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Neuromedin U-8 and U-25: Novel uterus stimulating and hypertensive peptides identified in porcine spinal cord
Vol. 130, No. 3, 1985 August
BIOCHEMICAL
15, 1985
NEUROMEDIN U-8
AND U-25: Naoto
Received
June
27,
NOVEL UTERUS STIMULATING AND HYPERTENSIVE PEPTIDES IDENTIFIED IN PORCINE SPINAL CORD
MINAMINO,
Department
AND BIOPHYSICAL RESEARCH COMMUNICATIONS Pages 1078-l 085
Kenji
KANGAWA and Hisayuki
MATSUO
of Biochemistry, Miyazaki Medical Kiyotake, Miyazaki 889-16, Japan
College,
1985
SUMMARY: Two novel peptides eliciting a potent stimulant effect on the rat uterus smooth muscle have been purified and identified in porcine spinal cord. These peptides were designated as neuromedin u-8 (8 amino acids long) and U-25 (25 amino acids long) refering to their uterus stimulating activity. Sequence analyses and syntheses revealed that neuromedin U-8 is a novel octapeptide with a C-terminal amide structure, while u-25 contains the U-8 sequence at its C-terminus, preceded by paired Arg residues, implicating their biosynthetic relationship. Their potent uterus stimulating activity and hypertensive effect, as well as their unique C-terminal amide structure are indicative of their specialized physiological function. @ 1985 Academic Press, Inc.
In a survey a
simple
preparations muscle
but
for
unidentified
sensitive
assay
successfully
stimulating "B" ,
enabled
peptides
comprising
and
the complete
amino
acids
uterus
activity,
Their
purified. be discussed
us
spinal "KM
acid
sequence
and 11U-25" by
hypertensive
in comparison
we present
long)
which those
effect
that
on smooth-muscle
a family
of novel
smooth-
cord, named as "neuromedins", "L" ckassinin-like) and "Nl!
the
identif
ication
in porcine
of two new neuromedins.
spinal
designated
(25 amino
acids
long)
peptides
have
been monitored
both
and smooth-muscle with
we have demonstrated
stimulant
to discover
in porcine Here
as IIU-!j'lt (8 amino stimulant
the
"C"(bombesin-like)?
(neurotensin-like)(l-5). cord
neuropeptides, for
of several
stimulant
activities
known bioactive
after will
their and also
peptides.
MATERIALS AND METHODS in the present purification were Purification: The starting materials used side fractions obtained in our previous purification of neuromedin B, C, K, L Porcine spinal cords (ca. 20kg obtained from 550 pigs) were and N (l-5). minced, heat-treated and extracted with 1M CH COOH containing 20mM HCl. After by acetone-precipitation an Amicon UH-2 membrane, aallowed desalting through was evaporated at a final concentration of 752, the supernatant --in vacua to
Abbreviations: TLC, thin layer substance. P; polypeptide: Mr,
RP-HPLC, reverse phase high performance liquid chromatography: TFA, trifluoroacetic acid; BK, bradykinin; SP, chromatography; vasoactive intestinal polypeptide: PP, pancreatic VIP, molecular weight.
0006-291X/85$1.50 Copyright AN rights
0 1985 by Academic Press, Inc. of reproduction in any form reserved.
1078
Vol.
130,
BIOCHEMICAL
No. 3, 1985
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
materials were dissolved in 1M CH COOH and then submitted to dryness. Dry ? m), pre-equilibrated with batchwise chromatography on SP-Sephadex C-25(H+-fo 1M CH COOH. Successive elutions with 1M CH COOK, 2M pyridine and 2M pyridineCH COdH (pH 5.0) yielded three fractions of’SP-I, SP-II and SP-III. The SP-III frdction containing basic peptides was separated by gel filtration on a column of Sephadex G-50 and then on a column of Sephadex G-25. An aliquot of each Uterus fraction was subjected to bioassay for rat uterus stimulant activity. activity was observed in a wide range of fractions A to F (Fig. la). Neuromedin 11-x and U-25 were isolated from fraction F and fraction 8, respectively. i) Neuromedin U-8: After lyophilization, fraction F was subjected to ion exchange HPLC (Fig. lb). The uterus active fraction eluted at 103-105 min was further purified by RP-HPLC to vield neuromedin U-3 in a pure state (Fig. lcl. ii) Nenromedin U-25: Fraction-B (Fig. la) was submitted to a preparative RP-HPLC to yield two peaks with uterus activity (Fig. 2a). The uterus active fraction eluted at 128-136 min was further purified by cation exchange HPLC to give a single bioactive peak eluted at 68-71 min (Fig. 2b). The active fraction obtained above was further separated by RP-HPLC on a Chemcosorb 7-diphenyl column (Chemco) and finally on a C-13 column to purify neuromedin U-25 to homogeneitv(Fig. 2~). Structure Analyses: i) Amino acid composition: Analyses were carried out with an amino acid analvzer (Hitachi-835), after acid hvdrolvsis of the purified neuromedins in 6M HCl containing 0.17:’ phenol and 0 .G27! 2-mercaptoethanol at 110°C for 20 hr. ii) Amino acid sequence: Neuromedin U-8 (ca. 200 pmol) and neuromedin U-25 (ca. 200 pmoll were each sequenced with a gas-phase sequencer (Applied Biosystems Model 47DAl (6), coupled with HPLC identification of the resulting PTH-amino acids (2). iii) C-Terminal analysis: The C-terminal amide structure W&S verified by trypsinization of the pept ide , followed by dansplat ion, in a manner similar to the method reported by Tatemoto and Mutt
(7). Syntheses : Neuromedin U-8 and U-25 were synthesized by solid phase techniques conducted on p-methyl-benzhydrylamine resin. Bioassay: i) Uterus stimulant activity: Assay was performed according to the described method (8) by using strips of rat uterus preparation freshly isolated in proestrous stage, in a modified Locke’s solution at 32°C. ii) Hypertensive effect: Systemic blood pressure was measured from the carotid artery in rats (000-4@Og) anesthetized with pentobarbital (5). Indicated amounts of peptides in 100-200 ul of 0.4’7 saline were administered through a cannula in the femoral vein. BK, SP and VIP were purchased from Protein Research Foundation. Bovine PP was kindly donated from Dr. A. Arimura, Tulane University School of Medicine.
RESULTS Neuromedin for
the
manner
to
peptide
that
used
Sephadex
of
G-50
further
uterus
to
collect
the
regions
(A-F). three
spinal fractions
purified subjected
was
(1).
The the
rat
spinal uterus
by
SP-Sephadex was
a Sephadex widely
(Fig.
of
C-25
to G-25
bioactive subsequent
Yr
1079
As in
peak
of
major
to
The
ca.
basicity purify
basic of
in
the on
daltons, shown
the
peak,
higher
assay
gel-filtration
5,000
F (tir the
RP-HPLC
(I-5).
by
column.
fraction
an
a similar
chromatography
separated
From
using in
neuromedins
distributed
lb).
cord
preparations
of
cord
HPLC
peaks
to
porcine
corresponding on
Cation-exchange bioactive
from
isolations
prepared
activity
DISCUSSION
isolate?
previous
rechromatographed
yielded
was
the
porcine
stimulant
previously
in
on
(SP-III!,
extract
were
purified
effect
fraction
acid
min
Us were
stimulant
AND
which
Fig.
la,
chromatographic 1,000
daltons)
neuromedin eluted neuromedin
B was at U-8
104 to
Vol.
130,
No. 3, 1985
BIOCHEMICAL
AND
BIOPHYSICAL
Abd---- B
C
DE
RESEARCH
COMMUNICATIONS
F&
L
0
10
40 number
30
20
Fraction
Time
50
60
70
(mtn)
C
-.
0
_- - _____
10
____-__-- ---
20
________--------
30
Tlme
_ __------ _______-------
40
‘i z II 0:
50
(mln)
Fig. 1 Purification of neuromedin u-8. a) filtration of SP-III on a Sephadex G-25(fine) column (7.5 x 135 cm). Eluent: 1M CH COOH. Fraction size: 100 ml/tube. Flow rate: 60 ml/hr b) Cation exe a ange HPLC of fraction F (l/3 portion) in Fig. la. Column: TSK IEX-530 CM (4.0 x 300 mm, Toyosoda). Flow rate: 1 ml/min. Solvent system: Linear gradient elution from A:B = 100: 0 to 85:15 for 48 min, followed by the second gradient from A:B = 85:15 to 50:50 for 48 min. (A) 1OmM HCOONHd(pH 6.5):CH3CN ; 9O:lO (v/v), (B) l.OM HCOONH4(pH 6.5):CH3CN = 9O:lO (v/v,. 1080
Vol.
130,
No. 3. 1985
homogeneity
BIOCHEMICAL
(Fig.
fraction
B in
Fig.
fraction
B on
a C-18
(Note
that
from
purified.) min
peak
2~).
II-6
and
using
1.05
a
for
U-5
and
3b).
in
The
were
verified
the
structures
native
proceeded
by
acid
of
showr (0)
comparison.
structure
been
has
PP.
(7).
*Neuromedin U-8: Asp 1.05(l), Pro Neuromedin (J-25: .Asp .1.07( n,, Ser Ile i?.30(1), Leu
the
the
related far
peptides observed As oc
C-terminal
exhibiting in
seen
I:ig.
uring
in
Leu
0.04
O.o711), 1.00(l),
Glu Tyr
3.89(4J, 0.92(11,
1).
the
peptides,
end
(Fig.
U-8
and
,ja U-25 of
the
of
complete
are
U-3
the
shown or
C-terminal
hormonal
the
pancreatic
(10)
neuromedin
or
releasing
and
U-25 amide
physiological factors
a partial II-‘,
of
and
C-terminal U-25 to
also
is
O.oOil),
Phe
2.0%?(2),
Arg
2.02(?).
Pro
2.27(Z),
Phe
4.04(41,
Gly Lys
1.00(l), l.O5il),
Val Arg
1.74(2), 4.14(4)
Tyr
known
is
structure
c) Final purification of neuromedin U-8 by RP-HPLC. Column: Chemcosorb SODS-H (4.0 x 250 mm, Chemco). Flow rate: 1 ml/min. Solvent: Linear gradient elution from (A) to (B) for 80 min. Hz0 : CH3CN : 10% TFA = (A) 90 : 10 : 1, (8) 40 : 60 : 1 (v/v). uterus activity (Fig.la,b) and uterus active fraction (Fig.lc) are shown by black bars. BSA, bovine serum albumin; SPO, SP sulfoxide; gNE, cyneo-endorphin; SS, snmatostatin; LE, Leu-enkephalin; R6LE, [Ax-g I-Leuenkephalin; LHRH, luteinizing hormone releasing hormone; Dyn8, dynorphin[l-81. 1081
acid Edman
unambiguously
sequences
neuromedin
of
confirmation
been
3c .
for
sequences
PTH-amino
Thus,
to
acid
nmol
0.84
comparison
hypothalamic in
column
analysis.
neuromedin
have
by
amino
carboxyl
identified.
asparaginamide
1.00(l),
of
polypeptidc(VIPI
highly so
25
Positive
known
C-15
the
neuromedin
the
ones.
intestinal
of been
-Arg-Pro-Arg-X-CONH, But )
where
each
of
of
(J-25
a
acid
chromatographic
and
state
as
of
the
(71.
synthetic C-8
peptides
feature often
hormones of
the
pmol step
Mutt by
corresponding
.Tc .
pm01
upto
a pure
and
Amino
structure and
provided
vasoactive
150
3
128-1.16 From
on
estimated
first
amide
sequences in
a unique
gastrointestinal
in
and
200
yields
Tatemoto
Fig.
with
the
repetitive
was
pigs.
About at
neuromedin in
found
as
sequence
sequencer.
also
200
in
at
was
2b).
footnote)*,
comprise
Za).
peptide
finally (see
of
(Fig.
eluted
isolated
and
were from
determined
of
(Fig.
from
RP-HPLC
releasing peak
to
isolated
peaks
activity was
was
daltons.
bioactive
data
yields
starting
Although
is
their
above their
polppeptide(PP)
activities,
found
asparagine
with
as
never
were
high
sequences
established,
above
method
deduced
peptides
amino
the
hioactive
column,
peptide
C-terminal
two
U-25
analyses
automated each
gave
first
acid
were
from
the
amino
U-25, U-25
a gas-phase
of
diphenyl
the
3,000
gastrin
neuromedin
and
nmol
degradation
found
on
ca.
later,
COMMUNICATIONS
U-25
Mr
stimulating
above,
purified
generated
have
HPLC
respectively,
and
neuromedin
for
uterus
on
II-25
residues,
and
of
obtained
Based
to
eluted
RESEARCH
neuromedin
column, peak
peak
BIOPHYSICAL
hand,
corresponding
second
RP-HPLC
(Fig.
other
preparative
the
a single
successive
was
la,
Cation-exchange
gave
binactive
U-8
On the
ICI.
AND
occur
Vol. 130, No. 3, 1985
8lOCHEMlCAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Tlme
b
2 1 J
5 J
g 0.05
H 5 J
(min)
L JJ
a% JJ
___----
_----
-
8 p‘1
--___----
ii x i %
'
O;-; 0
20
40
60 (mln)
Tlme
0.15
80
100
c
I
P 0GO,lO_---
______--
----
________--
------
_____----
______- -----
_______--
-----
E 0" g 0.05 % I O-
I 10
60 20
30 Time
(mln)
40
50
Fig. 2. Purification of neuromedin U-25. a) Preparative RP-HPLC of fraction B (l/7 portion) in Fig. la. c01uml: TSK ODS-120A (2.0 x 25 cm, Toyosoda). Flow rate: 5 ml/min. Solvent system: Linear gradient elution from A:B =90:10 to A:B = 30:70 for 250 min. Solvents A and B were as in Fig. lc. b) Cation exchange HPLC of uterus active fraction (l/2 portion) cluted at 128-136 min in Fig. 2a. Column: TSK CM-2SW (4.6 x 250 mm, Toyosada). Flow rate: 1 ml/min. Solvent system: Linear gradient elution from A:8 = 100:0 to A:B 2 SO:50 for 100 min. Solvents A and B were as in Fig. lb.
1082
Vol.
130.
BIOCHEMICAL
No. 3, 1985
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
b
10
5
15
20
25
Cycle
number
8
4
J
Tyr-Phe-Leu-Phe-Arg-Pro-Arg-Asn-NH2
: NMU-8
Phe-Lys-Val-Asp-Glu-Glu-Phe-Gln-Giy-Pm-Ile-Val-Ser-G1n-Asn-Arg-Arg-Tyr-Phe-Leu-Phe-Arg-Pro-Arg-Asn-NH~ -
: NMU-25
----Ala-Ala-Glu-Leu-Arg-Arg-Tyr-Ile-Asn-Met-Leu-Thr-Arg-Pro-Arg-Tyr-NH~ ---_--
: PP
----Leu-Arg-Lys-Gln-Met-Ala-Val-Lys-Lys-Tyr-Leu-Asn-Ser-Ile-Leu-~* -----_
: VIP
-
Fig. 3. Amino acid sequences of neuromedin U-8 and neuromedin a) Yield of PTH-amino acid generated from neuromedin u-8. b) Yield of PTH-amino acid generated from neuromedin U-25. c) Complete amino acid sequences of neuromedin U-8(NMU-8) compared with porcine PP and VIP. Homologous sequences are line indicates the paired basic signal for processing.
only
in
VIP.
The
and
neuromedin
U-25
processing
signal
most may
likely take
residues
in
generate
rat
systemic
blood
substance
P(SP)
(Fig.
basis), U-25
neuromedin is
repeated Furthermore,
three
times
twitching U-2j
of
as
were
4).
With
is
approximately
potent
of
uterus
was
found
to
at
so
with
far
of
rat
sensitivity
-la),
which
paired
basic as
of
contrcation
bradykinin(BK)
and
activity BK.
while
neuromcdin 11-25
while of
(molar
(J-8 rat
induced did
uterus
c) Final purification of neuromedin U-25 by RP-HPLC. Column : Chemcosorb 30DS-H (4.6 x 75 mm, Chemco). Flow rate: 1 ml/min. Temperature: Solvent system: Linear gradient elution from A:B = 8@:20 45°C. to A:B = 0:lOO for 192 min. Solvents A and B were as in Fig. ic. Relative uterus contractile activity (Fig. 2a,b) and uterus active fraction (Fig. 2~) were shown by black bars. 1083
is
amides
uterus
neuromedin (Fig.
typical
procrssinc
peptide
those
of
identified.
stimulating with
a U-6
site
been
Interestingly,
increase
is
a similar
the
Us on
uterus
C-terminus
neuromedin that
equipotent BK.
the
C-terminal
not
compared
preparation to
PP
neuromedin
regard
as
of
truncated have
at
which
suggests
and
they
pressure
u-8
occurence
respective
activities
located
and U-25(NMU-25) underlined. Dashed
structure.
[I-25
family
though
is
Ax-g-Arg
natural
VIP/PHI
even
biological
a
neuromedin
their
entities, The
The from
also
sequence
by
(11,12).
place to
C-8
preceded
processed
endogenous
and
neuromedin
U-25.
not. to
Vol.
130,
No. 3, 1985
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
a BK 1.0
-
NMU-8 1.0 nM
nM
\-
. 0
NMU-25
NMU-25 0.7 ntl
0.35
nM
0
2
4
and
11-25
. 2
4
.
- 0
2
4 Time
0
2
4
rat
uterus
imln)
b
Time
Fig.
4.
-
Biological effects blood pressure.
systemic
neuromedin
IIs.
essential part
for
These
of neuromedin
activity. fact
they
Furthermore, anesthetized
rats
hypotensive
effect. in
systolic
(J-25 was longer It
should
amide rat
be mentioned
C-terminus
at the or on
is
important
neuromedin
a concentration
blood
900
elicit
stimulation.
of
that
exerting
nM, t;ith
times
no appreciable
indicating that its biological
a contractile which
hut
effect
(I-8,
SP and HK show potent 1084
blood
short-lived
LI-5 (Fig.
4b).
lacking
an c1-
biological
on guinea
to
15 mmHg of neuromedin
than
the amide activities.
Ils.
about
effect
more potent
the
nmol/kg) arterial
induced
des-amid+neuromedin
, showed
pressure,
v-8
of the despite
in
strong
The hypertensive
three
the N-terminal
(1.0
increase
nmol/kg,
may he
neuromedin
(1-q
have
rat
prolongation
with
neuromedin which
of 3.0
synthetic
C-terminus for
uterine
and sustained
pressure.
U elicited of
not
RK and SF,
and about
and that and
similarity
and
U-h sequence
reinforcement
structural
a dose
blood
lasting
structure
uterus
neither
At
uterus.
for
a rapid
from
on
the neuromedin
on rat
injection
produced
differing
increase
some
u-8
that
effect
PP and VTP did have
intravenous
pressure,
indicate
stimulant
11-25 may serve
Note that that
of neuromedin
results
exerting
(min)
effects
on
structure at the Tncidentally, pig
ileum
stimulant
even at activity
BIOCHEMICAL
Vol. 130, No. 3, 1985
(0.4-1.0
nM).
The pharmacological
of SP and BK, function
--in vivo
strongly
suggest
as neuropeptides
AND BIOPHYSICAL
spectra that
of neuromedin
neuromedin
RESEARCH COMMUNICATIONS
Us distinct their
Us may have
from those specialized
or hormones.
This work was supported in part by a Grant-in-Aid from the ACKNOWLEDGEMENTS: Science and Culture of Japan. We sincerely thank Ministry of Education, Tamayo Hatoh and Masuyo Hiranaga of our Department for their Tetsuji Sudoh, technical assistance. REFERENCES 1. Minamino, N., Kangawa, K. & Matsuo, H. Biochem. Biophys. Res. Commun. 114, 541-548 (1983). 2. Gamine, N., Kangawa, K. & Matsuo, H. Biochem. Biophys. Res. Commun. 9, 14-20 (1984). 3. Kangawa, K., Minamino, N., Fukuda, A. & Matsuo, H. Biochem. Biophys. Res. Commun. 114, 533-540 (1983). 4. Minamino, N., Kangawa, K., Fukada, A. & Matsuo, H. Neuropeptides 4, 157-166 (1984). 5. Minamino, N., Kangawa, K. & Matsuo, H. Biochem. Biophys. Res. Commun. 122, 542-549 (1984). 6. Hewick, R.M., Hunkapiller, M.W., Hood, L.E. & Dreyer, W.J. J. Biol. Chem. 256, 7990-7997 (1981). (1978). 7. Tatemoto,K. & Mutt,V. Proc. Natl. Acad. Sci. U.S.A. 75, 4115-4119 8. Carraway, R. & Leeman, S. J. Biol. Chem. 248, 6854-68iil (1973). 9. Floyd, J.C. Jr., Fajans, S.S., Pek, S. & Chance, R.E. Recent Prog. Horm. Res. 33, 519-570 (1977). 10. Bodanszky, M., Klausner, Y.S. & Said, S.I. Proc. Natl. Acad. Sci. U.S.A. 70, 383-384 (1973). 11. Nakanishi, S. et al. Nature 3, 423-427 (1979). 12, Steiner, D.F. Quinn, P.S., Chan, S.J., Marsh, J. &. Tager, H.S. Ann. N-Y. Acad. Sci. 343, 1-16 (1980).
1085
BIOCHEMICAL
15, 1985
NEUROMEDIN U-8
AND U-25: Naoto
Received
June
27,
NOVEL UTERUS STIMULATING AND HYPERTENSIVE PEPTIDES IDENTIFIED IN PORCINE SPINAL CORD
MINAMINO,
Department
AND BIOPHYSICAL RESEARCH COMMUNICATIONS Pages 1078-l 085
Kenji
KANGAWA and Hisayuki
MATSUO
of Biochemistry, Miyazaki Medical Kiyotake, Miyazaki 889-16, Japan
College,
1985
SUMMARY: Two novel peptides eliciting a potent stimulant effect on the rat uterus smooth muscle have been purified and identified in porcine spinal cord. These peptides were designated as neuromedin u-8 (8 amino acids long) and U-25 (25 amino acids long) refering to their uterus stimulating activity. Sequence analyses and syntheses revealed that neuromedin U-8 is a novel octapeptide with a C-terminal amide structure, while u-25 contains the U-8 sequence at its C-terminus, preceded by paired Arg residues, implicating their biosynthetic relationship. Their potent uterus stimulating activity and hypertensive effect, as well as their unique C-terminal amide structure are indicative of their specialized physiological function. @ 1985 Academic Press, Inc.
In a survey a
simple
preparations muscle
but
for
unidentified
sensitive
assay
successfully
stimulating "B" ,
enabled
peptides
comprising
and
the complete
amino
acids
uterus
activity,
Their
purified. be discussed
us
spinal "KM
acid
sequence
and 11U-25" by
hypertensive
in comparison
we present
long)
which those
effect
that
on smooth-muscle
a family
of novel
smooth-
cord, named as "neuromedins", "L" ckassinin-like) and "Nl!
the
identif
ication
in porcine
of two new neuromedins.
spinal
designated
(25 amino
acids
long)
peptides
have
been monitored
both
and smooth-muscle with
we have demonstrated
stimulant
to discover
in porcine Here
as IIU-!j'lt (8 amino stimulant
the
"C"(bombesin-like)?
(neurotensin-like)(l-5). cord
neuropeptides, for
of several
stimulant
activities
known bioactive
after will
their and also
peptides.
MATERIALS AND METHODS in the present purification were Purification: The starting materials used side fractions obtained in our previous purification of neuromedin B, C, K, L Porcine spinal cords (ca. 20kg obtained from 550 pigs) were and N (l-5). minced, heat-treated and extracted with 1M CH COOH containing 20mM HCl. After by acetone-precipitation an Amicon UH-2 membrane, aallowed desalting through was evaporated at a final concentration of 752, the supernatant --in vacua to
Abbreviations: TLC, thin layer substance. P; polypeptide: Mr,
RP-HPLC, reverse phase high performance liquid chromatography: TFA, trifluoroacetic acid; BK, bradykinin; SP, chromatography; vasoactive intestinal polypeptide: PP, pancreatic VIP, molecular weight.
0006-291X/85$1.50 Copyright AN rights
0 1985 by Academic Press, Inc. of reproduction in any form reserved.
1078
Vol.
130,
BIOCHEMICAL
No. 3, 1985
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
materials were dissolved in 1M CH COOH and then submitted to dryness. Dry ? m), pre-equilibrated with batchwise chromatography on SP-Sephadex C-25(H+-fo 1M CH COOH. Successive elutions with 1M CH COOK, 2M pyridine and 2M pyridineCH COdH (pH 5.0) yielded three fractions of’SP-I, SP-II and SP-III. The SP-III frdction containing basic peptides was separated by gel filtration on a column of Sephadex G-50 and then on a column of Sephadex G-25. An aliquot of each Uterus fraction was subjected to bioassay for rat uterus stimulant activity. activity was observed in a wide range of fractions A to F (Fig. la). Neuromedin 11-x and U-25 were isolated from fraction F and fraction 8, respectively. i) Neuromedin U-8: After lyophilization, fraction F was subjected to ion exchange HPLC (Fig. lb). The uterus active fraction eluted at 103-105 min was further purified by RP-HPLC to vield neuromedin U-3 in a pure state (Fig. lcl. ii) Nenromedin U-25: Fraction-B (Fig. la) was submitted to a preparative RP-HPLC to yield two peaks with uterus activity (Fig. 2a). The uterus active fraction eluted at 128-136 min was further purified by cation exchange HPLC to give a single bioactive peak eluted at 68-71 min (Fig. 2b). The active fraction obtained above was further separated by RP-HPLC on a Chemcosorb 7-diphenyl column (Chemco) and finally on a C-13 column to purify neuromedin U-25 to homogeneitv(Fig. 2~). Structure Analyses: i) Amino acid composition: Analyses were carried out with an amino acid analvzer (Hitachi-835), after acid hvdrolvsis of the purified neuromedins in 6M HCl containing 0.17:’ phenol and 0 .G27! 2-mercaptoethanol at 110°C for 20 hr. ii) Amino acid sequence: Neuromedin U-8 (ca. 200 pmol) and neuromedin U-25 (ca. 200 pmoll were each sequenced with a gas-phase sequencer (Applied Biosystems Model 47DAl (6), coupled with HPLC identification of the resulting PTH-amino acids (2). iii) C-Terminal analysis: The C-terminal amide structure W&S verified by trypsinization of the pept ide , followed by dansplat ion, in a manner similar to the method reported by Tatemoto and Mutt
(7). Syntheses : Neuromedin U-8 and U-25 were synthesized by solid phase techniques conducted on p-methyl-benzhydrylamine resin. Bioassay: i) Uterus stimulant activity: Assay was performed according to the described method (8) by using strips of rat uterus preparation freshly isolated in proestrous stage, in a modified Locke’s solution at 32°C. ii) Hypertensive effect: Systemic blood pressure was measured from the carotid artery in rats (000-4@Og) anesthetized with pentobarbital (5). Indicated amounts of peptides in 100-200 ul of 0.4’7 saline were administered through a cannula in the femoral vein. BK, SP and VIP were purchased from Protein Research Foundation. Bovine PP was kindly donated from Dr. A. Arimura, Tulane University School of Medicine.
RESULTS Neuromedin for
the
manner
to
peptide
that
used
Sephadex
of
G-50
further
uterus
to
collect
the
regions
(A-F). three
spinal fractions
purified subjected
was
(1).
The the
rat
spinal uterus
by
SP-Sephadex was
a Sephadex widely
(Fig.
of
C-25
to G-25
bioactive subsequent
Yr
1079
As in
peak
of
major
to
The
ca.
basicity purify
basic of
in
the on
daltons, shown
the
peak,
higher
assay
gel-filtration
5,000
F (tir the
RP-HPLC
(I-5).
by
column.
fraction
an
a similar
chromatography
separated
From
using in
neuromedins
distributed
lb).
cord
preparations
of
cord
HPLC
peaks
to
porcine
corresponding on
Cation-exchange bioactive
from
isolations
prepared
activity
DISCUSSION
isolate?
previous
rechromatographed
yielded
was
the
porcine
stimulant
previously
in
on
(SP-III!,
extract
were
purified
effect
fraction
acid
min
Us were
stimulant
AND
which
Fig.
la,
chromatographic 1,000
daltons)
neuromedin eluted neuromedin
B was at U-8
104 to
Vol.
130,
No. 3, 1985
BIOCHEMICAL
AND
BIOPHYSICAL
Abd---- B
C
DE
RESEARCH
COMMUNICATIONS
F&
L
0
10
40 number
30
20
Fraction
Time
50
60
70
(mtn)
C
-.
0
_- - _____
10
____-__-- ---
20
________--------
30
Tlme
_ __------ _______-------
40
‘i z II 0:
50
(mln)
Fig. 1 Purification of neuromedin u-8. a) filtration of SP-III on a Sephadex G-25(fine) column (7.5 x 135 cm). Eluent: 1M CH COOH. Fraction size: 100 ml/tube. Flow rate: 60 ml/hr b) Cation exe a ange HPLC of fraction F (l/3 portion) in Fig. la. Column: TSK IEX-530 CM (4.0 x 300 mm, Toyosoda). Flow rate: 1 ml/min. Solvent system: Linear gradient elution from A:B = 100: 0 to 85:15 for 48 min, followed by the second gradient from A:B = 85:15 to 50:50 for 48 min. (A) 1OmM HCOONHd(pH 6.5):CH3CN ; 9O:lO (v/v), (B) l.OM HCOONH4(pH 6.5):CH3CN = 9O:lO (v/v,. 1080
Vol.
130,
No. 3. 1985
homogeneity
BIOCHEMICAL
(Fig.
fraction
B in
Fig.
fraction
B on
a C-18
(Note
that
from
purified.) min
peak
2~).
II-6
and
using
1.05
a
for
U-5
and
3b).
in
The
were
verified
the
structures
native
proceeded
by
acid
of
showr (0)
comparison.
structure
been
has
PP.
(7).
*Neuromedin U-8: Asp 1.05(l), Pro Neuromedin (J-25: .Asp .1.07( n,, Ser Ile i?.30(1), Leu
the
the
related far
peptides observed As oc
C-terminal
exhibiting in
seen
I:ig.
uring
in
Leu
0.04
O.o711), 1.00(l),
Glu Tyr
3.89(4J, 0.92(11,
1).
the
peptides,
end
(Fig.
U-8
and
,ja U-25 of
the
of
complete
are
U-3
the
shown or
C-terminal
hormonal
the
pancreatic
(10)
neuromedin
or
releasing
and
U-25 amide
physiological factors
a partial II-‘,
of
and
C-terminal U-25 to
also
is
O.oOil),
Phe
2.0%?(2),
Arg
2.02(?).
Pro
2.27(Z),
Phe
4.04(41,
Gly Lys
1.00(l), l.O5il),
Val Arg
1.74(2), 4.14(4)
Tyr
known
is
structure
c) Final purification of neuromedin U-8 by RP-HPLC. Column: Chemcosorb SODS-H (4.0 x 250 mm, Chemco). Flow rate: 1 ml/min. Solvent: Linear gradient elution from (A) to (B) for 80 min. Hz0 : CH3CN : 10% TFA = (A) 90 : 10 : 1, (8) 40 : 60 : 1 (v/v). uterus activity (Fig.la,b) and uterus active fraction (Fig.lc) are shown by black bars. BSA, bovine serum albumin; SPO, SP sulfoxide; gNE, cyneo-endorphin; SS, snmatostatin; LE, Leu-enkephalin; R6LE, [Ax-g I-Leuenkephalin; LHRH, luteinizing hormone releasing hormone; Dyn8, dynorphin[l-81. 1081
acid Edman
unambiguously
sequences
neuromedin
of
confirmation
been
3c .
for
sequences
PTH-amino
Thus,
to
acid
nmol
0.84
comparison
hypothalamic in
column
analysis.
neuromedin
have
by
amino
carboxyl
identified.
asparaginamide
1.00(l),
of
polypeptidc(VIPI
highly so
25
Positive
known
C-15
the
neuromedin
the
ones.
intestinal
of been
-Arg-Pro-Arg-X-CONH, But )
where
each
of
of
(J-25
a
acid
chromatographic
and
state
as
of
the
(71.
synthetic C-8
peptides
feature often
hormones of
the
pmol step
Mutt by
corresponding
.Tc .
pm01
upto
a pure
and
Amino
structure and
provided
vasoactive
150
3
128-1.16 From
on
estimated
first
amide
sequences in
a unique
gastrointestinal
in
and
200
yields
Tatemoto
Fig.
with
the
repetitive
was
pigs.
About at
neuromedin in
found
as
sequence
sequencer.
also
200
in
at
was
2b).
footnote)*,
comprise
Za).
peptide
finally (see
of
(Fig.
eluted
isolated
and
were from
determined
of
(Fig.
from
RP-HPLC
releasing peak
to
isolated
peaks
activity was
was
daltons.
bioactive
data
yields
starting
Although
is
their
above their
polppeptide(PP)
activities,
found
asparagine
with
as
never
were
high
sequences
established,
above
method
deduced
peptides
amino
the
hioactive
column,
peptide
C-terminal
two
U-25
analyses
automated each
gave
first
acid
were
from
the
amino
U-25, U-25
a gas-phase
of
diphenyl
the
3,000
gastrin
neuromedin
and
nmol
degradation
found
on
ca.
later,
COMMUNICATIONS
U-25
Mr
stimulating
above,
purified
generated
have
HPLC
respectively,
and
neuromedin
for
uterus
on
II-25
residues,
and
of
obtained
Based
to
eluted
RESEARCH
neuromedin
column, peak
peak
BIOPHYSICAL
hand,
corresponding
second
RP-HPLC
(Fig.
other
preparative
the
a single
successive
was
la,
Cation-exchange
gave
binactive
U-8
On the
ICI.
AND
occur
Vol. 130, No. 3, 1985
8lOCHEMlCAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Tlme
b
2 1 J
5 J
g 0.05
H 5 J
(min)
L JJ
a% JJ
___----
_----
-
8 p‘1
--___----
ii x i %
'
O;-; 0
20
40
60 (mln)
Tlme
0.15
80
100
c
I
P 0GO,lO_---
______--
----
________--
------
_____----
______- -----
_______--
-----
E 0" g 0.05 % I O-
I 10
60 20
30 Time
(mln)
40
50
Fig. 2. Purification of neuromedin U-25. a) Preparative RP-HPLC of fraction B (l/7 portion) in Fig. la. c01uml: TSK ODS-120A (2.0 x 25 cm, Toyosoda). Flow rate: 5 ml/min. Solvent system: Linear gradient elution from A:B =90:10 to A:B = 30:70 for 250 min. Solvents A and B were as in Fig. lc. b) Cation exchange HPLC of uterus active fraction (l/2 portion) cluted at 128-136 min in Fig. 2a. Column: TSK CM-2SW (4.6 x 250 mm, Toyosada). Flow rate: 1 ml/min. Solvent system: Linear gradient elution from A:8 = 100:0 to A:B 2 SO:50 for 100 min. Solvents A and B were as in Fig. lb.
1082
Vol.
130.
BIOCHEMICAL
No. 3, 1985
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
b
10
5
15
20
25
Cycle
number
8
4
J
Tyr-Phe-Leu-Phe-Arg-Pro-Arg-Asn-NH2
: NMU-8
Phe-Lys-Val-Asp-Glu-Glu-Phe-Gln-Giy-Pm-Ile-Val-Ser-G1n-Asn-Arg-Arg-Tyr-Phe-Leu-Phe-Arg-Pro-Arg-Asn-NH~ -
: NMU-25
----Ala-Ala-Glu-Leu-Arg-Arg-Tyr-Ile-Asn-Met-Leu-Thr-Arg-Pro-Arg-Tyr-NH~ ---_--
: PP
----Leu-Arg-Lys-Gln-Met-Ala-Val-Lys-Lys-Tyr-Leu-Asn-Ser-Ile-Leu-~* -----_
: VIP
-
Fig. 3. Amino acid sequences of neuromedin U-8 and neuromedin a) Yield of PTH-amino acid generated from neuromedin u-8. b) Yield of PTH-amino acid generated from neuromedin U-25. c) Complete amino acid sequences of neuromedin U-8(NMU-8) compared with porcine PP and VIP. Homologous sequences are line indicates the paired basic signal for processing.
only
in
VIP.
The
and
neuromedin
U-25
processing
signal
most may
likely take
residues
in
generate
rat
systemic
blood
substance
P(SP)
(Fig.
basis), U-25
neuromedin is
repeated Furthermore,
three
times
twitching U-2j
of
as
were
4).
With
is
approximately
potent
of
uterus
was
found
to
at
so
with
far
of
rat
sensitivity
-la),
which
paired
basic as
of
contrcation
bradykinin(BK)
and
activity BK.
while
neuromcdin 11-25
while of
(molar
(J-8 rat
induced did
uterus
c) Final purification of neuromedin U-25 by RP-HPLC. Column : Chemcosorb 30DS-H (4.6 x 75 mm, Chemco). Flow rate: 1 ml/min. Temperature: Solvent system: Linear gradient elution from A:B = 8@:20 45°C. to A:B = 0:lOO for 192 min. Solvents A and B were as in Fig. ic. Relative uterus contractile activity (Fig. 2a,b) and uterus active fraction (Fig. 2~) were shown by black bars. 1083
is
amides
uterus
neuromedin (Fig.
typical
procrssinc
peptide
those
of
identified.
stimulating with
a U-6
site
been
Interestingly,
increase
is
a similar
the
Us on
uterus
C-terminus
neuromedin that
equipotent BK.
the
C-terminal
not
compared
preparation to
PP
neuromedin
regard
as
of
truncated have
at
which
suggests
and
they
pressure
u-8
occurence
respective
activities
located
and U-25(NMU-25) underlined. Dashed
structure.
[I-25
family
though
is
Ax-g-Arg
natural
VIP/PHI
even
biological
a
neuromedin
their
entities, The
The from
also
sequence
by
(11,12).
place to
C-8
preceded
processed
endogenous
and
neuromedin
U-25.
not. to
Vol.
130,
No. 3, 1985
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
a BK 1.0
-
NMU-8 1.0 nM
nM
\-
. 0
NMU-25
NMU-25 0.7 ntl
0.35
nM
0
2
4
and
11-25
. 2
4
.
- 0
2
4 Time
0
2
4
rat
uterus
imln)
b
Time
Fig.
4.
-
Biological effects blood pressure.
systemic
neuromedin
IIs.
essential part
for
These
of neuromedin
activity. fact
they
Furthermore, anesthetized
rats
hypotensive
effect. in
systolic
(J-25 was longer It
should
amide rat
be mentioned
C-terminus
at the or on
is
important
neuromedin
a concentration
blood
900
elicit
stimulation.
of
that
exerting
nM, t;ith
times
no appreciable
indicating that its biological
a contractile which
hut
effect
(I-8,
SP and HK show potent 1084
blood
short-lived
LI-5 (Fig.
4b).
lacking
an c1-
biological
on guinea
to
15 mmHg of neuromedin
than
the amide activities.
Ils.
about
effect
more potent
the
nmol/kg) arterial
induced
des-amid+neuromedin
, showed
pressure,
v-8
of the despite
in
strong
The hypertensive
three
the N-terminal
(1.0
increase
nmol/kg,
may he
neuromedin
(1-q
have
rat
prolongation
with
neuromedin which
of 3.0
synthetic
C-terminus for
uterine
and sustained
pressure.
U elicited of
not
RK and SF,
and about
and that and
similarity
and
U-h sequence
reinforcement
structural
a dose
blood
lasting
structure
uterus
neither
At
uterus.
for
a rapid
from
on
the neuromedin
on rat
injection
produced
differing
increase
some
u-8
that
effect
PP and VTP did have
intravenous
pressure,
indicate
stimulant
11-25 may serve
Note that that
of neuromedin
results
exerting
(min)
effects
on
structure at the Tncidentally, pig
ileum
stimulant
even at activity
BIOCHEMICAL
Vol. 130, No. 3, 1985
(0.4-1.0
nM).
The pharmacological
of SP and BK, function
--in vivo
strongly
suggest
as neuropeptides
AND BIOPHYSICAL
spectra that
of neuromedin
neuromedin
RESEARCH COMMUNICATIONS
Us distinct their
Us may have
from those specialized
or hormones.
This work was supported in part by a Grant-in-Aid from the ACKNOWLEDGEMENTS: Science and Culture of Japan. We sincerely thank Ministry of Education, Tamayo Hatoh and Masuyo Hiranaga of our Department for their Tetsuji Sudoh, technical assistance. REFERENCES 1. Minamino, N., Kangawa, K. & Matsuo, H. Biochem. Biophys. Res. Commun. 114, 541-548 (1983). 2. Gamine, N., Kangawa, K. & Matsuo, H. Biochem. Biophys. Res. Commun. 9, 14-20 (1984). 3. Kangawa, K., Minamino, N., Fukuda, A. & Matsuo, H. Biochem. Biophys. Res. Commun. 114, 533-540 (1983). 4. Minamino, N., Kangawa, K., Fukada, A. & Matsuo, H. Neuropeptides 4, 157-166 (1984). 5. Minamino, N., Kangawa, K. & Matsuo, H. Biochem. Biophys. Res. Commun. 122, 542-549 (1984). 6. Hewick, R.M., Hunkapiller, M.W., Hood, L.E. & Dreyer, W.J. J. Biol. Chem. 256, 7990-7997 (1981). (1978). 7. Tatemoto,K. & Mutt,V. Proc. Natl. Acad. Sci. U.S.A. 75, 4115-4119 8. Carraway, R. & Leeman, S. J. Biol. Chem. 248, 6854-68iil (1973). 9. Floyd, J.C. Jr., Fajans, S.S., Pek, S. & Chance, R.E. Recent Prog. Horm. Res. 33, 519-570 (1977). 10. Bodanszky, M., Klausner, Y.S. & Said, S.I. Proc. Natl. Acad. Sci. U.S.A. 70, 383-384 (1973). 11. Nakanishi, S. et al. Nature 3, 423-427 (1979). 12, Steiner, D.F. Quinn, P.S., Chan, S.J., Marsh, J. &. Tager, H.S. Ann. N-Y. Acad. Sci. 343, 1-16 (1980).
1085