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Candidacidal activity of myeloperoxidase: Characterization of myeloperoxidase-yeast complex formation
Vol.
154,
No.
July
29,
1988
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
COMMUNICATIONS Pages
CANDIDACIDAL
ACTIVITY
Clifford
D. Wright'
Departments
.June 20,
CHARACTERIZATION
OF MYELOPEROXIDASE:
MYKLOPEROXIDASE-YEAST
Received
RESEARCH
809-817
OF
COMPLEX FORMATION D. Nelson I,2
and Robert
of Microbiology1 and Surgery2 University of Minnesota Minneapolis, MN 55455
1988
demonstrated the ability of human FxJmlARY : We have previously -neutrophil myeloperoxidase to bind to cell wall mannan polysaccharide isolated :Erom Candida albicans. This binding capacity provides for association of the enzyme with target yeast which is essential for In this report, we further consider the efficient candidacidal activity. role of the mannan-binding property of myeloperoxidase in the Solubilized mannan antagonizes candidacidal activity of the enzyme. binding o:E the enzyme to yeast, suggesting that mannan may be a primary component of the fungal cell wall which serves as a target for binding of Myeloperoxidase is shown to form complexes with both myeloperoxidase. solubilized mannan and Candida yeast, with Kds of 0.97 x lo-' M and 1.2 x lo-' M, respectively. The interaction between myeloperoxidase and mannan does not allow the enzyme to readily dissociate from the surface of target yeast. As a result, the enzyme may be unable to dissociate from dead yeast to become available for binding to additional fungal targets. 0 1988 ncademlc Press. 1°C.
The microbicidal halide
system
activity
(1)
is
microorganisms.
This
Escherichia -- coli: Candida albicans _ -_
(4).
myelopero'xidase acid
(5)
of this
of the
optimized phenomenon
(2),
Actinobacillus It
enzyme is
has been
at the microbial
thereby
(6,7)
to the for
and its
that for
of
(3),
binding
and
of
generation
of hypochlorous
minimizing
both
interaction
target
killing
actinomycetecomitans allows
surface,
oxidant
peroxide-
bound
demonstrated
has been proposed
to microorganisms
cytotoxic
myeloperoxidase-hydrogen
when the
with
the
dilution
alternate
substrates. We have previously C. albicans interaction
through
was shown
myeloperoxidase 'Current Company,
demonstrated cell
address:
wall
to be ionic,
(p1 = 10.2)
(11)
Pharmacology
Pharmaceutical
that
mannan
Research
myeloperoxidase
polysaccharide
rather and the
Department, Division,
than
binds
to
(4,8,9,10). lectin-like,
phosphate
The between
groups
of the
mannan
Parke-Davis/Warner-Lambert Ann Arbor,
MI
48105 0006-291X/88
809
$1.50
Copyright 0 1988 by Academic Press. Inc. All rights of reproduction in any form reserved.
Vol.
154,
outer
No.
2, 1988
chain
(8).
has also
been
The purpose myeloperoxidase of the
BIOCHEMICAL
Binding
shown
BIOPHYSICAL
of myeloperoxidase
to be a mannan-specific
of this
report
to mannan
is
required
RESEARCH
interaction
to further
COMMUNICATIONS
to A. actinomycetecomitans (3).
characterize
to promote
the
candidacidal
the binding
of
activity
enzyme. MATERIALS
Isolation
AND
AND METHODS
of Myeloperoxidase
Human neutrophils were isolated from anti-coagulant treated whole blood according to the procedure of Ferrante and Thong (12). Myeloperoxidase was isolated from human neutrophils according to the method of Andrews and Krinsky (13). The partially purified enzyme had an R. 2. value of 0.62. Myeloperoxidase activity was quantitated in terms of pyrogallol units as described by Baggiolini, et al, (14). The candidacidal activity of the enzyme preparation was characterized in vitro. Candidacidal activity was shown to be both hydrogen peroxideand chloride ion-dependent. Inhibitors of myeloperoxidase activity (0.1 mM azide, 0.1 mM cyanide) and a scavenger of hypochlorous acid (1 mM I-methionine) also effectively inhibited killing of target yeast (4). Isolation
of Mannan
Candida albicans 2252 (ATC 44806) was grown to stationary yeast nitrogen base minimal medium (15). Mannan was isolated Fehling's solution as copper complexes from citrate-extracted described by Peat, et al, (16). Assay
of Myeloperoxidase-Mannan
Complex
phase with yeast
in as
Formation
Myeloperoxidase (3.5 x 10e2 units) and mannan (4.0 mg) were incubated in Dulbecco's phosphate-buffered saline (PBS) (pH 7.4) for 30 minutes at 37%. The sample was then chromatographed on a Sephadex G-150 gel permeation column (18 x 1.5 cm) in distilled water. The elution profile of the myeloperoxidase-mannan reaction mixture was compared with those of isolated myeloperoxidase and mannan. Elution of myeloperoxidase was monitored by its catalytic activity at 435 nm (14). Elution of mannan was monitored by the phenol-sulfuric acid assay for carbohydrates at 490 nm (17). Assay
of Myeloperoxidase-Yeast
Complex
Formation
C. albicans 2252 was incubated overnight in yeast nitrogen base mini&l media at 37%. Following three washes in PBS, the yeast suspension was adjusted to a final optical density of 1.0 at 660 nm (Asso) of 1.0 equals approximately 2 x lo7 yeast per ml. A 0.1 ml aliquot of yeast was incubated with 1.1 x 10e3 units of myeloperoxidase in a final volume of 0.5 ml at 37%. After 30 minutes, the reaction mixture was centrifuged and the amounts of free and yeast-bound myeloperoxidase were determined. Binding of myeloperoxidase to yeast compared in the presence and absence of 2 mg/ml mannan. Dissociation Constants Yeast Interactions
of Myeloperoxidase-Mannan
The dissociation constant of.myeloperoxidase-mannan determined by incubation of varying concentrations 810
and Myeloperoxidasecomplexes was of myeloperoxidase
was
Vol.
154,
No.
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
with 12 mg of C. albicans 2252 mannan in PBS. After a 30 minute incubation at 37OC, the reaction mixture was chromatographed on a G-150 Sephadex gel permeation column (18 x 1.5 cm) in distilled water to separate free myeloperoxidase from mannan-bound enzyme. The peak areas of the chromatographed myeloperoxidase fractions were used to determine the amount of bound and free enzyme for use in Scatchard analysis (18). The dissociation constant of myeloperoxidase-yeast complexes was determined by incubation of varying concentrations of myeloperoxidase with C. albicans 2252. Overnight cultures of C. albicans 2252 were One ml aliquots of the yeast suspension prepared as described above. were centrifuged and resuspended to a final volume of 0.6 ml with a 30-minute incubation at 37OC, the myeloperoxidase in PBS. After reaction mixture was centrifuged and the amount of myeloperoxidase remaining free in the supernate was quantified for use in Scatchard analysis. Molecular
Weight
Determinations
of Candida
mannan
The molecular weight of C. albicans 2252 mannan was determined by meniscus depletion equilibration using a Spinco model E analytical centrifuge with interference optics (19). Samples were prepared at 0.5 mg/ml in 0.1 M KHsPO4, pH 4.7. The sample was centrifuged at 14,000 rpm at 18OC. The mean molecular weight of mannan from two runs was detennined. Assay
of Myeloperoxidase-Mediated
Candidacidal
Activity
2252 were prepared as described Overnight cultures of C. albicans above. A 0.1 ml aliquot ofyeast was incubated with 1.1 x lop3 units of myelopero.xidase at 4nC for 30 minutes. Following preincubation, hydrogen peroxidas,e was added to give a concentration of 0.02 mM in a final All reagents were diluted in PBS to provide a reaction -volume of 1.0 ml. final chl'oride concentration of 0.14 M. The reaction mixture was incubated at 37OC on a rotating table. Myeloperoxidase-mediated killing was stopped by transferring the reaction tube to ice water. Yeast viability was determined by pour plate methodology using yeast extract peptone dextrose agar (15). Control experiments verified that the observed candidacidal activity was generated by the myeloperoxidase-hydrogen peroxide-chloride antimicrobial system (1). RESULTS Myeloperoxidase-Mannan Binding mannan
Complex
was assessed
by gel
of myeloperoxidase of its
catalytic
of the
column.
phenol-sulfuric volume.
myeloperoxidase allow
from
In contrast, acid
association
(435
run),
of the
C. albicans
chromatography G-150
column,
occurred
elution
carbohydrate
and a 4.0
to solubilized
permeation
a Sephadex
activity
The chromatograph
elution did not
Formation
of human myeloperoxidase
monitored
within
of mannan, assay
(490
nm),
of 3.5
mg of mannan
preincubated
showed
the
a shift
volume
by the
occurred
in the
void
of
30 minutes
to
of the peroxidase
peak to the void volume. Binding of myeloperoxidase inhibit the catalytic activity of the enzyme. This 811
Elution
as a function
x 10e2 units for
1).
inclusion
monitored
of a mixture reactants
(Figure
2252
to mannan shift in the
Vol.
154,
No.
2, 1988
BIOCHEMICAL
0.4
-
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
"0 i
0.3
-
:
MPO + mannan 435nm
Iii e
2
MPCJ 435nm
0.2 -
:
II, 0.1
R
-
&!.!L&.
5
10
15
20
25
30
Elution
35
40
Volume
45
50
55
6C
(ml)
FIGIJBE 1. Myeloperoxidase-mannan complex formation. Elution patterns of myeloperoxidase (MPO), -~ C. albicans 2252 mannan, and an MPO-mannan reaction mixture from a Sephadex G-150 gel permeation column are illustrated. Elution of myeloperoxidase was monitored as a function of its catalytic activity at 435 am. Elution of mannan was monitored by the phenol-sulfuric acid carbohydrate assay at 490 nm. Vo, void volume. elution
pattern
for
peroxidase
activity
is
expected
for
an enzyme-mannan
complex. Myeloperoxidase-Yeast Binding
Complex
determining
the
30-minute
incubation
amount
1.1 x 10-e
units
68 percent
of the
corresponding association binding
with that
involves
with enzyme. with
myeloperoxidase
yeast.
in a dose-dependent displace
Analysis
Myeloperoxidase-Candida The dissociation myeloperoxidase-Candida
incubation
Candida
yeast, with
of the
solubilized enzyme with
binding
interaction
of myeloperoxidase
Solubilized
(4).
enzyme.
to solubilized
These
mannan
of the
mannan
was also
results
suggest
and to yeast
of the enzyme.
of Myeloperoxidase-Mannan
and
Interactions constants
(Kds)
interactions
for were
812
myeloperoxidase-mannan determined
the
a common
antagonized
yeast-bound
function
whether
involved
Preincubation
of a
to determine
and yeast
with
manner
a
After
was preincubated
inhibits
of myeloperoxidase
a common binding
In order
by
following
cell-associated
completely
Mannan
2).
2 x lo6
mannan
of yeast. mannan
was assessed
enzyme
(Figure
enzyme became
in free
to addition
to effectively binding
Binding
available
of solubilized
yeast
shown
and yeast-bound
of myeloperoxidase
decrease
to target
to C. albicans
reagents
of myeloperoxidase
mannan prior enzyme
of free of the
function,
2 mg/ml
Formation
of human myeloperoxidase
by Scatchard
and
Vol.
154,
No.
2, 1988
BIOCHEMICAL
120
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
-
FIGURE 2. Influence of soluble mannan on myeloperoxidase-Candida comlplex formation. Binding of myeloperoxidase (MPO) to yeast was compared in the presence and absence of soluble mannan (mean 2 S.E.M., n = 3).
analysis
of binding
data
of myeloperoxidase permeation bound
with
enzyme.
of binding
allowed
Scatchard
sites
analysis
available (Figure
myeloperoxidase
with
activity,
allowed
Scatchard
analysis
complexes per results
yeast
cell
3A).
of varying
for
was used of 0.97
for
indicate
to determine
wall-associated
a Kd for
of mannan
interaction
Incubation
of varying
of free 4.12
interactions the
and mannan-
milligram
to determine
that
of free 1.95
of 1.2 x 10e5 M with yeast
concentrations by gel
x 10e5 M with
a determination
was used
followed
determination
2252 stationary -C. albicans and analysis of the supernatant
centrifugation
available
per
Incubation 2252 mannan,
for
complexes
myeloperoxidase
These
3).
albicans
chromatography
myeloperoxidase-mannan
yeast
(Figure C 2
with binding
mannan
for
moles with
concentrations phase
medium
yeast, for
of followed
by
enzyme
and yeast-bound
a Kd for
enzyme.
myeloperoxidase-Candida
x lo-l3
mM of binding
myeloperoxidase affinities
and for
x lo-'
sites
(Figure
3B).
of myeloperoxidase
solubilized
mannan
are
for nearly
identical. In order mannan determined equilibrium
to determine
the
and myeloperoxidase, by analytical method
(19),
stoichiometry
the
molecular
centrifugation. the
Candida
of the weight
of
Using
the
interaction the mannan meniscus
mannan was determined 813
of Candida was
depletion to have
a
Vol. 154,
No.
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
A *O 1
0
10
20
Bound I 15
25
20
Nmoles
30
40
50
60
(micromolar) , 30
Added
Nmoles
Added
FIGURE 3. Binding of myeloperoxidase to Candida mannan (Panel A) and Candida yeast (Panel B). A 30 minute incubation at 37OC allowed for maximal binding of myeloperoxidase to mannan or yeast.
molecular
weight
sites
milligram
per
approximately
of approximately
Capacity
We have yeast.
with
conditions.
viability yeast
units
population
candidacidal under
available
from
for were activity
a lack
peroxide-halide 1.1 x 10-a concentration
is
next
to target performed
resulted
from
of sufficient of myeloperoxidase
of 0.02
yeast
mM to
that
the
percent target
as percent dose
yeast
fungal
shows that
to kill
Thus,
the
Candida optimal
of myeloperoxidase
target
ratio per
These
results
suggest
that
is
limited
by the
amount
for
yeast the of
yeast. to verify a lack
cofactors system
capacity
fungicidal
of available
has a capacity
of myeloperoxidase
of
to the
enzyme was incubated
data
1.4 x lo*.
activity absorbed
optimal
number
7.9 x 1Om8 units
antimicrobial units
of
candidacidal
3, indicate
of the
conditions. binding
is
the
under
of initial
of approximately
Experiments candidacidal
of a plot
logarithm
candidacidal
enzyme
of purified
as the
of myeloperoxidase
activity
ratio
of myeloperoxidase.
characterize
in Figure
increased
experimental
candidacidal
than
the
the
of Candida
illustrated yeast
activity
these
enzyme
to further
Extrapolation versus
1.1 x 10-a
that
concentrations Data
of enzyme binding
to a binding
molecule
when the
1.1 x 10d3 units
of target
decreased.
per
effective
In order
decreasing
killing
equates
of mannan
demonstrated
is most
of myeloperoxidase,
The number
of Myeloperoxidase
previously
myeloperoxidase target
of polysaccharide
two molecules
Candidacidal
280,000.
that
the
of sufficient for
(Table
of
enzyme
rather
the myeloperoxidase-hydrogen 1).
and hydrogen
1 x 10" Candida
limitation
yeast
Simultaneous peroxide
addition
of
to a final
in PBS resulted
in
less
Vol.
154,
No.
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
TABLE I Characterization
of Myeloperoxidase-Mediated
Condition
Candidacidal
Supplements Ml'0 a + HzOz b MPO + HzOz + MPO + Hz02 + MPO + HzOz +
1 2 3
4
Yeast Viability
+ Cl-' (-MPO preincubation) Cl (+MPO preincubation) Cl- + (Hz02 at T = 30') Cl- + (MPO at T = 30')
*p
than at
a one percent 37'C
(Fig.
yeast
at
yeast
viability
decrease
4).
4cC for
30 minutes after
(p < 0.01).
Binding
of hydrogen
peroxide
Incubation
(4).
hydrogen reduction treated
provided
a 30-minute
for
of myeloperoxidase is
not
for
of yeast
an additional
viability.
yeast
to kill yeast
with
with
target in
peroxide in
target
the
absence
microorganisms aliquot
resulted
incubation
However,
incubation
reduction
yeast
the
2.5 0.7" 2.0 1.6"
with
hydrogen
a second
30 minutes
an additional
enzyme
percent
with
to Candida
sufficient
a 30 min.
the
a 23.1
f + 2 f
(%)
2 0.02 mM;
after of
incubation
99.0 76.9 80.5 63.5
condition peroxide,
viability
preincubation
of enzyme-treated
peroxide target
in yeast
In contrast,
Activity
of
in no further
of the
1.1 x 10S3 units
previously of
100 90 i
T ~
80-
C. albicans
2252
]
z-l 70.g =.nr 60; 508 40t L 3020-
IO-
4.0
log yeast I
1 1 0.125
0.25
Yeast
5.0
0.5 Concentration
6.0
concentration
1.0 (per
ml x10-9
FIGURE 4. Effect of yeast concentration on myeloperoxidase-mediated candidacidal activity. Percent viability of varying concentrations of C.aLbicans 2252 after incubation with 1.1 mU of myeloperoxidase and -___ 0.012 mM hydrogen peroxide in PBS is illustrated in linear and semilogarithmic plots (mean f S.E.M., n = 3).
815
Vol.
154,
No.
2, 1988
myeloperoxidase after
BIOCHEMICAL
reduced
a 30 minute
myeloperoxidase
activity
Additional
suggest of its
under
from
conditions hour
incubation
availability
the
is
performed
remained
of the
of additional
to desorb
fungal
of
since
a six
incubation
After
a similar
yeast,
the
amount
suggest
may be limited
killed
yeast
not
fungicidal
observations
activity
of this did
hour
optimal
Candida
These
cause
limitation
activity.
from
peroxide
factor the
This
with
candidacidal
enzyme
limiting
under
constant.
percent
of
to determine
enzyme,
catalytic
13.4
conditions.
activity.
on its
COMMUNICATIONS
of hydrogen
the
experimental
peroxide
myeloperoxidase-mediated killing
that
of myeloperoxidase
enzyme
inability
aliquot
hydrogen
had no effect
yeast-bound
by an additional
of the
with
RESEARCH
a second
candidacidal
of myeloperoxidase six
were
autoinactivation
BIOPHYSICAL
substrates
these
experiments
myeloperoxidase-limited result
with
results and not
candidacidal
viability
incubation
These
(p <0.05).
yeast
AND
of
that
by an
to participate
in
targets. DISCUSSION
Myeloperoxidase its
the
cytotoxic
agent
bind
walls
acid. Mannan
of myeloperoxidase that
weight
this
of the
Interaction occurs
without
result,
the
carbohydrate
cell the
provide
for
would
result, yeast.
of a minimum limitation
would
result,
the
may be limited
available
fail
availability by its
to form
is
able
to
cell as a target
as evidenced
for
by the
30 to 50 percent
Candida
through
activity
cell
of the
to this
of the
fungal
of the
both
cell
of the
mannan As a
surface acid
Such localized
dilution
wall
enzyme.
of hypochlorous cells.
candidacidal dose
an inability
activity
of the of the
of myeloperoxidase
also
ion
(20,21).
generation
effective
from
Targeting
mannan
with
in close generation
oxidant
appears
enzyme
of myeloperoxidase-mediated
in part,
chloride
for
of
and its
substrates.
Myeloperoxidase-mediated apparent
essential capable
myeloperoxidase
yeast
with
minimize
alternative
with
may compose
catalytic
components
acid with
readily
of myeloperoxidase
would
of hypochlorous
binding
wall
of myeloperoxidase
to target
interaction
is
is
interaction
to Candida
affecting binding
Second,
polysaccharide
fungal
properties
peroxide
by specific
mannan.
observation
two unique myeloperoxidase
of hydrogen
hypochlorous cell
wall-associated
proximity
First,
reaction
to fungal
binding
to have
activity.
catalyzing
dry
appears
candidacidal
affinity
for
enzyme
between
of myeloperoxidase mannan. 816
to target
candidacidal
to Candida
to discriminate
to require
for
cell
The
activity
to desorb
live
yeast. from
may
killed
wall-associated and dead yeast.
binding
to target
As a yeast
Vol.
154,
No.
2, 1988
We beI.ieve
that
mannan
represents
activity
of the
determine targets
whether for
BIOCHEMICAL
the
ability
additional
interaction
BIOPHYSICAL
RESEARCH
of myeloperoxidase
an essential enzyme.
AND
mechanism
Continued
research
microbial
to
involved must
interact
in the
with
other
with
candidacidal
be performed
polysaccharides
of myeloperoxidase
COMMUNICATIONS
to
may serve
as
microbial
pathogens. ACKNOWLEDGMENT This
work
was supported
in part
by Public
Health
Service
Grant
AI 16785.
REFERENCES 1.
2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21.
Klebanoff, S. J. (1968) J. Bacterial. 95, 2131-2138. Selvaraj, R. J., Zgliczynski, J. M., Paul, B. B., and Sbarra, A. J. (1978) J. Infect. Dis. 137, 481-485. Miyasaki, K. T., Zambon, J. J., Jones, C. A., and Wilson, M. E. (1987) Infect. Immun. 55, 1029-1036. Wright, C. D., Bowie, J. U., Gray, G. R., and Nelson R. D. (1983) Infect. Immun. 42, 76-80. Agner, K. (1972) Structure and function of oxidation reduction enzymes. In A. Akeson and A. Ehrenberg (Eds.), pp. 329-335. Pergamon Press, Oxford. Albrich, J. M., McCarthy, C. A., and Hurst, J. K. (1981) Proc. Natl. Acad. Sci. USA 78, 210-214. Sips, H. J. and Hamers, M. N. (1981) Infect. Immun. 31, 11-16. Wright, C. D., Bowie, J. U., and Nelson, R. D. (1984) Infect. Immun. 43, 467-471. Wright, C. D., Herron, M. J., Gray, G. R., Holmes, B., and Nelson, R. D. (1981) Infect. Immun. 32, 731-738. Wright, C. D. and Nelson, R. D. (1985) Infect. Immun. 47, 363-365. Agner, K. (1941) Acta Physiol. Stand. (Suppl. 8) 2, l-62. Ferrante, A. and Thong, Y.H. (1978) J. Immunol. Methods 24, 389-393. Andrews, P. C. and Krinsky, N. I. (1981) J. Biol. Chem. 258, 4211-4218. Baggiolini, M., Hirsch, J. G., and deDuve, C. (1969) J. Cell Biol. 40, 529-541. Fink, G. (1970) Methods Ezymol. 17A, 59-78. Peat, S., Whelan, W. J., and Edwards, T. E. (1961) 3. Chem. Sot. p. 29-34. Dubois, M., Gilles, K. A., Hamilton, J. K., Rebers, P. A., and Smith, F. (1956) Anal. Chem. 28, 350-356. Scatchard, G. (1949) Ann. N.Y. Acad. Sci. 51, 660-672. Nakajima, T. and Ballou, C. E. (1974) J. Biol. Chem. 249, 7679-7684. Chattawa, F. W., Holmes, M. R., and Barlow, A. J. E. (1968) J. Gen. Microbial. 51, 367-376. McMurrough, I. and Rose, A. H. (1967) Biochem. J. 105, 189-203.
817
154,
No.
July
29,
1988
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
COMMUNICATIONS Pages
CANDIDACIDAL
ACTIVITY
Clifford
D. Wright'
Departments
.June 20,
CHARACTERIZATION
OF MYELOPEROXIDASE:
MYKLOPEROXIDASE-YEAST
Received
RESEARCH
809-817
OF
COMPLEX FORMATION D. Nelson I,2
and Robert
of Microbiology1 and Surgery2 University of Minnesota Minneapolis, MN 55455
1988
demonstrated the ability of human FxJmlARY : We have previously -neutrophil myeloperoxidase to bind to cell wall mannan polysaccharide isolated :Erom Candida albicans. This binding capacity provides for association of the enzyme with target yeast which is essential for In this report, we further consider the efficient candidacidal activity. role of the mannan-binding property of myeloperoxidase in the Solubilized mannan antagonizes candidacidal activity of the enzyme. binding o:E the enzyme to yeast, suggesting that mannan may be a primary component of the fungal cell wall which serves as a target for binding of Myeloperoxidase is shown to form complexes with both myeloperoxidase. solubilized mannan and Candida yeast, with Kds of 0.97 x lo-' M and 1.2 x lo-' M, respectively. The interaction between myeloperoxidase and mannan does not allow the enzyme to readily dissociate from the surface of target yeast. As a result, the enzyme may be unable to dissociate from dead yeast to become available for binding to additional fungal targets. 0 1988 ncademlc Press. 1°C.
The microbicidal halide
system
activity
(1)
is
microorganisms.
This
Escherichia -- coli: Candida albicans _ -_
(4).
myelopero'xidase acid
(5)
of this
of the
optimized phenomenon
(2),
Actinobacillus It
enzyme is
has been
at the microbial
thereby
(6,7)
to the for
and its
that for
of
(3),
binding
and
of
generation
of hypochlorous
minimizing
both
interaction
target
killing
actinomycetecomitans allows
surface,
oxidant
peroxide-
bound
demonstrated
has been proposed
to microorganisms
cytotoxic
myeloperoxidase-hydrogen
when the
with
the
dilution
alternate
substrates. We have previously C. albicans interaction
through
was shown
myeloperoxidase 'Current Company,
demonstrated cell
address:
wall
to be ionic,
(p1 = 10.2)
(11)
Pharmacology
Pharmaceutical
that
mannan
Research
myeloperoxidase
polysaccharide
rather and the
Department, Division,
than
binds
to
(4,8,9,10). lectin-like,
phosphate
The between
groups
of the
mannan
Parke-Davis/Warner-Lambert Ann Arbor,
MI
48105 0006-291X/88
809
$1.50
Copyright 0 1988 by Academic Press. Inc. All rights of reproduction in any form reserved.
Vol.
154,
outer
No.
2, 1988
chain
(8).
has also
been
The purpose myeloperoxidase of the
BIOCHEMICAL
Binding
shown
BIOPHYSICAL
of myeloperoxidase
to be a mannan-specific
of this
report
to mannan
is
required
RESEARCH
interaction
to further
COMMUNICATIONS
to A. actinomycetecomitans (3).
characterize
to promote
the
candidacidal
the binding
of
activity
enzyme. MATERIALS
Isolation
AND
AND METHODS
of Myeloperoxidase
Human neutrophils were isolated from anti-coagulant treated whole blood according to the procedure of Ferrante and Thong (12). Myeloperoxidase was isolated from human neutrophils according to the method of Andrews and Krinsky (13). The partially purified enzyme had an R. 2. value of 0.62. Myeloperoxidase activity was quantitated in terms of pyrogallol units as described by Baggiolini, et al, (14). The candidacidal activity of the enzyme preparation was characterized in vitro. Candidacidal activity was shown to be both hydrogen peroxideand chloride ion-dependent. Inhibitors of myeloperoxidase activity (0.1 mM azide, 0.1 mM cyanide) and a scavenger of hypochlorous acid (1 mM I-methionine) also effectively inhibited killing of target yeast (4). Isolation
of Mannan
Candida albicans 2252 (ATC 44806) was grown to stationary yeast nitrogen base minimal medium (15). Mannan was isolated Fehling's solution as copper complexes from citrate-extracted described by Peat, et al, (16). Assay
of Myeloperoxidase-Mannan
Complex
phase with yeast
in as
Formation
Myeloperoxidase (3.5 x 10e2 units) and mannan (4.0 mg) were incubated in Dulbecco's phosphate-buffered saline (PBS) (pH 7.4) for 30 minutes at 37%. The sample was then chromatographed on a Sephadex G-150 gel permeation column (18 x 1.5 cm) in distilled water. The elution profile of the myeloperoxidase-mannan reaction mixture was compared with those of isolated myeloperoxidase and mannan. Elution of myeloperoxidase was monitored by its catalytic activity at 435 nm (14). Elution of mannan was monitored by the phenol-sulfuric acid assay for carbohydrates at 490 nm (17). Assay
of Myeloperoxidase-Yeast
Complex
Formation
C. albicans 2252 was incubated overnight in yeast nitrogen base mini&l media at 37%. Following three washes in PBS, the yeast suspension was adjusted to a final optical density of 1.0 at 660 nm (Asso) of 1.0 equals approximately 2 x lo7 yeast per ml. A 0.1 ml aliquot of yeast was incubated with 1.1 x 10e3 units of myeloperoxidase in a final volume of 0.5 ml at 37%. After 30 minutes, the reaction mixture was centrifuged and the amounts of free and yeast-bound myeloperoxidase were determined. Binding of myeloperoxidase to yeast compared in the presence and absence of 2 mg/ml mannan. Dissociation Constants Yeast Interactions
of Myeloperoxidase-Mannan
The dissociation constant of.myeloperoxidase-mannan determined by incubation of varying concentrations 810
and Myeloperoxidasecomplexes was of myeloperoxidase
was
Vol.
154,
No.
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
with 12 mg of C. albicans 2252 mannan in PBS. After a 30 minute incubation at 37OC, the reaction mixture was chromatographed on a G-150 Sephadex gel permeation column (18 x 1.5 cm) in distilled water to separate free myeloperoxidase from mannan-bound enzyme. The peak areas of the chromatographed myeloperoxidase fractions were used to determine the amount of bound and free enzyme for use in Scatchard analysis (18). The dissociation constant of myeloperoxidase-yeast complexes was determined by incubation of varying concentrations of myeloperoxidase with C. albicans 2252. Overnight cultures of C. albicans 2252 were One ml aliquots of the yeast suspension prepared as described above. were centrifuged and resuspended to a final volume of 0.6 ml with a 30-minute incubation at 37OC, the myeloperoxidase in PBS. After reaction mixture was centrifuged and the amount of myeloperoxidase remaining free in the supernate was quantified for use in Scatchard analysis. Molecular
Weight
Determinations
of Candida
mannan
The molecular weight of C. albicans 2252 mannan was determined by meniscus depletion equilibration using a Spinco model E analytical centrifuge with interference optics (19). Samples were prepared at 0.5 mg/ml in 0.1 M KHsPO4, pH 4.7. The sample was centrifuged at 14,000 rpm at 18OC. The mean molecular weight of mannan from two runs was detennined. Assay
of Myeloperoxidase-Mediated
Candidacidal
Activity
2252 were prepared as described Overnight cultures of C. albicans above. A 0.1 ml aliquot ofyeast was incubated with 1.1 x lop3 units of myelopero.xidase at 4nC for 30 minutes. Following preincubation, hydrogen peroxidas,e was added to give a concentration of 0.02 mM in a final All reagents were diluted in PBS to provide a reaction -volume of 1.0 ml. final chl'oride concentration of 0.14 M. The reaction mixture was incubated at 37OC on a rotating table. Myeloperoxidase-mediated killing was stopped by transferring the reaction tube to ice water. Yeast viability was determined by pour plate methodology using yeast extract peptone dextrose agar (15). Control experiments verified that the observed candidacidal activity was generated by the myeloperoxidase-hydrogen peroxide-chloride antimicrobial system (1). RESULTS Myeloperoxidase-Mannan Binding mannan
Complex
was assessed
by gel
of myeloperoxidase of its
catalytic
of the
column.
phenol-sulfuric volume.
myeloperoxidase allow
from
In contrast, acid
association
(435
run),
of the
C. albicans
chromatography G-150
column,
occurred
elution
carbohydrate
and a 4.0
to solubilized
permeation
a Sephadex
activity
The chromatograph
elution did not
Formation
of human myeloperoxidase
monitored
within
of mannan, assay
(490
nm),
of 3.5
mg of mannan
preincubated
showed
the
a shift
volume
by the
occurred
in the
void
of
30 minutes
to
of the peroxidase
peak to the void volume. Binding of myeloperoxidase inhibit the catalytic activity of the enzyme. This 811
Elution
as a function
x 10e2 units for
1).
inclusion
monitored
of a mixture reactants
(Figure
2252
to mannan shift in the
Vol.
154,
No.
2, 1988
BIOCHEMICAL
0.4
-
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
"0 i
0.3
-
:
MPO + mannan 435nm
Iii e
2
MPCJ 435nm
0.2 -
:
II, 0.1
R
-
&!.!L&.
5
10
15
20
25
30
Elution
35
40
Volume
45
50
55
6C
(ml)
FIGIJBE 1. Myeloperoxidase-mannan complex formation. Elution patterns of myeloperoxidase (MPO), -~ C. albicans 2252 mannan, and an MPO-mannan reaction mixture from a Sephadex G-150 gel permeation column are illustrated. Elution of myeloperoxidase was monitored as a function of its catalytic activity at 435 am. Elution of mannan was monitored by the phenol-sulfuric acid carbohydrate assay at 490 nm. Vo, void volume. elution
pattern
for
peroxidase
activity
is
expected
for
an enzyme-mannan
complex. Myeloperoxidase-Yeast Binding
Complex
determining
the
30-minute
incubation
amount
1.1 x 10-e
units
68 percent
of the
corresponding association binding
with that
involves
with enzyme. with
myeloperoxidase
yeast.
in a dose-dependent displace
Analysis
Myeloperoxidase-Candida The dissociation myeloperoxidase-Candida
incubation
Candida
yeast, with
of the
solubilized enzyme with
binding
interaction
of myeloperoxidase
Solubilized
(4).
enzyme.
to solubilized
These
mannan
of the
mannan
was also
results
suggest
and to yeast
of the enzyme.
of Myeloperoxidase-Mannan
and
Interactions constants
(Kds)
interactions
for were
812
myeloperoxidase-mannan determined
the
a common
antagonized
yeast-bound
function
whether
involved
Preincubation
of a
to determine
and yeast
with
manner
a
After
was preincubated
inhibits
of myeloperoxidase
a common binding
In order
by
following
cell-associated
completely
Mannan
2).
2 x lo6
mannan
of yeast. mannan
was assessed
enzyme
(Figure
enzyme became
in free
to addition
to effectively binding
Binding
available
of solubilized
yeast
shown
and yeast-bound
of myeloperoxidase
decrease
to target
to C. albicans
reagents
of myeloperoxidase
mannan prior enzyme
of free of the
function,
2 mg/ml
Formation
of human myeloperoxidase
by Scatchard
and
Vol.
154,
No.
2, 1988
BIOCHEMICAL
120
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
-
FIGURE 2. Influence of soluble mannan on myeloperoxidase-Candida comlplex formation. Binding of myeloperoxidase (MPO) to yeast was compared in the presence and absence of soluble mannan (mean 2 S.E.M., n = 3).
analysis
of binding
data
of myeloperoxidase permeation bound
with
enzyme.
of binding
allowed
Scatchard
sites
analysis
available (Figure
myeloperoxidase
with
activity,
allowed
Scatchard
analysis
complexes per results
yeast
cell
3A).
of varying
for
was used of 0.97
for
indicate
to determine
wall-associated
a Kd for
of mannan
interaction
Incubation
of varying
of free 4.12
interactions the
and mannan-
milligram
to determine
that
of free 1.95
of 1.2 x 10e5 M with yeast
concentrations by gel
x 10e5 M with
a determination
was used
followed
determination
2252 stationary -C. albicans and analysis of the supernatant
centrifugation
available
per
Incubation 2252 mannan,
for
complexes
myeloperoxidase
These
3).
albicans
chromatography
myeloperoxidase-mannan
yeast
(Figure C 2
with binding
mannan
for
moles with
concentrations phase
medium
yeast, for
of followed
by
enzyme
and yeast-bound
a Kd for
enzyme.
myeloperoxidase-Candida
x lo-l3
mM of binding
myeloperoxidase affinities
and for
x lo-'
sites
(Figure
3B).
of myeloperoxidase
solubilized
mannan
are
for nearly
identical. In order mannan determined equilibrium
to determine
the
and myeloperoxidase, by analytical method
(19),
stoichiometry
the
molecular
centrifugation. the
Candida
of the weight
of
Using
the
interaction the mannan meniscus
mannan was determined 813
of Candida was
depletion to have
a
Vol. 154,
No.
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
A *O 1
0
10
20
Bound I 15
25
20
Nmoles
30
40
50
60
(micromolar) , 30
Added
Nmoles
Added
FIGURE 3. Binding of myeloperoxidase to Candida mannan (Panel A) and Candida yeast (Panel B). A 30 minute incubation at 37OC allowed for maximal binding of myeloperoxidase to mannan or yeast.
molecular
weight
sites
milligram
per
approximately
of approximately
Capacity
We have yeast.
with
conditions.
viability yeast
units
population
candidacidal under
available
from
for were activity
a lack
peroxide-halide 1.1 x 10-a concentration
is
next
to target performed
resulted
from
of sufficient of myeloperoxidase
of 0.02
yeast
mM to
that
the
percent target
as percent dose
yeast
fungal
shows that
to kill
Thus,
the
Candida optimal
of myeloperoxidase
target
ratio per
These
results
suggest
that
is
limited
by the
amount
for
yeast the of
yeast. to verify a lack
cofactors system
capacity
fungicidal
of available
has a capacity
of myeloperoxidase
of
to the
enzyme was incubated
data
1.4 x lo*.
activity absorbed
optimal
number
7.9 x 1Om8 units
antimicrobial units
of
candidacidal
3, indicate
of the
conditions. binding
is
the
under
of initial
of approximately
Experiments candidacidal
of a plot
logarithm
candidacidal
enzyme
of purified
as the
of myeloperoxidase
activity
ratio
of myeloperoxidase.
characterize
in Figure
increased
experimental
candidacidal
than
the
the
of Candida
illustrated yeast
activity
these
enzyme
to further
Extrapolation versus
1.1 x 10-a
that
concentrations Data
of enzyme binding
to a binding
molecule
when the
1.1 x 10d3 units
of target
decreased.
per
effective
In order
decreasing
killing
equates
of mannan
demonstrated
is most
of myeloperoxidase,
The number
of Myeloperoxidase
previously
myeloperoxidase target
of polysaccharide
two molecules
Candidacidal
280,000.
that
the
of sufficient for
(Table
of
enzyme
rather
the myeloperoxidase-hydrogen 1).
and hydrogen
1 x 10" Candida
limitation
yeast
Simultaneous peroxide
addition
of
to a final
in PBS resulted
in
less
Vol.
154,
No.
2, 1988
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
TABLE I Characterization
of Myeloperoxidase-Mediated
Condition
Candidacidal
Supplements Ml'0 a + HzOz b MPO + HzOz + MPO + Hz02 + MPO + HzOz +
1 2 3
4
Yeast Viability
+ Cl-' (-MPO preincubation) Cl (+MPO preincubation) Cl- + (Hz02 at T = 30') Cl- + (MPO at T = 30')
*p
than at
a one percent 37'C
(Fig.
yeast
at
yeast
viability
decrease
4).
4cC for
30 minutes after
(p < 0.01).
Binding
of hydrogen
peroxide
Incubation
(4).
hydrogen reduction treated
provided
a 30-minute
for
of myeloperoxidase is
not
for
of yeast
an additional
viability.
yeast
to kill yeast
with
with
target in
peroxide in
target
the
absence
microorganisms aliquot
resulted
incubation
However,
incubation
reduction
yeast
the
2.5 0.7" 2.0 1.6"
with
hydrogen
a second
30 minutes
an additional
enzyme
percent
with
to Candida
sufficient
a 30 min.
the
a 23.1
f + 2 f
(%)
2 0.02 mM;
after of
incubation
99.0 76.9 80.5 63.5
condition peroxide,
viability
preincubation
of enzyme-treated
peroxide target
in yeast
In contrast,
Activity
of
in no further
of the
1.1 x 10S3 units
previously of
100 90 i
T ~
80-
C. albicans
2252
]
z-l 70.g =.nr 60; 508 40t L 3020-
IO-
4.0
log yeast I
1 1 0.125
0.25
Yeast
5.0
0.5 Concentration
6.0
concentration
1.0 (per
ml x10-9
FIGURE 4. Effect of yeast concentration on myeloperoxidase-mediated candidacidal activity. Percent viability of varying concentrations of C.aLbicans 2252 after incubation with 1.1 mU of myeloperoxidase and -___ 0.012 mM hydrogen peroxide in PBS is illustrated in linear and semilogarithmic plots (mean f S.E.M., n = 3).
815
Vol.
154,
No.
2, 1988
myeloperoxidase after
BIOCHEMICAL
reduced
a 30 minute
myeloperoxidase
activity
Additional
suggest of its
under
from
conditions hour
incubation
availability
the
is
performed
remained
of the
of additional
to desorb
fungal
of
since
a six
incubation
After
a similar
yeast,
the
amount
suggest
may be limited
killed
yeast
not
fungicidal
observations
activity
of this did
hour
optimal
Candida
These
cause
limitation
activity.
from
peroxide
factor the
This
with
candidacidal
enzyme
limiting
under
constant.
percent
of
to determine
enzyme,
catalytic
13.4
conditions.
activity.
on its
COMMUNICATIONS
of hydrogen
the
experimental
peroxide
myeloperoxidase-mediated killing
that
of myeloperoxidase
enzyme
inability
aliquot
hydrogen
had no effect
yeast-bound
by an additional
of the
with
RESEARCH
a second
candidacidal
of myeloperoxidase six
were
autoinactivation
BIOPHYSICAL
substrates
these
experiments
myeloperoxidase-limited result
with
results and not
candidacidal
viability
incubation
These
(p <0.05).
yeast
AND
of
that
by an
to participate
in
targets. DISCUSSION
Myeloperoxidase its
the
cytotoxic
agent
bind
walls
acid. Mannan
of myeloperoxidase that
weight
this
of the
Interaction occurs
without
result,
the
carbohydrate
cell the
provide
for
would
result, yeast.
of a minimum limitation
would
result,
the
may be limited
available
fail
availability by its
to form
is
able
to
cell as a target
as evidenced
for
by the
30 to 50 percent
Candida
through
activity
cell
of the
to this
of the
fungal
of the
both
cell
of the
mannan As a
surface acid
Such localized
dilution
wall
enzyme.
of hypochlorous cells.
candidacidal dose
an inability
activity
of the of the
of myeloperoxidase
also
ion
(20,21).
generation
effective
from
Targeting
mannan
with
in close generation
oxidant
appears
enzyme
of myeloperoxidase-mediated
in part,
chloride
for
of
and its
substrates.
Myeloperoxidase-mediated apparent
essential capable
myeloperoxidase
yeast
with
minimize
alternative
with
may compose
catalytic
components
acid with
readily
of myeloperoxidase
would
of hypochlorous
binding
wall
of myeloperoxidase
to target
interaction
is
is
interaction
to Candida
affecting binding
Second,
polysaccharide
fungal
properties
peroxide
by specific
mannan.
observation
two unique myeloperoxidase
of hydrogen
hypochlorous cell
wall-associated
proximity
First,
reaction
to fungal
binding
to have
activity.
catalyzing
dry
appears
candidacidal
affinity
for
enzyme
between
of myeloperoxidase mannan. 816
to target
candidacidal
to Candida
to discriminate
to require
for
cell
The
activity
to desorb
live
yeast. from
may
killed
wall-associated and dead yeast.
binding
to target
As a yeast
Vol.
154,
No.
2, 1988
We beI.ieve
that
mannan
represents
activity
of the
determine targets
whether for
BIOCHEMICAL
the
ability
additional
interaction
BIOPHYSICAL
RESEARCH
of myeloperoxidase
an essential enzyme.
AND
mechanism
Continued
research
microbial
to
involved must
interact
in the
with
other
with
candidacidal
be performed
polysaccharides
of myeloperoxidase
COMMUNICATIONS
to
may serve
as
microbial
pathogens. ACKNOWLEDGMENT This
work
was supported
in part
by Public
Health
Service
Grant
AI 16785.
REFERENCES 1.
2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20. 21.
Klebanoff, S. J. (1968) J. Bacterial. 95, 2131-2138. Selvaraj, R. J., Zgliczynski, J. M., Paul, B. B., and Sbarra, A. J. (1978) J. Infect. Dis. 137, 481-485. Miyasaki, K. T., Zambon, J. J., Jones, C. A., and Wilson, M. E. (1987) Infect. Immun. 55, 1029-1036. Wright, C. D., Bowie, J. U., Gray, G. R., and Nelson R. D. (1983) Infect. Immun. 42, 76-80. Agner, K. (1972) Structure and function of oxidation reduction enzymes. In A. Akeson and A. Ehrenberg (Eds.), pp. 329-335. Pergamon Press, Oxford. Albrich, J. M., McCarthy, C. A., and Hurst, J. K. (1981) Proc. Natl. Acad. Sci. USA 78, 210-214. Sips, H. J. and Hamers, M. N. (1981) Infect. Immun. 31, 11-16. Wright, C. D., Bowie, J. U., and Nelson, R. D. (1984) Infect. Immun. 43, 467-471. Wright, C. D., Herron, M. J., Gray, G. R., Holmes, B., and Nelson, R. D. (1981) Infect. Immun. 32, 731-738. Wright, C. D. and Nelson, R. D. (1985) Infect. Immun. 47, 363-365. Agner, K. (1941) Acta Physiol. Stand. (Suppl. 8) 2, l-62. Ferrante, A. and Thong, Y.H. (1978) J. Immunol. Methods 24, 389-393. Andrews, P. C. and Krinsky, N. I. (1981) J. Biol. Chem. 258, 4211-4218. Baggiolini, M., Hirsch, J. G., and deDuve, C. (1969) J. Cell Biol. 40, 529-541. Fink, G. (1970) Methods Ezymol. 17A, 59-78. Peat, S., Whelan, W. J., and Edwards, T. E. (1961) 3. Chem. Sot. p. 29-34. Dubois, M., Gilles, K. A., Hamilton, J. K., Rebers, P. A., and Smith, F. (1956) Anal. Chem. 28, 350-356. Scatchard, G. (1949) Ann. N.Y. Acad. Sci. 51, 660-672. Nakajima, T. and Ballou, C. E. (1974) J. Biol. Chem. 249, 7679-7684. Chattawa, F. W., Holmes, M. R., and Barlow, A. J. E. (1968) J. Gen. Microbial. 51, 367-376. McMurrough, I. and Rose, A. H. (1967) Biochem. J. 105, 189-203.
817