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Infection and Immunity, March 1999, p. 1317-1322, Vol. 67, No. 3
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Cryptosporidium parvum Sporozoite
Pellicle Antigen Recognized by a Neutralizing Monoclonal Antibody Is a
-Mannosylated Glycolipid
Michael W.
Riggs,1,*
Michael R.
McNeil,2
Lance E.
Perryman,3
Alice L.
Stone,1
Michael S.
Scherman,2 and
Roberta
M.
O'Connor4
Department of Veterinary Science and
Microbiology, University of Arizona, Tucson, Arizona
857211; Department of Microbiology,
Colorado State University, Fort Collins, Colorado
805232; Department of Microbiology,
Pathology, and Parasitology, North Carolina State University,
Raleigh, North Carolina 276063; and
Department of Pathobiology, University of Florida,
Gainesville, Florida 326114
Received 1 October 1998/Returned for modification 6 December
1998/Accepted 21 December 1998
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ABSTRACT |
The protozoan parasite Cryptosporidium parvum is an
important cause of diarrhea in humans, calves, and other mammals
worldwide. No approved vaccines or parasite-specific drugs are
currently available for the control of cryptosporidiosis. To
effectively immunize against C. parvum, identification and
characterization of protective antigens are required. We previously
identified CPS-500, a conserved, neutralization-sensitive antigen of
C. parvum sporozoites and merozoites defined by monoclonal
antibody 18.44. In the present study, the biochemical characteristics
and subcellular location of CPS-500 were determined. CPS-500 was
chloroform extractable and eluted with acetone and methanol in silicic
acid chromatography, consistent with being a polar glycolipid.
Following chloroform extraction and silicic acid chromatography,
CPS-500 was isolated by high-pressure liquid chromatography for
glycosyl analysis, which indicated the presence of mannose and
inositol. To identify which component of CPS-500 comprised the
neutralization-sensitive epitope recognized by 18.44, the ability of
the monoclonal antibody to bind CPS-500 treated with proteases, or with
- or 
-glycosidases, was determined. Monoclonal antibody 18.44 did
not bind antigen treated with -D-mannosidase but did
bind antigen treated with -D-mannosidase, other - or
-glycosidases, or a panel of proteases. These data indicated that
the target epitope was dependent on terminal
-D-mannopyranosyl residues. By immunoelectron
microscopy, 18.44 binding was localized to the pellicle and an
intracytoplasmic tubulovesicular network in sporozoites. Monoclonal
antibody 18.44 also bound to antigen deposited and released onto
substrate over the course travelled by gliding sporozoites and
merozoites. Surface localization, adhesion and release during
locomotion, and neutralization sensitivity suggest that CPS-500 may be
involved in motility and invasion processes of the infective zoite stages.
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INTRODUCTION |
Cryptosporidium parvum is
an apicomplexan parasite that causes the diarrheal disease
cryptosporidiosis in humans and economically important food animals
throughout the world (10, 34). Despite progress, prevention
and treatment of the disease remain limited by the absence of approved
vaccines or immunotherapies and by the lack of safe and effective
parasite-specific drugs (6, 24). Because C. parvum infection is controlled by normal immune responses,
immunologic strategies for prevention and treatment are being
investigated (reviewed in reference 24). Central to such investigations is the structural and functional characterization of candidate target antigens.
Apical organelle and surface-exposed molecules of apicomplexan
parasites are involved in the pathogenesis of infection and present
rational targets for immunologic intervention (18, 28, 29).
We previously reported that monoclonal antibody (MAb) 18.44, prepared
against whole C. parvum, binds to sporozoites and merozoites and neutralizes their infectivity in a time-dependent manner (5, 21, 26). The antigen defined by MAb 18.44 has been designated CPS-500. Because this antigen is expressed in both infective life cycle
stages, contains one or more neutralization-sensitive epitopes, and is
conserved among geographically diverse human and bovine C. parvum isolates (33), it likely has an important
biological role. Therefore, CPS-500 is a candidate target antigen for
active or passive immunization against cryptosporidiosis. In initial experiments to characterize the antigen, CPS-500 migrated with the dye
front in sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), eluted in the void volume of a Bio-Gel-A column with an
exclusion limit of 500 kDa, was not radiolabelled by biosynthetic incorporation of [35S]methionine, and did not contain
iodinatable tyrosine residues (26). In addition, preparative
electrophoresis-isolated CPS-500 was weakly immunogenic in mice,
rabbits, and hens immunized for preparation of MAbs or polyclonal
antibodies (23). These observations, taken together,
suggested that CPS-500 was nonproteinaceous, thereby complicating
recombinant approaches for its production and characterization. For
these reasons, experiments to biochemically characterize CPS-500 and
the target epitope recognized by MAb 18.44 were performed. In the
present study, CPS-500 was classified as a polar glycolipid based on
its chloroform extractability and elution properties in silicic acid
chromatography. Most importantly, it was determined that the
neutralization-sensitive epitope recognized by MAb 18.44 is dependent
on terminal -D-mannopyranosyl residues based on -D-mannosidase susceptibility, an observation consistent
with the identification of mannose by glycosyl analysis of
high-pressure liquid chromatography (HPLC)-isolated CPS-500. A possible
function for CPS-500 in the motility of the infective stages is
suggested by its immunoelectron microscopic localization to the
sporozoite pellicle and its deposition on substrate by viable
sporozoites and merozoites during locomotion. We conclude that CPS-500
is a candidate molecular target for immunologic control of
cryptosporidiosis. While its glycolipid composition may preclude
standard recombinant approaches for subunit production, chemical
synthesis of the target epitope or anti-idiotypic antibody approaches
may lead to CPS-500-based vaccines for cryptosporidiosis.
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MATERIALS AND METHODS |
Oocyst, sporozoite, and merozoite isolation.
The Iowa
C. parvum isolate (13), used for all experiments,
was passaged bimonthly in newborn Cryptosporidium-free
Holstein calves to obtain parasite material (27). Oocysts
were separated from calf feces by sucrose density gradient
centrifugation and stored in 2.5% KCr2O7
(4°C) for up to 2 months prior to use (3). Oocysts were
treated with hypochlorite prior to excystation, after which sporozoites
were isolated by anion-exchange chromatography (27).
Merozoites were isolated by Percoll density gradient centrifugation of
intestinal contents from neonatal BALB/c mice at 65 h post-oocyst inoculation as previously described (25).
CPS-500 isolation.
In initial experiments to isolate
CPS-500, MAb 18.44-affinity chromatography using CNBr-activated
Sepharose, hydrazide Fc linkage matrix, or matrix with
carbon chain spacers was unsuccessful (data not shown).
Chloroform-methanol extraction of whole C. parvum was then
performed to isolate the lipid fraction (7). Prior to
extraction, oocysts (1.1 × 109) were excysted, then
solubilized in lysis buffer (50 mM Tris, 5 mM EDTA, 5 mM iodoacetamide,
0.1 mM N-p-tosyl-L-lysine chloromethyl ketone
[TLCK], 1 mM phenylmethylsulfonyl fluoride [PMSF], 0.01 mM
leupeptin, 0.01 mM pepstatin A) by five rapid freeze-thaw cycles and
sonication (4°C) (25). All glassware used in the
subsequent extraction procedure was pretreated with concentrated HCl
(12 M), rinsed with distilled water (dH2O), cleaned in
PCC-54 detergent (50°C) (Pierce, Rockford, Ill.), rinsed with
dH2O, dried (100°C), and siliconized. Standard measures
to prevent contamination or degradation of lipids were implemented
during all stages of extraction and storage (15). Following
solubilization, the excysted oocyst preparation (4 volumes) was
combined with glass-distilled chloroform (5 volumes) and methanol (10 volumes) (Burdick & Jackson, Muskegon, Mich.) to form a monophasic
solution. After vortexing (30 min at 21°C), chloroform (5 volumes)
and deionized water (5 volumes) (NANOpure; Barnstead, Dubuque, Iowa)
were added to the monophasic solution (19 volumes) to form a diphasic
solution. The diphasic solution was vortexed (for 30 min at 21°C) and
then centrifuged (at 2,250 × g), after which the
chloroform phase was collected. The methanol-water phase was
back-extracted twice with chloroform, and the fractions were collected.
Chloroform-extracted fractions and methanol-water fractions were
filtered (Teflon membrane; 0.2-µm pore size; Nalge-Nunc, Rochester,
N.Y.), dried under N2 (final volume, 0.5 ml), and stored at
80°C prior to analysis. To determine which fraction(s) contained
CPS-500, samples of each were examined by dot immunoblot assay
(33). In brief, samples were dotted onto nitrocellulose,
incubated with MAb 18.44 immunoglobulin G3 (IgG3) or an isotype-matched
control MAb of irrelevant specificity (each at 4 µg
ml
1), washed, and incubated with affinity-purified
alkaline phosphatase-conjugated rabbit anti-mouse IgG3 (Zymed, South
San Francisco, Calif.) followed by substrate. To determine the
(glyco)protein content of each fraction, samples were resolved in 10 to
20% gradient SDS-PAGE gels under reducing conditions and were silver
stained (Bio-Rad, Hercules, Calif.) (28). Molecular weight
standards (Bio-Rad) included myosin (200 kDa), phosphorylase B (97.4 kDa), bovine serum albumin (BSA) (66.2 kDa), ovalbumin (45 kDa),
carbonic anhydrase (31 kDa), and soybean trypsin inhibitor (21.5 kDa).
Following identification of CPS-500 in the chloroform-extracted
fraction, the extract (0.5 ml) was applied to a chloroform-equilibrated 9- by 45-mm BioSil-A silicic acid (Bio-Rad) column, which was then
sequentially eluted with chloroform (7 column volumes), acetone (28 column volumes), and methanol (7 column volumes) (15).
Eluate fractions were examined for the presence of CPS-500 by dot
immunoblot assay as described above. Fractions containing CPS-500 were
combined, dried under N2 (final volume, 0.5 ml), and stored
at 80°C prior to use. To determine the (glyco)protein content in
the combined CPS-500 fractions, samples were resolved in SDS-PAGE and
silver stained as described above.
Silicic acid column-isolated CPS-500 was further purified by HPLC as
follows (
15). A mixture of chloroform (2 parts) and
methanol
(1 part) was added to N
2-dried CPS-500 obtained from
2.6 × 10
9 excysted oocysts, and the preparation was
then injected onto
an HPLC (Beckman, Fullerton, Calif.) with a 250- by
7-mm Econosil
silica column (10-µm bead size; Alltech Scientific,
Deerfield,
Ill.). Solvent A was HPLC-grade chloroform, and solvent B
was
anhydrous methanol (flow rate, 2 ml/min). After an initial 2 min
at
0% B, a linear gradient was started, resulting in 100% B at
30 min.
Twenty fractions (2 ml each) were collected into anhydrous
methanol-cleaned glass tubes over a 40-min elution period. Aliquots
(100 µl) of each fraction were dried under N
2,
reconstituted in
phosphate-buffered saline (PBS) containing 0.1%
(wt/vol) SDS,
sonicated (4°C), and examined for CPS-500 by a dot
immunoblot
assay as described above. Fraction 16 reacted strongly with
MAb
18.44 and was used for glycosyl analysis (described
below).
Epitope characterization.
The ability of MAb 18.44 to bind
CPS-500 treated with proteases (Sigma, St. Louis, Mo.), sodium
periodate, or glycosidases was determined by a dot immunoblot assay as
described above. For pepsin, trypsin, or papain treatment, purified
sporozoites (7.5 × 107; 95 µg of protein
[bicinchoninic acid assay; Pierce]) were solubilized (in 100 µl of
PBS containing 0.5% [wt/vol] SDS and 0.5% [wt/vol] octylglucoside) and incubated with pepsin (0.85 U/µg of sporozoite protein for 1 h at 38°C; pH 4.7), trypsin (3.4 U/µg of
sporozoite protein for 12 h at 38°C; pH 7.6), or papain (2.1 U/µg of sporozoite protein, with 0.05% [wt/vol] cysteine, for
12 h at 25°C; pH 6.2). Sporozoites were also solubilized in
borate buffer (0.1 M sodium borate, 0.03% [wt/vol]
CaCl2, 0.5% [wt/vol] SDS, 0.5% [wt/vol] octylglucoside) and incubated with pronase (0.001 U/µg of sporozoite protein, for 12 h at 38°C; pH 7.0), or they were solubilized in TNE buffer (0.01 M Tris, 0.1 M NaCl, 0.001 M EDTA, 0.5% [wt/vol] SDS, 0.5% [wt/vol] octylglucoside) and incubated with proteinase K
(0.004 U/µg of sporozoite protein, for 1 h at 50°C; pH 7.0). For each treatment, control sporozoite protein was incubated
identically in buffer lacking protease. Following incubation, protease
inhibitors (1.0 mM PMSF and 0.1 mM TLCK) were added to each
preparation. For periodate treatment, silicic acid column-isolated
CPS-500 (from 5 × 107 excysted oocysts/treatment) was
reconstituted in PBS containing 0.1% (wt/vol) SDS, dotted onto
nitrocellulose, and incubated with sodium periodate (1 to 10 mM) or
control buffer lacking periodate (36). For glycosidase
treatment, silicic acid column-isolated CPS-500 (from 107
excysted oocysts/treatment) was incubated (at 37°C for 12 h; pH
7.5) in PBS with or without a glycosidase preparation from Turbo
cornutus (final concentration, 25 mg ml1) (ICN,
Costa Mesa, Calif.) containing -L-fucosidase,
-xylosidase, - and -mannosidase, - and -glucosidase,
- and -galactosidase, - and
-N-acetylglucosaminidase, and - and
-N-acetylgalactosaminidase. Following observations that
MAb 18.44 did not bind CPS-500 after incubation with mixed glycosidases
from T. cornutus, treatments were repeated with component
glycosidases (Sigma) as follows. Silicic acid column-isolated CPS-500
(from 107 excysted oocysts/treatment) was incubated (at
37°C for 12 h) in buffer (50 mM sodium acetate, pH 4.5) with or
without (i) a combination of -D-mannosidase (1 U),
-D-galactosidase (0.1 U), -L-fucosidase
(0.01 U), and -D-glucosidase (1 U) or (ii) a combination of -D-mannosidase (0.5 U), -D-xylosidase
(0.05 U), and -D-glucosidase (1 U). Following
observations that MAb 18.44 bound to CPS-500 which had been treated
with the -glycosidase combination, but not with the -glycosidase
combination, treatments were repeated with component -glycosidases
as follows. Silicic acid column-isolated CPS-500 was incubated as
described above in buffer with or without -D-mannosidase
(0.5 U), -D-xylosidase (0.05 U), or
-D-glucosidase (1 U) to determine which enzyme altered
the epitope recognized by MAb 18.44.
Glycosyl analysis.
The glycosyl composition of whole
C. parvum (106 excysted oocysts) and
HPLC-isolated CPS-500 (fraction 16; 10% [vol/vol]) was determined by
methanolysis, re-N-acetylation, trimethysilation, and gas
chromatography-mass spectrometry (GC-MS) (model 5970; Hewlett-Packard,
Avondale, Pa.) (8). To minimize the introduction of any
contaminating sugars, reaction vessels (500-µl Reacti-Vials; Pierce)
were preconditioned (at 70°C for 3 h) with methanolic HCl (3 M;
0.5 ml) and methyl acetate (125 µl). Positive displacement glass
capillary tube pipettors and sterile Eppendorf pipettors were used for
all organic and aqueous reagents, respectively. Samples and standards
were derivatized as described elsewhere (8) except that
scyllo-inositol was used as the internal standard. GC-MS
detection and quantitation of derivatized samples was performed by
using the selective ion monitoring mode at m/z
204 (hexoses, pentoses, and 6-deoxyhexoses), 173 (N-acetyl
amino sugars), and 318 (inositols).
Electron microscopy.
To localize CPS-500 ultrastructurally,
sporozoites were examined by immunoelectron microscopy using MAb 18.44 as follows. Purified sporozoites (5 × 107) were
suspended (for 25 min at 4°C) in an isotonic phosphate-buffered fixative (40 mM NaH2PO4 · H2O-160 mM Na2HPO4 containing 2%
[wt/vol] formaldehyde, 0.5% [vol/vol] glutaraldehyde, and 1%
[wt/vol] tannic acid), washed with phosphate buffer, and centrifuged
(at 1,850 × g for 5 min) into agarose. The sample was
then dehydrated through a series of ethanol solutions (30 to 100%
ethanol) while the temperature was progressively lowered (4 to
20°C), and it was embedded (20°C) in LR White resin. Sections
were mounted on nickel grids, blocked (with 0.1% [vol/vol] Tween
20), incubated (for 30 min at 37°C) with protein A-purified MAb 18.44 or an isotype-matched control MAb (each at 50 µg ml1),
washed, incubated with affinity-purified rabbit anti-mouse IgG (Zymed),
washed, and incubated with affinity-purified colloidal gold-conjugated
goat anti-rabbit IgG (5 nm; electron microscopy grade; Zymed).
Following additional washing, sections were postfixed (4% [wt/vol]
formaldehyde-1% [vol/vol] glutaraldehyde) and stained with a
saturated solution of uranyl acetate. Samples were observed and
photographed with a Philips 420 transmission electron microscope at 80 kV.
Exoantigen characterization.
To determine if CPS-500 is an
exoantigen, two assays were performed. First, viable sporozoites or
merozoites in PBS containing 0.5% (wt/vol) BSA were applied to
poly-L-lysine-coated multiwell glass slides, incubated (at
37°C for 15 min), air dried, and gently heat fixed (4).
Slides were processed for an indirect immunofluorescence assay (IFA)
using MAb 18.44, the C. parvum P23-reactive MAb 7D10 (20), or isotype-matched control MAbs; then they were
examined by epifluorescence microscopy. In a second assay, viable
sporozoites (2 × 107 in Hank's balanced salt
solution) were incubated in suspension (under 10% CO2 for
1.5 h at 37°C), then centrifuged (at 5,000 × g
at 4°C for 30 min) to separate sporozoites and incubation medium.
Pelleted sporozoites were solubilized in lysis buffer containing 1%
(wt/vol) octylglucoside by freeze-thawing and sonication (4°C).
Following removal of insoluble material (at 100,000 × g at 4°C for 45 min), the soluble fractions from
sporozoites and incubation medium were examined for the presence of
CPS-500 by a dot immunoblot assay as described above.
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RESULTS |
CPS-500 is a chloroform-extractable glycolipid.
On the basis
of the inability to purify CPS-500 by MAb 18.44 affinity
chromatography, and of previous observations suggesting that the
molecule was nonproteinaceous (26), the lipid fraction from
whole C. parvum was extracted and examined. CPS-500 was
identified in chloroform extracts, but not in the methanol-water
fraction (Fig. 1). In silicic acid
chromatography of the chloroform extract, CPS-500 eluted in acetone and
methanol (Fig. 1), suggesting a polar glycolipid composition
(15). Chloroform-extracted, silicic acid
chromatography-isolated CPS-500 was relatively free of protein and glycoprotein contamination (Fig. 2)
and was considered appropriate for use in characterizing the epitope
recognized by MAb 18.44. The preparation was further purified by HPLC
to characterize the glycosyl composition of CPS-500. Glycosyl analysis
was first performed on excysted oocyst preparations to obtain general
knowledge of the sugar composition in whole C. parvum and
for comparison to that in HPLC-isolated CPS-500. A substantial amount
of N-acetylgalactosamine was identified in whole C. parvum (Table 1). Other sugars
expected in eucaryotic organisms were also identified (Table 1)
(35). In HPLC-isolated CPS-500 (fraction 16), mannose and
inositol (~1:1) were identified as the major sugars (Table 1). Small
amounts of glucose and galactose were also detected. In contrast to
whole C. parvum, no N-acetylgalactosamine was
identified.
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FIG. 1.
Dot immunoblot demonstrating chloroform extractability
and isolation of CPS-500 from whole C. parvum. Shown are an
excysted oocyst preparation before extraction (lanes 1 and 6),
chloroform (lanes 2 and 7) and methanol (lanes 3 and 8) extracts, and
chloroform extract following successive silicic acid chromatography
(lanes 4 and 9) and HPLC (lanes 5 and 10) isolation steps. Lanes 1 through 5 were probed with MAb 18.44, and lanes 6 through 10 were
probed with isotype control MAb. Serial twofold dilutions of each
preparation are dotted from top to bottom.
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FIG. 2.
Silver-stained SDS-PAGE gel of CPS-500 at successive
stages of isolation from whole C. parvum, demonstrating
relative freedom from protein and glycoprotein contamination. Shown are
an excysted oocyst preparation (5 × 106 oocysts)
prior to chloroform-methanol extraction (lane 2), the
methanol-water-extracted phase (lane 4), and the chloroform-extracted
phase before (lane 5) and after (lane 3) silicic acid chromatography.
Lane 1 was loaded with sample buffer to identify silver stain
artifacts.
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-D-Mannose comprises a neutralization-sensitive
CPS-500 epitope.
Treatment of solubilized sporozoites with
individual proteases did not affect the binding of MAb 18.44 to CPS-500
(data not shown). When CPS-500 was treated with periodate, mixed
glycosidases from T. cornutus, or mixed -glycosidases,
the binding of MAb 18.44 was substantially reduced or eliminated (Fig.
3 and 4). Treatment with mixed -glycosidases did not affect the binding of MAb
18.44 (Fig. 4). When glycosidase treatments were repeated by using
individual enzymes present in the mixed preparations, -D-mannosidase, but not -D-mannosidase or
other glycosidases, eliminated the binding of MAb 18.44 to CPS-500
(Fig. 4). These findings are consistent with glycosyl composition data
and indicated that CPS-500 contains a terminal
-D-mannopyranosyl residue essential for recognition by
MAb 18.44.
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FIG. 3.
Dot immunoblot detection of the CPS-500 epitope
recognized by MAb 18.44 before (lanes 1 and 5) and after treatment with
1 mM (lane 2), 5 mM (lane 3), or 10 mM (lane 4) periodate or with mixed
glycosidases from T. cornutus (lane 7). Lane 6 (untreated
CPS-500) and lane 8 (CPS-500 treated with mixed glycosidases) were
probed with an isotype control MAb. Serial twofold dilutions of CPS-500
are dotted from top to bottom.
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FIG. 4.
Dot immunoblot detection of the CPS-500 epitope
recognized by MAb 18.44 before (lane 1) and after treatment with mixed
-glycosidases (lane 3), mixed -glycosidases (lane 4),
-D-glucosidase (lane 5), -D-xylosidase
(lane 6), or -D-mannosidase (lane 7). Lane 2 contains
untreated CPS-500 probed with an isotype control MAb. Serial twofold
dilutions of CPS-500 are dotted from top to bottom.
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CPS-500 exposed on the pellicle surface is bound and released onto
substrate during sporozoite and merozoite motility.
Although the
glycolipid composition of CPS-500 precluded optimal fixation and
processing for ultrastructural studies, immunoelectron microscopy
localized MAb 18.44 binding to the sporozoite pellicle (Fig.
5). This finding is consistent with the
binding of MAb 18.44 to viable sporozoites (26) and
merozoites (5) in an IFA, and it confirmed surface exposure
of the target epitope. MAb 18.44 binding was also observed in a
tubulovesicular pattern in the sporozoite cytoplasm but was not
localized to any discernible organelle (Fig. 5).
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FIG. 5.
Immunoelectron photomicrographs of sporozoites probed
with MAb 18.44 (A) or an isotype-matched control MAb (B). Note
immunogold labelling of the sporozoite pellicle and intracytoplasmic
material by MAb 18.44 (arrows). Bars, 0.1 µm.
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In an IFA, MAb 18.44 and the P23-reactive MAb 7D10 detected prominent
trails of antigen deposited on substrate over the path
travelled by
motile sporozoites (Fig.
6) and
merozoites (data
not shown). Sporozoite antigen deposits detected by
each MAb were
morphologically similar (Fig.
6). Following incubation of
viable
sporozoites in suspension, CPS-500 was detected by MAb 18.44 in
immunoblots of the sporozoite fraction but not in the soluble
phase of
incubation medium (data not shown).
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FIG. 6.
Immunofluorescence reactivity of MAb 18.44 (A) and MAb
7D10 (B) with sporozoites. Note MAb detection of CPS-500 (A) and P23
(B) antigen deposits emanating from the posterior sporozoite and
demarcating the gliding path (arrows). Bars, 5 µm.
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DISCUSSION |
In the present study, the biochemical properties, subcellular
location, and possible function of the neutralization-sensitive C. parvum zoite antigen CPS-500 were characterized.
Information related to these subjects was essential to ongoing
investigations on the utility of this antigen for passive or active
immunoprophylaxis against cryptosporidiosis (24). Other
studies have reported that the antigenic composition of C. parvum is biochemically complex (17, 19) and suggested
that parasite carbohydrates or glycoconjugates are important targets of
the humoral immune response (5, 14, 17, 22, 26, 28, 32).
Accordingly, the general biochemical composition of CPS-500 was
determined, and the specific target epitope recognized by MAb 18.44 was
characterized. This was of paramount interest because of the ability of
MAb 18.44 to neutralize the infectivity of both sporozoites and
merozoites (5, 26) and to significantly reduce C. parvum infection in oocyst-challenged mice when coadministered
with other neutralizing MAb (21). In addition, conservation
of the target epitope among different C. parvum isolates
(33), and in both infectious stages (5, 26), suggests an important biological role. Finally, hyperimmune bovine polyclonal antibodies, which neutralize C. parvum sporozoite
infectivity and significantly reduce infection in oocyst-challenged
mice, recognize sporozoite and merozoite antigens comigrating with
CPS-500 in SDS-PAGE (25). This observation suggests that
cattle are able to respond to CPS-500 when immunized with whole
C. parvum; thereby CPS-500 satisfies a fundamental criterion
for consideration as a vaccine candidate.
Initial biochemical characterization of CPS-500 indicated a glycolipid
composition based on chloroform extractability, and susceptibility to
periodate and mixed glycosidases. Following HPLC isolation of CPS-500
from chloroform-extracted, silicic acid chromatography-enriched
preparations, glycosyl analysis identified mannose and inositol as the
predominant residues, suggesting that the antigen may be a mannosylated
inositol. Glucose and galactose were also identified, but in much
smaller amounts than mannose or inositol, suggesting that they may not
be components of CPS-500. Relatively small amounts of native CPS-500
were recoverable for analysis in the present study. Isolation of
CPS-500 in quantity will be required to determine its complete
molecular structure and whether inositol, glucose, and galactose are components.
In studies to characterize the neutralization-sensitive CPS-500 epitope
recognized by MAb 18.44, resistance to serine-, thiol-, acid-, and
metalloproteases confirmed and extended previous observations that the
epitope was not likely peptide dependent (26). A
carbohydrate-dependent epitope was initially suggested by the IgG3
isotype of MAb 18.44, in that this isotype often predominates in murine
antibody responses to carbohydrate epitopes (11). The
rationale for determining if the epitope contained mannose was twofold.
First, glycosyl analysis identified mannose as a major sugar in
CPS-500. Second, a mixed-glycosidase preparation which contained -
and -mannosidases destroyed the epitope. Subsequent studies using
individual glycosidases of defined specificity led to the critical
observation that the epitope was susceptible to
-D-mannosidase but not to -D-mannosidase or other glycosidases. This finding provided unequivocal evidence that
the target epitope was dependent on terminal
-D-mannopyranosyl residues. Importantly, because
glycoconjugates in mammals are essentially devoid of terminal
-D-mannopyranosyl residues (35), the CPS-500
epitope composition identified herein may facilitate targeted
disruption of a parasite-specific molecule known to have a role in the
pathogenesis of infection. In relation to this, the weak immunogenicity
of native CPS-500 observed in immunized animals may be accounted for by
its biochemical properties (1) identified in the present
study. Indeed, when coupled to methylated BSA or keyhole limpet
hemocyanin, CPS-500 was highly immunogenic based on antibody responses
in immunized mice and hens (23). Further, orally
administered CPS-500-reactive mouse MAbs, and polyclonal monospecific
hen egg yolk antibodies derived from animals immunized with carrier
protein-coupled CPS-500, provided highly significant passive protection
against C. parvum oocyst challenge in mice (23).
Immunoelectron microscopic localization of CPS-500 to the sporozoite
pellicle and IFA identification of antigen bound and released onto
substrate by gliding sporozoites and merozoites suggest that CPS-500
has a role in the motility of the infective stages. Previous studies
have shown that sporozoites deposit surface antigens of 15 (GP15)
(12, 31), 23 (P23) (4, 9, 31), and 38 or >900
(12) kDa on substrate or epithelial-cell monolayers during
gliding motility in vitro. Deposition of GP15 and P23, antigens which
are known to express neutralization-sensitive epitopes (2, 9, 20,
32), was detected in these studies by using MAbs specific for
each antigen, including C6B6 (P23). Antigen deposits were
morphologically similar to those described previously for the
circumsporozoite protein of Plasmodium sp. (30),
suggesting that specific C. parvum surface molecules may be
involved in motility and invasion. In the present study, the
P23-reactive MAb 7D10 detected antigen deposited by motile sporozoites
and merozoites. We previously reported that MAb 7D10, prepared against
C6B6 affinity chromatography-isolated native P23, significantly reduces
C. parvum infection in mice and recognizes a
neutralization-sensitive epitope which is different from that defined
by MAb C6B6 (20). Therefore, recognition of a second
distinct epitope by MAb 7D10 in P23 deposits further supports the
hypothesis that surface antigen binding and release during
infective-stage motility in vitro has probable biological relevance in
vivo. Deposition of surface antigens other than the preceding by motile
C. parvum sporozoites has not been previously reported. The
results presented herein demonstrate that CPS-500, or a portion thereof
containing the neutralization-sensitive epitope recognized by MAb
18.44, is bound and released onto substrate by motile sporozoites and,
additionally, by merozoites. This finding is consistent with the
surface location of CPS-500 and suggests a functional role for the
molecule. Indeed, if the binding and release of CPS-500, P23, and GP15
are required for zoite motility and invasion, a probable mechanism for
the neutralizing activity of MAbs against these antigens would be suggested.
With regard to the foregoing, we recently reported the identification
of an ~1,300-kDa apical and surface glycoprotein of C. parvum zoites designated CSL (28). CSL is a soluble
exoantigen released into the incubation medium by sporozoites, and it
contains a repetitive carbohydrate-dependent epitope recognized by MAbs which elicit the circumsporozoite precipitate-like reaction
(28). MAbs which elicit this reaction neutralize sporozoite
infectivity in vitro and provide passive protection against oocyst
challenge in vivo (16, 28). On the basis of the
characteristics of CSL and the inability of 18.44, 7D10, or other
neutralizing MAbs against CPS-500 and P23 to elicit the
circumsporozoite precipitate-like reaction (24), it was of
interest to determine if CPS-500 is a soluble exoantigen. Although
CPS-500 was bound and released during zoite motility and was identified
in sporozoites after incubation in suspension, it was not detected in
the incubation medium. These findings suggest that CPS-500, unlike CSL,
is not a soluble exoantigen and that its release may require adhesion to a substrate during zoite motility. Alternatively, if CPS-500 is
constitutively released by sporozoites, lack of detection in the
incubation medium may relate to its glycolipid composition and
immiscibility with the aqueous phase used for immunoblots. The
relationships between C. parvum zoite surface molecules
deposited during motility, released as soluble exoantigens, or bound by MAbs in the circumsporozoite precipitate-like reaction remain to be defined.
In this report we have characterized the biochemical properties and
possible function of CPS-500, the neutralization-sensitive C. parvum zoite antigen defined by MAb 18.44. Of most significance, -D-mannose has been identified as the specific sugar
conferring carbohydrate dependency on the target epitope recognized by
MAb 18.44. These findings now provide the rationale for determining the
complete molecular structure of CPS-500 and for investigating the
utility of chemically synthesized -mannosides or anti-idiotype-18.44 antibodies in vaccination strategies against cryptosporidiosis.
| |
ACKNOWLEDGMENTS |
This work was supported by Public Health Service grant AI 30223 from the National Institutes of Health, U.S. Department of Agriculture
NRICGP grant 94-37204-0496, and funds from the Agricultural Experiment
Station, Colorado State University.
We thank Beth A. Auerbach for excellent technical assistance and
preparation of figures, and David L. Bentley for valuable advice on
ultrastructural localization of glycolipid antigens.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Veterinary Science and Microbiology, Veterinary Science and
Microbiology Bldg., University of Arizona, Tucson, AZ 85721. Phone:
(520) 621-8445. Fax: (520) 621-6366. E-mail:
mriggs{at}u.arizona.edu.
Editor:
T. R. Kozel
| |
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Infection and Immunity, March 1999, p. 1317-1322, Vol. 67, No. 3
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
