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Estrogen-induced increase in phosphohexose isomerase activity in the rat uterus
Estrogen-Induced Increase in Phosphohexose Isonlerase Activity in the Rat Uterus
The effects
of administration
of estradiol-
17~ on the activity of phosphohexose isomerase have been studied in the rat titerus. In ovariectomized rats, the activity of uterine phosphohexose isomerase was decreased to 49 per cent when compared to that of normal, unoperated rats. A single injection of estradiol-17/3 caused a marked increase in the enzyme activity which was detectable in 4 hours (153 per cent) and reached a maximum level (246 per cent) 16 hours after adof the hormone. Doseministration response studies indicated that 0.50 pg. of estradiol/lOO Gm. was sufficient to induce a statistically significant increase in uterine phosphohexose isomerase activity (158 per cent). Enzyme activity was maximally elevated to 278 per cent with the 20 pg./100 Gm. dose. Treat-
ment of estradiol injected rats with actinomycin, puromycin or ethionine, inhibitors of RNA and protein synthesis. completely blocked estradiolthe induced increase in the activity of uterine phosphohexose isomerase. Methionine, given concurrently with ethionine caused a complete reversal of ethionine inhibition of estradiol-induced rise in phosphohexose isomerase activity. The results suggest that the estradiol-induced increase in uterine phosphohexose isomerase activity represents enzyme biosynthesis de novo. The data are discussed in the light of current views regarding biochemical mechanisms underlying estrogenic action in the rat uterus. (Metabolism 16: No. 0, March, 271-278, 1967)
Control HOURS
2 AFTER
4
8
IN. JECTION
16
24 OF
E STRADI
OL
SINt31.41,.
VALADAHES
AND
LINC
Fig. 2.-Effect of varying d oses ’ of estradiol-17p on uterine phosphohexose isomerase (dose-response study). Bars represent the III~;~IISand st;dartl errors of 0 wluea rats of IO-12 m~ariectoinized c,acli obtained lw pooling lIteri Front :3-4 I-ats. hllp” were gi\.erl a sii;glc injection of estradiol-I’iP ii) (loses wr\-ing from 0. I O-:30.0 pg. 100 (;in. and sacrificed after 16 11011~s.Eirz\mr ;Icti\-it\, \xis calcl~l;~tctl per 100 (Gun. TIIC Id\. weight aird expressed as pcrumtage~ of controlk taken as IO0 per wrh asterisks indicate sigilific;wt alterations statisticall\ different from \~Llllrs of tllct C’oIt1ro1 rats. (1’ =
lh.~l~~xose
isomcwse
121, 124 and dfects
uctivitv
105 pr
of c~thioninr
versed
by rthioniw
(221
pc’r crnt)
and
Thus,
niiir gest
synthc,sis
that
the
phoh~~xosr Thy
of
and/or followiiig control thw
c~xprini~nt
anv
s&d
onlv
port
to thk
of ukrine
;~pprwial~k
\vas
view
carrid
out.
wtinomycin studies
1,~ hlurllc~r horniom~s
HNA
and
wnts
wtrogenic
protck
co-work+’
activitv.
inliil,itioii
rcacwltlv rcsvcwecl
wtivitv
Of synthrsis
of cstroqcnic I
alouS
id cutain
1)iosvntlicsis. of s&l,lc-l
our
that
~idi;iinistratit,11 into
l
<;ol-ski
csstratliol
in rat uterus
data
the, suggrstion
1jrc’;111(l
c;~I~s~~(~
and
that
olww~atioi~s
l~hospl~ol~~xosc
ot
utcbriirr>
cwnpl<~tc~ly
lvith
prc\ious
arc’ ii1 lines \vith
1’r(L-
prcuuwrs
lwcwnt
in ukrine \I.ith
sup-
ill the, ;lcti\it\.
tllis
011 thcs isorncw~c~
on
phosph0-
that
ri~ki!’ 1~1 one’ of thcs prim;ir\
stilnllac+ioi~s
hormones.
oiltht>ir rcsccwt studic,s, a&on
of this
is l~~lic~~d
dclition~~l
l
trc~atment
ethos
iiicrcaasc.
in this kssucl
ill tllc~ rat
iii stcpa. First, cstrogcw target tissue, i.c*., uterus. wtivit\,
promvcin,
~iintl promvcin
r(i-
Furthermore,
of l~NA-l”)lvrnc.r~~s~,
h\,
to
and
yiizvmC
of
of
ant1 \fy’r(’ failed
as \vc,ll as pm‘omy~in that
th(, ntyri
activitv
lrncls
sho\ln
r~sponsw.““‘)”
tllca
aclmixiti~g
incwas[~
of DNA-cliwctcyl
cl~moiistrat~d
in the activitv
Such
incorporatiol~
of tlwse
of rstroSnl-intlu~~~l
fi&okinasr~
Bawd
thci
from
at the l&e1
his groiq~1i~2” lla\,e
Actinomycin
lw
actinomvcin
estrogen
and
ilr viva.
incwase could
inhibitor
c7i~vmc’
Accordingly.~
of wzvmc’
clrs nova
bvnthcsis
phos-
~~lios~~liolic~xos~~
proportions
obwrvation
wpscwts
in ukrinc,
Supernatants in carving
This
protc+n
stimulate>
Iwthio-
of prc-existing
~stroS~n-indL1~c.d
acwleration hail
a marked
lation
inhibits
II is ;I pvcrful
ckstropic
incrwsc
olwr\x~cl isoniwiw
puromvcin
rrprtd
that
tk nova.
consicl~wcl.
or inhil~ition
summation.
tlw
phosl~holiexos~
\\‘hereas \ioiis
that
c~stradiol inliihitioit
\\‘a
in utrrinca
furth(~r
\vc‘w mix&
activation
in the ~xpctd
\\ith
increases
inckcwcs
:~ssa~~~l for phosl~l~ol~esose~xos~isom(‘rasc
produce
treatd
of dhiollinc~
cluck to an activation
\vas
rc’-
on mrtisoiw ~ilicl rc&dingsug~iizviiws. lCi Thescn findings
svnthcssis
~,strt,R~n-induc~~~l
c.str~~diol-tre~it~~~l rats
wml~lrt~l\~
also liavc~ sliomm
hqxitic
06 im inhildor.
in vitro and
at
of ~tliioirinc~
mav lw tlu~ to enzvme
tlic rrmc;\al
arc
p2iosphofructo~ili~~s(~
estradiol-iliducctl
~oulcl liavc, lwrn
rwn~tinrd th(a inhihitor\~
injcckd comurr;~lItl\rcWrncd complrtV1;~
of rats
co-nwrkc~rs
important
ohwr\wl
that
activitv
that
iiicrcucs
r(~vcwal
uteriw
c4kts
of wveral
possibilit\r
in utui
nidiioninc~
\Vc~lx~r aid
prrwntlv
isoiiwr;~s~
isoiwraw
lw
svnthesis
can rc’vc’rsC thrs inhibitory
induced
~ii%vm~
lrvclohscyvcd
In a&lit&
of rats
~strogen-trc,~\t(~~l rats pliosl~hollc~xost~ isoni(wsc
cent ). A similar
of c,str~~diol-iiiduc~~l pviously.”
:3 groups
It is intcwsting
in
mdhioninc~,
to the
(228 per
alonr~
of thwc
on t,stradiol-inducc,~l
mrd~ionine.
with
in uteri
cent. ‘reqwctiwly.
that
r~ccptor this
utrrus iiit(wc+s
<&ski
protc,in
co-\\~orkc~rs2i
stay
;IS a rcwlt
intcwdiolI
invol\yhs
ha\.cs sll~gc~st~~(] t]lilt
consiclrrcyl
st;~r~,o-sl”.‘.it~~,ll~~
Tllcb sCcont1
primarv
aid
inki\‘ 1~5 arl)itraril\,
\\.itll ;i changy
of its intcwction is rc’po~~sil)lt~
;~s ()ccllrrillg
;k rcyy,l)tor
ill ttlc.
iu tllc- l)i()logic,;il \\ith
cLstrogc%It. It
for ;m i~l~rc~;~s(~itI g1~1.
c’osc’ m~tal~olisni, lipid, and ’ liN.4 svlltllcxsis. Tlrcwa authors” ha\ c’ suggrstc,tl that syntliclsis Of r,cdain sp~dic ciizvmc’s iIi;i\’ l)c~ ill\~ol\;~tl in iilc,rcylsillg t]lcbxc’ \.ital iwt~~holi~ procywc~s. sinccl c,ctrog[~i1-iiltlLl~(,~t rc~sl>o~~sty ;ir(’ ill1l,lO~!dYl
I:‘L‘lQIINt: I’HOSI’HOHEXOSE
ISOhlEIMSI~:
277
lw actinomycin and puromycin at a time when no c+fec% is noted on overall protein synthesis. Estradiol has been sho\vn to incrraw thcb activity of se\wal Ilterine enzvmes2:i.2i hut whether or not the olwxvecl increases represent c’nzvmc &thesis remains to 1)~ demonstrated. Previous studies by Wallas ani co-w&kerslzi have shown that glycolysis in isolatecl uterine muscle is grcaatlv enhanced hy treatmrnt of the rat \\ith estrogen. Our present obsc~vations on estradiol-induced increases in uterine phosphohexose isomerase. together with those reported earlier for l~l~ospl~ofructokinasr”-‘x art’ in agrectmcwt \\.ith thta above views of Corski and co-workers.“’ It is tempting to specwlate that the increased glycolysis observed in the rat uterus following cstrogrn treatment may be associated with an incrwwcl rate of synthesis of specific enzvrn~~s. Further studies on c,stladiol-induction of other uterine enzymes in\wlvc,cl in flucwr mctalx~lisni ;w curwntlv in progrws in this lal,oratorv. ACKNOWLEDGMENTS enc. ot ,,b (KIS) js gl.at&11 to I’I.ofcswr continilcd intrrrst. encowngen~rrlt for twhnic;ll assistance ant1 Dr.
(hxgc \C’rhr of Indiana rtlivcrsit! ;~ntl xlvivt~. Thth ;~llthors thnk Airs. Xhriette (;c~)rgr Howr clt \lrrck. Shat-p ;~rltl Doh~~rc~ for
gift< of .~c%incm~\.ci~l D. REFERENCES
for
lli\
%icdillski
ynt~r~~~~
1:3. \Vall;~s.
0..
~l’allu.
E.. antI
I.iikW,
I;.:
Ef+‘ect of oestratliol n~onolxmmatc. 011 the nWtal,olislr~ of rat lltcrinr~ mllscle. .kta Endocrinol. 10:201-21 1. 19Ti2. 14. Kennv.
F.
T.,
and
Flora,
Ii.
hl.:
In-
t\.rosin~-tr-~~~t(~~lll~~~r~lte dllction of transnminasc~ in rat liver. 1. Biol. Ch?111. 7:36:%99-~703, 1% 1 1.5. M:el)er, C:.. ant1 Singhal. K. I,.: Rtrl<~ of cnz~mcs it1 homeostasis \‘I. Elf’td of triamcinolonr antI 0thc.r strroitls on rnzymes involxd ill ~lucorleogenc~sis. 13iochem. 1’11arm:~~ol. I:i: 117:316. -.
1187. 1964. Banrrjee. <:.. untl Brcmdvilr. S. 13.: Selective intlnctiml ;mtl sllplxcssiolr of Ii\ t’r c1nx\.,11(’ I)ios\~nthvsis. :Zmer. J, Physiol. 2ob: 1:37-14i, 196-7.
17. IlerrarWn. A.. ;mtl hlllell~~r. (i. c.: Ellcct of estradiol on thr metalx~lisnr of \erine-3-C’-’ in s,lr\ il,irly: Iltcrine
1956. ler\,ell. K. I’.. DiniT, C. Ii.. ant1 ~lucllrr. C:. C.: E;~rlv t~lfecta of cstr;ldid
on
nllclric
acid
mc~t;~l~olisln
in
thr mt uterlls. J. Hiol. Chc~. 2:31: 94Yj-959. 1958. 19. \lueller, (G. C.. llerrancll, A.. ant1 Jvrvell. I;. I’.: Studies on th(L lllechxiism Prop. 40. -,
of action of fdrogens. Hvc. Hormone Krs. 14395-1339. 19.58. Y.: Thr Corski. J.? ant1 Aizawa,
role of protein avnthrsis rstrogen action. l’roc. NatI. IT, S. 47:104-169. 1961. 21.
ill (WI\ :\catl. SC;.
(kn&. J., Notelx)onr. 11’. I>., ant1 Kicolettt~. J. :\.: Estroi_‘cn control of
The effects
of administration
of estradiol-
17~ on the activity of phosphohexose isomerase have been studied in the rat titerus. In ovariectomized rats, the activity of uterine phosphohexose isomerase was decreased to 49 per cent when compared to that of normal, unoperated rats. A single injection of estradiol-17/3 caused a marked increase in the enzyme activity which was detectable in 4 hours (153 per cent) and reached a maximum level (246 per cent) 16 hours after adof the hormone. Doseministration response studies indicated that 0.50 pg. of estradiol/lOO Gm. was sufficient to induce a statistically significant increase in uterine phosphohexose isomerase activity (158 per cent). Enzyme activity was maximally elevated to 278 per cent with the 20 pg./100 Gm. dose. Treat-
ment of estradiol injected rats with actinomycin, puromycin or ethionine, inhibitors of RNA and protein synthesis. completely blocked estradiolthe induced increase in the activity of uterine phosphohexose isomerase. Methionine, given concurrently with ethionine caused a complete reversal of ethionine inhibition of estradiol-induced rise in phosphohexose isomerase activity. The results suggest that the estradiol-induced increase in uterine phosphohexose isomerase activity represents enzyme biosynthesis de novo. The data are discussed in the light of current views regarding biochemical mechanisms underlying estrogenic action in the rat uterus. (Metabolism 16: No. 0, March, 271-278, 1967)
Control HOURS
2 AFTER
4
8
IN. JECTION
16
24 OF
E STRADI
OL
SINt31.41,.
VALADAHES
AND
LINC
Fig. 2.-Effect of varying d oses ’ of estradiol-17p on uterine phosphohexose isomerase (dose-response study). Bars represent the III~;~IISand st;dartl errors of 0 wluea rats of IO-12 m~ariectoinized c,acli obtained lw pooling lIteri Front :3-4 I-ats. hllp” were gi\.erl a sii;glc injection of estradiol-I’iP ii) (loses wr\-ing from 0. I O-:30.0 pg. 100 (;in. and sacrificed after 16 11011~s.Eirz\mr ;Icti\-it\, \xis calcl~l;~tctl per 100 (Gun. TIIC Id\. weight aird expressed as pcrumtage~ of controlk taken as IO0 per wrh asterisks indicate sigilific;wt alterations statisticall\ different from \~Llllrs of tllct C’oIt1ro1 rats. (1’ =
lh.~l~~xose
isomcwse
121, 124 and dfects
uctivitv
105 pr
of c~thioninr
versed
by rthioniw
(221
pc’r crnt)
and
Thus,
niiir gest
synthc,sis
that
the
phoh~~xosr Thy
of
and/or followiiig control thw
c~xprini~nt
anv
s&d
onlv
port
to thk
of ukrine
;~pprwial~k
\vas
view
carrid
out.
wtinomycin studies
1,~ hlurllc~r horniom~s
HNA
and
wnts
wtrogenic
protck
co-work+’
activitv.
inliil,itioii
rcacwltlv rcsvcwecl
wtivitv
Of synthrsis
of cstroqcnic I
alouS
id cutain
1)iosvntlicsis. of s&l,lc-l
our
that
~idi;iinistratit,11 into
l
<;ol-ski
csstratliol
in rat uterus
data
the, suggrstion
1jrc’;111(l
c;~I~s~~(~
and
that
olww~atioi~s
l~hospl~ol~~xosc
ot
utcbriirr>
cwnpl<~tc~ly
lvith
prc\ious
arc’ ii1 lines \vith
1’r(L-
prcuuwrs
lwcwnt
in ukrine \I.ith
sup-
ill the, ;lcti\it\.
tllis
011 thcs isorncw~c~
on
phosph0-
that
ri~ki!’ 1~1 one’ of thcs prim;ir\
stilnllac+ioi~s
hormones.
oiltht>ir rcsccwt studic,s, a&on
of this
is l~~lic~~d
dclition~~l
l
trc~atment
ethos
iiicrcaasc.
in this kssucl
ill tllc~ rat
iii stcpa. First, cstrogcw target tissue, i.c*., uterus. wtivit\,
promvcin,
~iintl promvcin
r(i-
Furthermore,
of l~NA-l”)lvrnc.r~~s~,
h\,
to
and
yiizvmC
of
of
ant1 \fy’r(’ failed
as \vc,ll as pm‘omy~in that
th(, ntyri
activitv
lrncls
sho\ln
r~sponsw.““‘)”
tllca
aclmixiti~g
incwas[~
of DNA-cliwctcyl
cl~moiistrat~d
in the activitv
Such
incorporatiol~
of tlwse
of rstroSnl-intlu~~~l
fi&okinasr~
Bawd
thci
from
at the l&e1
his groiq~1i~2” lla\,e
Actinomycin
lw
actinomvcin
estrogen
and
ilr viva.
incwase could
inhibitor
c7i~vmc’
Accordingly.~
of wzvmc’
clrs nova
bvnthcsis
phos-
~~lios~~liolic~xos~~
proportions
obwrvation
wpscwts
in ukrinc,
Supernatants in carving
This
protc+n
stimulate>
Iwthio-
of prc-existing
~stroS~n-indL1~c.d
acwleration hail
a marked
lation
inhibits
II is ;I pvcrful
ckstropic
incrwsc
olwr\x~cl isoniwiw
puromvcin
rrprtd
that
tk nova.
consicl~wcl.
or inhil~ition
summation.
tlw
phosl~holiexos~
\\‘hereas \ioiis
that
c~stradiol inliihitioit
\\‘a
in utrrinca
furth(~r
\vc‘w mix&
activation
in the ~xpctd
\\ith
increases
inckcwcs
:~ssa~~~l for phosl~l~ol~esose~xos~isom(‘rasc
produce
treatd
of dhiollinc~
cluck to an activation
\vas
rc’-
on mrtisoiw ~ilicl rc&dingsug~iizviiws. lCi Thescn findings
svnthcssis
~,strt,R~n-induc~~~l
c.str~~diol-tre~it~~~l rats
wml~lrt~l\~
also liavc~ sliomm
hqxitic
06 im inhildor.
in vitro and
at
of ~tliioirinc~
mav lw tlu~ to enzvme
tlic rrmc;\al
arc
p2iosphofructo~ili~~s(~
estradiol-iliducctl
~oulcl liavc, lwrn
rwn~tinrd th(a inhihitor\~
injcckd comurr;~lItl\rcWrncd complrtV1;~
of rats
co-nwrkc~rs
important
ohwr\wl
that
activitv
that
iiicrcucs
r(~vcwal
uteriw
c4kts
of wveral
possibilit\r
in utui
nidiioninc~
\Vc~lx~r aid
prrwntlv
isoiiwr;~s~
isoiwraw
lw
svnthesis
can rc’vc’rsC thrs inhibitory
induced
~ii%vm~
lrvclohscyvcd
In a&lit&
of rats
~strogen-trc,~\t(~~l rats pliosl~hollc~xost~ isoni(wsc
cent ). A similar
of c,str~~diol-iiiduc~~l pviously.”
:3 groups
It is intcwsting
in
mdhioninc~,
to the
(228 per
alonr~
of thwc
on t,stradiol-inducc,~l
mrd~ionine.
with
in uteri
cent. ‘reqwctiwly.
that
r~ccptor this
utrrus iiit(wc+s
<&ski
protc,in
co-\\~orkc~rs2i
stay
;IS a rcwlt
intcwdiolI
invol\yhs
ha\.cs sll~gc~st~~(] t]lilt
consiclrrcyl
st;~r~,o-sl”.‘.it~~,ll~~
Tllcb sCcont1
primarv
aid
inki\‘ 1~5 arl)itraril\,
\\.itll ;i changy
of its intcwction is rc’po~~sil)lt~
;~s ()ccllrrillg
;k rcyy,l)tor
ill ttlc.
iu tllc- l)i()logic,;il \\ith
cLstrogc%It. It
for ;m i~l~rc~;~s(~itI g1~1.
c’osc’ m~tal~olisni, lipid, and ’ liN.4 svlltllcxsis. Tlrcwa authors” ha\ c’ suggrstc,tl that syntliclsis Of r,cdain sp~dic ciizvmc’s iIi;i\’ l)c~ ill\~ol\;~tl in iilc,rcylsillg t]lcbxc’ \.ital iwt~~holi~ procywc~s. sinccl c,ctrog[~i1-iiltlLl~(,~t rc~sl>o~~sty ;ir(’ ill1l,lO~!dYl
I:‘L‘lQIINt: I’HOSI’HOHEXOSE
ISOhlEIMSI~:
277
lw actinomycin and puromycin at a time when no c+fec% is noted on overall protein synthesis. Estradiol has been sho\vn to incrraw thcb activity of se\wal Ilterine enzvmes2:i.2i hut whether or not the olwxvecl increases represent c’nzvmc &thesis remains to 1)~ demonstrated. Previous studies by Wallas ani co-w&kerslzi have shown that glycolysis in isolatecl uterine muscle is grcaatlv enhanced hy treatmrnt of the rat \\ith estrogen. Our present obsc~vations on estradiol-induced increases in uterine phosphohexose isomerase. together with those reported earlier for l~l~ospl~ofructokinasr”-‘x art’ in agrectmcwt \\.ith thta above views of Corski and co-workers.“’ It is tempting to specwlate that the increased glycolysis observed in the rat uterus following cstrogrn treatment may be associated with an incrwwcl rate of synthesis of specific enzvrn~~s. Further studies on c,stladiol-induction of other uterine enzymes in\wlvc,cl in flucwr mctalx~lisni ;w curwntlv in progrws in this lal,oratorv. ACKNOWLEDGMENTS enc. ot ,,b (KIS) js gl.at&11 to I’I.ofcswr continilcd intrrrst. encowngen~rrlt for twhnic;ll assistance ant1 Dr.
(hxgc \C’rhr of Indiana rtlivcrsit! ;~ntl xlvivt~. Thth ;~llthors thnk Airs. Xhriette (;c~)rgr Howr clt \lrrck. Shat-p ;~rltl Doh~~rc~ for
gift< of .~c%incm~\.ci~l D. REFERENCES
for
lli\
%icdillski
ynt~r~~~~
1:3. \Vall;~s.
0..
~l’allu.
E.. antI
I.iikW,
I;.:
Ef+‘ect of oestratliol n~onolxmmatc. 011 the nWtal,olislr~ of rat lltcrinr~ mllscle. .kta Endocrinol. 10:201-21 1. 19Ti2. 14. Kennv.
F.
T.,
and
Flora,
Ii.
hl.:
In-
t\.rosin~-tr-~~~t(~~lll~~~r~lte dllction of transnminasc~ in rat liver. 1. Biol. Ch?111. 7:36:%99-~703, 1% 1 1.5. M:el)er, C:.. ant1 Singhal. K. I,.: Rtrl<~ of cnz~mcs it1 homeostasis \‘I. Elf’td of triamcinolonr antI 0thc.r strroitls on rnzymes involxd ill ~lucorleogenc~sis. 13iochem. 1’11arm:~~ol. I:i: 117:316. -.
1187. 1964. Banrrjee. <:.. untl Brcmdvilr. S. 13.: Selective intlnctiml ;mtl sllplxcssiolr of Ii\ t’r c1nx\.,11(’ I)ios\~nthvsis. :Zmer. J, Physiol. 2ob: 1:37-14i, 196-7.
17. IlerrarWn. A.. ;mtl hlllell~~r. (i. c.: Ellcct of estradiol on thr metalx~lisnr of \erine-3-C’-’ in s,lr\ il,irly: Iltcrine
1956. ler\,ell. K. I’.. DiniT, C. Ii.. ant1 ~lucllrr. C:. C.: E;~rlv t~lfecta of cstr;ldid
on
nllclric
acid
mc~t;~l~olisln
in
thr mt uterlls. J. Hiol. Chc~. 2:31: 94Yj-959. 1958. 19. \lueller, (G. C.. llerrancll, A.. ant1 Jvrvell. I;. I’.: Studies on th(L lllechxiism Prop. 40. -,
of action of fdrogens. Hvc. Hormone Krs. 14395-1339. 19.58. Y.: Thr Corski. J.? ant1 Aizawa,
role of protein avnthrsis rstrogen action. l’roc. NatI. IT, S. 47:104-169. 1961. 21.
ill (WI\ :\catl. SC;.
(kn&. J., Notelx)onr. 11’. I>., ant1 Kicolettt~. J. :\.: Estroi_‘cn control of