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Infection and Immunity, March 2000, p. 1649-1654, Vol. 68, No. 3
Department of Microbiology, Montana State
University, Bozeman, Montana 59717-3520
Received 13 August 1998/Returned for modification 7 October
1999/Accepted 26 October 1999
We previously reported that a liposome-mannan vaccine (L-mann) of
Candida albicans induces production of mouse antibodies that protect against disseminated candidiasis and vaginal infection. Immunoglobulin M (IgM) monoclonal antibody (MAb) B6.1, specific for a
C. albicans cell surface In experimental animals, host
defense against cryptococcosis and candidiasis involves virtually all
aspects of the immune system, including antibodies (7). The
role of antibodies in defense against these diseases in humans is not
known, but suggestive evidence has been obtained that certain
antibodies may be protective (6, 7, 19). Because of the
possible utility in prevention and treatment of human fungal diseases,
continued efforts are needed for gaining a clear definition of
protective antibodies. In studies on experimental cryptococcosis, both
antibody specificity and isotype are apparently important
considerations. Monoclonal antibodies (MAbs) specific for
epitopes within the glucuronoxylomannan capsular structure are
protective. However, whereas immunoglobulin M (IgM) and IgG1 MAbs
specific for the glucuronoxylomannan protect against experimental
disease, an IgG3 MAb does not protect even though all three antibodies
have identical levels of epitope recognition (25, 26).
We have been investigating the role of Candida-specific
antibodies in host defense against various forms of candidiasis. Using an intravenous (i.v.) immunization route for administering liposomes containing Candida albicans surface mannan complexes, mice
responded by making a protective antibody response against both
disseminated candidiasis (11, 12) and Candida
vaginal infection (14). Recently, we developed a more
efficient vaccine formula made of mannan-protein conjugates. The
conjugate vaccine requires fewer boosters and is administered by an
intraperitoneal (i.p.) route (15). Both vaccines induced
protective antibody responses that could be passively transferred to
naive animals. During this work, we isolated an IgM MAb, termed MAb
B6.1, which enhances resistance of normal, SCID, and neutropenic mice
against disseminated disease (11, 12) and protected the
animals against Candida vaginal infection (14).
MAb B6.1 is specific for a In this study, we compared the protective efficacies of the IgM MAb
B6.1 and an IgG3 MAb, termed C3.1, against experimental candidiasis. We
show that the two MAbs are specific for the same mannotriose and both
are protective against candidiasis in mice.
Organism and culture conditions.
C. albicans CA-1 was
started from frozen glycerol stocks, grown at 37°C, washed and
suspended in cold Dulbecco's phosphate-buffered saline (DPBS; Sigma
Chemical Co., St. Louis, Mo.), and used to infect mice as previously
described (11, 14, 18).
Mice.
BALB/c female mice (NCI Animal Production Program,
Frederick Cancer Research Center, Frederick, Md.) 6 to 8 weeks old were used throughout the study. In all experiments, mice were maintained in
accordance with institutional regulations in an Association for
Assessment and Accreditation of Laboratory Animal Care-certified animal
facility at Montana State University.
Anti-C. albicans MAbs C3.1 and B6.1.
MAb C3.1
was one of several MAbs, including the protective MAb B6.1, which were
isolated through hybridoma techniques from mice vaccinated with a
mannan-liposome preparation as described elsewhere (11). MAb
C3.1 was produced from a hybridoma clone grown in the absence of
antibiotics either in RPMI 1640 (Sigma) plus 10% fetal bovine serum or
in serum-free medium (HB101 Liquid kit; Irvine Scientific, Santa Ana,
Calif.) without antibiotics. The MAb was concentrated by precipitation
in 50% ammonium sulfate. MAb B6.1, which served as a positive control
antibody, was produced by LigoCyte Pharmaceuticals, Inc. (Bozeman,
Mont.) as before, and both MAbs were quantified as described previously
(12, 14).
ELISA titer of MAbs.
Wells of a polystyrene microtiter plate
(Costar 96-well microtiter plate; Costar Corning, Corning, N.Y.) were
coated with mannan extract by adding to each well 100 µl of mannan
(10 µg of mannan/ml) solubilized in 0.06 M carbonate buffer (pH 9.6), with incubation for 3 h at 37°C and at 4°C overnight. The
wells were washed with deionized water, and each received 250 µl of 0.01 M Tris-buffered saline (0.01 M TBS) (0.01 M Trizma-HCl [Sigma] plus 0.15 N NaCl [pH 7.4]) with 3% bovine serum albumin (BSA) (fraction V; Sigma) for 1 h at 21 to 23°C. The buffer was
replaced by 50 µl of either MAb appropriately diluted in 0.01 M
TBS-BSA for 1 h at 37°C, washed three times with 0.01 M TBS
containing 0.05% Tween 20 (0.01 M TBST), and washed three times with
0.01 M TBS. The 0.01 M TBS was replaced by 50 µl of
peroxidase-conjugated anti-mouse polyvalent Igs (1.6 mg/ml; diluted
1:1,000 in 0.01 M TBS-BSA; Sigma) for 1 h at 21 to 23°C, washed
with 0.01 M TBS, and replaced by 100 µl of substrate. The substrate
was a solution made of 25 ml of 0.1 M citrate buffer (pH 5.0), 0.5 ml
of a water solution of o-phenylenediamine (50 mg/ml; Sigma),
and 10 µl of 30% H2O2. The color was allowed
to develop for 30 min, at which time 100 µl of 10%
H2SO4 was added as a stop to each well, and the
optical density (OD) for each was determined at 490 nm in a microtiter
plate reader (model 450; Bio-Rad, Richmond, Calif.). Negative control
wells that were coated with or without the mannan extract,
respectively, received only diluent (0.01 M TBS-BSA) instead of the
test MAbs, and the remaining steps of the procedure were exactly as
described above. Background absorbance from the negative control wells
was subtracted from the test well to obtain final OD readings. The
enzyme-linked immunosorbent assay (ELISA) titer was taken as the
reciprocal of the last antibody dilution that gave a positive OD reading.
Standardization of antibody concentrations.
Antibodies were
titered by agglutination against either whole C. albicans
yeast cells or mannan-coated latex beads (11, 14) and by
ELISA (14) as described above. By these various measures,
the antibody concentrations and titers were determined, and working
solutions of each were prepared as follows. MAb C3.1 prepared at 2.14 mg/ml gave the same agglutinin and ELISA titers as MAb B6.1 prepared at
0.21 mg/ml (40 and 2,000, respectively). For the protection assays in
mice, each animal received 0.5 ml of these antibody preparations.
SDS-PAGE.
MAb C3.1 was evaluated by sodium dodecyl
sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (12.5%
polyacrylamide) analysis under reducing ( Isotyping of MAb C3.1.
The isotype of MAb C3.1 was
determined by a capture ELISA as follows. One half of the wells in a
polystyrene microtiter plate (Costar 3396 EIA/RIA plate) received 100 µl of affinity-purified heavy-chain-specific goat, rabbit, or rat
anti-mouse Ig. All anti-mouse Igs used in these assays were prepared at
10 µg/ml in 0.06 M carbonate buffer (pH 9.6). Anti-mouse IgA was
purchased from Zymed (San Francisco, Calif.), IgE was obtained from
Southern Biotechnology Associates, Inc. (Birmingham, Ala.), and
anti-mouse IgG and IgM were obtained from Sigma. For negative controls,
each of the remaining wells received 100 µl of the carbonate buffer
solution. The plate was incubated at 21 to 23°C for 3 h. The
wells were washed with Trizma (Sigma)-buffered saline solution (0.05 M
Trizma-HCl [Sigma] plus 0.15 mM NaCl [pH 7.5]) three times, blocked
with 1% BSA and 5% nonfat dry milk in TBST (blocking buffer), and
incubated at 5 to 8°C overnight. The wells were washed once with TBST
and then three times with TBS. One hundred microliters of MAb C3.1
(diluted 1:200 in blocking buffer) was added to the appropriate wells, which were then incubated at 21 to 23°C for 2 h. Negative
control wells received only 100 µl of blocking buffer. After the
wells were washed with TBST and TBS as described above, 100 µl of
heavy-chain-specific biotinylated goat anti-mouse Ig (diluted 1:4,000
in blocking buffer) was put into the appropriate wells. Biotinylated
anti-mouse IgE was obtained from Southern Biotechnology Associates,
biotinylated anti-mouse IgA and IgM were from Sigma, and the remaining
biotin-conjugated anti-mouse IgG, IgG1, IgG2a, IgG2b, and IgG3 were
from Zymed. The wells were washed with TBST and TBS as described above,
100 µl of streptavidin-alkaline phosphatase (diluted 1:1,000 in TBST; Zymed) was added to each, and the plate was incubated at 21 to 23°C
for 1 h and washed as described above. For these experiments, the
substrate was prepared by dissolving 50 mg of p-nitrophenol phosphate (Sigma) in 1 ml of distilled water and diluting the solution
1:100 in substrate buffer (8.2% diethanolamine [Fisher Scientific,
Fair Lawn, N.J.], 60 mM HCl, 1 mM MgCl2). One hundred microliters of substrate was added to each well, the plate was incubated in the dark at 21 to 23°C for 15 min for color development, and the results were read at 405 nm in a microtiter plate reader (model
450; Bio-Rad). As positive controls, MAb B6.1 (IgM) and a mouse IgG3
(Zymed) were used under conditions identical to those described above.
In some tests, an IgG3 and an IgG1 specific for a Cryptococcus
neoformans capsular glucuronoxylomannan epitope (a generous gift
from A. Casadevall) (8) were used as positive controls.
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Protection against Candidiasis by an Immunoglobulin
G3 (IgG3) Monoclonal Antibody Specific for the Same Mannotriose as an
IgM Protective Antibody
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-1,2-mannotriose, protects mice against both infections. Another IgM MAb, termed B6, which is specific
for a different cell surface mannan epitope, does not protect against
disseminated candidiasis. The B6.1 epitope is displayed homogeneously
over the entire cell surface, compared to a patchy distribution of the
B6 epitope. To determine if protection is restricted to an IgM class of
antibody, we tested an IgG antibody. MAb C3.1 was obtained from
L-mann-immunized mice. By results of sodium dodecyl
sulfate-polyacrylamide gel electrophoresis analysis, capture
enzyme-linked immunosorbent assay, and immunodiffusion tests, MAb C3.1
is an IgG3 isotype. By epitope inhibition assays, we determined that
MAb C3.1 is specific for same mannotriose as MAb B6.1. As expected by
the results of the inhibition assays, immunofluorescence microscopy
showed that the C3.1 epitope is distributed on the yeast cell surface
in a pattern identical to that of the B6.1 epitope. Kidney CFU and mean
survival times of infected mice pretreated with MAb C3.1 indicated that
the antibody enhanced resistance of mice against disseminated
candidiasis. Mice in pseudoestrus that were given MAb C3.1 prior to
vaginal infection developed fewer vaginal Candida CFU than
control animals that received buffered saline instead of the antibody.
The finding that an IgG3 antibody is protective is consistent with our
hypothesis that epitope specificity and complement activation are
related to the ability of an antibody to protect against candidiasis.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-1,2-mannotriose (13), which
is an acid-labile component of the phosphomannan complex (PMC) of the
C. albicans cell walls (23, 24). This oligomannosyl epitope appears to be expressed uniformly over the entire
cell surface (13). In contrast to MAb B6.1, a nonprotective IgM MAb, termed MAb B6, has a patchy distribution over the cells (13). The B6 epitope is apparently associated with the
acid-stable part of the PMC (13). Whereas these data show
that antibody specificity is a key consideration, they do not address
the relevance of Ig isotype to protection. In view of the critical role
that antibody isotype plays in protection against cryptococcosis, as cited above, and in other diseases, including those due to group B
streptococci (16), we investigated whether an IgG MAb can protect against experimental candidiasis. The results of these studies
should help in the elucidation of mechanisms by which protective
antibodies assist the host in defense against candidiasis.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-mercaptoethanol)
conditions to determine sizes of heavy and light chains of the
antibody. The sizes were compared to those of known IgG MAb 54.1, specific for human neutrophil cytochrome b (a gift from Jim
Burritt and Al Jesaitis, Montana State University), and IgM MAb B6.1,
specific for C. albicans cell wall mannan (LigoCyte).
Locations of the protein bands were determined by silver staining and
compared to known molecular markers (Sigma) of 205-, 116-, 97-, 66-, 45-, and 29-kDa molecules corresponding to myosin, -galactose,
phosphorylase b, albumin (bovine plasma), albumin (egg), and
carbonic anhydrase, respectively.
Mannan extraction, acid hydrolysis, and identification of MAb
C3.1 epitope.
The same batch of affinity column-purified PMC, acid
hydrolysate of the PMC, and P-2 column-fractionated components of the hydrolysate were used in these experiments as described previously for
work on the identification of the B6.1 epitope (13). The individual fractions from the P-2 column, each of which represented a
predominance of one size of a -1,2-linked oligomannoside, were tested for the ability to react with MAb C3.1 by the mannotriose inhibition assay described for identification of the epitope recognized by MAb B6.1 (13). That is, solutions containing various
amounts of each fraction per milliliter were prepared in DPBS
containing 1% BSA and 0.02% sodium azide. Each fraction (10 µl) at
the indicated concentrations was mixed with 10 µl of MAb C3.1 (4.3 mg/ml; 1:20 diluted in DPBS). Following mixing in solution of the
various fractions with antibody, 10 µl of mannan-coated latex beads
(30 × 107 beads per ml) was added to the solutions,
mixed, and observed for agglutination of the beads. As a positive
control for agglutination, antibody was mixed with the mannan-coated
latex beads in the absence of the column fractions. As controls for
specificity, the irrelevant sugars raffinose (a triose; Sigma) and
stachyose (a tetraose; Sigma) were tested for the ability to inhibit
agglutination of the latex-mannan beads. Concentrations of the
irrelevant sugars used were the same as those indicated with the
fractions above.
Fluorescence microscopy.
Distribution of the C3.1 epitope on
yeast cells was determined by indirect immunofluorescence. Two hundred
microliters of MAb C3.1 (at 107.5 µg/ml of DPBS) was added to a
pellet of C. albicans hydrophilic yeast cells (5 × 106) that were prewashed with cold DPBS three times. The
yeast cells were suspended in the antibody solution and incubated on
ice for 30 min. During the incubation, the suspension was mixed by
inverting the tube every 3 min. The yeast cells were washed with cold
DPBS three times, suspended in 200 µl of goat anti-mouse IgG
(
-chain specific; Sigma) (stock solution, 0.8 mg/ml; working
solution, 26.7 µg/ml of DPBS) and incubated on ice as described
above. After washing, the yeast cells were suspended in 500 µl of
fluorescein-labeled anti-goat IgG (heavy and light chains; 1:200
diluted in DPBS; Jackson ImmunoResearch Lab, West Grove, Pa.) and
incubated on ice for 20 min. The yeast cells were washed and suspended
in 200 µl of cold DPBS. The cells were observed by fluorescence and
phase-contrast microscopy (model Labophot, series no. 234142; Nikon,
Tokyo, Japan). The distribution of the C3.1 epitope on the yeast cell
surface was compared to that obtained with yeast cells fluorescently
stained for detection of the B6.1 epitope as described previously
(13).
Protection against Candida infections by passive transfer. MAbs C3.1 and B6.1 were used without pretreatment, pretreated at 56°C for 30 min before use, or absorbed with C. albicans yeast cells (11, 14, 15). Untreated and treated MAbs C3.1 and B6.1 were compared for the ability to protect mice against experimental disseminated candidiasis and Candida vaginal infection as previously described (11, 12, 14, 15) with one modification. Test animals were given antibody only before infection with C. albicans, rather than 4 h before and 20 h after infection. Specifically, for testing against disseminated candidiasis, the MAbs (0.5 ml) were given to mice by an i.p. route 4 h before the animals were infected by an i.v. route with yeast cells (5 × 105 per mouse). Forty-eight hours after antibody treatment, groups of animals were sacrificed and their kidneys were assessed for CFU as before (11, 12, 15). Other groups of mice were monitored for determination of mean survival times.
For testing against vaginal infection, each mouse was pretreated with 0.5 mg of estradiol (Sigma) subcutaneously. Seventy-two hours later, these mice received MAb C3.1 by an i.p. (0.5 ml/mouse) or intravaginal (i.vg.; 10 µl/mouse) route. Four hours later, the animals were infected i.vg. with yeast cells (5 × 105 per mouse in a 10-µl volume); 48 h after infection, vaginal CFU were enumerated as previously described (14). The protective effect of MAb B6.1 given i.p. was previously tested in the mouse vaginal infection model (14), but in the present study this antibody was tested only by the i.vg. route at a dose of 10 µl/mouse.Statistical analyses. In all cases, the minimum number of animals per group was five, and each experiment was repeated at least three times. Statistical significance of differences of survival times was measured by use of the Kaplan-Meier test (Systat 7.0; SPSS Inc., Chicago, Ill.). Survival experiments were terminated at day 27. For calculation of mean survival time, survivors were assigned a survival time of 27 days. For other analyses, Student's t test was used. P values were considered statistically significant if they were less than 0.05.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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MAb C3.1 is an IgG3. SDS-PAGE run under reducing conditions revealed molecular sizes of heavy and light chains of MAb C3.1 of approximately 50 and 27 kDa, respectively (gels not shown), the former of which is consistent with the expected size of an IgG heavy chain (2). Under identical electrophoretic conditions, MAb B6.1 produced heavy and light chains of 76 and 25 kDa, the former of which is consistent with the expected size of an IgM heavy chain.
Results of the capture ELISA and double immunodiffusion in agar showed that the isotype of MAb C3.1 is an IgG3. By ELISA, MAb C3.1 gave a color development of about 0.77 OD unit at 405 nm when interacted with anti-IgG3, whereas the OD was <0.02 following an interaction of MAb C3.1 with anti-IgM, anti-IgG1, anti-IgG2a, anti-IgG2b, anti-IgA, and anti-IgE. The control antibody, MAb B6.1 (IgM), reacted specifically with anti-IgM (OD405 of approximately 1.0). Results obtained for MAb C3.1 were the same as those for the IgG3 MAb specific for a glucuronoxylomannan capsular epitope from C. neoformans. The double immunodiffusion (gels not shown) was confirmatory in that visible precipitin bands occurred between the well containing MAb C3.1 and peripheral wells containing whole anti-IgG and anti-IgG3 but not with the peripheral well containing anti-IgM. The pooled mouse IgG control produced obvious precipitin bands with whole anti-IgG, anti-IgG1, and anti-IgG2b but not with anti-IgM.Identification of the MAb C3.1 epitope.
For isolation of the
epitope recognized by MAb C3.1 (i.e., the C3.1 epitope), the same PMC
preparation was used in these studies as in those for identification of
the B6.1 epitope (13). That is, the PMC was hydrolyzed in 10 mM HCl to release the acid-labile oligomannosyl residues from the
remaining acid-stable part. The resulting oligomannosyl residues were
separated on a P-2 column. The column resolved four acid-stable
fractions and seven oligomannosyl acid-labile peaks (fractions I to
VII). Acid-labile fractions III and IV inhibited agglutination of
mannan-coated latex beads (Table 1),
whereas none of the other acid-labile moieties or the acid-stable part
of the PMC inhibited agglutination. Likewise, raffinose (triose) and
stachyose (tetraose) did not affect the agglutination (Table 1). These
results are identical to those obtained on studies of the epitope
recognized by MAb B6.1, indicating that MAb C3.1 is also specific for
-1,2-mannotriose.
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Cell surface distribution of the C3.1.
Immunofluorescence
microscopy was used to approximate the cell surface distribution
pattern of the C3.1 epitope. Stationary-phase yeast cells displayed a
uniform distribution of epitope over the entire cell surface of
C. albicans (Fig. 1). This
distribution was essentially identical to the distribution of the B6.1
epitope (13). Comparing yeast cells observed by bright-field
microscopy with those that fluoresced showed that some yeast cells and
all of the blastoconidia were nonreactive with MAb C3.1. These results are also identical to those with MAb B6.1.
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MAb C3.1 transfers protection against disseminated
candidiasis.
BALB/c mice were given unheated MAb C3.1 (C3.1), MAb
C3.1 heated at 56°C for 30 min (H-C3.1), C. albicans-absorbed MAb C3.1 (A-C3.1), or DPBS (buffer diluent) by
an i.p. route and were then infected with viable yeast cells i.v. (Fig.
2A). In other experiments, mice were
given C3.1, MAb B6.1, or DPBS to compare the prophylactic potentials of
the two MAbs (Fig. 2B). Susceptibility to disseminated disease was
assessed by determining kidney CFU (Fig. 2A) and by survival curves
(Fig. 2B). The mean CFU values (105) per gram of
kidney ± standard error for mice given C3.1, H-C3.1, or A-C3.1,
and DPBS were 30 ± 6, 25 ± 6, 200 ± 50, and 210 ± 25. That is, mice that received either C3.1 or H-C3.1 had 86 and
88% fewer CFU, respectively, than control mice that received DPBS (P < 0.001). Mice that were given the A-C3.1 developed
almost the same number of CFU as the control animals. Analyses of mean survival times (Fig. 2B) showed that mice given C3.1 had extended survival times similar to those for animals given MAb B6.1. These survival times were significantly longer than those for animals given
DPBS (P < 0.05).
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MAb C3.1 has a prophylactic effect against Candida
vaginal infection.
Pseudoestrus mice were given MAb C3.1 i.p. or
i.vg. before an i.vg. infection with 5 × 105 yeast
cells (Fig. 3). Vaginal CFU counts were
compared with CFU from animals that were given unheated C3.1, H-C3.1,
A-C3.1, or DPBS (diluent). Mice that received MAb C3.1 or H-C3.1 i.p.
developed 60 and 49% fewer CFU, respectively, than DPBS control mice.
Mice that received A-C3.1 developed CFU to levels similar to those for
control mice that received DPBS i.vg. prior to infection (Fig. 3A).
Mice that received either C3.1, H-C3.1, or MAb B6.1 developed approximately 86% fewer CFU than DPBS control mice (Fig. 3B). The
differences between antibody-treated mice and DPBS controls were
significant (P < 0.05), whereas mice that received
A-C3.1 developed approximately the same number of vaginal CFU as the DPBS-treated mice.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The hybridoma cell line that produces MAb C3.1 was obtained from the splenocyte-myeloma fusion that yielded the IgM MAb B6.1-producing cell line (11). At that time, the C3.1 hybridoma was cloned twice by limiting dilution, the isotype class was determined as an IgG (unpublished data), and the clone was stored in liquid nitrogen. Interest in the C3.1 clone peaked with current speculation on mechanisms by which MAb B6.1 protects experimental animals against both hematogenously disseminated candidiasis and vaginal infection. In work on the IgM antimannan MAbs B6.1 and B6, we clearly established that antibody specificity is a critical criterion for consideration of a protective antibody against candidiasis (11, 13, 14).
Based on suggestive evidence that MAb B6.1 was found to enhance neutrophil candidacidal activity only in the presence of complement (4) and other unpublished observations, we have hypothesized that rapid complement activation is critical to the protective activity by the antibody. A prediction based on this hypothesis is that an IgG3 antibody, which is also a potent activator of complement (21), should be protective. The purpose of this report was to establish the rationale for using MAb C3.1 to extend our knowledge of mechanisms by which antibodies protect against candidiasis. These studies necessitated establishing the identity of the isotype subclass of MAb C3.1, comparing its specificity with that of MAb B6.1, and testing MAb C3.1 for protective activities.
By different measures, the subtype of MAb C3.1 was unequivocally an
IgG3. SDS-PAGE analysis gave a heavy-chain molecular size consistent
with that reported for an IgG molecule (2). The IgG3
subclass was established by similar results obtained through a capture
ELISA and by an Ouchterlony double-diffusion test. Both analyses showed
that the C3.1 hybridoma clone produced immune globulin reactive with
antibody specific for the 3 heavy chain but not with antibodies that
recognize other IgG subtypes or other Ig isotypes. These results were
not surprising. The splenocytes used in the fusion that yielded the
C3.1 clone were obtained from animals immunized against a cell wall
extract rich in PMC (11). Although the subclass isotype of
MAb C3.1 was not previously determined, an IgG3 would be expected
because this may be the predominant IgG subclass produced by mice in
response to polysaccharide antigens (5, 10, 20).
A strategy similar to that used for identification of the B6.1 epitope
was used for identification of C3.1 specificity. The basis of this
analysis is that the PMC is composed of 
- and -mannan (24), the latter of which is phosphodiester linked to the
former. The phosphodiester bond is readily hydrolyzed by 10 mM HCl,
which results in release of the -oligomannosyl chains from the
-mannan. The -oligomannosyl chains are of varying lengths based
on the number of mannose units of each, but -1,2-glycosidic bonds
connect all of the mannose units regardless of length. Because these
chains are readily released from the PMC by acid hydrolysis, these
-1,2-linked oligomannosyl residues are referred to as acid-labile
parts of the complex; the -mannan is called the acid-stable part
(17, 22). Following acid hydrolysis, each part of the PMC
and the various -1,2-linked oligomannosyl residues may be separated
by size exclusion column chromatography. In previous work, mass
spectroscopy was used to confirm the molecular mass and purity of each
of the column fractions (13). The various parts of the
complex may be tested for reactivity with antibodies by mixing each of
the column fractions with antibody and determining which prevents the
antibody from agglutinating latex beads coated with nonhydrolyzed phosphomannan. By this approach, the B6.1 epitope was defined as an
acid-labile component composed specifically of a -1,2-mannotriose (13). By an identical analysis, we determined that this is
the same oligomannoside that is recognized by MAb C3.1. As suggestive confirmatory evidence, we tested the C3.1 epitope distribution on the
surface of C. albicans. Our expectation was that the
distribution should be uniform as with the B6.1 epitope, rather than
punctate and patchy as with the B6 epitope (13). By the same
immunofluorescence analysis that was used for distribution studies of
the B6.1 and B6 epitopes, we found that the C3.1 epitope distribution
is identical to that of the B6.1 epitope display on the yeast cell
surface. By these various findings, we concluded that MAb C3.1 is an
IgG3 and the antibody is specific for the same oligomannoside as MAb B6.1. MAb C3.1 was then tested for its ability to protect mice against
candidiasis to determine whether an IgM isotype (i.e., MAb B6.1) is
required for this activity.
The preventive or prophylactic activity of MAb C3.1 against disseminated candidiasis was compared to that of MAb B6.1. The concentrations of each antibody were standardized on the basis of agglutination titer and previous dose response information from other studies (12, 14). A significant departure from these studies compared to our previous work is that a single dose of either antibody was given i.p. 4 h before infection with live C. albicans yeast cells, rather than one dose 4 h before infection and another 24 h after the first dose (11, 14). Based on mean survival times, both antibodies showed similar protective activities. As with MAb B6.1, MAb C3.1 protective activity was resistant to pretreatment at 56°C, but the activity was removed by preabsorption with yeast cells. Both of these characteristics are consistent with antibody properties and tend to rule out nonspecific protective factors that might be present in the antibody preparations.
In addition to enhancing protection against hematogenously disseminated candidiasis, MAb B6.1 was previously shown to enhance resistance against vaginal infection in mice (14). For effective results, the antibody could be given either i.p., as above in the disseminated candidiasis studies, or i.vg. 4 h before infection. By use of the same concentration of MAb C3.1 as was used in the disseminated disease studies involving this antibody, significant protective effects were observed when MAb C3.1 was given either i.p. or i.vg. prior to a vaginal infection with viable yeast cells.
Our results show that experimental animals can be protected against
candidiasis by antibodies with specificity for a -1,2-mannotriose, but the protective antibody may be either an IgM or an IgG3. Since interleukin-12 administration to mice causes enhanced IgG3 responses to
antigens presented in the presence of alum (9), it will be
interesting to examine the efficacy of our mannan-protein vaccine (15) administered as an alum preparation to mice given
multiple doses of the cytokine.
Our finding that an IgG3 antibody is protective is in contrast to the reported findings that an IgG1 but not an IgG3 MAb protects against cryptococcosis (25, 26). In addition, protective and nonprotective IgG3 MAbs have been described in studies on experimental rickettsial (1) and Pseudomonas aeruginosa infections (3). Obviously, the key consideration is the underlying mechanism of protection. In our work, an IgG3 protective response is consistent with our findings and hypothesis that complement activation may be involved in the mechanism of resistance against disseminated disease. Regardless of the mechanism, the immediate implication of these findings is that it should be possible to develop an immunization protocol that leads to memory B-cell responses and long-term immunity against various forms of candidiasis.
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ACKNOWLEDGMENTS |
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The technical assistance of Soo Kyung Han and Sheila E. Beery is gratefully acknowledged.
This work was supported by grants RO1 AI24912 and PO1 AI37194 from the National Institute of Allergy and Infectious Diseases.
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FOOTNOTES |
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* Corresponding author. Mailing address: Montana State University, Department of Microbiology, Lewis Hall 109, Bozeman, MT 59717-3520. Phone: (406) 994-2373. Fax: (406) 994-4926. E-mail: umbic{at}montana.edu.
Editor: T. R. Kozel
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Infection and Immunity, March 2000, p. 1649-1654, Vol. 68, No. 3
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Copyright © 2000, American Society for Microbiology. All rights reserved.
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