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Infection and Immunity, December 1998, p. 6027-6029, Vol. 66, No. 12
Department of Microbiology and the Cell and
Molecular Biology Program, School of Medicine, University of Nevada,
Reno, Nevada 89557,1 and
Department of
Microbiology, Montana State University, Bozeman, Montana
597172
Received 29 June 1998/Returned for modification 12 August
1998/Accepted 17 September 1998
Polyclonal antimannan immunoglobulin G (IgG) activates the
classical complement pathway and accelerates initiation of the alternative pathway by Canidida albicans. This dual role
was assessed for two antimannan IgM monoclonal antibodies (MAbs). MAb
B6.1 is specific for an epitope on the acid-labile portion of C. albicans phosphomannan; MAb B6 is specific for an epitope on the
acid-stable region. Both MAbs were potent activators of the classical
pathway but poor facilitators of alternative pathway initiation.
Candida albicans
activates the human complement system via both the classical and the
alternative pathways, leading to deposition of opsonic complement
fragments on the yeast cell surface (8, 10, 18). In previous
studies, we described a critical role for naturally occurring
antimannan immunoglobulin G (IgG) in complement activation by C. albicans. Those studies used a kinetic assay for C3 deposition on
the yeast and immunofluorescence evaluation of the sites of C3 binding
(10, 17, 18). Deposition of C3 onto C. albicans
cells incubated in normal human serum (NHS) occurs rapidly via the
classical pathway and can be detected within the first 2 min of
incubation. If the classical pathway is blocked by chelation of
Ca2+ with EGTA, C3 deposition occurs via the alternative
pathway, but C3 deposition is delayed and a 6-min incubation is
required before bound C3 is readily detectable on the yeast surface.
Removal of naturally occurring antimannan IgG from the serum by mannan absorption profoundly delays accumulation of C3 on the yeast cell surface, with 12 min or more of incubation being required before appreciable amounts of bound C3 are detected. However, this 12-min delay can be overcome by supplementation of the mannan-absorbed serum
with affinity-purified human antimannan IgG in the absence of EGTA to
mediate classical pathway initiation or shortened to 6 min in the
presence of EGTA to allow antibody-facilitated activation of the
alternative pathway. These observations demonstrate a dual role for
antimannan IgG in serum from healthy adults in complement activation by
C. albicans. Antimannan IgG mediates activation of the
classical pathway and facilitates initiation of the alternative pathway
(17, 18).
In studies described above, we used polyclonal antimannan IgG purified
from pooled human plasma. Since C. albicans cells express a
number of immunodominant mannan components recognized by rabbits (15, 16), the human polyclonal antimannan IgG likely
contains a range of specificities for distinct mannan determinants. It has been shown that rabbit antibodies that are reactive with three different cell wall determinants of group A streptococci display differential abilities to activate the classical or alternative pathway
(2). Although the antibodies specific for three different cell wall epitopes all activated the classical pathway, only antibody specific for the N-acetyl-D-glucosamine epitope
activated the alternative pathway (2). In a separate study,
capsular as well as noncapsular antibodies were found to direct
classical-pathway-mediated killing of Haemophilus influenzae
type b, whereas only the capsular antibodies promoted killing by the
alternative pathway (12). These studies provide evidence
that epitope specificity may influence the ability of an antibody to
activate the alternative pathway and prompted us to examine whether
antibodies that recognize different mannan determinants are able to
mediate activation of the classical and alternative pathways by
C. albicans.
Two IgM monoclonal antibodies (MAbs) that recognize distinct mannan
determinants were compared for their abilities to activate the
classical or alternative pathway. MAb B6.1 is specific for an
acid-labile component of the Candida phosphomannan complex, and MAb B6 is specific for an acid-stable component (5). The MAbs were produced commercially (Montana ImmunoTech, Inc., Bozeman, Mont.).
C. albicans CA-1 was grown as yeast forms to stationary
phase in glucose (2%)-yeast extract (0.3%)-peptone (1%) broth for 24 h at 37°C as described elsewhere (4, 6, 10). The
mannan of CA-1 yeast was purified as described previously (7,
18) and coupled to CNBr-Sepahrose 4B (Pharmacia Biotech, Uppsala, Sweden) (18).
Pooled NHS was prepared from peripheral blood from at least 10 healthy
adult donors and stored at Kinetics of C3 binding were assayed by the method of Kozel et al.
(10). To determine whether MAb B6 or B6.1 activates the classical pathway, 2 × 106 yeast cells were incubated
at 37°C in 1 ml of a complement binding medium that contained (i)
40% NHS, mannan-absorbed serum, or mannan-absorbed serum supplemented
with MAb B6 or B6.1, (ii) sodium Veronal (5 mM)-buffered saline (142 mM, pH 7.3) containing 0.1% gelatin, 1.5 mM CaCl2, and 1 mM MgCl2, and (iii) 125I-labeled C3. To study
whether MAb B6 or B6.1 plays a role in alternative pathway initiation,
yeast cells were incubated in the manner described above except that
the binding medium was not supplemented with Ca2+ and
contained 5 mM EGTA and 5 mM MgCl2. At various time
intervals from 2 to 16 min, 50-µl samples were withdrawn in duplicate
and added to 200 µl of phosphate-buffered saline-0.1% sodium
dodecyl sulfate-20 mM EDTA in Millipore MABX-N12 filter plates fitted with BV 1.2-µm-pore-size filter membranes (Millipore, Bedford, Mass.). The cells were washed with phosphate-buffered saline-0.1% sodium dodecyl sulfate, and filter-bound radioactivity was determined with a gamma counter. Nonspecific binding was estimated from cells incubated in NHS containing EDTA and was subtracted from the total counts.
Mannan absorption of serum profoundly delayed C3 accumulation on yeast
from 2 min to approximately 10 min (Fig. 1 and
2). However, addition of either MAb B6 or MAb B6.1 at 50 µg per ml of
reaction mixture to the absorbed serum generated rapid activation kinetics characteristic of C3 deposition via the classical pathway (Fig. 1) (10, 17, 18). This observation was not unexpected, as polyvalent IgM is known to be a potent activator of the classical pathway.
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Contrasting Roles of Mannan-Specific Monoclonal
Immunoglobulin M Antibodies in the Activation of Classical and
Alternative Pathways by Candida albicans
ABSTRACT
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80°C. C3 was isolated from frozen human
plasma (9, 13) and stored at 80°C until used. C3 was
labeled with 125I as described previously (3) by
use of IODO-GEN reagent (Pierce, Rockford, Ill.). NHS was absorbed with
mannan-Sepharose 4B to remove antimannan antibodies (18).
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FIG. 1.
Effect of MAb B6 or B6.1 on the kinetics of C3
deposition on C. albicans cells via the classical pathway.
Yeast cells were incubated in a C3 binding medium containing (i) 40%
NHS ( 
), (ii) 40% mannan-absorbed NHS (
), (iii) 40%
mannan-absorbed NHS supplemented with MAb B6 (
), or (iv) 40%
mannan-absorbed NHS supplemented with MAb B6.1 (
) at 50 µg per ml
of reaction mixture. C3 deposition patterns from three independent
assays were similar; results from one representative assay are shown.
View larger version (26K):
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FIG. 2.
Effect of MAb B6 or B6.1 on the kinetics of C3
deposition on C. albicans cells via the alternative pathway.
Yeast cells were incubated in a C3 binding medium containing (i) 40%
NHS ( ), (ii) 40% NHS-EGTA (
), (iii) 40% mannan-absorbed NHS
containing EGTA (), (vi) 40% mannan-absorbed NHS containing EGTA
supplemented with MAb B6 (), or (iv) 40% mannan-absorbed NHS
supplemented with MAb B6.1 () at 50 µg per ml of reaction mixture.
C3 deposition patterns from four independent assays were similar;
results from one representative assay are shown.
The effects of MAbs B6 and B6.1 on activation of the alternative pathway were assessed by addition of the antibodies to mannan-absorbed serum in the presence of EGTA. The results (Fig. 2) showed that neither MAb B6 nor MAb B6.1 at 50 µg per ml of reaction mixture altered the alternative pathway activity of the mannan-absorbed serum. To determine whether the inability of MAb B6 or B6.1 to facilitate initiation of the alternative pathway was influenced by antibody concentration, the experiment represented in Fig. 2 was repeated with mannan-absorbed serum that was supplemented with 10 to 160 µg of MAb B6 or B6.1 per ml. These antibody concentrations were chosen because in our previous studies we found that affinity-purified human antimannan IgG activates both the classical and alternative pathways (17). However, at 10, 40, or 160 µg per ml of reaction mixture, both antibodies failed to enhance alternative pathway activity of mannan-absorbed serum but promoted classical pathway activity (data not shown).
The observation that both MAbs were unable to enhance alternative pathway activity was unexpected. Our previous studies showed that addition of polyclonal antimannan IgG to mannan-absorbed NHS containing EGTA produced C3 binding kinetics that were indistinguishable from the kinetics observed with nonabsorbed NHS containing EGTA (17). We further demonstrated IgG-dependent initiation of the alternative pathway by C. albicans using the six purified alternative pathway proteins (17).
There are at least three possible explanations for the failure of MAbs B6 and B6.1 to facilitate activation of the alternative pathway. First, it is possible that antimannan antibodies of the IgM class are unable to enhance C3 deposition via the alternative pathway. However, there is evidence that polyclonal IgM is able to enhance alternative pathway-mediated lysis of rabbit erythrocytes by NHS (11, 14). Second, the ability of an antibody to facilitate deposition of C3 via the alternative pathway could be epitope specific; MAbs B6 and B6.1 could have the wrong epitope specificity. As noted above, Eisenberg and Schwab (2) found that polyclonal antibodies specific for one antigen found on group A streptococcal cell walls were able to facilitate initiation of the alternative pathway, whereas antibodies specific for two other antigens were not. If antibody-facilitated activation of the alternative pathway is dependent on epitope specificity, such a finding might influence strategies for induction of protective immunity to Candida. Optimal immunization may require an immunogen that induces antibodies with epitope specificities needed to facilitate activation of the alternative pathway. Finally, we cannot exclude the possibility that human antimannan antibodies are able to facilitate activation of the alternative pathway, whereas mouse antibodies lack this capability.
In studies involving a murine model of disseminated candidiasis, MAb B6.1 was shown to be protective, whereas MAb B6 was not (4). However, the protection mechanisms remain to be elucidated. In an in vitro assay, MAb B6.1 but not MAb B6 was found to enhance candidacidal activity of polymorphonuclear leukocytes in the presence of fresh mouse serum, suggesting the involvement of mouse complement in the killing (1). Although assessing the role of complement in MAb B6.1-mediated protection was beyond the scope of this study, our observation that the two antibodies mediate similar kinetics of C3 deposition for C. albicans does not preclude the possibility that the composition and/or accessibility of opsonic complement fragments bound to the yeast cells might differ following complement activation by these two antibodies. Alternatively, the concerted action of several protective functions, including activation of the complement system, may be required for MAb B6.1-mediated protection.
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ACKNOWLEDGMENTS |
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This work was supported in part by National Institutes of Health grants AI 14209, AI 37194, and AI 24912.
We thank Kevin Wall for technical assistance.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology, School of Medicine, University of Nevada, Reno, NV 89557. Phone: (702) 784-6161. Fax: (702) 784-1620. E-mail: mzhang{at}med.unr.edu.
Editor: V. A. Fischetti
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