupling
chloroplasts is
solution
carrier
of Azotobacter. is
summarized
treatment)
was passed
0.02
M IBIPES (E-2-hydroxy-
pH 7.2.
in
through
Most of the electron
Vol. 38, No. 5, 1970
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
from 10, 20, 30, and 4.0 coleoptiles, water bath before incubation
reduced the lowering
from 15.2% of the unheated pellet These findings
respectively.
Heating
of the pellzt
of viscosity
on a
in 15 minutes
to 2.546, and in 30 minutes to O.O$.
are in agreement with the conclusion
that the decrease in
TAEUI Detiranase Activity in Pellets of 20 Avena Coleoptile Sections from Normal and Decapitated Plants by Vises of Dextran Solutions After 4 Eonrs' Incubation, as Flow in S&Wds and Percentage Decrease of Flowtime as Compared to Control Substrate. Each Figure is the Average of !Puo Viscosity Runs Which Varied Less Ehan 2 Seconds.
IWl. Substrate
alone
447
4$and 2$Dextran mol. wt. 2 million
2$ Dextran
Wt. 20-30 IBillion 450
444
460
475
260
423
-
-
475
247
Substrate digest with pellet frQmnormel coleoptile %h crease Substrate with pellet fmm decapitated coleoptile %= crease
l!miE
II
Dextranase Activity in Pellets Of 20 Avena Coleaptile Sections, Which Have Been Previously Treated or Rot Treated with Auxin. Each Figure is the Average or Two Viscosity Runs Which Varied Less Than 2 Seconds. a.
Substrate
Coleoptiles in water
410
alone
410
Substrrte with pellet fzvm hormone-treated sections %- crea6e Substrate with pellet untreated sections $ Decrease
froln 391
!m 834
b.
ColeQptiles w
352
-
317 lo.os
348
Vol. 38, No. 5, 1970
viscosity
BIOCHEMICAL
is due to the activity
term ndextranase" activity
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
of an enzyme acting on dextran.
will
therefore
In order to study the effect
The general
be used for this effect.
of the presence of the hormone, auxin, a
comparison was madebetween the activity
of pellets
from sections of normal
plants with those of plants that had been decapitated about 2& hours prior the preparation tissue.
of the pellet,
so as to decrease the hormone content of the
From Table I it is seen that the activity
is much less than that of normal coleoptiles. decapitation,
and 6.6
to
3% hours after
of the decapitated coleoptiles
The activity
decapitation.
is 0.6
2$ hours after
The higher value after
&
hours is no doubt due to the known regeneration of a hormone-producing tip. The effect
of the hormone was further
sections which had been placed for lor auxin (Table II,a),
studied by comparing the activity
of
2 hours in water with or without 8 ppm
and of sections which remsined in the dry state,
of which
the tips had been powdered with sometalcum with or without someindole In each of the two sets of two experiments the
acetic acid (Table 11,b). activity viscosity
of the hormone-treated plant8 was larger, being 24 seconds or about 6$.
flowtime with 4 comparable pellets
!Pheaverage deviation
from normal coleoptiles,
with 3 cc of a samedextran solution,
cell valls.
incubated for 4 hour8
of a pure dextran and of
of the natural dextran,
dextranase are given in Table III. of glucose.
The mobilities
!jOB, by a purified Rg are represented as frac-
By comparing these mobilities
pure sugars, the products of degradation by the purified fiea as ieomaltose, isomaltotriose,
consisting of substances of very low mobility
enzyme could be iaenti-
In addition,
linkages.
for normal dextranase activity
835
a spot
was seen. These substances must
someof which contain the d-1,3-
products observed are typical
with those of
and in somecases also isomaltotetrose.
Glucose was only present in a very low concentration.
be poly8accharides,
from the mean
The results of the paper chromatographic analysis of
the products of hydrolysis
tions of the mobility
in
was 3 seconds (0, 2, 4, 6 seconds).
Chromatography of dextranase hydrolyzates coleoptile
the average difference
The degradation (8,
9, 10, 11, 12).
BIOCHEMICAL
Vol. 38, No. 5, 1970
AND 8lOPHYSlCAL
RESEARCH COMMUNICATIONS
TABLEIII Rydrolysis Products of a Natural Dextran and of Cell Wall Material of Coleoptiles Acted on by a Purified Dextranase. Dextran mol.wt. 20-30 million
Component Rg
Oligosacchgricles
weak
weak
0.13
Isomaltotetrose
weak
none
0.26
Isomaltotriose
weak
medium
0.52
Isomaltose
strong
strong
1.00
Glucose
weak
medium
0.66
none
weak
1.13
none
mdium
Unidentified Rs. Rf3
Coleoptile cell walls
spots:
In order to determine whether or not substances are present in the cell walls of these coleoptiles pellets
which can be broken down by dextranase, cell wall
were digested for 4 or 12 hours at 45oC with the purified
The sameproducts of hydrolysis
resulted from the digestion of the pellets
from the digestion of pure dextrans by this enzyme (Table XII). the isomaltotriose hyarolyzate.
dextranase.
spot was clearly
as
Particularly
marked in the chromatogram from the pellet
In addition to the spots of the isomaltose series, two unidenti-
fied weaker spots were present. From these findings it may be concluded that dextran-like
polysaccharides
occur in these cell walls and that these substances can be acted upon by dextranase. CONCLUSIOR From the above experiments it may be concluded that dextranase activity present in coleoptiles
of Avena, and that the enzyme is sensitive
of auxin, being higher at higher auxin concentration. coleoptiles
contain dextran-like
to the presence
The cell walls of the
substances in which the dextranase can
836
is
act.
Vol, 38, No. 5, 1970
l?atural
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
dextrans are generally
highly branched.
substances probably form a continuous network.
In the cell wall these
The above experiments suggest
that this network is broken down under the influence of the dextranase acting on Fhe cell wall.
This will
lower the plasticity
similar to the lowering of the viscosity It is concluded that a specific
of the dextran solutions investigated.
enzyme has been found which meets the two
main requirements of an intermediate auxin-regulated.cell
of the cell wall in a way
in the plasticization
elongation in coleoptiles
of the cell wall in
of Avena.
REFmmcEs 1.
Hey-n, A. 19. J., Proc. Setherl.
2.
Heyn, A. H. J., Rec. Trav. Rot. Nkerl. 28, 113 (1931).
3.
Heyn, A. B. J., Rot. Review 6, 515 (190).
4.
Heyn, A. B. J., Arch. Biochem. and Biophy8. B,
5.
Jeanes, A., I?. C. Haynes, J. C. Wilham, E. H. Bankin, E. H. Melvin, A. J. Austin, J. C. Cluakiey, B. E. Fisher, H. M. Tsuchiya, and C. E. Blst, J. Am. Chem. Sm. 76, 5041 (19%).
6.
Bovey, F. A., J. Polymer
7.
Granath, K. A., J. couoia
8.
Jamon, J.-Chriater, and J. Porath in "M&hods in Enzymology" (E. F. Seufleld and V. Ginsburg ede. j %?a. x111, p. 615. AC~L&&C PF~SS, Bew York, 1966.
sci.
Roy. Aced. Sci. &
474, (1931).
442 (1969).
s
167, 183 (1959).
sci. l&
308 (1958).
9* Bowrne, E. J., D. H. Hutson, and H. Weigel, Biochem. J. &,.158
(1962).
10.
Bourne, E. J., D. H. Ilutson, and H. Weigel, Biochem. J. 86, 555 (1963).
11.
Hutson, D. H., and H. Welgel, Bioohem. J. s
L-2.
Reese, E. T., and F. W. Parrish,
588 (1963).
Biopolymers h 1043 (1966).
837
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
DExTRANAsEAC~ITyAlpDAuxM-INDUCEDCELI,ELoncATIoB IlVCOLMlP!PILgSOFAVlU?A Anton IV. J. Eeyn Department of Biological Sciences Louisiana State University in Iiew Orleans, La.
Received December 8, 1969 Dextranase activity, so far only found in microorganisms and animals, is found to be associated with coleoptiles of Avena. Dextranase breaks down&glucans in which the glucose residues are mainly linked byi$1,6linkages. This enzyme is found to be sensitive to the plant moreover, are growth hormone, auxin. The cell walls of the coleoptiles, found to contain dextran-lib o(Tglucans which can be brolotn down by dextranase . This enzyme, therefore, seemsto meet two main requirements of an intermediate in the plasticieation of the cell wall in auxin-regulated cell elongation in coleoptiles. A knowledge of enzymes which occur in elongating plant cells and which can act on cell wall substances is of interest cell wall and its plasticity
in connection with the role of the
(1, 2, 3) in auxin-regulated
cell elongation.
A
systematic study has therefore been undertaken of such enzymes in coleoptlles Avena, the traditional a previous article
of
material for studies on auxin-induced cell elongation.
(4) four different/-glucanases
enzymes, however , probably do not participate tion because they are not sensitive
have been studied.
In
These
in hormone regulated cell elonga-
to the presence of the hormone in the
tissue. The present coxnunlcation material of an#-glucanaee,
deals with the occurrence and behavior in this
Itdextranase."
the glucose residues are linked by&1,6dextrana .
This enzyme act6 on glucans in which aad c(-1,3- bonds, so-called
It is also shownthat in the cell walls of coleoptiles,
occur which can be broken down by pure dextranaee. lngs for a further
polysacchariden
The importance of these flnd-
analysis of the meahanlemof cell elongation Is discussed.
831
BIOCHEMICAL
Vol. 38, No. 5, 1970
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
MATi-imALs
Am MEYmms
Coleoptiles of Avena sativa were grown in the dark. --
When the coleoptiles
measured about 2$ cm long, sections of 1 cm long were taken 4 zznbelow the tip. 'Ihe sections were ground or homogenized under standard conditions, fuged at 2290 x g with intermittent
washing in water.
twice eentri-
The pellets
so obtained
mainly consist of cell wall materials and were found to contain the enzyme activity,
just as in the case of the/?-glucanases studied before (4).
The specific
substrate used for demonstrating dextranase
natural dextran produced by Leuconostoc mesenteroides sample was received courtesy of Dr. A. Jeanes.
constitute
was a
NRRLB512(F), 50B. This
It had a high purity
and a
This dextran is reported to contain about
molecular weight of 20-30 million. 95s of&l,%
activity
bonds, the remaining bonds areq-1,3-
linkages, which mainly
One percent of the branches would be very long,
the branch points.
the remaining branches are believed to be as short as 1 glucose residue (5, 6). In addition,
a commercial dextran (Worthington Biochemical Corporation)
molecular weight of 2 million
of a
was used.
Two percent solutions of these dextrans were incubated with the pellet derived from 20 or 30 coleoptile
sections at 45OC and p3 5.0.
An incubation
time of 4 hours was found to be the most suitable. !l!he depolymerization
of the dextran molecule was studied viscometrically
in the usual way (6, 7) by the decrease in flowtime.
A semi-micro viscomater
of the Cannon-Manning type for volw~~a of 1 ml was used at 25.0:
Duplicate
determinations did not vary more than 2 seconds. The flowtime of the solvent (water) was 68 seconds. The products of the enzymatic degradation were studied by descending paper chromatography.
The hydrolyzates
streaked across the paper. isopropanol-acetic The locations
were concentrated from 3 ml to 0.2 ml ana
The ChmmatOgramSwere developedwith
acid-water
(54:8:18)
in the conventional manner
of the Products of hydrolysis
samples of isomaltose, isomaltotriose,
used for sugars.
were compared with those of pure
and glucose, which are the final 832
products
Vol. 38, No. 5, 1970
8lOCHEMlCAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Table
1
EFFECT OF BEATING AND OXYGEN ON THE STABILITY AND NITROGENASE ACTIVITY Treatment
of bacteroid
Electron carrier Dithionite-dependent activity1 nitrogenase activity (Ethylene produced (mumoles/min))
extract
None lOO$ 0, for Heating
34.1
92.5
4.6
0.5
34.8
2.0
2 hours
at 60'
for
OF ELECTRON CARRIER
OF RHIZOBIUM BACTEROID EXTRACTS
10 min (under
IThe electron carrier activity ability to support acetylene nitrogenase system described
argon)
of the treated extract was measured reduction in the coupled chloroplastby Yoch and Arnon (1969).
by its
The reaction mixture used to measure dithionite-dependent nitrogenase activity of the Rhizobium bacteroid extract contained, in addition to bacteroid extract (3.75 mg protein), treated as indicated, the following in urnoles: HEPES buffer, pH 7.4, 50; Mg", 5; creatine phosphate, 40; ATP, phosphokinase, 0.05 mg; and sodium dithionite, 20. To measure 4; creatine electron carrier activity, the above reaction mixture was modified by adding a washed A. vinelandii nitrogenase (4.6 mg protein) and replacing the sodium dithionite by spinach chloroplasts (300 ug chlorophyll); ascorbate, 10 umoles; and 2,6-dichlorophenol indophenol, 0.05 umoles. Final volume, 1.5 ml. Light intensity, 9,000 foot-candles. Gas phase, 7;t$ argon and 27s acetylene. The reaction was carried out at JO0 for 30 min.
The supernatant effectiveness
cant
which activity
the crude a rate
bacteroid
parallel
2.
for
contained
of
added
the washed
extract
gave a marked
column
ethylpiperazine-N'-2-ethanesulfonic
increase nitrogenase
of the bacteroid solution previously
(after
the heat
equilibrated acid)
840
buffer,
with
had an
The crude
bacteroid
showed
signifi-
the addition
of carrier
to
in nitrogenase
activity,
at
activity
electron
nitrogenase
nitrogenase
carrier
Its spinach
bacteroid
carrier.
Nevertheless,
carrier.
by illuminated
Azotobacter
and electron
to the carrier-dependent purification
generated
electron
nitrogenase carrier.
of the electron
and to the native
the bacteroid both
The supernatant
a DEAE-cellulose
power
nitrogenase
Activity
without
A further Table
1.
requirement
extract
the reducing
to Azotobacter
shown in Fig.
absolute
was used as the source
in coupling
chloroplasts is
solution
carrier
of Azotobacter. is
summarized
treatment)
was passed
0.02
M IBIPES (E-2-hydroxy-
pH 7.2.
in
through
Most of the electron
Vol. 38, No. 5, 1970
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
from 10, 20, 30, and 4.0 coleoptiles, water bath before incubation
reduced the lowering
from 15.2% of the unheated pellet These findings
respectively.
Heating
of the pellzt
of viscosity
on a
in 15 minutes
to 2.546, and in 30 minutes to O.O$.
are in agreement with the conclusion
that the decrease in
TAEUI Detiranase Activity in Pellets of 20 Avena Coleoptile Sections from Normal and Decapitated Plants by Vises of Dextran Solutions After 4 Eonrs' Incubation, as Flow in S&Wds and Percentage Decrease of Flowtime as Compared to Control Substrate. Each Figure is the Average of !Puo Viscosity Runs Which Varied Less Ehan 2 Seconds.
IWl. Substrate
alone
447
4$and 2$Dextran mol. wt. 2 million
2$ Dextran
Wt. 20-30 IBillion 450
444
460
475
260
423
-
-
475
247
Substrate digest with pellet frQmnormel coleoptile %h crease Substrate with pellet fmm decapitated coleoptile %= crease
l!miE
II
Dextranase Activity in Pellets Of 20 Avena Coleaptile Sections, Which Have Been Previously Treated or Rot Treated with Auxin. Each Figure is the Average or Two Viscosity Runs Which Varied Less Than 2 Seconds. a.
Substrate
Coleoptiles in water
410
alone
410
Substrrte with pellet fzvm hormone-treated sections %- crea6e Substrate with pellet untreated sections $ Decrease
froln 391
!m 834
b.
ColeQptiles w
352
-
317 lo.os
348
Vol. 38, No. 5, 1970
viscosity
BIOCHEMICAL
is due to the activity
term ndextranase" activity
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
of an enzyme acting on dextran.
will
therefore
In order to study the effect
The general
be used for this effect.
of the presence of the hormone, auxin, a
comparison was madebetween the activity
of pellets
from sections of normal
plants with those of plants that had been decapitated about 2& hours prior the preparation tissue.
of the pellet,
so as to decrease the hormone content of the
From Table I it is seen that the activity
is much less than that of normal coleoptiles. decapitation,
and 6.6
to
3% hours after
of the decapitated coleoptiles
The activity
decapitation.
is 0.6
2$ hours after
The higher value after
&
hours is no doubt due to the known regeneration of a hormone-producing tip. The effect
of the hormone was further
sections which had been placed for lor auxin (Table II,a),
studied by comparing the activity
of
2 hours in water with or without 8 ppm
and of sections which remsined in the dry state,
of which
the tips had been powdered with sometalcum with or without someindole In each of the two sets of two experiments the
acetic acid (Table 11,b). activity viscosity
of the hormone-treated plant8 was larger, being 24 seconds or about 6$.
flowtime with 4 comparable pellets
!Pheaverage deviation
from normal coleoptiles,
with 3 cc of a samedextran solution,
cell valls.
incubated for 4 hour8
of a pure dextran and of
of the natural dextran,
dextranase are given in Table III. of glucose.
The mobilities
!jOB, by a purified Rg are represented as frac-
By comparing these mobilities
pure sugars, the products of degradation by the purified fiea as ieomaltose, isomaltotriose,
consisting of substances of very low mobility
enzyme could be iaenti-
In addition,
linkages.
for normal dextranase activity
835
a spot
was seen. These substances must
someof which contain the d-1,3-
products observed are typical
with those of
and in somecases also isomaltotetrose.
Glucose was only present in a very low concentration.
be poly8accharides,
from the mean
The results of the paper chromatographic analysis of
the products of hydrolysis
tions of the mobility
in
was 3 seconds (0, 2, 4, 6 seconds).
Chromatography of dextranase hydrolyzates coleoptile
the average difference
The degradation (8,
9, 10, 11, 12).
BIOCHEMICAL
Vol. 38, No. 5, 1970
AND 8lOPHYSlCAL
RESEARCH COMMUNICATIONS
TABLEIII Rydrolysis Products of a Natural Dextran and of Cell Wall Material of Coleoptiles Acted on by a Purified Dextranase. Dextran mol.wt. 20-30 million
Component Rg
Oligosacchgricles
weak
weak
0.13
Isomaltotetrose
weak
none
0.26
Isomaltotriose
weak
medium
0.52
Isomaltose
strong
strong
1.00
Glucose
weak
medium
0.66
none
weak
1.13
none
mdium
Unidentified Rs. Rf3
Coleoptile cell walls
spots:
In order to determine whether or not substances are present in the cell walls of these coleoptiles pellets
which can be broken down by dextranase, cell wall
were digested for 4 or 12 hours at 45oC with the purified
The sameproducts of hydrolysis
resulted from the digestion of the pellets
from the digestion of pure dextrans by this enzyme (Table XII). the isomaltotriose hyarolyzate.
dextranase.
spot was clearly
as
Particularly
marked in the chromatogram from the pellet
In addition to the spots of the isomaltose series, two unidenti-
fied weaker spots were present. From these findings it may be concluded that dextran-like
polysaccharides
occur in these cell walls and that these substances can be acted upon by dextranase. CONCLUSIOR From the above experiments it may be concluded that dextranase activity present in coleoptiles
of Avena, and that the enzyme is sensitive
of auxin, being higher at higher auxin concentration. coleoptiles
contain dextran-like
to the presence
The cell walls of the
substances in which the dextranase can
836
is
act.
Vol, 38, No. 5, 1970
l?atural
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
dextrans are generally
highly branched.
substances probably form a continuous network.
In the cell wall these
The above experiments suggest
that this network is broken down under the influence of the dextranase acting on Fhe cell wall.
This will
lower the plasticity
similar to the lowering of the viscosity It is concluded that a specific
of the dextran solutions investigated.
enzyme has been found which meets the two
main requirements of an intermediate auxin-regulated.cell
of the cell wall in a way
in the plasticization
elongation in coleoptiles
of the cell wall in
of Avena.
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837