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Clinical and Diagnostic Laboratory Immunology, January 1998, p. 50-57, Vol. 5, No. 1
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Cincinnati Veterans Affairs Medical
Center,1
Department of Internal
Medicine,
Received 29 May 1997/Returned for modification 31 July
1997/Accepted 2 October 1997
The major surface glycoprotein (MSG) of Pneumocystis
carinii f. sp. carinii consists of a heterogeneous
family of proteins that are encoded by approximately 100 unique genes.
A genomic expression library was screened with a panel of MSG-specific
monoclonal antibodies (MAbs) to identify conserved and rare epitopes.
All of the antibodies reacted with epitopes that are encoded within the
5' end of MSG. The results from the expression screening identified antibodies that recognize highly conserved, moderately conserved, and
rare epitopes. Four MAbs (MAbs RA-F1, RA-E7, RA-G10, and RB-E3) reacted
with a maltose binding protein-MSG-B fusion protein
(MBPMSG-B41-1065) by immunoblotting and
enzyme-linked immunosorbent assay. Three of the MAbs (MAbs RA-F1,
RA-G10, and RA-E7) reacted with the same continuous epitope that was
localized to amino acids 278 to 290 of MSG-B. Comparison of the
sequence of the RA-F1-, RA-G10-, and RA-E7-reactive epitope to the
deduced amino acid sequences of multiple MSGs demonstrated that it is
highly conserved. The reactivity of RB-E3 with MSG-B was shown to be
dependent on amino acids 184 to 192, which may comprise a portion of a
discontinuous epitope.
Pneumocystis carinii f.
sp. hominis is an important cause of pneumonia in patients
with human immunodeficiency virus infection, cancer, and organ
transplantation and in other immunocompromised hosts. The host factors
that predispose individuals to the development of P. carinii
f. sp. hominis pneumonia involve impaired cellular and
humoral immunity; however, the specific immune defects are poorly
understood. All forms of P. carinii that have been examined contain a 95,000- to 140,000-kDa glycoprotein, termed either the major
surface glycoprotein (MSG) or glycoprotein A (gpA), which plays an
important role in the immunobiology of the organism (12, 17, 20,
34, 42, 50). MSG is highly immunogenic and stimulates the
production of various cytokines, contains protective B- and T-cell
epitopes, and facilitates the interaction of P. carinii with
host cells (9, 30, 33, 43, 44, 54).
MSG actually consists of a heterogeneous family of proteins encoded by
about 100 genes. DNA sequence analysis of MSG cDNAs and/or genes has
demonstrated that the gene family encodes many distinct MSG isoforms,
which are very similar in size but whose sequences vary (10, 18,
21, 26, 48).
Transcription of MSG genes appears to occur only within a single
telomeric expression site (7, 39, 49). The isolation of
multiple unique MSG cDNAs from a single P. carinii f. sp.
carinii-infected rat lung suggests that multiple MSG mRNAs
and proteins may be present at the same time within a population of
P. carinii f. sp. carinii (26). The
ability to alter the expression of different MSG molecules raises the
possibility of antigenic variation occurring in P. carinii
f. sp. carinii.
MSG appears to be involved in both the cellular and the humoral immune
responses of the host to P. carinii f. sp.
carinii. Spleen cells isolated from rats environmentally
exposed to P. carinii f. sp. carinii proliferate
in response to MSG, and sera from these animals contain MSG-specific
antibodies (44). MSG is also recognized by humans exposed to
P. carinii f. sp. hominis. MSG-specific
antibodies have been detected in approximately 30 to 70% of human
serum specimens that contain P. carinii f. sp. hominis antibodies (28, 31). Animals generate a
vigorous immune response against MSG upon immunization with purified
antigens or P. carinii f. sp. carinii
preparations (7). Passive immunotherapy with MSG-specific
monoclonal antibodies (MAbs) and/or hyperimmune polyclonal antiserum
has also been shown to modulate P. carinii infection in
ferrets, rats, and mice with severe combined immunodeficiency, supporting the significance of MSG in the host response to P. carinii (13, 14, 35). The involvement of MSG in the
host immune response suggests that immunization with it may provide protection against P. carinii infection. Because multiple
isoforms of MSG can be expressed within a population of P. carinii, it will be important to identify immunoreactive regions
common to all MSGs.
Several groups have described the production and characterization of
P. carinii-specific MAbs (11, 16, 19, 23, 24, 27,
29). MSG-specific MAbs have also used to distinguish rat P. carinii f. sp. carinii and P. carinii f. sp.
ratti strains at a phenotypic level (47). A MAb
specific to MSG purified from P. carinii f. sp.
hominis has been used in the development of a new method of
diagnosis of P. carinii f. sp. hominis pneumonia by radioimmunodetection (15).
In the study described in this paper we have characterized a panel of
MSG-specific MAbs on the basis of the frequency with which their
epitopes are encoded and expressed within a population of P. carinii f. sp. carinii. This analysis demonstrated the
presence of conserved epitopes that appear to be present on the
majority of MSGs and epitopes that appear to be present on a restricted number of MSGs. A single MSG isoform was expressed in a bacterial vector and was used to identify the epitopes recognized by two of the
MAbs that recognize conserved epitopes. Detailed characterization of
MSG-specific MAb reactivities and identification of epitopes recognized
by the MAbs will greatly improve their usefulness in the analysis of
the expression of different MSG isoforms.
Pneumocystis nomenclature.
The
Pneumocystis nomenclature proposed at the 3rd International
Workshop on Pneumocystis in Cleveland, Ohio, in June 1994 will be used in this report (32). Provisional tripartite
names denoting the mammal of origin were given to the organism
populations isolated from various mammalian hosts.
Pneumocystis isolated from rats will be referred to as
either P. carinii f. sp. carinii, designated the
prototype, or P. carinii f. sp. ratti, designated a variant; the organism from human beings will be referred to as
P. carinii f. sp. hominis.
Source of organisms.
P. carinii f. sp.
carinii pneumonia was induced by corticosteroid treatment of
rats, and the organisms were recovered from infected lungs and were
quantitated as described previously (4). Briefly, infected
lungs were removed en bloc, minced, and homogenized. The homogenate was
centrifuged at 1,000 × g for 10 min at 4°C, and the
resulting pellet was treated with 0.85% ammonium chloride to lyse the
erythrocytes. The pellet was washed twice, and the organisms were
resuspended in phosphate-buffered saline.
Source of antibodies.
MSG-specific MAbs were produced and
characterized as described previously (27). Three different
P. carinii antigen preparations were used to produce the
MAbs used in this study: (i) P. carinii f. sp.
carinii, (ii) MSG purified from P. carinii f. sp.
carinii, and (iii) detergent-solubilized P. carinii f. sp. hominis (Table 1). Mice were immunized three times
subcutaneously with the antigen preparations, and antigen preparations
were then injected intraperitoneally 3 days prior to fusion. Spleen
cells from the mice were fused to a myeloma cell line, and hybrids were
selected by previously described methods. The resulting hybridomas were
screened for P. carinii-specific reactivity by
immunoblotting or enzyme-linked immunosorbent assay (ELISA). Polyclonal
antibodies to P. carinii f. sp. carinii MSG were
prepared by immunizing rabbits with purified MSG. Polyclonal rabbit
anti-maltose binding protein (anti-MBP) serum was obtained from New
England Biolabs, Beverly, Mass. Enzyme-conjugated antibodies were
obtained from Kirkegaard & Perry, Gaithersburg, Md.
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
TABLE 1.
Characterization of MSG-specific MAbs and frequency of
epitope expression
Hybridization and screening of the 
gt11 genomic expression
library.
The bacteriophage gt11 genomic library was generated
by insertion of randomly sheared P. carinii f. sp.
carinii DNA into gt11, and hybridizations were performed
by standard methods (36). The gt11 library was screened
with MAbs as described previously (10). To determine the
number of plaques to be screened, the library was first evaluated by
hybridization of the gt11 library to four different single-copy gene
probes and to an MSG gene probe. The single-copy gene probes used were
the TATA box binding protein (40), thymidylate synthase
(8), alpha-tubulin (53), and 55-kDa antigen
(37). Approximately 20,000 plaques were screened with each
gene probe. Four positive plaques were detected with the 55-kDa antigen
gene probe, and five positive plaques were found with the other gene
probes. These data suggested that 4,000 to 5,000 plaques contain one
genome equivalent in this library. This is reasonably close to the
theoretical value calculated from the size of the genome, which is
approximately 107 bp (5). A genome of this size
would be contained in 4 × 103 phages, each carrying a
2.5-kb insert. The gt11 library was generated with randomly sheared
P. carinii f. sp. carinii DNA that ranged in size
from 1 to 4 kb.
Analysis of MAb RA-F1-reactive gt11 clones.
Four clones
reactive with MAb RA-F1 were plaque purified by standard techniques
(36). The reactivities of each of these clones were
determined with the other MAbs as described previously. Phage DNA from
all four clones was isolated by the Wizard lambda prep kit (Promega,
Madison, Wis.). Partial sequences from both insert ends were obtained
by using a PCR sequencing kit with the gt11 forward and reverse
primers by following the manufacturer's standard protocol (Life
Technologies, Inc., Gaithersburg, Md.). The sequences from each clone
were aligned with the DNANALYZE program (51) to MSG-B
(41) to determine the location of the beginning and end of
each of the inserts. Primer C5 (5'-CATGAAAGACTTGAGAAATGT-3') was used in the PCR cycle sequencing of clones 1 and 4 in order to compare sequences from the same area from all four RA-F1-reactive clones.
Cloning of the msg-b gene.
A gene encoding a
single species of MSG, designated msg-b, was amplified from
Rp3-1 template DNA; Rp3-1 is a 16-kb fragment containing repetitive
elements cloned from the P. carinii f. sp. carinii genome (38, 39, 41). Primers
msg1+ and msg3801
(Table
2) were designed to amplify the entire
msg-b gene. MunI sites were engineered into these
primers in order to ligate the products directly into an
EcoRI site. PCR was performed by standard methods. Reactions
were amplified for two cycles of 94°C for 1 min, 45°C for 1 min,
and 72°C for 3 min and were then amplified for 30 cycles of 94°C
for 1 min, 50°C for 1 min, and 72°C for 3 min. Amplified DNA was
purified by using the Wizard PCR Preps system (Promega) according to
the manufacturer's instructions. Ligation of the MunI-cut
msg-b PCR product into the EcoRI site of pMALc2
was unsuccessful. Therefore, restriction sites that were compatible
with sites in the pMALc2 polylinker were identified within the
msg-b sequence. Digestion of an AvaI site present
at base 124 and a HindIII site located downstream of the
stop codon at base 3366 allowed ligation of the msg-b PCR
product between the SalI and HindIII sites of
the pMALc2 polylinker. This construct, designated
pMAL/msg-b123-3366, contains the entire msg-b gene lacking the initial 122 bp ligated in frame with the MBP that is
encoded by pMALc2.
|
Exonuclease digestion-generated MSG-B truncations. In order to produce a linear construct with 5' and 3' 4-base overhanging ends, a 24-bp oligonucleotide containing a KpnI site was cloned into the 3' end of the pMAL/msg-b123-3366 construct. After digestion with KpnI and SalI (Promega), the linearized DNA was subjected to unidirectional digestion with exonuclease III (ExoIII; New England Biolabs) as described previously (2, 6).
Amplification and cloning of internal msg-b fragments. Eight overlapping MBPMSG-B fusion proteins were produced by amplifying the target regions of msg-b by PCR and cloning the products into pMAL-c2. Primers were either constructed to correspond to flanking regions of the target MSG-B region or to sequences within pMAL-c2 (Table 2). PCR products were digested with AvaI and HindIII and were then ligated into the polylinker of pMAL-c2 between the SalI and HindIII sites. Direct cloning of some of the PCR products into pMAL-c2 was unsuccessful; therefore, these products were initially cloned into a PCR cloning vector, pGEM-T (Promega). Ligation and transformation of pGEM-T was carried out as described by the manufacturer. The PCR products were excised from pGEM-T by restriction digestion. The inserts were gel purified and ligated into the polylinker of pMAL-c2 digested with the corresponding restriction enzymes.
The recombinant pMAL/msg-b clones were sequenced by a modified double-stranded DNA sequencing technique (Sequenase, version 2.0, U.S. Biochemicals). A mutation was detected in pMAL/msg-b579-966. A point mutation at bp 966 (T
A)
created a stop codon that resulted in the expression of a fusion
protein that extends from amino acids 193 to 322 with a predicted
molecular weight of 60,000 (MBPMSG193-322).
Analysis of the DNA sequence of pMAL/msg-b375-576 revealed
following base 576 a frameshift mutation that altered the MSG-B
amino acid sequence starting at amino acid 192 and that created a stop
codon at base 709. Thus, the resulting fusion protein had a predicted
molecular weight of 62,957, but the MSG-B amino acid sequence extended
only from residues 125 to 192 (MBPMSG125-192).
The remaining six constructs were cloned in the correct reading frame
with MBP and contained no mutations.
Fusion protein expression and purification.
The pMAL/msg-b
plasmids were used to transform electrocompetent Escherichia
coli in an Electroporator II apparatus (Invitrogen, San Diego,
Calif.) according to the manufacturer's instructions. Positive
transformants were picked and grown overnight at 37°C in 25-ml
cultures of Luria-Bertani liquid broth supplemented with 50 µg of
ampicillin per ml (LB-amp). On the following day, the overnight
cultures were used to inoculate new 1-liter cultures of LB-amp which
were then grown to an optical density at 600 nm (OD600) of
0.5 to 0.7. Fusion protein production was induced by the addition of
isopropyl-
-D-thiogalactopyranoside to a final concentration of 0.5 mM. After 3 h of induction at 37°C, the
cultures were centrifuged at 4,000 × g for 20 min and
bacterial pellets were reconstituted in 25 ml of amylose column buffer
(20 mM Tris-HCl [pH 7.0], 200 mM NaCl, 1 mM EDTA).
20°C, cell suspensions were thawed and
sonicated for five cycles of 15-s bursts followed by 15 s on ice.
Sonicates were centrifuged at 10,000 × g for 30 min, and MBPMSG-B fusion proteins were purified from the
supernatants by using an amylose resin column (New England Biolabs)
according to the manufacturer's instructions.
SDS-PAGE and immunoblotting.
Proteins were solubilized in
2× lysis buffer (125 mM Tris-HCl [pH 6.8], 4.0% sodium dodecyl
sulfate (SDS), 20% glycerol, 10% -mercaptoethanol) for analysis by
SDS-polyacrylamide gel electrophoresis (PAGE) (22, 25). The
proteins were transferred electrophoretically from the
SDS-polyacrylamide gel to a nitrocellulose membrane, and immunoblotting
was performed as described previously (25, 45).
ELISA. Purified fusion proteins from the deletion constructs were diluted to 20 µg/ml in coating buffer from the ELISAmate reagent kit (Kirkegaard & Perry), and 50 µl was used to sensitize 96-well polyvinyl ELISA plates (Dynatech, Chantilly, Va.) overnight at 4°C. All subsequent steps were performed at room temperature. The wells were washed twice with ELISAmate wash buffer and were blocked with ELISAmate bovine serum albumin blocking reagent for 2 h. The wells were washed four times with wash buffer, incubated with the MAb for 2 h, washed four times with wash buffer, and then incubated with goat anti-mouse immunoglobulin G-horseradish peroxidase conjugated antibody (Kirkegaard & Perry) at a 1:1,000 dilution in ELISAmate diluent buffer for 2 h. The wells were washed four times in wash buffer and developed with ELISAmate ABTS peroxidase substrate. The optical densities of the wells were monitored at 405 nm on a 96-well plate reader (Bio-Tek Instruments, Winooski, Vt.).
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Assessment of MAb epitope prevalence in the MSG family.
A
panel of MAbs known to react with MSG had been generated previously
(27). To estimate the number of MSG isoforms recognized by
each of these MAbs, we used a genomic expression library that had been
made by insertion of random fragments from the P. carinii f.
sp. carinii genome into gt11. A genomic expression
library could be used because previous studies had shown that MSG genes lack introns (41). It was determined that 4,000 to 5,000 plaques contain one genome equivalent in this library. However, because the inserts in the library are in random orientations and reading frames with respect to the vector DNA sequence, only one of six MSG
gene fragments would be expected to be capable of expressing an MSG
epitope. Therefore, 24,000 plaques would be expected to express every
unique epitope at least once.
|
gt11 library screen (fewer than 23 plaques) (Table 1). The remaining seven MAbs each reacted with at least
one RA-F1-positive phage (Fig. 1). Three MAbs (MAbs RA-F1, RA-E7, and
RA-G10) reacted with all four clones, suggesting that they recognize
the same epitope, and subsequent studies (described below) showed that
this was the case. The reactivities of MAbs RA-F1, RA-E7, RA-G10,
RA-C1, RA-C6, and RB-C8 with clone 2 indicates that the epitopes for these MAbs are contained within the region from amino acids 227 to 660. The location of the epitopes for MAbs RB-E3 and RB-F9 could be
localized to the first 600 amino acids of MSG on the basis of their
reactivities with clone 3.
Localization of two MSG-specific MAb epitopes. To facilitate identification of the MAb epitopes, the msg-b isoform was produced in a bacterial expression system as described in the Materials and Methods. The MBPMSG-B fusion protein (MBPMSG-B41-1065) was assayed by immunoblot analysis for its reactivity to the 12 MAbs (data not shown), and it was found to be reactive with MAbs RA-F1, RA-E7, RA-G10, and RB-E3 (Fig. 1).
An epitope mapping strategy was designed to monitor the loss of reactivity of the MAbs with truncated forms of the MBPMSG-B fusion protein. MAb RA-E7 was chosen to represent the RA-F1, RA-E7, and RA-G10 group because of the availability of sufficient quantities of this MAb for epitope mapping studies. RB-E3 was selected because it appeared to recognize a unique epitope. The regions of MSG-B recognized by MAbs RA-E7 and RB-E3 were initially localized by expression of truncated MBPMSG-B fusion proteins produced by digestion of pMAL/msg-b124-3366 with ExoIII. MAbs RA-E7 and RB-E3 remained reactive with the two shortest ExoIII-generated truncations that stopped at MSG-B amino acids 563 (MBPMSG41-563) and 373 (MBPMSG-B41-373) (Fig. 2 and 3, lanes 3 and 4). These results indicated that the epitopes were contained in the region from amino acids 41 to 373. Further attempts to produce shorter proteins by ExoIII digestion were unsuccessful.
|
|
Analysis of the epitope regions in additional MSG isoforms. The availability of reactive and nonreactive phages provided a means of comparing the epitopes in these clones to the epitopes identified in MSG-B. The regions corresponding to those encoding the epitope in MSG-B reactive with MAbs RA-F1, RA-G10, and RA-E7 were amplified from phage clones 2 and 4, both of which produced plaques that were reactive with MAb RA-E7. The PCR products were cloned into pGEM-T, and the DNA was sequenced. Analysis of the deduced amino acid sequence revealed that the sequence of clone 2 matched the MSG-B sequence exactly and the sequence of clone 4 matched at 10 of 11 of the MSG-B amino acids (Fig. 4A). This finding supports the idea that the region reactive with MAb RA-E7 is highly conserved among MSG isoforms. The 12-amino-acid binding site for MAb RA-E7 was also well conserved among five additional MSG sequences predicted from previously published DNA sequences (Fig. 4A). A similar analysis of the putative epitope reactive with MAb RB-E3 yielded a more complex picture (Fig. 4B). While only clone 3 produced reactive phage plaques, the predicted amino acid sequences of both clones 1 and 3 were similar to the MSG-B sequence, and within the epitope there were no obvious amino acid substitutions that may account for the variation of reactivity between clones 1 and 3. Therefore, amino acids 185 to 192 appear to be essential for the reactivity of MAb RB-E3 with MSG-B, but additional amino-terminal residues may be involved in the presentation of the epitope to the antibody.
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| |
DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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The identification of conserved and variable epitopes on MSG molecules provides a method of studying the expression of different isoforms through the use of either polyclonal antiserum produced against peptides or MSG-specific MAbs. Previously, three different MSG variants were identified in a single lobe of an infected lung with epitope-specific polyclonal antisera by immunohistochemistry (1). In another study two MSG-specific MAbs (MAbs RA-C6 and RA-C11) were able to identify antigenic differences between genetically distinct P. carinii f. sp. carinii and P. carinii f. sp. ratti populations and within a genetically defined population of P. carinii f. sp. carinii. Two additional MAbs (MAbs RA-F1 and RA-C7) reacted with all P. carinii f. sp. carinii and P. carinii f. sp. ratti populations examined (47).
In this study MSG-specific MAbs were initially characterized on the basis of the frequency with which their epitopes are encoded within the P. carinii f. sp. carinii genome by screening an expression library made by insertion of randomly sheared genomic P. carinii f. sp. carinii DNA. The MAbs could be separated into four groups on the basis of the number of plaques that each one recognized. MAb RA-F1 appeared to react with a conserved epitope on the basis of its reactivity with 738 plaques. MAbs RB-E3, RB-2F9, and RB-C8 each recognized between 100 and 300 plaques, suggesting that these epitopes are encoded in multiple MSG genes. The three MAbs in the third group (MAbs RA-C6, RA-C7, and RA-C1) reacted with 46, 23, and 55 plaques, respectively. This group of MAbs appeared to recognize a less conserved epitope. The final group of MAbs (MAbs HB-G6, RA-C11, and RB-F8) recognized a rare epitope on the basis of the low number (three to seven) of plaques that they detected.
In addition to characterizing the frequency with which MAb epitopes are
expressed in the Pneumocystis genome, analysis of reactive
gt11 phage established that the MAbs react with MSG. Characterization of the MSG-specific MAbs was previously based on their
reactivity with a 116,000-molecular-weight glycoprotein that was
specific to Pneumocystis (27). The reactivities
of the MAbs with MSG were confirmed through DNA sequence analysis of
the gt11 clones. The four reactive clones that were analyzed by DNA
sequencing all contained pieces of DNA that were homologous with
previously identified msg genes.
The reactivities of four MAbs with recombinant MSG provided a method
for mapping their epitopes. The epitope reactive with MAbs RA-F1,
RA-G10, and RA-E7 was localized to a highly conserved region in the
amino-terminal end of MSG-B and was identified as amino acids 278 to
290. Comparison of the identified epitope with deduced amino acids from
previously cloned msg genes, cDNAs, or cloned regions of MSG
from reactive gt11 phage demonstrated that this sequence is highly
conserved. The reactivity of MAb RB-E3 was also localized in the
amino-terminal portion of MSG-B approximately 100 amino acids upstream
from the epitope reactive with MAbs RA-F1, RA-G10, and RA-E7. Amino
acids 185 to 192 of MSG-B were determined to be required for reactivity
with MAb RB-E3. Comparison of the amino acid sequence of the epitope
reactive with MAb RB-E3 with that of previously cloned msg
genes demonstrated that this region is not as well conserved as the
epitope reactive with MAbs RA-F1, RA-G10, and RA-E7. Alignment of the
amino acids in the RB-E3-reactive epitope regions from a reactive
gt11 phage and a nonreactive gt11 phage did not reveal the
presence of critical residues that would be essential for reactivity.
There are two basic types of epitopes, continuous and discontinuous (3, 46). Continuous epitopes consist of short linear sequences of amino acids. Discontinuous epitopes involve distant residues brought together by protein folding. The immunoblotting, ELISA, and sequence comparison data indicate that MSG-B amino acids 279 to 290 represent the epitope reactive with MAbs RA-F1, RA-G10, and RA-E7, and deletion of these amino acids clearly results in the loss of MAb reactivity. In addition, the high degree of conservation of the epitope among other MSGs indicates that it is a continuous epitope. The functional identification of the RB-E3-reactive epitope by immunoblotting and ELISA suggests that it is continuous; however, the lack of a correlation of MAb reactivity with the conservation of specific amino acids indicates that additional residues may be required for high-affinity binding of MAb RB-E3. The decreased reactivity of the MBPMSG-B171-349 fusion protein also indicates that additional amino acids removed from the epitope region are required for antibody recognition. The presence of a cysteine at residue 187 that could be involved in the folding of MSG through the formation of disulfhydryl bonds is noteworthy. The location of cysteine residues is maintained among all MSGs analyzed to date (26, 52). The conservation of the cysteine positions suggests the importance of disulfhydryl bonds in maintaining a conserved higher-order structure that could be critical to the function of MSG.
MSG has been implicated in the binding of P. carinii to host cells and molecules. The extracellular MSG domains involved in these interactions have not been identified, and little is known about the position or orientation of MSG within the cell membrane or cell wall of P. carinii. As described previously, MAbs RA-E7, RA-G10, RA-F1, RB-E3, RA-C1, RA-C6, RB-C8, and RB-F9 react with the surface of P. carinii f. sp. carinii by immunofluorescence (27). Localization of the MAb reactivity within the first 600 amino acids demonstrates that at least portions of the amino terminus of MSG are exposed on the surface of P. carinii f. sp. carinii. These results suggest that the surface-exposed amino terminus of MSG may also be involved in binding to host proteins.
The presence of hundreds of MSG genes in the genome suggests that P. carinii is capable of undergoing a form of antigenic variation and that the ability to alter this abundant surface protein is critical to its survival. The MAbs characterized in these studies will provide useful tools for analyzing the expression of particular MSG isoforms on P. carinii.
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ACKNOWLEDGMENTS |
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This work was supported by the Medical Research Service of the U.S. Department of Veterans Affairs and Public Health Service contract AI 25139 and grant AI 36701 from the National Institutes of Health.
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FOOTNOTES |
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* Corresponding author. Mailing address: VA Medical Center, 3200 Vine St., Cincinnati, OH 45220. Phone: (513) 861-3100, extension 4423. Fax: (513) 475-6415. E-mail: mjl19{at}juno.com.
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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