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Increased spermidine or spermine level is essential for hepatocyte growth factor-induced DNA synthesis in cultured rat hepatocytes
GASTROENTEROLOGY 1994;106:1024-1031
Increased Spermidine or Spermine Level is Essential for Hepatocyte Growth Factor-Induced DNA Synthesis in Cultured Rat Hepatocytes IKKO HIGAKI,* ISA0 and SHUZO OTANI*
MATSUI-YUASA,’
MASANOBU
TERAKURA,*
HIROAKI
KINOSHITA,§
*Second Department of Biochemistry, Osaka City University Medical School; ‘Department of Food and Nutrition, Faculty of Science of Living, Osaka City University; and “Second Department of Surgery, Osaka City University Medical School, Osaka, Japan
Background/Aims: Hepatocyte growth factor is a potent mitogen for mature hepatocytes and seems to act as a trigger for liver regeneration. Hepatocyte growth factor was first purified from human and rabbit plasma and rat platelets. Additionally, putrescine, spermidine, and spermine are widely distributed in many different cells; intracellular concentrations of these polyamines are closely related to cell proliferation. The present study examined whether polyamine metabolism is involved in hepatocyte growth factor-induced DNA synthesis in primary cultured rat hepatocytes. Methods: Hepatocy-tes were isolated from rats by the collagenase perfusion method. Ornithine decarboxylase and Sadenosylmethionine decarboxylase activities were measured as the release of 14C02 from L-[1-14C]ornithine and Sadenosyl-L-[carboxyI-14C]methionine, respectively. Results: a-Difluoromethylornithine inhibited hepatocyte growth factor-induced DNA synthesis by only 21%. On the other hand, methylglyoxal bis(guanylhydrazone) completely inhibited hepatocyte growth factorinduced DNA synthesis to nontreated control level. The inhibitory effect of methylglyoxal bis(guanylhydrazone) on hepatocyte growth factor-induced DNA synthesis was reversed by exogenously added spermidine or spermine. Conclusions: Spermidine or spermine is essential for hepatocyte growth factor-induced DNA synthesis in primary cultured rat hepatocytes.
many
different
polyamines
H
for mature
factor
hepatocytes
(HGF)
and seems
for liver regeneration
after various
purified
and rabbit
based
from
on its ability
tocytes.“2 with
human
HGF
hepatic
animals
with
kinetics
of this
round
of DNA
gesting
that
levels
experimentally response synthesis HGF
plays
stimuli.
regeneration
forms
of liver injury,
ischemia,”
nine
HGF
in a time-
of rat hepa-
in the plasma
in the
plasma3
induced is rapid during a key
and
liver damage. precedes
the
in initiating
of The first sugthis
process.3*4 Putrescine,
spermidine,
and
spermine
the
after
activities
of
S-adenosylmethiokey
enzymes
in mammalian
many
liver
and polyamines The
and
pathway
many
different
of the cells, are
growth-pro-
reported
and
that HGF
dose-dependent
rat hepatocytes.13
ined
the
role
of ODC,
of polyamine and
is essential cultured
inhibitor
in primary study,
cul-
we exam-
by
using
a-
inhibi-
bis(guanylhydrazone) of SAMDC,
and
level of spermidine
for HGF-induced
activity
an irreversible
methylglyoxal
cellular
ODC
metabolism
(DFMO),
a reversible
that an increased
fashion
In the present
difluoromethylornithine (MGBG),
induced
DNA
found
or spermine
synthesis
in primary
rat hepatocytes.
Materials and Methods Materials Male Wistar rats weighing 150-200 g were used for preparation of hepatocytes. The protocol of the experiment was by the Animal
Research
care of the animals of this institution
Committee
of Osaka City
was in accordance
Osaka City University). Insulin, dexamethasone, spermidine, spermine, and S-adenosyl-L-methionine products
of Sigma Chemical
with
the
(Guide for AnimaL Experimentation, putrescine, were the
Co. (St. Louis, MO). MGBG
was
of patients or serum*
liver regeneration, role
increased
tured
standards
was first
regeneration. (ODC)
from
hepatectomy,‘.”
stimuli.5~6”2
We recently
tor
for recovery
(SAMDC),
biosynthetic
of these
proliferation.5.6
liver injury,‘“*”
for liver
decarboxylase
moting
cell
such as partial
decarboxylase
dramatically
to
is important
are responsible
polyamine
concentrations
related
and chemical
ornithine
University;
and rat platelets
mitogenesis
increase and
mitogen
to act as a trigger
plasma
to stimulate
failure’
is a potent
closely
Liver
approved growth
epatocyte
cells; intracellular are
are found
in
Abbreviations used in this paper DFMO, adifluoromethylornithine; HGF, hepatocyte growth factor; MGBG, methylglyoxal bis(guanylhydrazone); ODC, ornithine decarboxylase; PCNA, proliferating cell nuclear antigen; PVDF, polyvinyldifluoride; rhHGF, recombinant human hepatocyte growth factor: SAMDC, Sadenosylmethionine decarboxylase; SDS, sodium dodecyl sulfate; TBST, Tris-buffered saline containing 0.05% Tween 20. 0 1994 by the American Gastroenterological Association 0016-5065/94/$3.00
April 1994
POLYAMINE
purchased
from Aldrich
L-[l-‘“C]otnithine methionine
from Nippon
cell nuclear antigen
(Arkansas)
was from
human Ltd.
growth
(Tokushima,
Research
Japan)
Institute,
Hepatocyte Male cytes judged
from
Viability by ttypan
purity
immu-
> 99%) (Mettell
1 X lo-’
L dexamethasone. in a humidified changing
in the absence hours.
Then
thHGF
were
was
and harvested
Protein
CO,
concentrations
of radioactivity
as
as described counts
in 35-
DNA
from
The
a tubber
policeman
containing ylene
in 300
diaminetettaacetic
air. After
for additional
fresh
medium
thiothteitol. minutes
and were
at 4°C.
Then
16
0.25
and 80 nmol of L-otnithine stopper
syringe
needle.
350 absorbed transferred
(5 pL). The
on the paper disk, Daiichi
was measured 5801; mined
Beckman,
Tokyo,
by the release
‘“Clmethionine.‘”
The
was trapped
incubated
was sealed syringe
nee-
(Sigma
to
protein
Chemical
(Packon the
sodium
(SDS),
0.15
scintillation
SAMDC
were
The
as
amount
of Button.“.‘”
were washed
1% Nonidet
deoxycholate, mol/L NaCl,
of
Calf thy-
for 3 minutes
to PVDF
membrane
was blocked
albumin).
the PVDF
Tween (1:500
lin G conjugated After
developed
of SDS Protein
protein
Twenty
once
with
assay kit
micrograms gels and casein.
Ttis-buffeted
saline
TBST
with a chemiluminescent
and incu-
and 0.2%
with the primary three
times
with
bovine
antibody,
with
with anti-mouse
washing
transfer,
0.5%
(5 minutes)
in 0.05%
was washed
with
TBST
(5
immunoglobu-
with horse radish petoxidase
extensive
gel electto-
of Laemmli.”
at 4°C
20 (TBST)
each) and incubated
Cells
in the presence
After electtophotetic
After incubation
membrane
at 4°C.
SDS-polyactylamide
overnight
was washed
Co.), sulfate
and 2 mmol/L
by a Bio-Rad
membrane.
bated in anti-PCNA serum
PAGE
as a standard.
was run on 12.5%
0.05%
Chemical dodecyl
minutes
to the method
transferred
phos-
at 100,OOOg for 30 minutes
buffet.
of protein
containing
(Sigma EDTA,
for 30
with
in SDS-polyactylamide
sample
the paper
times
10 mmol/L Ttis-HCl
sodium
1 mmol/L
fluoride
were measured
Then
P-40
by centtifugation
(PAGE)
three
with
0.1%
concentrations
(1:2500
TBST,
detection
in 0.5%
the blots
were
system.
Measurement of Polyamine Concentrations
(LS
was detet-
washed
was measured
was expressed
of DNA.
saline and disrupted
according
The incubated
S-adenosyl-L-[catboxyl-
cells
incorporation
fluid
counter
activity
The incorporation
Co.) was used as a standard.
was performed
Radioactivity
scintillation
from
photesis
TBST).
by the Soluene-
Japan).
Fraction
fraction
by the method
hepatocytes
0.5%
minutes
and the paper disk was then
liquid
Japan).
di-
(5 FL)
IL) was impaled
Tokyo,
of 14C02
7.5)
was added to
test tube
The
using bovine serum albumin
at 30,OOOg for 20
5 mL toluene
Chemicals,
in a Beckman
(pH
50 PL Soluene-350
Grove,
The CO* released
with
mmol/L
with a disposable
to a vial containing
(Omnifluot;
Ttis
PCi of L-El-‘*C]otnithine
Co., Downers
washed
by three cycles of freezing
dle. A paper disk (8 mm) containing ard Instrument
were
and 2.5
centrifuged
equipped
The
was added to the cell cul-
pet microgram
(pH 7.5) containing
and boiled
0.1 mmol/L eth-
90 PL of the supetnatant
a glass tube containing with a tubber
cells
phosphate,
(EDTA),
then
PL). similar
of [3H]Thymidine Into Acid-Insoluble
previously.”
Rat
with
saline and harvested
The cells were disrupted
and thawing
(5
of 14C02 pto-
by a Bio-Rad
into the acid-insoluble
phate-buffeted
by the release of ‘“CO2
/.LLof 50 mmol/L
acid
tube
Western Blot Analysis
cells were cultured
incubated
200 pmol/L pytidoxal
at 4°C.
to a glass
VA) using bovine serum albu-
(1 PCiidish)
was determined
mus DNA
times.
was determined
L-[1-‘4C]ornithine.‘5
were measured
Richmond,
pet minute
moli
of Enzyme Activities
three times with phosphate-buffeted
and thawing
by estimation
ture 4 hours before the cells were harvested.
were pelleted
activity
was added
The
used in assay of ODC activity.
phenylmethylsulfonyl
ODC
of freezing
S-adenosyl-L-methionine
{‘H]Thymidine
the
>95%
and 95%
in the
at the indicated
Measurement
2.8
phosphate.
from S-adenosyl-L-[catboxyl-‘4C]methionine
at 37°C for 24 hours
and hormones
cultured
pytidoxal
cycles
phosphate
dithiothteitol,
at 30,OOOg for 20 minutes
was measured
min as a standard.
perfusion
and 1 X lo-’
with fresh medium,
of the serum cells
nmol
Dow
Hepato-
collagenase
The cells were cultured
the medium
20
activity
assay kit (Bio-Rad,
before
The cells were plated
of 5%
by three
Measurement Incorporation
water freely.
mol/L insulin,
atmosphere
and
duced
mmol/L
1025
PCi S-adenosyl-L-[catboxyl-‘4C]methionine
Co.
mm collagen-coated dishes at a density of 5 X lo4 cells.0.2 mL-’ . cm-’ m Williams’ medium E supplemented with 5% fetal calf serum,
PL)
the method
and
1.1
and 200 PmoliL
0.125
SAMDC
te-
Pharmaceutical
hepatocytes
blue exclusion.
(5
was from
for 18 hours
by the
of isolated
containing
PL of the supetnatant
containing
and Culture
to drink
tats
in 300 PL of 55 mmol/L sodium
7.5)
were disrupted 90
PROLIFERATION
respectively.
tats were fasted
isolated
[mouse])
IN HEPATOCYTE
and were then centrifuged Then
Recombinant
P. McCann
OH),
but were allowed
were
method.”
and Dr.
Preparation
Wistat
experiments
MA).
by Otsuka
Cincinnati,
was
proliferating
anti-mouse
factor (thHGF;
supplied
(pH
cells
petoxidase
(Boston,
policeman
buffet
(Buckinghammembrane
blot chemiluminescence
NEN
tubber
mmol/L puttescine,
anti-PCNA
Denmark);
and Western
were kindly
and
(31 Ci/mmol)
Japan);
with horseradish
DuPont
hepatocyte
DFMO
(PVDF)
(monoclonal
(Glosttup,
G conjugated
Pel-Fteet
International
Co. Ltd. (Tokyo,
(PCNA)
was from Dakopatts
agent
and [6-3H]thymidine
Polyvinyldifluotide
Genetics
WI),
S-adenosyl-L-[catboxyl-‘“C]-
from Ametsham
England).
noglobulin
Co. (Milwaukee,
Ciimol),
(57 Ci/mol),
were purchased shire,
Chemical
(53
METABOLISM
with
a
liceman
in 300
cells were harvested
PL of ice-cold
with a tubber
5% ttichlotoacetic
po-
acid centti-
1026
HIGAKI
GASTROENTEROLOGY
ET AL.
fuged for removal
of the protein.
amine
in the acid extract
liquid
chromatography
Japan)
equipped
of polyamine
(Shimadzu
with fluorescence
was performed
150 mm; particle
The concentration
was analyzed
detector.*’ Shimadzu
ric acid as solvent A and solvent A-methanol was eluted
with solvent
solvent
B at 4°C for 3 minutes
solvent
gradient
The gradient 22 minutes concentrations
using
The separation (4.6 X
Techno-Research of 10 mmol/L
l-
changed
(1:3) as solvent
A at 96°C and with
and then with a programmed
the linear
gradient
curve number
from 4°C to 55°C with
at a flow rate of 0.7 mlimin. were expressed
as picomoles
Various
Kyoto,
acid sodium salt- 100 mmol/L sodium perchlo-
B. The sample
Results
of poly-
LC-6A; Shimadzu,
Inc., Kyoto, Japan) with a solvent composed hexanesulfonic
No. 4
by high-performance
on a STR ODS-II column
size, 5 pmol/L;
Vol. 106,
solvent
cells, and the activities
of ODC (Figure
B in of
DNA.
1A) and SAMDC
6 hours after the addition (Figure 1B) were determined in primary cultured rat hepatocytes. Both of the enzyme activities
began
to increase
reached a maximum
with
with
1 ng/mL
5 ng/mL
(Figure activity
increased
and
HGF. 4 hours
of HGF and peaked at 8 hours; thereaf-
2A). To determine is required
we used DFMO.
HGF
(60 pmol/L)
Figure 2A shows that ODC activity after the addition
ter it decreased and returned 0.
The polyamine per micrograms
of HGF were added to the
concentrations
to O-hour level by 16 hours whether
an increase
for HGF-induced
Five millimolars
DNA
of DFMO
inhibited
the increase
in ODC activity
inhibited
HGF-induced
C3H]thymidine
in ODC synthesis,
completely
(Figure
2A) but
incorporation
by
Statistical Analysis The results are expressed cance of differences t test. Differences
as means t SD. The signifi-
in assay values was evaluated
by Student’s
with P values < 0.05 were considered
sig-
nificant.
“0
Figure 1. Effect of HGF on (A) ODC and (6) SAMDC activity in primary cultured rat hepatocytes. The cells were cultured as described in Materials and Methods. The culture medium was changed with the addition of HGF at the various concentrations, and cells were cultured for 6 hours. Values are expressed as means + SD of five dishes. *P < 0.01 compared with 0 ng/mL HGF. **P < 0.05 compared with 0 ng/mL HGF.
4
(I
1ime
12
16
:
P.
after HGF (hr)
figure 2. (A) Time course of ODC activity in primary cultured rat hepatocytes after the addition of HGF and DFMO. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence (0) or presence (0) of 5 mmol/L DFMO. Values are expressed as means 2 SD of five dishes. *P < 0.01 compared with the presence of DFMO. **P i 0.05 compared with the presence of DFMO. (6) Effect of exogenously added putrescine, spermidine, or spermine on [3H]thymidine incorporation in primary cultured rat hepatocytes treated with DFMO. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of 5 mmol/L DFMO. At 8 hours, 0.1 mmol/L putrescine (Put), 0.1 mmol/L spermidine (Spd), or 0.1 mmol/L spermine (Spm) was added. A 4-hour pulse of [3H)thymidine (1 pCi/dish) was begun 20 hours after the addition of HGF. Incorporation is expressed as means 2 SD of five dishes. “P < 0.01 compared with control; “P < 0.01 compared with the addition of HGF: ‘P < 0.01 compared with the addition of HGF in the presence of DFMO.
POLYAMINE METABOLISM
April 1994
only 21% (Figure
2B). The inhibitory
on HGF-induced
13H]thymidine
versed by exogenously
added 0.1 mmol/L
was re-
putrescine,
mmol/L spermidine, or 0.1 mmol/L spermine after HGF and DFMO addition (Figure 2B). As shown in Figure
3A, SAMDC
hours after the addition remained
at a high
L spermine
effect of DFMO
incorporation
activity
0.1
8 hours
increased
3
of HGF, peaked by 6 hours, and
level until
12 hours.
Thereafter
it
addition To
IN HEPATOCY-TE PROLIFERATION
was added exogenously
8 hours after MGBG
3B).
(Figure determine
HGF-induced
which
DNA
polyamine
synthesis,
addition
of DFMO
addition
and MGBG
of 5 mmol/L
DFMO
completely
inhibited
corporation
to nontreated
is
(Figure
control
level;
spermine
crease in SAMDC
DFMO
and MGBG
caused by HGF MGBG
HGF-induced
{3H]thymidine
treated
level; these inhibitory
control
were reversed when 0.1 mmol/L
(Figure
completely incorporation
3A).
inhibited to
non-
effects of MGBG
spermidine
or 0.1 mmoli
addition.
when 0.1 mmol/L
levels of PCNA (Figure showed
DNA
HGF-induced
spermidine hepatocyte
leled that seen in Figure Dose responses
proliferation.
inhibition
at 20 pmol/L.
amine concentrations tine concentration
Figure 3. (A) Time course of SAMDC activity in primary cultured rat hepatocytes after the addition of HGF and MGBG. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence (0) or presence (0) of 20 umol/L MGBG. Values are expressed as means 2 SD of five dishes. *P < 0.01 compared with the presence of MGBG. (8) Effect of exogenously added spermidine or spermine on [3H]thymidine incorporation in primary cultured rat hepatocytes treated with MGBG. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of 20 pmol/L MGBG (MGBGzO) or 30 pmol/L MGBG (MGBG,O). At 8 hours, 0.1 mmol/L spermidine or 0.1 mmol/L spermine was added. A 4-hour pulse of [3Hjthymidine (1 @/dish) was begun 20 hours after the addition of HGF. Values are expressed as means 2 SD of five dishes. aP < 0.01 compared with control; bP i 0.01 compared with the addition of HGF; ‘P < 0.01 compared with the addition of HGF in the presence of MGBG (20 pmol/L): dP < 0.01 compared with the addition of HGF in the presence of MGBG (30 umol/L).
also for
This result paral-
effects on SAMDC
activity
are shown in Figure 6A displaying
7.5 pmol/L
MGBG
The effects of HGF and polyamine Time after HGF (hr)
of PCNA is necessary
4.
incorporation
at roughly
protein
of cell proliferation
blot analysis
and B. Both curves are similar, inhibition
reversed
is important
we measured
or spermine
of MGBG
and [iHfthymidine
or spermine marker
5A and B). Western that
the inhibitory
was added exogenously.
synthesis,
as another
or 0.1
8 hours after
was not completely
that spermidine
for HGF-induced
in-
spermidine
In contrast,
putrescine
MGBG
the inhibitory
was added exogenously
effect of DFMO and MGBG To confirm
4). Combined
[‘H)thymidine
mmol/L
activity
for
combined
and 20 pmol/L
HGF-induced
effect was reversed when 0.1 mmol/L
20 and 30 pmol/L
essential
we examined
decreased and returned to O-hour level by 18 hours. Twenty-micromolar MGBG completely inhibited the inBoth
1027
half-maximal and maximal
inhibitors
on poly-
are shown in Figure 7. The putrespeaked
by 8 hours and decreased
by
16 hours after the addition
of HGF.
The addition
mmol/L
inhibited
the increase in the
DFMO
completely
of 5
Figure 4. Effect of exogenously added putrescine, spermidine, or spermine on [3H]thymidine incorporation in primary cultured rat hepatocytes treated with DFMO and MGBG. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of DFMO (5 mmol/L) and MGBG (20 pmol/L). At 8 hours, 0.1 mmol/L putrescine, 0.1 mmol/L spermidine, or 0.1 mmol/L spermine was added. A 4-hour pulse of [3H]thymidine (1 uCi/dish) was begun 20 hours after the addition of HGF. Values are expressed as means -t SD of five dishes. aP < 0.01 compared with control; bP < 0.01 compared with the addition of HGF; ‘P < 0.01 compared with the addition of HGF in the presence of DFMO and MGBG.
1028
HIGAKI
putrescine
GASTROENTEROLOGY
ET AL.
concentration
caused by HGF. In contrast,
by 8 hours and peaked by 16 hours after the addition HGF.
The addition
MGBG dine
completely
concentration
spermine
of 5 mmol/L inhibited caused
concentration
DFMO
by HGF
increased
of HGF. inhibited
spermine
concentration
mmol/L
DFMO
Changes
caused
did not inhibit
in polyamine
(Figure
by HGF. it (Figure
concentrations
However, after
are shown in Table
nously
added putrescine,
spermidine,
exoge-
1. Exoge-
or spermine
in cells, but each polyamine
5
7C).
added polyamines
converted
of 20
the increase in the
nously
accumulated
7B). The
The addition
spermine
polyamines
are widely
were
added was not
into the other polyamines.
-*
116kD
-
66kD
-
42kD
-
30kD
-
after various
documented 1 ng/mL
that DNA
HGF
HGF
induced
dependent
ODC
manner
In the present mine
metabolism
using
inhibitors
et a1.23 previously
began to increase with
cultured
trescine
and
was reversed
and SAMDC
rat hepatocytes.
activities
in a dose-
similar to that seen in DNA synthesis. study,
we examined
in HGF-induced
DNA DFMO
concentrations
DNA synthesis
synthesis
by
enzymes decreased but
in pu-
inhibited
by only 21%. The inhibi-
on HGF-induced
by exogenously
DNA
synthesis
added putrescine,
spermi-
On the other
caused the accumulation
the role of polya-
biosynthetic
rat hepatocytes.
spermidine
or spermine.
with 5 ng/mL
cultured
of polyamine
primary
dine,
synthesis
ODC ac-
fashion in primary
Nakamura
in primary
tory effect of DFMO . , .;
stimuli.‘-”
HGF and reached its maximum
(60 pmol/L)
is associated
shown that HGF induced
rat hepatocytes.13
cells
and differentia-
synthesis
in a time- and dose-dependent
cultured
and
in many different
that polyamine
We have recently tivity
spermidine,
role in cell growth
with liver regeneration
HGF-induced 200kD
putrescine,
distributed
and play an essential tion.22 It is known
by 8 hours and peaked
I6 hours after the addition completely
or 20 pmol/L
the increase in the spermi-
pmol/L
MGBG
The
of
No. 4
Discussion
the
addition of MGBG increased the putrescine concentration (Figure 7A). The spermidine concentration increased
Vol. 106,
hand,
of putrescine
MGBG,
which
and decreased
in
A
B Figure 5. Western blot analysis of PCNA levels in primary cultured rat hepatocytes. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of DFMO (5 mmol/L) and MGBG (20 pmol/L). At 8 hours, 0.1 mmol/L putrescine. 0.1 mmol/L spermidine, or 0.1 mmol/L spermine was added. Cells were harvested 24 hours afterthe addition of HGF, and cellular proteins (20 pg) were separated by acrylamide gel electrophoresis. (A) lmmunoblot analysis of PCNA. Lanes: M, marker proteins; 1, control; 2, HGF: 3, HGF + DFMO + MGBG; 4. HGF + DFMO + MGBG + putrescine; 5, HGF + DFMO + MGBG + spermidine; 6, HGF + DFMO + MGBG + spermine. (6) Densitometric analysis of relative amounts of PCNA.
Figure 6. Dose responses of (A) MGBG effects on SAMDC activity and (8) [3H]thymidine incorporation in primary cultured rat hepatocytes. SAMDC activity and [3H]thymidine incorporation were measured at 6 and 24 hours, respectively. A 4hour pulse of [3Hjthymidine (1 uCi/ dish) was begun 20 hours after the addition of HGF. Values are expressed as means 2 SD of five dishes. *P < 0.01 compared with 0 pmol/L MGBG. **P < 0.05 compared with 0 pmol/L MGBG.
POLYAMINE METABOLISM
April 1994
marker
IN HEPATOCYTE PROLIFERATION
of cell proliferation.
as a nonhistone correlates
directly
and DNA synthesis.24-27 the onset of DNA ing S phase.““s
Elevated levels of PCNA appear
synthesis
and become
Exogenously
protein
paralleled
added putrescine,
those obtained
spermidine,
but each polyamine
converted
into the other polyamines.
putrescine
is a potent
stimulator
or sperm-
added was not
It is known
of SAMDC
increases in the spermidine
and spermine
were not observed
putrescine.
The reason for this is not obvious. of transgenic
the human ODC gene.‘“-‘” elevated
et al. who recently
enhanced
and spermine
ODC activity
between putrescine
attributable
to an inhibition
are compatible
and
levels, the concentraremained virtually
altered in the tissue of the transgenic ent blockage
Similar
mice over-expressing
tissue putrescine
tions of spermidine
added
In spite of the fact that these
animals display a strikingly grossly
con-
after exogenously
findings were reported by Halmekyto a number
that
activity.*’
centrations
generated
dur-
incorporation.
ine was accumulated,
However,
before
maximum
The present study showed that changes
by [‘H}thymidine (hr)
proliferation
late G, phase immediately
in the levels of PCNA after HGF
has been described
whose level of synthesis
with the rate of cellular
in the nucleus during
Tie
PCNA
nuclear protein
1029
mice.”
and spermidine
of SAMDC.‘”
un-
The apparwas not
These results
with the views expressed by Davis et a1.34
in their recent review that one of the major functions the polyamine
homeostatic
is to prevent
an excessive
polyamines tylation,
spermidine the extent
which DNA
of inhibition polyamine synthesis,
inhibited control
HGF-induced DNA
synthesis
added spermidine DFMO
DNA
level. The inhibitory
induced
and MGBG was reversed
added exogenously. DFMO
and MGBG
putrescine
or spermine. completely when
to nontreated on HGF-
by exogenously
Combined inhibited
addition
of
HGF-induced
control level; the inhibitory
spermidine
In contrast,
or spermine
the inhibitory
was not completely
was added exogenously.
midine or spermine synthesis,
synthesis
completely
effect of MGBG
was reversed
DNA synthesis to nontreated effect
concentrations,
is important
was
effect of
reversed when
To confirm that sperfor HGF-induced
DNA
we measured protein levels of PCNA as another
of inhibition
after HGF
These
of SAMDC
or spermine
and MGBG synthesis
activity.
for HGF-induced (0.1 - 100 pmol/
The extent
to that of spermine
of recovery of spermi-
(data not shown).
that an increased
or spermine,
cellular
rather than putrescine,
DNA
are essential
for liver
Luk8 showed that the administration inhibitor,
DFMO,
pletely prevented exogenously
to partially
is essen-
added putrescine.
lation
of putrescine
spermine
without
accumulation
tion of DNA
synthesis
regeneration. rats, com-
this was reversed by
Nishiguchi
of interferon
in par-
of a specific ODC
hepatectomized
liver regeneration;
that administration
level of
synthesis.
Previous studies have reported that polyamines, putrescine,
to the
To determine
were added exogenously
addition.
tial for HGF-induced ticular
ace-
synthesis
was similar
by various concentrations
results suggest
spermidine
of DNA
of MGBG
is more important
dine was similar and spermine
cells
of the higher
by excretion,
various concentrations
L) of spermidine of DNA
the spermidine
and spermine
by various concentrations extent
in mammalian
or both.
Moreover, flgure 7. Time course of polyamine concentrations: (A) putrescine, (8) spermidine, and (C) spermine in primary cultured rat hepatocytes. The culture medium was changed with the addition of HGF (10 ng/ mL) in the absence of inhibitors (0) and in the presence of 5 mmol/ L DFMO (0) or 20 pmol/L MGBG (A). Values are expressed as means ? SD of five dishes. *P < 0.01 compared with no inhibitors. **P < 0.05 compared with no inhibitors.
system
accumulation
of
et a1.35 showed
suppressed the accumu-
affecting
spermidine
and also suppressed
and
the stimula-
in the liver induced
by partial
1030 HIGAKI ET AL.
GASTROENTEROLOGY Vol. 106, No. 4
Table1. Changes in Polyamine
Concentrations
After Exogenously
Added Polyamines
in Primary Cultured
Rat Hepatocytes
Polyamine concentrations (pmo//pg DNA) Addition
Putrescine
Spermidine
Spermine
Control
2.7 -t 0.4
196.8 2 12.9
105.7
HGF HGF + DFMO HGF + DFMO + Put HGF + DFMO + Spd
2.8 + 0.6 2.0 k 0.2
369.7 253.6
183.7 t 8.1” 171.4 5 15.1
HGF HGF HGF HGF HGF
+ + + + +
260.5 5 24.1
71.8 2 10.7”
404.3
2.1 5 0.2 2.1 67.5 62.8 74.2 63.6
DFMO + Spm MGBG MGBG + Spd MGBG + Spm MGBG + Spd + Spm
2 + 2 ? 2
+ 13.4” k 27/Ib 2 17.3’
249.0 2 23.2 249.7 2 6.2’ 423.8 2 10.0’ 231.1 5 21.1 386.6 -c 13.2’
0.2 5.6b 12.1 8.3 7.6
+ 18.3
161.3 t 5.7
165.3 k 5.4 263.9 96.1 79.8 248.9 269.2
+ 2 % ? 2
12.3” 13.6b 14.3 13.2’ 41.0’
NOTE. After a change to fresh medium, cells were cultured in HGF (10 ng/mL) with or without 5 mmol/L DFMO or 20 pmol/L MGBG. At 8 hours, 0.1 mmol/L putrescine (Put), 0.1 mmol/L spermidine (Spd), or 0.1 mmol/L spermine (Spm) was added. Polyamine concentrations were measured 16 hours after the addition of HGF. Values are expressed as means t SD of five dishes. “P < 0.01 compared with control. *P < 0.01 compared with HGF. ‘P < 0.01 compared with HGF + DFMO. dP < 0.01 compared with HGF + MGBG.
also, the suppression
hepatectomy; completely
nous putrescine regeneration
portant
Furthermore,
exoge-
used to stimulate
liver
1. Gohda E, Tsubouchi H, Nakayama H, Hirono S, Sakiyama 0,
and
in animal models of acute liver failure”
alcohol-induced putrescine,
was successfully
References
of DNA synthesis was
reversed by putrescine.
liver injury.36 These results suggest that
rather than spermidine
for liver regeneration.
The
our results and previous
studies
explanation
between
is difference
or spermine,
is im-
difference
2.
between
is not clear; a possible in vitro and in vivo
3.
conditions. It has been documented dine are essential
that putrescine
for proliferating
and spermi-
rat hepatoma
tissue
culture cells.37,38 On the other hand, it has been reported that spermidine
or spermine is required for DNA synthethese results are similar
sis in lymphocytes39-41;
results with cultured rat hepatocytes. stood which polyamine although
is critical
to our
It is not well under-
for proliferating
it may depend on the type of cultured
cells, cells or
tissues. Recently, transient
it was shown that HGF
generation
biphasic production
of inositol
induced
of 1 ,2-diacylglycerol.42
in primary cultured
is important
for ODC
rat hepatoma
tissue culture
duction
in lymphocytes.”
induction
Moreover,
ODC and SAMDC
though
between
caused by HGF
not yet clear.
8.
it 9.
and
it is possible
Ca*+ concentration
volved in HGF-induced changes
7.
by
and that Ca*+
in lymphocytes45
Therefore,
6.
for HGF.*3,44 Ca2+
cells,46 and for SAMDC
an increase in the intracellular the relationship
and a
were induced
rat hepatocytes
acted as one of the second messengers
5.
an early
1,4,5-triphosphate
has been shown that Ca2+ oscillations HGF
4.
inthat
is in-
activity,
al11.
very early biochemical
and polyamine
10.
metabolism
is
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Received June 14, 1993. Accepted November 16, 1993. Address requests for reprints to: lkko Higaki, M.D., Second Depattment of Biochemistry, Osaka City University Medical School, 1454 Asahimachi, Abenoku, Osaka 545, Japan. Fax: (81) 66452030. The authors thank Dr. Tomoyoshi Nishino (Otsuka Pharmaceutical Co., Ltd., Tokushima, Japan) for providing recombinant human hepatocyte growth factor and Hisako Fujimoto, Toshiko Yoshimata, and Kumle Nagahama for their excellent technical assistance.
Increased Spermidine or Spermine Level is Essential for Hepatocyte Growth Factor-Induced DNA Synthesis in Cultured Rat Hepatocytes IKKO HIGAKI,* ISA0 and SHUZO OTANI*
MATSUI-YUASA,’
MASANOBU
TERAKURA,*
HIROAKI
KINOSHITA,§
*Second Department of Biochemistry, Osaka City University Medical School; ‘Department of Food and Nutrition, Faculty of Science of Living, Osaka City University; and “Second Department of Surgery, Osaka City University Medical School, Osaka, Japan
Background/Aims: Hepatocyte growth factor is a potent mitogen for mature hepatocytes and seems to act as a trigger for liver regeneration. Hepatocyte growth factor was first purified from human and rabbit plasma and rat platelets. Additionally, putrescine, spermidine, and spermine are widely distributed in many different cells; intracellular concentrations of these polyamines are closely related to cell proliferation. The present study examined whether polyamine metabolism is involved in hepatocyte growth factor-induced DNA synthesis in primary cultured rat hepatocytes. Methods: Hepatocy-tes were isolated from rats by the collagenase perfusion method. Ornithine decarboxylase and Sadenosylmethionine decarboxylase activities were measured as the release of 14C02 from L-[1-14C]ornithine and Sadenosyl-L-[carboxyI-14C]methionine, respectively. Results: a-Difluoromethylornithine inhibited hepatocyte growth factor-induced DNA synthesis by only 21%. On the other hand, methylglyoxal bis(guanylhydrazone) completely inhibited hepatocyte growth factorinduced DNA synthesis to nontreated control level. The inhibitory effect of methylglyoxal bis(guanylhydrazone) on hepatocyte growth factor-induced DNA synthesis was reversed by exogenously added spermidine or spermine. Conclusions: Spermidine or spermine is essential for hepatocyte growth factor-induced DNA synthesis in primary cultured rat hepatocytes.
many
different
polyamines
H
for mature
factor
hepatocytes
(HGF)
and seems
for liver regeneration
after various
purified
and rabbit
based
from
on its ability
tocytes.“2 with
human
HGF
hepatic
animals
with
kinetics
of this
round
of DNA
gesting
that
levels
experimentally response synthesis HGF
plays
stimuli.
regeneration
forms
of liver injury,
ischemia,”
nine
HGF
in a time-
of rat hepa-
in the plasma
in the
plasma3
induced is rapid during a key
and
liver damage. precedes
the
in initiating
of The first sugthis
process.3*4 Putrescine,
spermidine,
and
spermine
the
after
activities
of
S-adenosylmethiokey
enzymes
in mammalian
many
liver
and polyamines The
and
pathway
many
different
of the cells, are
growth-pro-
reported
and
that HGF
dose-dependent
rat hepatocytes.13
ined
the
role
of ODC,
of polyamine and
is essential cultured
inhibitor
in primary study,
cul-
we exam-
by
using
a-
inhibi-
bis(guanylhydrazone) of SAMDC,
and
level of spermidine
for HGF-induced
activity
an irreversible
methylglyoxal
cellular
ODC
metabolism
(DFMO),
a reversible
that an increased
fashion
In the present
difluoromethylornithine (MGBG),
induced
DNA
found
or spermine
synthesis
in primary
rat hepatocytes.
Materials and Methods Materials Male Wistar rats weighing 150-200 g were used for preparation of hepatocytes. The protocol of the experiment was by the Animal
Research
care of the animals of this institution
Committee
of Osaka City
was in accordance
Osaka City University). Insulin, dexamethasone, spermidine, spermine, and S-adenosyl-L-methionine products
of Sigma Chemical
with
the
(Guide for AnimaL Experimentation, putrescine, were the
Co. (St. Louis, MO). MGBG
was
of patients or serum*
liver regeneration, role
increased
tured
standards
was first
regeneration. (ODC)
from
hepatectomy,‘.”
stimuli.5~6”2
We recently
tor
for recovery
(SAMDC),
biosynthetic
of these
proliferation.5.6
liver injury,‘“*”
for liver
decarboxylase
moting
cell
such as partial
decarboxylase
dramatically
to
is important
are responsible
polyamine
concentrations
related
and chemical
ornithine
University;
and rat platelets
mitogenesis
increase and
mitogen
to act as a trigger
plasma
to stimulate
failure’
is a potent
closely
Liver
approved growth
epatocyte
cells; intracellular are
are found
in
Abbreviations used in this paper DFMO, adifluoromethylornithine; HGF, hepatocyte growth factor; MGBG, methylglyoxal bis(guanylhydrazone); ODC, ornithine decarboxylase; PCNA, proliferating cell nuclear antigen; PVDF, polyvinyldifluoride; rhHGF, recombinant human hepatocyte growth factor: SAMDC, Sadenosylmethionine decarboxylase; SDS, sodium dodecyl sulfate; TBST, Tris-buffered saline containing 0.05% Tween 20. 0 1994 by the American Gastroenterological Association 0016-5065/94/$3.00
April 1994
POLYAMINE
purchased
from Aldrich
L-[l-‘“C]otnithine methionine
from Nippon
cell nuclear antigen
(Arkansas)
was from
human Ltd.
growth
(Tokushima,
Research
Japan)
Institute,
Hepatocyte Male cytes judged
from
Viability by ttypan
purity
immu-
> 99%) (Mettell
1 X lo-’
L dexamethasone. in a humidified changing
in the absence hours.
Then
thHGF
were
was
and harvested
Protein
CO,
concentrations
of radioactivity
as
as described counts
in 35-
DNA
from
The
a tubber
policeman
containing ylene
in 300
diaminetettaacetic
air. After
for additional
fresh
medium
thiothteitol. minutes
and were
at 4°C.
Then
16
0.25
and 80 nmol of L-otnithine stopper
syringe
needle.
350 absorbed transferred
(5 pL). The
on the paper disk, Daiichi
was measured 5801; mined
Beckman,
Tokyo,
by the release
‘“Clmethionine.‘”
The
was trapped
incubated
was sealed syringe
nee-
(Sigma
to
protein
Chemical
(Packon the
sodium
(SDS),
0.15
scintillation
SAMDC
were
The
as
amount
of Button.“.‘”
were washed
1% Nonidet
deoxycholate, mol/L NaCl,
of
Calf thy-
for 3 minutes
to PVDF
membrane
was blocked
albumin).
the PVDF
Tween (1:500
lin G conjugated After
developed
of SDS Protein
protein
Twenty
once
with
assay kit
micrograms gels and casein.
Ttis-buffeted
saline
TBST
with a chemiluminescent
and incu-
and 0.2%
with the primary three
times
with
bovine
antibody,
with
with anti-mouse
washing
transfer,
0.5%
(5 minutes)
in 0.05%
was washed
with
TBST
(5
immunoglobu-
with horse radish petoxidase
extensive
gel electto-
of Laemmli.”
at 4°C
20 (TBST)
each) and incubated
Cells
in the presence
After electtophotetic
After incubation
membrane
at 4°C.
SDS-polyactylamide
overnight
was washed
Co.), sulfate
and 2 mmol/L
by a Bio-Rad
membrane.
bated in anti-PCNA serum
PAGE
as a standard.
was run on 12.5%
0.05%
Chemical dodecyl
minutes
to the method
transferred
phos-
at 100,OOOg for 30 minutes
buffet.
of protein
containing
(Sigma EDTA,
for 30
with
in SDS-polyactylamide
sample
the paper
times
10 mmol/L Ttis-HCl
sodium
1 mmol/L
fluoride
were measured
Then
P-40
by centtifugation
(PAGE)
three
with
0.1%
concentrations
(1:2500
TBST,
detection
in 0.5%
the blots
were
system.
Measurement of Polyamine Concentrations
(LS
was detet-
washed
was measured
was expressed
of DNA.
saline and disrupted
according
The incubated
S-adenosyl-L-[catboxyl-
cells
incorporation
fluid
counter
activity
The incorporation
Co.) was used as a standard.
was performed
Radioactivity
scintillation
from
photesis
TBST).
by the Soluene-
Japan).
Fraction
fraction
by the method
hepatocytes
0.5%
minutes
and the paper disk was then
liquid
Japan).
di-
(5 FL)
IL) was impaled
Tokyo,
of 14C02
7.5)
was added to
test tube
The
using bovine serum albumin
at 30,OOOg for 20
5 mL toluene
Chemicals,
in a Beckman
(pH
50 PL Soluene-350
Grove,
The CO* released
with
mmol/L
with a disposable
to a vial containing
(Omnifluot;
Ttis
PCi of L-El-‘*C]otnithine
Co., Downers
washed
by three cycles of freezing
dle. A paper disk (8 mm) containing ard Instrument
were
and 2.5
centrifuged
equipped
The
was added to the cell cul-
pet microgram
(pH 7.5) containing
and boiled
0.1 mmol/L eth-
90 PL of the supetnatant
a glass tube containing with a tubber
cells
phosphate,
(EDTA),
then
PL). similar
of [3H]Thymidine Into Acid-Insoluble
previously.”
Rat
with
saline and harvested
The cells were disrupted
and thawing
(5
of 14C02 pto-
by a Bio-Rad
into the acid-insoluble
phate-buffeted
by the release of ‘“CO2
/.LLof 50 mmol/L
acid
tube
Western Blot Analysis
cells were cultured
incubated
200 pmol/L pytidoxal
at 4°C.
to a glass
VA) using bovine serum albu-
(1 PCiidish)
was determined
mus DNA
times.
was determined
L-[1-‘4C]ornithine.‘5
were measured
Richmond,
pet minute
moli
of Enzyme Activities
three times with phosphate-buffeted
and thawing
by estimation
ture 4 hours before the cells were harvested.
were pelleted
activity
was added
The
used in assay of ODC activity.
phenylmethylsulfonyl
ODC
of freezing
S-adenosyl-L-methionine
{‘H]Thymidine
the
>95%
and 95%
in the
at the indicated
Measurement
2.8
phosphate.
from S-adenosyl-L-[catboxyl-‘4C]methionine
at 37°C for 24 hours
and hormones
cultured
pytidoxal
cycles
phosphate
dithiothteitol,
at 30,OOOg for 20 minutes
was measured
min as a standard.
perfusion
and 1 X lo-’
with fresh medium,
of the serum cells
nmol
Dow
Hepato-
collagenase
The cells were cultured
the medium
20
activity
assay kit (Bio-Rad,
before
The cells were plated
of 5%
by three
Measurement Incorporation
water freely.
mol/L insulin,
atmosphere
and
duced
mmol/L
1025
PCi S-adenosyl-L-[catboxyl-‘4C]methionine
Co.
mm collagen-coated dishes at a density of 5 X lo4 cells.0.2 mL-’ . cm-’ m Williams’ medium E supplemented with 5% fetal calf serum,
PL)
the method
and
1.1
and 200 PmoliL
0.125
SAMDC
te-
Pharmaceutical
hepatocytes
blue exclusion.
(5
was from
for 18 hours
by the
of isolated
containing
PL of the supetnatant
containing
and Culture
to drink
tats
in 300 PL of 55 mmol/L sodium
7.5)
were disrupted 90
PROLIFERATION
respectively.
tats were fasted
isolated
[mouse])
IN HEPATOCYTE
and were then centrifuged Then
Recombinant
P. McCann
OH),
but were allowed
were
method.”
and Dr.
Preparation
Wistat
experiments
MA).
by Otsuka
Cincinnati,
was
proliferating
anti-mouse
factor (thHGF;
supplied
(pH
cells
petoxidase
(Boston,
policeman
buffet
(Buckinghammembrane
blot chemiluminescence
NEN
tubber
mmol/L puttescine,
anti-PCNA
Denmark);
and Western
were kindly
and
(31 Ci/mmol)
Japan);
with horseradish
DuPont
hepatocyte
DFMO
(PVDF)
(monoclonal
(Glosttup,
G conjugated
Pel-Fteet
International
Co. Ltd. (Tokyo,
(PCNA)
was from Dakopatts
agent
and [6-3H]thymidine
Polyvinyldifluotide
Genetics
WI),
S-adenosyl-L-[catboxyl-‘“C]-
from Ametsham
England).
noglobulin
Co. (Milwaukee,
Ciimol),
(57 Ci/mol),
were purchased shire,
Chemical
(53
METABOLISM
with
a
liceman
in 300
cells were harvested
PL of ice-cold
with a tubber
5% ttichlotoacetic
po-
acid centti-
1026
HIGAKI
GASTROENTEROLOGY
ET AL.
fuged for removal
of the protein.
amine
in the acid extract
liquid
chromatography
Japan)
equipped
of polyamine
(Shimadzu
with fluorescence
was performed
150 mm; particle
The concentration
was analyzed
detector.*’ Shimadzu
ric acid as solvent A and solvent A-methanol was eluted
with solvent
solvent
B at 4°C for 3 minutes
solvent
gradient
The gradient 22 minutes concentrations
using
The separation (4.6 X
Techno-Research of 10 mmol/L
l-
changed
(1:3) as solvent
A at 96°C and with
and then with a programmed
the linear
gradient
curve number
from 4°C to 55°C with
at a flow rate of 0.7 mlimin. were expressed
as picomoles
Various
Kyoto,
acid sodium salt- 100 mmol/L sodium perchlo-
B. The sample
Results
of poly-
LC-6A; Shimadzu,
Inc., Kyoto, Japan) with a solvent composed hexanesulfonic
No. 4
by high-performance
on a STR ODS-II column
size, 5 pmol/L;
Vol. 106,
solvent
cells, and the activities
of ODC (Figure
B in of
DNA.
1A) and SAMDC
6 hours after the addition (Figure 1B) were determined in primary cultured rat hepatocytes. Both of the enzyme activities
began
to increase
reached a maximum
with
with
1 ng/mL
5 ng/mL
(Figure activity
increased
and
HGF. 4 hours
of HGF and peaked at 8 hours; thereaf-
2A). To determine is required
we used DFMO.
HGF
(60 pmol/L)
Figure 2A shows that ODC activity after the addition
ter it decreased and returned 0.
The polyamine per micrograms
of HGF were added to the
concentrations
to O-hour level by 16 hours whether
an increase
for HGF-induced
Five millimolars
DNA
of DFMO
inhibited
the increase
in ODC activity
inhibited
HGF-induced
C3H]thymidine
in ODC synthesis,
completely
(Figure
2A) but
incorporation
by
Statistical Analysis The results are expressed cance of differences t test. Differences
as means t SD. The signifi-
in assay values was evaluated
by Student’s
with P values < 0.05 were considered
sig-
nificant.
“0
Figure 1. Effect of HGF on (A) ODC and (6) SAMDC activity in primary cultured rat hepatocytes. The cells were cultured as described in Materials and Methods. The culture medium was changed with the addition of HGF at the various concentrations, and cells were cultured for 6 hours. Values are expressed as means + SD of five dishes. *P < 0.01 compared with 0 ng/mL HGF. **P < 0.05 compared with 0 ng/mL HGF.
4
(I
1ime
12
16
:
P.
after HGF (hr)
figure 2. (A) Time course of ODC activity in primary cultured rat hepatocytes after the addition of HGF and DFMO. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence (0) or presence (0) of 5 mmol/L DFMO. Values are expressed as means 2 SD of five dishes. *P < 0.01 compared with the presence of DFMO. **P i 0.05 compared with the presence of DFMO. (6) Effect of exogenously added putrescine, spermidine, or spermine on [3H]thymidine incorporation in primary cultured rat hepatocytes treated with DFMO. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of 5 mmol/L DFMO. At 8 hours, 0.1 mmol/L putrescine (Put), 0.1 mmol/L spermidine (Spd), or 0.1 mmol/L spermine (Spm) was added. A 4-hour pulse of [3H)thymidine (1 pCi/dish) was begun 20 hours after the addition of HGF. Incorporation is expressed as means 2 SD of five dishes. “P < 0.01 compared with control; “P < 0.01 compared with the addition of HGF: ‘P < 0.01 compared with the addition of HGF in the presence of DFMO.
POLYAMINE METABOLISM
April 1994
only 21% (Figure
2B). The inhibitory
on HGF-induced
13H]thymidine
versed by exogenously
added 0.1 mmol/L
was re-
putrescine,
mmol/L spermidine, or 0.1 mmol/L spermine after HGF and DFMO addition (Figure 2B). As shown in Figure
3A, SAMDC
hours after the addition remained
at a high
L spermine
effect of DFMO
incorporation
activity
0.1
8 hours
increased
3
of HGF, peaked by 6 hours, and
level until
12 hours.
Thereafter
it
addition To
IN HEPATOCY-TE PROLIFERATION
was added exogenously
8 hours after MGBG
3B).
(Figure determine
HGF-induced
which
DNA
polyamine
synthesis,
addition
of DFMO
addition
and MGBG
of 5 mmol/L
DFMO
completely
inhibited
corporation
to nontreated
is
(Figure
control
level;
spermine
crease in SAMDC
DFMO
and MGBG
caused by HGF MGBG
HGF-induced
{3H]thymidine
treated
level; these inhibitory
control
were reversed when 0.1 mmol/L
(Figure
completely incorporation
3A).
inhibited to
non-
effects of MGBG
spermidine
or 0.1 mmoli
addition.
when 0.1 mmol/L
levels of PCNA (Figure showed
DNA
HGF-induced
spermidine hepatocyte
leled that seen in Figure Dose responses
proliferation.
inhibition
at 20 pmol/L.
amine concentrations tine concentration
Figure 3. (A) Time course of SAMDC activity in primary cultured rat hepatocytes after the addition of HGF and MGBG. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence (0) or presence (0) of 20 umol/L MGBG. Values are expressed as means 2 SD of five dishes. *P < 0.01 compared with the presence of MGBG. (8) Effect of exogenously added spermidine or spermine on [3H]thymidine incorporation in primary cultured rat hepatocytes treated with MGBG. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of 20 pmol/L MGBG (MGBGzO) or 30 pmol/L MGBG (MGBG,O). At 8 hours, 0.1 mmol/L spermidine or 0.1 mmol/L spermine was added. A 4-hour pulse of [3Hjthymidine (1 @/dish) was begun 20 hours after the addition of HGF. Values are expressed as means 2 SD of five dishes. aP < 0.01 compared with control; bP i 0.01 compared with the addition of HGF; ‘P < 0.01 compared with the addition of HGF in the presence of MGBG (20 pmol/L): dP < 0.01 compared with the addition of HGF in the presence of MGBG (30 umol/L).
also for
This result paral-
effects on SAMDC
activity
are shown in Figure 6A displaying
7.5 pmol/L
MGBG
The effects of HGF and polyamine Time after HGF (hr)
of PCNA is necessary
4.
incorporation
at roughly
protein
of cell proliferation
blot analysis
and B. Both curves are similar, inhibition
reversed
is important
we measured
or spermine
of MGBG
and [iHfthymidine
or spermine marker
5A and B). Western that
the inhibitory
was added exogenously.
synthesis,
as another
or 0.1
8 hours after
was not completely
that spermidine
for HGF-induced
in-
spermidine
In contrast,
putrescine
MGBG
the inhibitory
was added exogenously
effect of DFMO and MGBG To confirm
4). Combined
[‘H)thymidine
mmol/L
activity
for
combined
and 20 pmol/L
HGF-induced
effect was reversed when 0.1 mmol/L
20 and 30 pmol/L
essential
we examined
decreased and returned to O-hour level by 18 hours. Twenty-micromolar MGBG completely inhibited the inBoth
1027
half-maximal and maximal
inhibitors
on poly-
are shown in Figure 7. The putrespeaked
by 8 hours and decreased
by
16 hours after the addition
of HGF.
The addition
mmol/L
inhibited
the increase in the
DFMO
completely
of 5
Figure 4. Effect of exogenously added putrescine, spermidine, or spermine on [3H]thymidine incorporation in primary cultured rat hepatocytes treated with DFMO and MGBG. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of DFMO (5 mmol/L) and MGBG (20 pmol/L). At 8 hours, 0.1 mmol/L putrescine, 0.1 mmol/L spermidine, or 0.1 mmol/L spermine was added. A 4-hour pulse of [3H]thymidine (1 uCi/dish) was begun 20 hours after the addition of HGF. Values are expressed as means -t SD of five dishes. aP < 0.01 compared with control; bP < 0.01 compared with the addition of HGF; ‘P < 0.01 compared with the addition of HGF in the presence of DFMO and MGBG.
1028
HIGAKI
putrescine
GASTROENTEROLOGY
ET AL.
concentration
caused by HGF. In contrast,
by 8 hours and peaked by 16 hours after the addition HGF.
The addition
MGBG dine
completely
concentration
spermine
of 5 mmol/L inhibited caused
concentration
DFMO
by HGF
increased
of HGF. inhibited
spermine
concentration
mmol/L
DFMO
Changes
caused
did not inhibit
in polyamine
(Figure
by HGF. it (Figure
concentrations
However, after
are shown in Table
nously
added putrescine,
spermidine,
exoge-
1. Exoge-
or spermine
in cells, but each polyamine
5
7C).
added polyamines
converted
of 20
the increase in the
nously
accumulated
7B). The
The addition
spermine
polyamines
are widely
were
added was not
into the other polyamines.
-*
116kD
-
66kD
-
42kD
-
30kD
-
after various
documented 1 ng/mL
that DNA
HGF
HGF
induced
dependent
ODC
manner
In the present mine
metabolism
using
inhibitors
et a1.23 previously
began to increase with
cultured
trescine
and
was reversed
and SAMDC
rat hepatocytes.
activities
in a dose-
similar to that seen in DNA synthesis. study,
we examined
in HGF-induced
DNA DFMO
concentrations
DNA synthesis
synthesis
by
enzymes decreased but
in pu-
inhibited
by only 21%. The inhibi-
on HGF-induced
by exogenously
DNA
synthesis
added putrescine,
spermi-
On the other
caused the accumulation
the role of polya-
biosynthetic
rat hepatocytes.
spermidine
or spermine.
with 5 ng/mL
cultured
of polyamine
primary
dine,
synthesis
ODC ac-
fashion in primary
Nakamura
in primary
tory effect of DFMO . , .;
stimuli.‘-”
HGF and reached its maximum
(60 pmol/L)
is associated
shown that HGF induced
rat hepatocytes.13
cells
and differentia-
synthesis
in a time- and dose-dependent
cultured
and
in many different
that polyamine
We have recently tivity
spermidine,
role in cell growth
with liver regeneration
HGF-induced 200kD
putrescine,
distributed
and play an essential tion.22 It is known
by 8 hours and peaked
I6 hours after the addition completely
or 20 pmol/L
the increase in the spermi-
pmol/L
MGBG
The
of
No. 4
Discussion
the
addition of MGBG increased the putrescine concentration (Figure 7A). The spermidine concentration increased
Vol. 106,
hand,
of putrescine
MGBG,
which
and decreased
in
A
B Figure 5. Western blot analysis of PCNA levels in primary cultured rat hepatocytes. The culture medium was changed with the addition of HGF (10 ng/mL) in the absence or presence of DFMO (5 mmol/L) and MGBG (20 pmol/L). At 8 hours, 0.1 mmol/L putrescine. 0.1 mmol/L spermidine, or 0.1 mmol/L spermine was added. Cells were harvested 24 hours afterthe addition of HGF, and cellular proteins (20 pg) were separated by acrylamide gel electrophoresis. (A) lmmunoblot analysis of PCNA. Lanes: M, marker proteins; 1, control; 2, HGF: 3, HGF + DFMO + MGBG; 4. HGF + DFMO + MGBG + putrescine; 5, HGF + DFMO + MGBG + spermidine; 6, HGF + DFMO + MGBG + spermine. (6) Densitometric analysis of relative amounts of PCNA.
Figure 6. Dose responses of (A) MGBG effects on SAMDC activity and (8) [3H]thymidine incorporation in primary cultured rat hepatocytes. SAMDC activity and [3H]thymidine incorporation were measured at 6 and 24 hours, respectively. A 4hour pulse of [3Hjthymidine (1 uCi/ dish) was begun 20 hours after the addition of HGF. Values are expressed as means 2 SD of five dishes. *P < 0.01 compared with 0 pmol/L MGBG. **P < 0.05 compared with 0 pmol/L MGBG.
POLYAMINE METABOLISM
April 1994
marker
IN HEPATOCYTE PROLIFERATION
of cell proliferation.
as a nonhistone correlates
directly
and DNA synthesis.24-27 the onset of DNA ing S phase.““s
Elevated levels of PCNA appear
synthesis
and become
Exogenously
protein
paralleled
added putrescine,
those obtained
spermidine,
but each polyamine
converted
into the other polyamines.
putrescine
is a potent
stimulator
or sperm-
added was not
It is known
of SAMDC
increases in the spermidine
and spermine
were not observed
putrescine.
The reason for this is not obvious. of transgenic
the human ODC gene.‘“-‘” elevated
et al. who recently
enhanced
and spermine
ODC activity
between putrescine
attributable
to an inhibition
are compatible
and
levels, the concentraremained virtually
altered in the tissue of the transgenic ent blockage
Similar
mice over-expressing
tissue putrescine
tions of spermidine
added
In spite of the fact that these
animals display a strikingly grossly
con-
after exogenously
findings were reported by Halmekyto a number
that
activity.*’
centrations
generated
dur-
incorporation.
ine was accumulated,
However,
before
maximum
The present study showed that changes
by [‘H}thymidine (hr)
proliferation
late G, phase immediately
in the levels of PCNA after HGF
has been described
whose level of synthesis
with the rate of cellular
in the nucleus during
Tie
PCNA
nuclear protein
1029
mice.”
and spermidine
of SAMDC.‘”
un-
The apparwas not
These results
with the views expressed by Davis et a1.34
in their recent review that one of the major functions the polyamine
homeostatic
is to prevent
an excessive
polyamines tylation,
spermidine the extent
which DNA
of inhibition polyamine synthesis,
inhibited control
HGF-induced DNA
synthesis
added spermidine DFMO
DNA
level. The inhibitory
induced
and MGBG was reversed
added exogenously. DFMO
and MGBG
putrescine
or spermine. completely when
to nontreated on HGF-
by exogenously
Combined inhibited
addition
of
HGF-induced
control level; the inhibitory
spermidine
In contrast,
or spermine
the inhibitory
was not completely
was added exogenously.
midine or spermine synthesis,
synthesis
completely
effect of MGBG
was reversed
DNA synthesis to nontreated effect
concentrations,
is important
was
effect of
reversed when
To confirm that sperfor HGF-induced
DNA
we measured protein levels of PCNA as another
of inhibition
after HGF
These
of SAMDC
or spermine
and MGBG synthesis
activity.
for HGF-induced (0.1 - 100 pmol/
The extent
to that of spermine
of recovery of spermi-
(data not shown).
that an increased
or spermine,
cellular
rather than putrescine,
DNA
are essential
for liver
Luk8 showed that the administration inhibitor,
DFMO,
pletely prevented exogenously
to partially
is essen-
added putrescine.
lation
of putrescine
spermine
without
accumulation
tion of DNA
synthesis
regeneration. rats, com-
this was reversed by
Nishiguchi
of interferon
in par-
of a specific ODC
hepatectomized
liver regeneration;
that administration
level of
synthesis.
Previous studies have reported that polyamines, putrescine,
to the
To determine
were added exogenously
addition.
tial for HGF-induced ticular
ace-
synthesis
was similar
by various concentrations
results suggest
spermidine
of DNA
of MGBG
is more important
dine was similar and spermine
cells
of the higher
by excretion,
various concentrations
L) of spermidine of DNA
the spermidine
and spermine
by various concentrations extent
in mammalian
or both.
Moreover, flgure 7. Time course of polyamine concentrations: (A) putrescine, (8) spermidine, and (C) spermine in primary cultured rat hepatocytes. The culture medium was changed with the addition of HGF (10 ng/ mL) in the absence of inhibitors (0) and in the presence of 5 mmol/ L DFMO (0) or 20 pmol/L MGBG (A). Values are expressed as means ? SD of five dishes. *P < 0.01 compared with no inhibitors. **P < 0.05 compared with no inhibitors.
system
accumulation
of
et a1.35 showed
suppressed the accumu-
affecting
spermidine
and also suppressed
and
the stimula-
in the liver induced
by partial
1030 HIGAKI ET AL.
GASTROENTEROLOGY Vol. 106, No. 4
Table1. Changes in Polyamine
Concentrations
After Exogenously
Added Polyamines
in Primary Cultured
Rat Hepatocytes
Polyamine concentrations (pmo//pg DNA) Addition
Putrescine
Spermidine
Spermine
Control
2.7 -t 0.4
196.8 2 12.9
105.7
HGF HGF + DFMO HGF + DFMO + Put HGF + DFMO + Spd
2.8 + 0.6 2.0 k 0.2
369.7 253.6
183.7 t 8.1” 171.4 5 15.1
HGF HGF HGF HGF HGF
+ + + + +
260.5 5 24.1
71.8 2 10.7”
404.3
2.1 5 0.2 2.1 67.5 62.8 74.2 63.6
DFMO + Spm MGBG MGBG + Spd MGBG + Spm MGBG + Spd + Spm
2 + 2 ? 2
+ 13.4” k 27/Ib 2 17.3’
249.0 2 23.2 249.7 2 6.2’ 423.8 2 10.0’ 231.1 5 21.1 386.6 -c 13.2’
0.2 5.6b 12.1 8.3 7.6
+ 18.3
161.3 t 5.7
165.3 k 5.4 263.9 96.1 79.8 248.9 269.2
+ 2 % ? 2
12.3” 13.6b 14.3 13.2’ 41.0’
NOTE. After a change to fresh medium, cells were cultured in HGF (10 ng/mL) with or without 5 mmol/L DFMO or 20 pmol/L MGBG. At 8 hours, 0.1 mmol/L putrescine (Put), 0.1 mmol/L spermidine (Spd), or 0.1 mmol/L spermine (Spm) was added. Polyamine concentrations were measured 16 hours after the addition of HGF. Values are expressed as means t SD of five dishes. “P < 0.01 compared with control. *P < 0.01 compared with HGF. ‘P < 0.01 compared with HGF + DFMO. dP < 0.01 compared with HGF + MGBG.
also, the suppression
hepatectomy; completely
nous putrescine regeneration
portant
Furthermore,
exoge-
used to stimulate
liver
1. Gohda E, Tsubouchi H, Nakayama H, Hirono S, Sakiyama 0,
and
in animal models of acute liver failure”
alcohol-induced putrescine,
was successfully
References
of DNA synthesis was
reversed by putrescine.
liver injury.36 These results suggest that
rather than spermidine
for liver regeneration.
The
our results and previous
studies
explanation
between
is difference
or spermine,
is im-
difference
2.
between
is not clear; a possible in vitro and in vivo
3.
conditions. It has been documented dine are essential
that putrescine
for proliferating
and spermi-
rat hepatoma
tissue
culture cells.37,38 On the other hand, it has been reported that spermidine
or spermine is required for DNA synthethese results are similar
sis in lymphocytes39-41;
results with cultured rat hepatocytes. stood which polyamine although
is critical
to our
It is not well under-
for proliferating
it may depend on the type of cultured
cells, cells or
tissues. Recently, transient
it was shown that HGF
generation
biphasic production
of inositol
induced
of 1 ,2-diacylglycerol.42
in primary cultured
is important
for ODC
rat hepatoma
tissue culture
duction
in lymphocytes.”
induction
Moreover,
ODC and SAMDC
though
between
caused by HGF
not yet clear.
8.
it 9.
and
it is possible
Ca*+ concentration
volved in HGF-induced changes
7.
by
and that Ca*+
in lymphocytes45
Therefore,
6.
for HGF.*3,44 Ca2+
cells,46 and for SAMDC
an increase in the intracellular the relationship
and a
were induced
rat hepatocytes
acted as one of the second messengers
5.
an early
1,4,5-triphosphate
has been shown that Ca2+ oscillations HGF
4.
inthat
is in-
activity,
al11.
very early biochemical
and polyamine
10.
metabolism
is
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Received June 14, 1993. Accepted November 16, 1993. Address requests for reprints to: lkko Higaki, M.D., Second Depattment of Biochemistry, Osaka City University Medical School, 1454 Asahimachi, Abenoku, Osaka 545, Japan. Fax: (81) 66452030. The authors thank Dr. Tomoyoshi Nishino (Otsuka Pharmaceutical Co., Ltd., Tokushima, Japan) for providing recombinant human hepatocyte growth factor and Hisako Fujimoto, Toshiko Yoshimata, and Kumle Nagahama for their excellent technical assistance.