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Purification of a human alternative complement pathway inhibitor from hemolymph of larval fall armyworm (Spodoptera frugiperda)
Vol. 122, No. 3, 1984
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
August 16, 1984
Pages
1426-1433
PURIFICATION OF A HUMAN ALTERNATIVE COMPLEMENT PATHWAY INHIBITOR HEMOLYMPH OF LARVAL FALL ARMYWORM (SPODOPTERA FRUGIPERDA) Osmond Cancer
Received
Research
July
J.M.
D’Cruz
Program, Oklahoma
13,
and
Noorbibi
K.
Oklahoma Medical City, Oklahoma
FROM
Day
Research 73104
Foundation,
1984
Larval Spodoptera frugiperda hemolymph contains a specific inhibitor of the alternative pathway of human complement. This inhibitor was purified from larval hemolymph (HL) by 50% (NH4)2SO4 precipitation, DEAE-Sephacel chromatography and sequential gel-filtration on Bio-Gel 1.5m, 0.5m and Sephacryl S-200. Purified HL protein (M, = 110,000) was composed of two M, 55,000 polypeptide chains. Addition of purified HL protein to human complement resulted in a dose-dependent inhibition of RaRBC lysis and clumping of cells. The protein inhibitor provides a new tool for investigating the regulation of human alternative complement pathway.
The specific
vertebrate
complement
immunity
considered
to
and have
immunoglobulin
evolved
vertebrate
been
demonstrable
from
some
venom
in
and
erythrocytes
in
More which
(3).
can
recent
in
larval
cells titrations,
potentiate
the
presence
HL of and (RaRBC)
we
either
inhibitor
by
human
us
have
C by
reported
to
shown
Using
the
the
mori
specific activity serum
(1,4).
interact of
insect
Using
both
the
presence
of
not HL
(5).
presence lysis
kinetic a classical
we detected of
of and
factors
C
C assay,
an
rabbit fixed C pathway
the
lowest
cobra
HL contain with
a kinetic
(6).
has
C components
interaction
ACP-mediated
the
sheep
terminal
the
of
purified
unsensitized
L)
of
However,
with
that
is
C reaction
(HL)
specific
(Bombyx for
serum
C-like
vertebrate
C pathway.
an
scale, in
of
reactions of
type
lysis
amplifier
immune
detected
shown
an
development
vertebrate
the
silkworm
also
been
been
of by
the
hemolymph
mammalian
of
activator
to
studies
component(s) the
has
as
of
evolutionary
A true
has
regulate
to
invertebrate
invertebrates
factor
the
(ACP)
both
effector
prior On
C pathway
primitive
system
non-specific
(1,2).
alternative
(C)
red point
yet
Vol.
122,
No.
modulator In
BIOCHEMICAL
3, 1984
in
this
the
paper
zation
of
discuss
the the
MATERIALS
HL
of
we
describe
HL
inhibitor
larval
AND
fall the
phylogenetic
AND
BIOPHYSICAL
armyworm
RESEARCH
(Spodoptera
purification
and
specific
for
the
implication
of
this
frugiperda)
preliminary
ACP novel
of
COMMUNICATIONS
human
(7).
characteriserum
and
xenogeneic
reaction.
METHODS
Smith) larvae mass reared on Insects: Spodoptera frugiperda (J.E. artificial diet (8) were obtained from the USDA Plant Sciences Research HL was collected from adult larvae in chilled Facility, Stillwater, OK. The cell-free HL tubes containing a few crystals of phenylthiourea. obtained after centrifugation (2000 rpm/lO min, 4°C) was used for fractionation of the ACP inhibitor. Assay of ACP inhibitor: One ml of a l:3 dilution of normal human serum (NHS) in G-VBS-8mM EGTAZmM Mg++ buffer, pH 7.3 (9) was preincubated at 37°C for 60 min with dilutions of HL fractions (100 ~1) or with PBS as control. 200 pl of rabbit red ceI1 suspension in G-VBS-EGTA-Mg buffer was then added to the reaction mixture (i: 0.7 at 700 nm) and the incubation continued at 37°C for 60 min. The degree of inhibition of hemolysis was monitored by recording the turbidity of the reaction mixture at 700 nm (IO). Isolation of the ACP inhibitor: 90 ml of cell-free HL obtained from nearly 3000 adult larvae was made to 50% (NH4)2SO4 fraction. The dissolved precipitate after dialysis was applied on a DEAE-Sephacel column (1.5 x 60 cm) equilibrated with 1OOmM sodium phosphate buffer, pH 7.2. Five ml fractions were collected. The bound proteins were eluted with a linear NaCl gradient (O-500mM). Aliquots (100 ~1) of the dialyzed fractions were tested for the classical C pathway inhibitor (7) as well as for the inhibition of RaRBC lysis in human serum. The ACP inhibitor fractions obtained from DEAE-Sephacel step were then sequentially gel-filtered on Bio-Gel 1.5m (2 x 150 cm), Bio-Gel 0.5m (2 x 150 cm) and Sephacryl S-200 (0.5 x 100 cm) in 1OOmM sodium phosphate buffer (pH 7.2) in presence of 150mM NaCl. Low molecular weight contaminants were removed by dialysis (MW cut off 60,000). Gradient PAGE: The active fractions obtained from each chromatographic step were tested on a 4-30% gradient PAGE run exactly as specified by the manufacturer's instructions (Pharmacia Fine Chemicals, Piscataway, NJ). Standard proteins used as markers included: thyroglobulin 669K, ferritin 440K, catalase 232K and bovine serum albumin 66K. SDS-PAGE: SDS-polyacrylamide gel electrophoresis was carried out on 10% slab gels according to the method of Laemmli (11). Reduction of desulfide bonds was achieved with 5% (v/v) 2-mercaptoethanol in the sample buffer. Molecular weight was estimated with a Bio-Rad (Richmond, CA) HMW kit consisting of myosin 2OOK, B-galactosidase ll6K, phosphorylase s92K, bovine serum albumin 66K and ovalbumin 45K as standards. Amino acid analysis: 100 ug of the purified protein was hydrolyzed in vacua with 200 ul of 6 N HCl and heated at 108°C for 24 hrs. Amino acid analysis was performed on a Durrum Model D-500 amino acid analyzer.
RESULTS DEAE-Sephacel Spodoptera their
HL charge
chromatography resulted
difference
in and
the
of
50%
separation further
(NH4)2SO4 of
purified 1427
two
fraction C inhibitors
independently
of based (Fig.
on la).
Vol.
122,
No.
3, 1984
BIOCHEMICAL
AND
BIOPHYSICAL
FRACTION
FRACTION
Pig.
NO.
of ACP gradient ACP inhibitor tion, II. Bio-Gel 1.5 m elution Bio-Gel 0.5 m elution. Sephacryl S-200 elution performed as outlined 280 nm. Active fractions
DEAE-Sephacel
(B)
CC) (D)
The
classical
was
obtained
C pathway in
DEAE-Sephacel of peak
this
gave
was
active from
Subsequent the
the
inhibitor
the
high
a homogeneous
the
on
active
peak
of 1.5m
weight
anionic
Bio-Gel
0.5m
Additional
the
The
range
Bio-Gel
molecular
1~).
by
fractions.
in on
gel-filtration (Fig.
detected
flowthrough
fraction
C inhibitor
NO
frac-
Assays for ACP inhibitor activitv were profile. Fraction size 5 ml, (0) absorbance at the text. were pooled as indicated by the horizontal bars.
inhibitor
eluted
FRACTION
NO.
inhibitor from Spodoptera HL elution profile: I. Classical fraction. profile of ACP inhibitor.
in
COMMUNICATIONS
NUMBER
FRACTION
Purification
(A)
RESEARCH
Id).
1428
ACP
lOO-3OOmM resolved
resulted
C2 assay
inhibitor
the
bound
minor
inhibitor
(Fig.
lb).
in
the on
(7) to
Gel-filtration
NaCl.
proteins
gel-filtration (Fig.
limited
enrichment
Sephacryl
of S-200
Vol.
122,
No.
3,
BIOCHEMICAL
1984
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
2OOK 1161 -* 92K e
t
66K
b
a
c
d
e
4 5K
-
669k
-
uok
-
232k
-
wk
4t
nrrg
*
03
02 Fig. 2 Track a, Track b, Track c, Track d, Track e,
4-30X gradient DEAE-Sephacel Rio-Gel 1.5 m Bio-Gel 0.5 m Sephacryl S-200 Marker proteins
PAGE of ACP inhibitor active fraction; active fraction; active fraction: eluted fraction: of known molecular
Fig. 3 SDS polyacryiamide Marker proteins Track A Unreduced protein Track B Track C Reduced protein SDS-PAGE was on a 10% slab R 250.
Fig.
2 shows
obtained (c)
and
by
Sephacryl apparent
daltons
on
SDS-lo%
mobility single
varied
on at subunit
PAGE
pH. Mr
and
staining
(Fig.
3,
track
gels
due
Following
= 55,000
of
was
ACP (a),
when
weight
was with
of
DEAE-Sephacel
columns
gradient
alkaline of
(d)
molecular
4-30%
gel
ACP inhibitor
enrichment on
S-ZOO
The
of
stepwise
chromatography
PAGE.
but
the
gel
weight.
B) to
1429
on
ACP under
1.5m
a 4-30%
(b),
0.5m
gradient was
non-reducing
110,000 conditions
electrophoretic
with (Fig.
blue
fraction
inhibitor
differential
reduction obtained
inhibitor Bio-Gel
tested the
Coomassie
2-mercaptoethanol, 3,
lane
C).
a Thus,
Vol.
122,
No.
3, 1984
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
-l
0
I
3
2 ACP Inhibitor
4
5
(Ng)
Fig. 4 Inhibition of ACP mediated lysis of RaRBC by HL protein 1 ml of a 1:12 dilution of NHS in G-VBS-EGTA-Mg buffer pH 7.3 was incubated with purified HL protein (0.5-5 up) at 37"C/60 min. Next, 200 ~1 of RaRBC suspension was added to the reaction mixture and incubation continued for another 60 min The turbidity of the reaction mixture was monitored at 700 "Ill. 1 ml of a I:12 dilution of NHS served as control.
the
110,000
species
disulfide
consists
bonds.
conditions (Fig.
3,
The
on
SDS-lo%
track
B)
dilution
of
inhibition ml
of
of
a 1:12
This
NHS
HL protein
also
The presented
layer
in
Table
residues.
The
noteworthy
is
I.
than
virtual
cell
of
acidic lack
the
and
with
a I:12
ug
of
of
RaRBC
protein
to
protein
is
chelated
(data
not
a
NHS with shown).
the
formation
of
ACP
inhibitor
is
a
clumps.
purified aspartic
basic
of
methionine
acid
residues
comprise
24%
1.8:1.
Also
is and
low
1
hemolysis.
HL
EGTA
toward
protein.
a dose-dependent
2.5
of of
by
35,000
native
vg)
of
M,
Spodoptera
to
1430
the
inhibition
purified
a tendency
Glutamine of
>90%
of
about
Preincubation
composition
ratio the
showed
of
(0.5-5
conglutination
rather
acid
the
band
brought
together
non-reducing
additional
Addition in
held
under
product
4).
ACP. in
RaRBC
amino
an
buffer
that
resulted
cell
inhibitor
resulted
human
polypeptides
HL protein
(Fig.
dilution
55,000
a degraded
purified
lysis
of
agglutinated
continuous
is
indicates
inhibitor
showed
G-VBS-EGTA-Mg
RaRBC
experiment
potent
The
in
two ACP
PAGE
of
NHS
purified
which
Preincubation
of
cysteine
of
content.
the
Vol.
122,
No.
BIOCHEMICAL
3, 1984
AND
Table
Amino
Acid
Composition
Amino
of
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
I
ACP Inhibitor
Isolated
from
Spodoptera
Amino Acid (residues/100
4cid
HL
Composition residues) 13.5 7.5 5.0 II .o 5.6 8.3 7.8 trace 7.2
Asp Thr Ser GlU Pro GAY Ala CYS Val net Ill.? LeLl TY~ Phe His LYS *G? Total acidics Total basics Acidicslbasics
4.5 8.2 2.2 4.5 2.0 6.7 4.7 24.5 13.4 1.82
DISCUSSION
In larval
this
paper
Spodoptera
inhibitor assay the
we
(a
HL.
In
the
classical product
human
C showed
a single
molecular
The
weight
HL
were
inhibitor
of
inhibitor
is From
isolated. human
to
converting
clumping
of
cells
lacked
the
ACP
by
adsorption ability
band
on
110,000
of
a reaction
to
hemagglutinating
a limited
C2
separated
of
lysis
PAGE
3 mg of
protein
conglutinin
by
with
an
PAGE.
two
inactive to
The
RaRBC
HL protein HL
from
DEAE-Sephacel.
a subunit
HL,
activity. 1431
C
SDS-lo%
revealed
Spodoptera
comparable
classical
gradient
on
cell-free
hemolytically
the
inhibit
a 4-30%
of
from
was to
composed
Preincubation
inhibitor
using
daltons
therefore
ACP
inhibitor
conditions
90 ml
RaRBC --
protein)
the
Purified
ACP.
addition
itself
of
reducing
chains.
inhibitor
on
stained
under
polypeptide
inhibitor
study,
based
of isolated
specific
inhibitor
enriched
Electrophoresis 55,000.
present
purification
previously
larval
C pathway
final
the
We have
C4-binding
(7).
apparent
describe
of
identical pure is
with also
M,
ACP a potent
human
C in
brought
about
(12).
The
Vol.
122,
No.
3,
The
1984
amino
inhibitors
acid
of
suggests
such
the
insect
control
polypeptide human
nature inactivator.
Three
probable
protein
of
the the
the
product
indicator
for
human
the
context
From inhibitors
of
The
fact
of
it
C3b
degradation.
of
C in
insect
HL
mammalian
C pathway
suggests
operative
in
HL,
assays.
Since
homologies highly in
insect C3
which
is
probable
for
C-like
reaction
existed
prior
inhibitors
components
molecules
mammalian
C in
insect
that
the
to
the have
appearance had
interact may
the
the
regulators of
a common
a C-type origin
structural (15),
it
C may
also
presence of
mammalian
of
other
inhibitors,
any
case,
a thorough
their
specificity
characterization and
mechanism 1432
of of
the action,
exist for
specific
C perhaps of
important
HL complement and
these metabolic
pathways. In
is
a detectable
Some
reaction. with
appropriate
substrates
absence of
either
be
require and
the in
with also
natural
Alternatively, HL
speculations:
vertebrate
be
a
specific
duplication
of
could
ii)
suggests
might
key
RaRBC.
specific
several
might
gene
the
with
two
sequence
with
from
C3b
and
of
which
HL
result
selectively
reactions of
insect
on
of
selectively
considerable
protein.
i.nhibitor
inhibitors
These
HL.
react
HL raises
detection
consistent
product
presence
similar
the
C3 convertase.
a sensitive
can
with
sites the
early
can
the
that
C4 have
these
an
two
could
acceptor C3 for
and
which
inhibition
or
provide
proteins
by
the
Spodoptera
the
also
that
Spodoptera
either
and
similarities
expected
which
from
shows
with
phylogeny,
mammalian
that
could
different
protein
protein
C3b
is
mammalian (14)
weight
with
inhibitor
inactivator
molecular
receptor
react
C3b
COMMUNICATIONS
from
the
be
compete
could
If
and
First,
C3b
could
degraded
i)
the
inhibitor
degradation.
can ACP.
differs
protein
HL
RESEARCH
inhibitor
inhibitor
mechanisms
inhibitor
ACP
H (13)
Spodoptera
either
BIOPHYSICAL
However,
mammalian
blocking
Third,
Factor ACP
of
inhibits
Second,
as
of
proteins.
C3b
AND
composition
ACP
that
mammalian
the
BIOCHEMICAL
their
Vol.
122,
No.
relationship
to
understand geneic
BIOCHEMICAL
3, 1984
the
insect significance
AND
metamorphotic of
BIOPHYSICAL
events these
(6)
phylogenetically
RESEARCH
is
required conserved
COMMUNICATIONS
to xeno-
reactions.
ACKNOWLEDGEMENTS This work was supported by grants Foundation (#PCM-8216557) and American thank Patricia Cook for her technical for typing the manuscript.
from the National Science Cancer Society (#IM-298). We assistance and Karen Deatherage
REFERENCES
2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15.
Gewurz, H., Finstad, J., Muschel, L.M., and Good, R.A. (1966) In: Phylogeny of Immunity, Eds. Smith, R.T., Miescher, P.A., and G%, 105-117, University of Florida Press, Gainvesville, FL. R.A., pp. Porter, R.R., and Reid, K.B.M. (1978) Nature 275, 699-704. Fujii, T., and Murakawa, S. (1981) Dev. Comp. immunol. 5, 251-258. Day, N.K., Gewurz, H., Johannsen, R., Finstad, J., and Good, R.A. (1970) J. Exp. Med. 132, 941-948. Day, N., Geiger, H., Finstad, J., and Good, R.A. (1972) J. Immunol. 109, 164-167. D'Cruz, O.J.M. (1983) Fed. Proc. 42, 1237. D'Cruz, O.J.M., and Day, N.K. (1984) Fed. Proc. 43, 1764. Burton, R.L. (1967) USDA Bulletin ARS 33-117. Platts-Mills, T.A.E., and Ishizaka, K. (1976) J. Immunol. 113, 348-358. Polhill, R.B., Pruitt, K.M., and Johnston, Jr., R.B. (1978) J. Tmmunol. 121, 363-370. Laemmli, U.K. (1970) Nature (London) 227, 680-685. Linscott, W.D., Raymond, R., and Triglia, R.P. (1978) J. Immunol. 121, 658-664. Sim, R.B., and Discipio, R.G. (1982) Biochem. J. 205, 285-293. Hsiung Li-min, A., Barclay, N., Brandon, M.R., Sim, E., and Porter, R.R. (1982) Biochem. J. 203, 293-298. Sackstein, R., Colton, H.R., and Woods, D.E. (1983) J. Biol. Chem. 258, 14693-14697.
1433
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
August 16, 1984
Pages
1426-1433
PURIFICATION OF A HUMAN ALTERNATIVE COMPLEMENT PATHWAY INHIBITOR HEMOLYMPH OF LARVAL FALL ARMYWORM (SPODOPTERA FRUGIPERDA) Osmond Cancer
Received
Research
July
J.M.
D’Cruz
Program, Oklahoma
13,
and
Noorbibi
K.
Oklahoma Medical City, Oklahoma
FROM
Day
Research 73104
Foundation,
1984
Larval Spodoptera frugiperda hemolymph contains a specific inhibitor of the alternative pathway of human complement. This inhibitor was purified from larval hemolymph (HL) by 50% (NH4)2SO4 precipitation, DEAE-Sephacel chromatography and sequential gel-filtration on Bio-Gel 1.5m, 0.5m and Sephacryl S-200. Purified HL protein (M, = 110,000) was composed of two M, 55,000 polypeptide chains. Addition of purified HL protein to human complement resulted in a dose-dependent inhibition of RaRBC lysis and clumping of cells. The protein inhibitor provides a new tool for investigating the regulation of human alternative complement pathway.
The specific
vertebrate
complement
immunity
considered
to
and have
immunoglobulin
evolved
vertebrate
been
demonstrable
from
some
venom
in
and
erythrocytes
in
More which
(3).
can
recent
in
larval
cells titrations,
potentiate
the
presence
HL of and (RaRBC)
we
either
inhibitor
by
human
us
have
C by
reported
to
shown
Using
the
the
mori
specific activity serum
(1,4).
interact of
insect
Using
both
the
presence
of
not HL
(5).
presence lysis
kinetic a classical
we detected of
of and
factors
C
C assay,
an
rabbit fixed C pathway
the
lowest
cobra
HL contain with
a kinetic
(6).
has
C components
interaction
ACP-mediated
the
sheep
terminal
the
of
purified
unsensitized
L)
of
However,
with
that
is
C reaction
(HL)
specific
(Bombyx for
serum
C-like
vertebrate
C pathway.
an
scale, in
of
reactions of
type
lysis
amplifier
immune
detected
shown
an
development
vertebrate
the
silkworm
also
been
been
of by
the
hemolymph
mammalian
of
activator
to
studies
component(s) the
has
as
of
evolutionary
A true
has
regulate
to
invertebrate
invertebrates
factor
the
(ACP)
both
effector
prior On
C pathway
primitive
system
non-specific
(1,2).
alternative
(C)
red point
yet
Vol.
122,
No.
modulator In
BIOCHEMICAL
3, 1984
in
this
the
paper
zation
of
discuss
the the
MATERIALS
HL
of
we
describe
HL
inhibitor
larval
AND
fall the
phylogenetic
AND
BIOPHYSICAL
armyworm
RESEARCH
(Spodoptera
purification
and
specific
for
the
implication
of
this
frugiperda)
preliminary
ACP novel
of
COMMUNICATIONS
human
(7).
characteriserum
and
xenogeneic
reaction.
METHODS
Smith) larvae mass reared on Insects: Spodoptera frugiperda (J.E. artificial diet (8) were obtained from the USDA Plant Sciences Research HL was collected from adult larvae in chilled Facility, Stillwater, OK. The cell-free HL tubes containing a few crystals of phenylthiourea. obtained after centrifugation (2000 rpm/lO min, 4°C) was used for fractionation of the ACP inhibitor. Assay of ACP inhibitor: One ml of a l:3 dilution of normal human serum (NHS) in G-VBS-8mM EGTAZmM Mg++ buffer, pH 7.3 (9) was preincubated at 37°C for 60 min with dilutions of HL fractions (100 ~1) or with PBS as control. 200 pl of rabbit red ceI1 suspension in G-VBS-EGTA-Mg buffer was then added to the reaction mixture (i: 0.7 at 700 nm) and the incubation continued at 37°C for 60 min. The degree of inhibition of hemolysis was monitored by recording the turbidity of the reaction mixture at 700 nm (IO). Isolation of the ACP inhibitor: 90 ml of cell-free HL obtained from nearly 3000 adult larvae was made to 50% (NH4)2SO4 fraction. The dissolved precipitate after dialysis was applied on a DEAE-Sephacel column (1.5 x 60 cm) equilibrated with 1OOmM sodium phosphate buffer, pH 7.2. Five ml fractions were collected. The bound proteins were eluted with a linear NaCl gradient (O-500mM). Aliquots (100 ~1) of the dialyzed fractions were tested for the classical C pathway inhibitor (7) as well as for the inhibition of RaRBC lysis in human serum. The ACP inhibitor fractions obtained from DEAE-Sephacel step were then sequentially gel-filtered on Bio-Gel 1.5m (2 x 150 cm), Bio-Gel 0.5m (2 x 150 cm) and Sephacryl S-200 (0.5 x 100 cm) in 1OOmM sodium phosphate buffer (pH 7.2) in presence of 150mM NaCl. Low molecular weight contaminants were removed by dialysis (MW cut off 60,000). Gradient PAGE: The active fractions obtained from each chromatographic step were tested on a 4-30% gradient PAGE run exactly as specified by the manufacturer's instructions (Pharmacia Fine Chemicals, Piscataway, NJ). Standard proteins used as markers included: thyroglobulin 669K, ferritin 440K, catalase 232K and bovine serum albumin 66K. SDS-PAGE: SDS-polyacrylamide gel electrophoresis was carried out on 10% slab gels according to the method of Laemmli (11). Reduction of desulfide bonds was achieved with 5% (v/v) 2-mercaptoethanol in the sample buffer. Molecular weight was estimated with a Bio-Rad (Richmond, CA) HMW kit consisting of myosin 2OOK, B-galactosidase ll6K, phosphorylase s92K, bovine serum albumin 66K and ovalbumin 45K as standards. Amino acid analysis: 100 ug of the purified protein was hydrolyzed in vacua with 200 ul of 6 N HCl and heated at 108°C for 24 hrs. Amino acid analysis was performed on a Durrum Model D-500 amino acid analyzer.
RESULTS DEAE-Sephacel Spodoptera their
HL charge
chromatography resulted
difference
in and
the
of
50%
separation further
(NH4)2SO4 of
purified 1427
two
fraction C inhibitors
independently
of based (Fig.
on la).
Vol.
122,
No.
3, 1984
BIOCHEMICAL
AND
BIOPHYSICAL
FRACTION
FRACTION
Pig.
NO.
of ACP gradient ACP inhibitor tion, II. Bio-Gel 1.5 m elution Bio-Gel 0.5 m elution. Sephacryl S-200 elution performed as outlined 280 nm. Active fractions
DEAE-Sephacel
(B)
CC) (D)
The
classical
was
obtained
C pathway in
DEAE-Sephacel of peak
this
gave
was
active from
Subsequent the
the
inhibitor
the
high
a homogeneous
the
on
active
peak
of 1.5m
weight
anionic
Bio-Gel
0.5m
Additional
the
The
range
Bio-Gel
molecular
1~).
by
fractions.
in on
gel-filtration (Fig.
detected
flowthrough
fraction
C inhibitor
NO
frac-
Assays for ACP inhibitor activitv were profile. Fraction size 5 ml, (0) absorbance at the text. were pooled as indicated by the horizontal bars.
inhibitor
eluted
FRACTION
NO.
inhibitor from Spodoptera HL elution profile: I. Classical fraction. profile of ACP inhibitor.
in
COMMUNICATIONS
NUMBER
FRACTION
Purification
(A)
RESEARCH
Id).
1428
ACP
lOO-3OOmM resolved
resulted
C2 assay
inhibitor
the
bound
minor
inhibitor
(Fig.
lb).
in
the on
(7) to
Gel-filtration
NaCl.
proteins
gel-filtration (Fig.
limited
enrichment
Sephacryl
of S-200
Vol.
122,
No.
3,
BIOCHEMICAL
1984
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
2OOK 1161 -* 92K e
t
66K
b
a
c
d
e
4 5K
-
669k
-
uok
-
232k
-
wk
4t
nrrg
*
03
02 Fig. 2 Track a, Track b, Track c, Track d, Track e,
4-30X gradient DEAE-Sephacel Rio-Gel 1.5 m Bio-Gel 0.5 m Sephacryl S-200 Marker proteins
PAGE of ACP inhibitor active fraction; active fraction; active fraction: eluted fraction: of known molecular
Fig. 3 SDS polyacryiamide Marker proteins Track A Unreduced protein Track B Track C Reduced protein SDS-PAGE was on a 10% slab R 250.
Fig.
2 shows
obtained (c)
and
by
Sephacryl apparent
daltons
on
SDS-lo%
mobility single
varied
on at subunit
PAGE
pH. Mr
and
staining
(Fig.
3,
track
gels
due
Following
= 55,000
of
was
ACP (a),
when
weight
was with
of
DEAE-Sephacel
columns
gradient
alkaline of
(d)
molecular
4-30%
gel
ACP inhibitor
enrichment on
S-ZOO
The
of
stepwise
chromatography
PAGE.
but
the
gel
weight.
B) to
1429
on
ACP under
1.5m
a 4-30%
(b),
0.5m
gradient was
non-reducing
110,000 conditions
electrophoretic
with (Fig.
blue
fraction
inhibitor
differential
reduction obtained
inhibitor Bio-Gel
tested the
Coomassie
2-mercaptoethanol, 3,
lane
C).
a Thus,
Vol.
122,
No.
3, 1984
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
-l
0
I
3
2 ACP Inhibitor
4
5
(Ng)
Fig. 4 Inhibition of ACP mediated lysis of RaRBC by HL protein 1 ml of a 1:12 dilution of NHS in G-VBS-EGTA-Mg buffer pH 7.3 was incubated with purified HL protein (0.5-5 up) at 37"C/60 min. Next, 200 ~1 of RaRBC suspension was added to the reaction mixture and incubation continued for another 60 min The turbidity of the reaction mixture was monitored at 700 "Ill. 1 ml of a I:12 dilution of NHS served as control.
the
110,000
species
disulfide
consists
bonds.
conditions (Fig.
3,
The
on
SDS-lo%
track
B)
dilution
of
inhibition ml
of
of
a 1:12
This
NHS
HL protein
also
The presented
layer
in
Table
residues.
The
noteworthy
is
I.
than
virtual
cell
of
acidic lack
the
and
with
a I:12
ug
of
of
RaRBC
protein
to
protein
is
chelated
(data
not
a
NHS with shown).
the
formation
of
ACP
inhibitor
is
a
clumps.
purified aspartic
basic
of
methionine
acid
residues
comprise
24%
1.8:1.
Also
is and
low
1
hemolysis.
HL
EGTA
toward
protein.
a dose-dependent
2.5
of of
by
35,000
native
vg)
of
M,
Spodoptera
to
1430
the
inhibition
purified
a tendency
Glutamine of
>90%
of
about
Preincubation
composition
ratio the
showed
of
(0.5-5
conglutination
rather
acid
the
band
brought
together
non-reducing
additional
Addition in
held
under
product
4).
ACP. in
RaRBC
amino
an
buffer
that
resulted
cell
inhibitor
resulted
human
polypeptides
HL protein
(Fig.
dilution
55,000
a degraded
purified
lysis
of
agglutinated
continuous
is
indicates
inhibitor
showed
G-VBS-EGTA-Mg
RaRBC
experiment
potent
The
in
two ACP
PAGE
of
NHS
purified
which
Preincubation
of
cysteine
of
content.
the
Vol.
122,
No.
BIOCHEMICAL
3, 1984
AND
Table
Amino
Acid
Composition
Amino
of
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
I
ACP Inhibitor
Isolated
from
Spodoptera
Amino Acid (residues/100
4cid
HL
Composition residues) 13.5 7.5 5.0 II .o 5.6 8.3 7.8 trace 7.2
Asp Thr Ser GlU Pro GAY Ala CYS Val net Ill.? LeLl TY~ Phe His LYS *G? Total acidics Total basics Acidicslbasics
4.5 8.2 2.2 4.5 2.0 6.7 4.7 24.5 13.4 1.82
DISCUSSION
In larval
this
paper
Spodoptera
inhibitor assay the
we
(a
HL.
In
the
classical product
human
C showed
a single
molecular
The
weight
HL
were
inhibitor
of
inhibitor
is From
isolated. human
to
converting
clumping
of
cells
lacked
the
ACP
by
adsorption ability
band
on
110,000
of
a reaction
to
hemagglutinating
a limited
C2
separated
of
lysis
PAGE
3 mg of
protein
conglutinin
by
with
an
PAGE.
two
inactive to
The
RaRBC
HL protein HL
from
DEAE-Sephacel.
a subunit
HL,
activity. 1431
C
SDS-lo%
revealed
Spodoptera
comparable
classical
gradient
on
cell-free
hemolytically
the
inhibit
a 4-30%
of
from
was to
composed
Preincubation
inhibitor
using
daltons
therefore
ACP
inhibitor
conditions
90 ml
RaRBC --
protein)
the
Purified
ACP.
addition
itself
of
reducing
chains.
inhibitor
on
stained
under
polypeptide
inhibitor
study,
based
of isolated
specific
inhibitor
enriched
Electrophoresis 55,000.
present
purification
previously
larval
C pathway
final
the
We have
C4-binding
(7).
apparent
describe
of
identical pure is
with also
M,
ACP a potent
human
C in
brought
about
(12).
The
Vol.
122,
No.
3,
The
1984
amino
inhibitors
acid
of
suggests
such
the
insect
control
polypeptide human
nature inactivator.
Three
probable
protein
of
the the
the
product
indicator
for
human
the
context
From inhibitors
of
The
fact
of
it
C3b
degradation.
of
C in
insect
HL
mammalian
C pathway
suggests
operative
in
HL,
assays.
Since
homologies highly in
insect C3
which
is
probable
for
C-like
reaction
existed
prior
inhibitors
components
molecules
mammalian
C in
insect
that
the
to
the have
appearance had
interact may
the
the
regulators of
a common
a C-type origin
structural (15),
it
C may
also
presence of
mammalian
of
other
inhibitors,
any
case,
a thorough
their
specificity
characterization and
mechanism 1432
of of
the action,
exist for
specific
C perhaps of
important
HL complement and
these metabolic
pathways. In
is
a detectable
Some
reaction. with
appropriate
substrates
absence of
either
be
require and
the in
with also
natural
Alternatively, HL
speculations:
vertebrate
be
a
specific
duplication
of
could
ii)
suggests
might
key
RaRBC.
specific
several
might
gene
the
with
two
sequence
with
from
C3b
and
of
which
HL
result
selectively
reactions of
insect
on
of
selectively
considerable
protein.
i.nhibitor
inhibitors
These
HL.
react
HL raises
detection
consistent
product
presence
similar
the
C3 convertase.
a sensitive
can
with
sites the
early
can
the
that
C4 have
these
an
two
could
acceptor C3 for
and
which
inhibition
or
provide
proteins
by
the
Spodoptera
the
also
that
Spodoptera
either
and
similarities
expected
which
from
shows
with
phylogeny,
mammalian
that
could
different
protein
protein
C3b
is
mammalian (14)
weight
with
inhibitor
inactivator
molecular
receptor
react
C3b
COMMUNICATIONS
from
the
be
compete
could
If
and
First,
C3b
could
degraded
i)
the
inhibitor
degradation.
can ACP.
differs
protein
HL
RESEARCH
inhibitor
inhibitor
mechanisms
inhibitor
ACP
H (13)
Spodoptera
either
BIOPHYSICAL
However,
mammalian
blocking
Third,
Factor ACP
of
inhibits
Second,
as
of
proteins.
C3b
AND
composition
ACP
that
mammalian
the
BIOCHEMICAL
their
Vol.
122,
No.
relationship
to
understand geneic
BIOCHEMICAL
3, 1984
the
insect significance
AND
metamorphotic of
BIOPHYSICAL
events these
(6)
phylogenetically
RESEARCH
is
required conserved
COMMUNICATIONS
to xeno-
reactions.
ACKNOWLEDGEMENTS This work was supported by grants Foundation (#PCM-8216557) and American thank Patricia Cook for her technical for typing the manuscript.
from the National Science Cancer Society (#IM-298). We assistance and Karen Deatherage
REFERENCES
2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15.
Gewurz, H., Finstad, J., Muschel, L.M., and Good, R.A. (1966) In: Phylogeny of Immunity, Eds. Smith, R.T., Miescher, P.A., and G%, 105-117, University of Florida Press, Gainvesville, FL. R.A., pp. Porter, R.R., and Reid, K.B.M. (1978) Nature 275, 699-704. Fujii, T., and Murakawa, S. (1981) Dev. Comp. immunol. 5, 251-258. Day, N.K., Gewurz, H., Johannsen, R., Finstad, J., and Good, R.A. (1970) J. Exp. Med. 132, 941-948. Day, N., Geiger, H., Finstad, J., and Good, R.A. (1972) J. Immunol. 109, 164-167. D'Cruz, O.J.M. (1983) Fed. Proc. 42, 1237. D'Cruz, O.J.M., and Day, N.K. (1984) Fed. Proc. 43, 1764. Burton, R.L. (1967) USDA Bulletin ARS 33-117. Platts-Mills, T.A.E., and Ishizaka, K. (1976) J. Immunol. 113, 348-358. Polhill, R.B., Pruitt, K.M., and Johnston, Jr., R.B. (1978) J. Tmmunol. 121, 363-370. Laemmli, U.K. (1970) Nature (London) 227, 680-685. Linscott, W.D., Raymond, R., and Triglia, R.P. (1978) J. Immunol. 121, 658-664. Sim, R.B., and Discipio, R.G. (1982) Biochem. J. 205, 285-293. Hsiung Li-min, A., Barclay, N., Brandon, M.R., Sim, E., and Porter, R.R. (1982) Biochem. J. 203, 293-298. Sackstein, R., Colton, H.R., and Woods, D.E. (1983) J. Biol. Chem. 258, 14693-14697.
1433