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Protein degradation during diauxic growth of Escherichia, coli
Vol. 20, No. 6, 1965
BiOCHEMlCAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
PROTHN DmRADATION DURIN@ DIAUXIC OabWTH OP ESCHERICHIA COLI
N. S. Wlllette national
Inetltute
for Medical Rerearoh,
all
Hill,
London, N.W.7.
Received August 3, 1966 The phenomenon of diauxlo (1945).
He gr8r B. &
and found that
in a
growth
wae fket
contalnlq
medium
demonetrated both glucose
there were tm pheree of growth
eeparated
during We
period en intermediary
and lactoee,
by a lag period.
A mechauiemproposed to explain this le that the cello flret glucose:
by &mod
utilized
the
metabollte me prodwed aoh
repreered the eyntheeie of the ensyma neceeeary for laotore utillratlon, even in the pre8ence of laetoee.
When the gluoore use exheueted, the aelle
had neither the entgmee neceseary for lactoee utilieatlon, for
their
nor amino aclde
Then emlno aoide were derived from Intracellular
eptherie.
breekdoun of protein
(We
lncmaeing in rate when growth rtopped) and ueed
for the aynthe8i~ of proteine -oh
Included the now denpmeed
neoerv
Exponential growth war then reeumed
for la&ore
utlllration.
erwue
(Maudeletem, 1963). A rimllu
growth 4
~110 were tmtaoferred fsotore thedse; nthlonine mixture
whbh
they
har
alm
to a m
wili\n
had the ge~typlo,
e.g. arglnlne
(tkwinl,
been okerred
In other -tam
fmm one eon-
but not pb~Qpie,
acide
and
growth
Ruth ability
to w
9undermn and Rurser, 19611, wmteiae and
(Bourgeois, Wan and UUnaehle~lle, of amlno
where
fadore
1960).
692
prement in a
1960); or the eo*er broth
medium(u,
BIOCHEMICAL
vol. zo,No.6,1965
pirect
conflrmstion
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
of the connection between di8uxic
growth
rind protein deg%sdatlon haa been obtained during growth of g. & on 8 mixtum of glucoosecud either lactate
E. Coli XL 328~ lsc+leu- w8e1grorar. in a synend Methoda. mm
Yeteriale thetic
medium(Mandelstem, 1960))
p&l),
or glycerol.
8nd containing
of Lv8llne
supplemented
nith
DLleudne
the carbon eouroee end different
described below.
Emline,
&iWL
At
extracted protein
end then followlng
the begimlq
Its liberation
ecid.
radioactivity
into the culture eemples were
acid (TCA) at 90’ C for 30 mln.
were flltered
on Oxoid membranefilters
eucceeeively ulth 5%TCA cont8iniq 1% acetic
cello nith radio-
of the experiment, culture
with 5% trichloroacetic preclpitatee
conoentrntiona
All lncubatione were at 35' C.
Protein degradation me measured by labelllng active
(300
Emline
( 150 v&l),
end nrarhed 5% TCA, and
They were then glued tc alundnium plenchettee end their
determlned, giving 8 measure of the original
of the cell protein.
radioactlvzlty
Culture remplee were t&en during the experiment,
oooled to 0’ C tc prevent further
metabolitm, end centrifuged.
rupenzatent w8e rexwed,
and ite emino aoidr adeorbed onto
diluted,
coluume of Zeo-K8rb 225 in the Ii+ form. with water tc remcve inorganic 0x080s of 2 2 EH,OH.
eelte,
The eclutionfi
8ud the amino 8cide eluted with en were evaporated to drgnsee at 100’
There were dried end their
radioactivity
menwureof the nmcunt of radioactive Comparison of thb eetimte
The
The columua were rrarrhed through
and the residue6 dieeclved in w8ter end trenefemd ettee.
The
Lv8llne
with the radioactivity
to 8lumlnlum planchdetermined, giving a
in the culture
mapernntnnt.
of the cell protein gave (UI
of protein degrpdation.
Prellmlmry experlmnte elmwed thet radioactive Lmline w8e Incorporated only into Lmline in the cell protein, end that cell lyeie followed by extracellular
protein
degmd8tion
002iditl0ar umd in theae l xperlmente.
693
C,
did
not occur under thg
The liber8tion
of intmmllul~
Vol. 20, No.6, 1965
BIOCHEMICAL AND BWHYSlCAl
&galaotoeidaee
Into
the culture
RESEARCH COMMUNICATIONS
medltm use umed ae en index of cell
lyrlr. Correotiona preparation
were mede for loor
of radioaotivlty
of the eamplee, end for their of their
detemination
radioaotirity
dudng
eelf-abeorptlon
duz%ng
(in an Automatlo Sample Changer
Counter with a thin end-ulndon Geiger tube dote&or).
Beeult8.
Cells were grownfroma
mallinoculum
mediumcontaining glucore (1 m&l) 0.1 p&l).
and L-f4CJ
(1%)
reeuepended in amediumcontaining (200 &l).
We latter
radloaatit&
(35 &ml;
valine
during exponentld
They were hamooted
inamediumcontalnlngL-valine
in the synthetic
growth, mahed tuioe
p&l)butno
carbon~ource,
gluaoee( 150 &l)arrcZ
Errline
wae included to prevent reinoorporation
L-saline liberated
culture
and -lea
a period of 9C min. for the detezmlnation of
deneity and protein
degradation.
almoot exhaueted, and the following to oulture(a)
of
by protein degradation.
Thl8 culture wae divided into eix part6 ((a) to (f)), t&en from eacshover
and
glucose wa8
Atthispolntthe
addltione uere tie:
eodiumla&ate(SCC
&I.)
n
(b) @y-=1
w
(0) no addition
W
(d) glwo-
w
(0) gluooee (SW p&l)
and eodium la&ate
n
(f)
and gl@erol
(@C M@)
(eo0 da)
glwo~e (see II&&
(WC &ml)
(sao 44.
The additions were delayed to eneure mlnlmel 8yntheslm of the en-0 fint
neoeeeaq for the utilleation
of laotate
or glycerol
drprine
the
growth period. Sampler were taken for
the determlnatlon of suture
and protein degradation for afurthor The result8
are
ohown in pig.
duuiw
150 min. 1.
694
Those
of experimnte
(d),
(e),
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Vol. 20, No. 6, 1965
$20 i c 35 I -10 5 =5 0a 0
12
3
4 TIME
Fig. 1. Protein degradation during growth on: A, end lactate (SO0 &ml); B, glucose (150 &ml) and p&l); C, glworo (150 p&l); D, &woee (950 with la&ate (SO0 pg/lil), or glyoerol (SO0 &ml). Symbole: 0, protein degradation; o , culture deneity.
and (f)
were similar,
neither
lactate
aud are shown In Fig.
nor glycerol
1, D.
per ee &fected
Thle indicated
the rate
that
of protein
degradation.
of protein
Comparison (c) aud (d)
&owe
expdnentially
degradation
that the rate
was slow (about
about 6% per hour)
and cell
of protein
0.6s
degradation
per hour),
when the glueore
there wae a diauxie
of expmential
growth.
at an lnureared
rate,
wherear
degraded at the #low rate Three reeulte intracellular ayntheeia
support
protein end that
of the wchaniam
In oelle
thi8
protein
of diauxlo
leg period,
both before
charaoterietlc
in experlmentm
rapidly
(to
euppllee
degradation growth.
695
uaa degraded
and aitmmrds
that
(a) and
the two perioda
protein
of grouiug
the mgge6tion
degradation
growing
WELBexhawted.
leg of about 30 ndn. between During
in experiments
but lnareased
When a eecood carbon Bource mu3 pxwent, (b),
growth
it
wea
oelle.
during
a diauxic
lag
the emlno a&de for protein
is therefore
an eeeential
part
Vol. 20, No. 6,1965
Aeknowledmaent. adrioe
throughout
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
The euthor rriehee to thank Dr J. kndeletem
for hie
this w*.
Referenaee. Ii. (1960) Bioehlm. Bourgeole, S., Whme, J. Y., and Lelouchler-Degrmlie, Biophye. Aota 38, 136. Gorini, L., Ounderaen, W., and Burger, Y. (1961) Cold Spr. Harb. Sump. quent. Blol. 26, 173. Maalgfe, 0. (1960) Symp. Soo. Oen. Hlcroblol. IO, 272. Meadeletem, J. (1960) Blochem. J. 6& 103. Mandeletem, J. (1963) Ann. I?. Y. Aead. 801. 102. 626. Mod, J. (1945) Ann. In&. Peeteur 111, 37.
BiOCHEMlCAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
PROTHN DmRADATION DURIN@ DIAUXIC OabWTH OP ESCHERICHIA COLI
N. S. Wlllette national
Inetltute
for Medical Rerearoh,
all
Hill,
London, N.W.7.
Received August 3, 1966 The phenomenon of diauxlo (1945).
He gr8r B. &
and found that
in a
growth
wae fket
contalnlq
medium
demonetrated both glucose
there were tm pheree of growth
eeparated
during We
period en intermediary
and lactoee,
by a lag period.
A mechauiemproposed to explain this le that the cello flret glucose:
by &mod
utilized
the
metabollte me prodwed aoh
repreered the eyntheeie of the ensyma neceeeary for laotore utillratlon, even in the pre8ence of laetoee.
When the gluoore use exheueted, the aelle
had neither the entgmee neceseary for lactoee utilieatlon, for
their
nor amino aclde
Then emlno aoide were derived from Intracellular
eptherie.
breekdoun of protein
(We
lncmaeing in rate when growth rtopped) and ueed
for the aynthe8i~ of proteine -oh
Included the now denpmeed
neoerv
Exponential growth war then reeumed
for la&ore
utlllration.
erwue
(Maudeletem, 1963). A rimllu
growth 4
~110 were tmtaoferred fsotore thedse; nthlonine mixture
whbh
they
har
alm
to a m
wili\n
had the ge~typlo,
e.g. arglnlne
(tkwinl,
been okerred
In other -tam
fmm one eon-
but not pb~Qpie,
acide
and
growth
Ruth ability
to w
9undermn and Rurser, 19611, wmteiae and
(Bourgeois, Wan and UUnaehle~lle, of amlno
where
fadore
1960).
692
prement in a
1960); or the eo*er broth
medium(u,
BIOCHEMICAL
vol. zo,No.6,1965
pirect
conflrmstion
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
of the connection between di8uxic
growth
rind protein deg%sdatlon haa been obtained during growth of g. & on 8 mixtum of glucoosecud either lactate
E. Coli XL 328~ lsc+leu- w8e1grorar. in a synend Methoda. mm
Yeteriale thetic
medium(Mandelstem, 1960))
p&l),
or glycerol.
8nd containing
of Lv8llne
supplemented
nith
DLleudne
the carbon eouroee end different
described below.
Emline,
&iWL
At
extracted protein
end then followlng
the begimlq
Its liberation
ecid.
radioactivity
into the culture eemples were
acid (TCA) at 90’ C for 30 mln.
were flltered
on Oxoid membranefilters
eucceeeively ulth 5%TCA cont8iniq 1% acetic
cello nith radio-
of the experiment, culture
with 5% trichloroacetic preclpitatee
conoentrntiona
All lncubatione were at 35' C.
Protein degradation me measured by labelllng active
(300
Emline
( 150 v&l),
end nrarhed 5% TCA, and
They were then glued tc alundnium plenchettee end their
determlned, giving 8 measure of the original
of the cell protein.
radioactlvzlty
Culture remplee were t&en during the experiment,
oooled to 0’ C tc prevent further
metabolitm, end centrifuged.
rupenzatent w8e rexwed,
and ite emino aoidr adeorbed onto
diluted,
coluume of Zeo-K8rb 225 in the Ii+ form. with water tc remcve inorganic 0x080s of 2 2 EH,OH.
eelte,
The eclutionfi
8ud the amino 8cide eluted with en were evaporated to drgnsee at 100’
There were dried end their
radioactivity
menwureof the nmcunt of radioactive Comparison of thb eetimte
The
The columua were rrarrhed through
and the residue6 dieeclved in w8ter end trenefemd ettee.
The
Lv8llne
with the radioactivity
to 8lumlnlum planchdetermined, giving a
in the culture
mapernntnnt.
of the cell protein gave (UI
of protein degrpdation.
Prellmlmry experlmnte elmwed thet radioactive Lmline w8e Incorporated only into Lmline in the cell protein, end that cell lyeie followed by extracellular
protein
degmd8tion
002iditl0ar umd in theae l xperlmente.
693
C,
did
not occur under thg
The liber8tion
of intmmllul~
Vol. 20, No.6, 1965
BIOCHEMICAL AND BWHYSlCAl
&galaotoeidaee
Into
the culture
RESEARCH COMMUNICATIONS
medltm use umed ae en index of cell
lyrlr. Correotiona preparation
were mede for loor
of radioaotivlty
of the eamplee, end for their of their
detemination
radioaotirity
dudng
eelf-abeorptlon
duz%ng
(in an Automatlo Sample Changer
Counter with a thin end-ulndon Geiger tube dote&or).
Beeult8.
Cells were grownfroma
mallinoculum
mediumcontaining glucore (1 m&l) 0.1 p&l).
and L-f4CJ
(1%)
reeuepended in amediumcontaining (200 &l).
We latter
radloaatit&
(35 &ml;
valine
during exponentld
They were hamooted
inamediumcontalnlngL-valine
in the synthetic
growth, mahed tuioe
p&l)butno
carbon~ource,
gluaoee( 150 &l)arrcZ
Errline
wae included to prevent reinoorporation
L-saline liberated
culture
and -lea
a period of 9C min. for the detezmlnation of
deneity and protein
degradation.
almoot exhaueted, and the following to oulture(a)
of
by protein degradation.
Thl8 culture wae divided into eix part6 ((a) to (f)), t&en from eacshover
and
glucose wa8
Atthispolntthe
addltione uere tie:
eodiumla&ate(SCC
&I.)
n
(b) @y-=1
w
(0) no addition
W
(d) glwo-
w
(0) gluooee (SW p&l)
and eodium la&ate
n
(f)
and gl@erol
(@C M@)
(eo0 da)
glwo~e (see II&&
(WC &ml)
(sao 44.
The additions were delayed to eneure mlnlmel 8yntheslm of the en-0 fint
neoeeeaq for the utilleation
of laotate
or glycerol
drprine
the
growth period. Sampler were taken for
the determlnatlon of suture
and protein degradation for afurthor The result8
are
ohown in pig.
duuiw
150 min. 1.
694
Those
of experimnte
(d),
(e),
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Vol. 20, No. 6, 1965
$20 i c 35 I -10 5 =5 0a 0
12
3
4 TIME
Fig. 1. Protein degradation during growth on: A, end lactate (SO0 &ml); B, glucose (150 &ml) and p&l); C, glworo (150 p&l); D, &woee (950 with la&ate (SO0 pg/lil), or glyoerol (SO0 &ml). Symbole: 0, protein degradation; o , culture deneity.
and (f)
were similar,
neither
lactate
aud are shown In Fig.
nor glycerol
1, D.
per ee &fected
Thle indicated
the rate
that
of protein
degradation.
of protein
Comparison (c) aud (d)
&owe
expdnentially
degradation
that the rate
was slow (about
about 6% per hour)
and cell
of protein
0.6s
degradation
per hour),
when the glueore
there wae a diauxie
of expmential
growth.
at an lnureared
rate,
wherear
degraded at the #low rate Three reeulte intracellular ayntheeia
support
protein end that
of the wchaniam
In oelle
thi8
protein
of diauxlo
leg period,
both before
charaoterietlc
in experlmentm
rapidly
(to
euppllee
degradation growth.
695
uaa degraded
and aitmmrds
that
(a) and
the two perioda
protein
of grouiug
the mgge6tion
degradation
growing
WELBexhawted.
leg of about 30 ndn. between During
in experiments
but lnareased
When a eecood carbon Bource mu3 pxwent, (b),
growth
it
wea
oelle.
during
a diauxic
lag
the emlno a&de for protein
is therefore
an eeeential
part
Vol. 20, No. 6,1965
Aeknowledmaent. adrioe
throughout
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
The euthor rriehee to thank Dr J. kndeletem
for hie
this w*.
Referenaee. Ii. (1960) Bioehlm. Bourgeole, S., Whme, J. Y., and Lelouchler-Degrmlie, Biophye. Aota 38, 136. Gorini, L., Ounderaen, W., and Burger, Y. (1961) Cold Spr. Harb. Sump. quent. Blol. 26, 173. Maalgfe, 0. (1960) Symp. Soo. Oen. Hlcroblol. IO, 272. Meadeletem, J. (1960) Blochem. J. 6& 103. Mandeletem, J. (1963) Ann. I?. Y. Aead. 801. 102. 626. Mod, J. (1945) Ann. In&. Peeteur 111, 37.