Previous Article | Next Article 
Infection and Immunity, June 2000, p. 3186-3192, Vol. 68, No. 6
Life Science Laboratory, Research and
Development Center, Nippon Zeon Co., Ltd., 1-2-1 Yako, Kawasaki-ku,
Kawasaki 210-8507, Japan
Received 13 December 1999/Returned for modification 7 February
2000/Accepted 26 February 2000
In order to identify antigenic proteins of Mycoplasma
gallisepticum, monoclonal antibodies (MAbs) against virulent
M. gallisepticum R strain were produced in mice. MAb 35A6
was selected for its abilities to inhibit both growth and metabolism of
M. gallisepticum in vitro. The MAb
recognized a membrane protein with an apparent molecular mass of 120 kDa. The corresponding gene, designated the mgc3 gene, was cloned from
an M. gallisepticum genomic DNA expression library and sequenced. The mgc3 gene is a homologue of the
ORF6 gene encoding 130-kDa protein in the P1 operon of M. pneumoniae and is localized downstream of the mgc1 gene, a homologue of the P1 gene. To assess the characteristics of MGC3 protein, all 10 TGA codons in the mgc3 gene, which encode a tryptophan in the Mycoplasma species, were replaced with TGG codons,
and recombinant fowlpox viruses (FPV) harboring the altered mgc3 gene were constructed. One of the recombinant FPVs was improved to express
MGC3 protein on the cell surface in which the signal peptide of MGC3
protein was replaced with one from Marek's disease virus gB.
These results should provide the impetus to develop a vaccine based on
MGC3 protein which can induce antibodies with both growth inhibition
and metabolic-inhibition activities using a recombinant FPV.
Mycoplasma
gallisepticum is the aetiologic agent of chronic
respiratory disease in chickens and infectious sinusitis in turkeys (37). The disease is characterized by nasal discharge,
respiratory rales, coughing, and airsacculitis. M. gallisepticum infection causes reduced feed
conversion and egg production, and the outbreaks remain a persistent
cause of severe economic loss for broiler and turkey production firms
(36). The best solution for controlling this disease may
reside in the development of safe and effective vaccines.
An attenuated strain, the F strain, can induce protective immune
responses and subsequently improve egg production in vaccinated chickens. However, the F strain is not completely apathogenic for young
chickens (25) and turkeys (20), and it may spread to M. gallisepticum-free chicken and turkey
farms. Other attenuated strains, ts11 (40) and 6/85
(7) have been used as vaccines in multi-age layers because
of lower virulence. These strains, however, confer somewhat less
protection than does the F strain (1). On the other hand,
for an inactivated vaccine, an experimental immunostimulating
complex (ISCOM) vaccine consisting of detergent-solubilized M. gallisepticum antigens and Quillaja
saponin induced protective immunity and significantly reduced lesion
scores in the air sac after challenge (31). The success of
the inactivated vaccine using the special adjuvant suggests that the
isolation of specific immunogens responsible for protective immunity
may lead to the development of effective vaccines without the adverse
side effects associated with the administration of whole organisms.
We have focused on the identification and structural analysis of
M. gallisepticum surface antigens which are
prominent targets of the chicken immune responses and may influence key
host interactions (27). The attachment of M. gallisepticum to mucosal epithelium of the
respiratory tract of birds is thought to be prerequisite for infection
and disease (19). Therefore, a vaccine designed to induce
inhibition responses to the attachment and the growth of M. gallisepticum in vivo should provide protective
immunity to the organism.
The present study describes the production of a mouse monoclonal
antibody (MAb) that inhibits both growth and metabolism of M. gallisepticum in vitro and the identification
of an antigen recognized by the MAb. The antigen,
designated MGC3, was a 120-kDa membrane protein and a homologue
of 130-kDa protein encoded by the ORF6 gene, which is a part of P1
operon of M. pneumoniae (30). Recently, the 40- and 90-kDa proteins from 130-kDa protein have been shown to be
responsible for the tip structure formation associated with P1
(17). Since we demonstrate for the first time that MGC3 protein possesses epitopes recognized by MAbs with growth inhibition and metabolic-inhibition activities, few attempts have so far been made
to use the 130-kDa protein or its homologues as vaccine candidates. It
is of interest to express the mgc3 gene and to determine whether MGC3
protein is important as a potential target of humoral responses in
chickens. For these purposes, we used a recombinant fowlpox virus (FPV)
expression system which has been established as a live viral vector for
use of vaccines against avian viruses such as Newcastle disease virus
(13, 24) and Marek's disease virus (MDV) (23, 35,
38) in our laboratory. Based on the recombinant FPV technology,
MGC3 protein expressed by recombinant FPVs was analyzed in chicken
fibroblast embryo (CEF) cells.
Strains and growth conditions.
The sources of M. gallisepticum strains R, F, S6, and KP13 have been
described elsewhere (10, 16). These M. gallisepticum strains were grown statically at
37°C for 3 days in Chanock's modified medium (5).
M. gallisepticum strains were filter cloned according to the recommendations of the Subcommittee on the Taxonomy of
Mollicutes (14, 33) and subsequently freeze-dried. CEF cells
were maintained in Leibovitz-McCoy medium (Life Technologies, Inc.,
Rockville, Md.) supplemented with 4% calf serum and antibotics. A
large plaque variant of cell culture-attenuated FPV (22) was used as the parental virus from which recombinants were constructed.
Production of MAbs.
Six-week-old BALB/c mice were immunized
subcutaneously with 100 µg of whole M. gallisepticum R strain protein emulsified in Freund's complete adjuvant. Three weeks later, the mice were injected intraperitoneally with the same antigen concentration in Freund's incomplete adjuvant. Three days later, serum was collected, and spleen
cells were fused with P3X63Ag8.U1 myeloma cells (American Type Culture
Collection, Rockville, Md.), using an established procedure
(4). Hybridoma clones were screened by enzyme-linked immunosorbent assay (ELISA) using the whole M. gallisepticum R strain (3).
ELISA-positive hybridoma clones were used for preparation of M. gallisepticum-specific antibody-producing tumors
in pristane (2,6,10,14-tetramethylpentadecane)-primed BALB/c mice.
Ascites fluids containing MAbs were clarified by centrifugation at
2,000 × g for 10 min and stored at SDS-PAGE and immunoblotting.
Whole-cell preparations of
M. gallisepticum strains used in this study
were separately suspended at a protein concentration of 1 mg/ml in
sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)
lysis buffer (50 mM Tris-HCl [pH 6.8], 2% SDS, 10% glycerol, 2%
Growth inhibition assay.
The growth inhibition assay without
complement was performed essentially as described previously
(27). In brief, M. gallisepticum R strain was grown in Chanock's modified medium at 37°C for 3 days,
filtered through a 0.45-µm (pore-size) membrane filter, and diluted
to 1.2 × 103 CFU/ml. Three hundred CFU of the
suspension cells were cultured in the presence of 50 µg of MAbs or
serum dilutions of 1:10 in a volume of 300 µl. The cultures were
incubated at 37°C for 3 days. To determine the number of CFU, six
serial 10-fold dilutions in modified Chanock's medium were performed
in duplicate. Aliquots of 10 or 100 µl were plated on modified
Chanock's agar medium following gentle passing of the cultures through
a 0.45-µm filter. After 6 to 7 days of incubation at 37°C, the
number of CFU was counted under a stereomicroscope (Leitz).
Metabolic inhibition assay.
The complement-independent
inhibition of glucose metabolism by MAbs resulting in the reduction of
an acidity shift in the medium pH was analyzed in microtiter plates as
described previously (32). Twenty-five microliters of MAbs
(5 mg/ml) or sera was serially diluted in a microtiter plate.
Color-changing units (CCU), representing the number of mycoplasmas,
were determined by serial dilution with tubes containing phenol red.
One CCU of M. gallisepticum R strain in 150 µl of culture medium containing phenol red was added to each well.
When cells proliferated, the medium turned yellow because of the
presence of phenol red in the medium. After 3 days of incubation at
37°C, the color of the culture medium was checked. When the medium
remained red at the maximum dilution of antibodies, the concentration
was determined as the metabolism inhibition titer.
Flow cytometoric analysis.
For analysis of the expression of
a 120-kDa protein on the cell surface, 105 M. gallisepticum cells were incubated either with MAb
35A6 or control MAb 1AN86 (29) for 45 min on ice. After a
washing, the cells were incubated with fluorescein isothiocyanate
(FITC)-conjugated goat anti-mouse IgG (Pharmingen, San Diego, Calif.)
for 45 min on ice. After a second washing, the cells were analyzed by
FACScan (Becton Dickinson, San Jose, Calif.).
Preparation of polyclonal antisera.
For the preparation of
chicken polyclonal anti-M. gallisepticum R
strain serum, 5-week-old specific-pathogen-free chickens (line M;
Institute of Nippon Biological Science, Tokyo, Japan) were immunized
subcutaneously in the right thigh with 100 µg of M. gallisepticum R strain whole cells emulsified in
Freund's complete adjuvant. Two subsequent boosters of the same
antigen concentration in Freund's incomplete adjuvant were
administered at 2-week intervals. Sera were collected 2 weeks after the
final booster and used to immunoscreen an M. gallisepticum genomic DNA expression library.
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Identification and Expression of a Mycoplasma
gallisepticum Surface Antigen Recognized by a Monoclonal Antibody
Capable of Inhibiting Both Growth and Metabolism
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
20°C. The
immunoglobulin concentration of each ascites fluid was measured with a
IgG Mouse ELISA Quantitation Kit (Bethyl Laboratories, Inc.). The
immunoglobulin class and subclass were typed with the MonoAB-ID EIK kit
A (Zymed).
-mercaptoethanol, 0.1% bromophenol blue), heated in a boiling water
bath for 3 min, and stored at 20°C until used. Mycoplasma proteins
were separated by SDS-8% PAGE, and the gel was either stained with
Coomassie brilliant blue or electrophoretically transferred to
Immobilon Transfer Membrane (Millipore, Bedford, Mass.) for
immunoblotting. The membrane was treated with MAb 35A6 followed by
alkaline phosphatase-conjugated goat anti-mouse immunoglobulin G (IgG;
Promega, Madison, Wis.). Polypeptide bands recognized by the MAb were
visualized by using nitroblue tetrazolium chloride plus
5-bromo-4-chloro-3-indolyphosphate p-toluidine salt.
Construction and screening of an M. gallisepticum genomic DNA expression library.
M. gallisepticum genomic DNA was extracted
as described previously (15). The genomic DNA of M. gallisepticum R strain was partially digested with
AluI and size-selected (1 to 3 kb) DNA fragments were
ligated to 
gt11 arm DNA (Stratagene GmbH, Heidelberg, Germany) and
packaged using Gigapack gold packaging extract (Stratagene) according
to the manufacturer's instructions, resulting in a primary genomic
library with a size of 106 PFU. The library was
immunoscreened with chicken polyclonal anti-M. gallisepticum R strain serum. Positive clones were
pooled and reimmunoscreened with the mouse polyclonal
anti-120-kDa-protein serum.
DNA cloning and sequencing.
A gt11 phage DNA was
extracted from a plaque that reacted with the mouse polyclonal
anti-120-kDa-protein serum. An insert DNA fragment was amplified from
the phage DNA by PCR. To obtain a full-length gene encoding 120-kDa
protein, the PCR products were radiolabeled with
[
-32P]dCTP and used as a probe for Southern blot
analysis (28). DNA fragments identified by Southern blot
analysis were cloned into pUC18 by a standard procedure (2).
DNA sequencing was performed on double-stranded plasmid by the Dye
Terminator Cycle Sequencing FS Ready Reaction Kit (Applied Biosystems,
Inc., Foster City, Calif.). DNA sequence data was analyzed with the
GENETYX-MAC software package, as well as the GenBank and Swissprot
databases, for comparison of the 120-kDa protein predicted amino acid
sequence with database entries.
Replacement of TGA codons with TGG codons. To express the mgc3 gene by recombinant FPVs, all 10 TGA codons in the mgc3 gene were replaced with TGG codons using the PCR with a total of 15 primers. The sequence of each primer contains restriction enzyme recognition sites which are created without amino acid substitution. The PCRs were performed as described above except for the use of M11-1, M11-2, and M11-3 clones as templates (see Fig. 2). The PCR products were digested with appropriate restriction enzymes and then inserted into pUC18 to construct the altered mgc3 gene, designated pUC-MGC3.
Generation of recombinant FPVs. Transfer vector pNZ29RMGC3 was constructed by inserting a 3,228-bp BamHI-SphI fragment from pUC-MGC3 into the BamHI-SphI site of insertion vector pNZ1829R (24). Transfer vector pNZ29RMGC3-S was constructed by replacing the 5' terminus encoding the MGC3 predicted signal sequence with the 5' terminus encoding the MDV glycoprotein B (gB) signal sequence. The 5'-terminal fragment encoding MDV gB signal sequence was obtained from plasmid pNZ29RMDgB (35) by PCR using primers pgB-1 (5'-CCCCAGGATCCAATCATGCACTATTTTAGG-3'; a BamHI site is underlined) and pgB-2 (5'-CCCCCAGAGCTCCTCGAGATGTCACATTTTGGGTACTCGGAGA-3'; a newly created SacI site is underlined). This set of primers had a restriction site flanked by five additional bases to protect the site and facilitate enzyme digestion. Transfer vector pNZ29RMGC3-S was constructed by replacing a 67-bp BamHI-SacI fragment from pNZ29RMGC3 with a 105-bp BamHI-SacI fragment of the PCR products. The procedure for transfection of FPV-infected cells with the transfer vectors by electroporation and generation of recombinant FPVs was described previously (24, 35). The resulting FPVs were designated recFPV-MGC3 and recFPV-MGC3-S.
Expression of the mgc3 gene by recombinant FPVs. (i) Immunoprecipitation. CEF cells were infected with recombinant FPVs at a multiplicity of infection of 5 PFU/cell. Cell labeling with [35S]methionine and immunoprecipitation with MAb 35A6 were performed as described previously (38).
(ii) Endo H treatment. Immunoprecipitated proteins were digested with endoglycosidase H (Endo H; Boehringer-Mannheim) and PNGase F (Boehringer-Mannheim) as described previously (38).
(iii) Immunofluorescence.
Indirect immunofluorescence was
performed on monolayers of CEF cells grown on eight-chambered tissue
culture slides (Miles Scientific, Division of Miles Laboratories, Inc.,
Naperville, Ill.) infected with recombinant FPVs. At 16 h
postinfection, cells were fixed with 100% methanol at 20°C for 10 min or with 3% paraformaldehyde in phosphate-buffered saline (PBS) for
15 min and then blocked with 4% bovine serum albumin in PBS. The
slides were incubated with MAb 35A6 for 1 h at room temperature.
Bound MAb was detected with FITC-conjugated goat anti-mouse IgG (Life
Technologies, Inc.) by fluorescence microscopy.
Nucleotide sequence accession number. The nucleotide sequence of the mgc3 gene has been deposited with GenBank under accession number AB023292.
| |
RESULTS |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Production of MAbs capable of inhibiting growth and
metabolism.
Hybridoma supernatants derived from mice immunized
with whole M. gallisepticum R strain were
screened by ELISA. Hybridoma cells secreting high levels of antibodies
to M. gallisepticum R strain were selected
to produce ascites fluids. The growth inhibition and
metabolic-inhibition activities against M. gallisepticum R strain by the representative MAbs
are shown in Table 1. MAbs 30G8, 35A6,
and 34H1 had very strong growth inhibition activities. The percentages
of cell growth in the presence of these MAbs compared with control MAb
1AN86 are even less than 0%, indicating that these MAbs inhibit cell
multiplication completely for 3 days after incubation. The highest
metabolic inhibition was obtained in the presence of MAb 35A6. On the
other hand, MAbs 30G8 and 34H1 that strongly inhibited M. gallisepticum growth were less effective in
inhibiting metabolism of the organism than MAb 35A6. As a positive control, the mouse polyclonal anti-M.
gallisepticum R strain serum displayed a modest
level of both growth inhibition and metabolic-inhibition activities,
whereas normal mouse serum or a control MAb, 1AN86, did not have growth
inhibition and metabolic-inhibition activities. MAb 35A6 is a IgG2a
isotype, and it recognizes the multiple bands with molecular sizes
(Mr) of 105 to 120 kDa from a M. gallisepticum lysate (Fig.
1). The prominent band in the complexity
of the binding pattern is a 120-kDa protein. Thus, we found MAb 35A6 to
be a valuable tool for the identification of immunogenic antigens of M. gallisepticum.
|
|
Cloning of a gene encoding 120-kDa protein.
In an attempt to
identify a gene encoding a 120-kDa protein, a gt11 genomic DNA
library of M. gallisepticum was constructed. In an earlier study, no positive clone was obtained by immunoscreening with MAb 35A6 from the library. Since the most outstanding feature in
the codon usage of mycoplasma species is that the TGA stop codon is
utilized for tryptophan (34), a gene encoding an epitope recognized by the MAb would never be obtained from the
Escherichia coli expression system, such as a gt11
library, if the epitope is located on or following TGA codons unless an
opal suppressor mutant is used (21). We therefore made a
mouse polyclonal anti-120-kDa-protein serum because the polyclonal
antiserum was considered to be more reliable. As expected, the
polyclonal antiserum had both growth inhibition and
metabolic-inhibition activities (Table 1). By immunoscreening with
chicken polyclonal anti-M. gallisepticum R
strain serum, which had both growth inhibition and metabolic-inhibition activities (Table 1), 100 positive clones were obtained from the
library. Of these clones, a single positive clone (#100), which
contained an insertion of 2.8 kb, was obtained by reimmunoscreening with the mouse polyclonal anti-120-kDa-protein serum. In fact, the
#100 clone did not react with MAb 35A6.
|
Analysis of deduced amino acid sequence.
The nucleotide
sequence of a 4-kbp fragment containing the #100 insert DNA has an
ORF which comprises 3,186 bp, and the predicted primary translation
products would be a protein of 1,062 amino acids with a predicted size
of 115.8 kDa. The gene has 10 TGA codons encoding tryptophan.
Hydropathic analysis indicates that the protein contains characteristic
features of membrane proteins, namely, a 5' hydrophobic signal sequence
at the N-terminal end between positions 1 and 22, an external
hydrophilic surface domain, a hydrophobic membrane-spanning domain, and
a basic, highly charged cytoplasmic domain (data not shown). The
predicted size of the gene product following a signal sequence cleavage
(113.5 kDa) is in good agreement with the 120-kDa protein as estimated
by SDS-PAGE.
|
Cell surface localization of MGC3 protein in M. gallisepticum.
On the basis of the predicted amino
acid sequence of the mgc3 gene, MGC3 protein was expected to be located
on the cell surface as a membrane protein. To address this, the freshly
harvested organisms were treated with MAb 35A6 and analyzed for cell
surface expression by flow cytometry. Strong immunofluorescent staining was detected when MAb 35A6 was used (Fig.
4). This observation is consistent with
the previous report that the ORF6 gene product was a
membrane-associated protein expressing a surface-exposed region
(18).
|
Reactivities of MAb 35A6 for different strains.
MGC3 protein
was affinity-purified with MAb 35A6 and inoculated into mice to produce
a polyclonal antiserum to this protein. These sera were found to have
high antibody titers against M. gallisepticum and also inhibited the growth and
metabolism of M. gallisepticum in vitro
(Table 1). To examine the reactivity of MAb 35A6 with other strains,
Western blotting analysis was performed on M. gallisepticum strains R, S6, F, and KP13. M. gallisepticum R, S6, and KP13 possessed the
120-kDa protein as recognized by MAb 35A6, whereas M. gallisepticum F strain, an avirulent vaccine strain, was not recognized (Fig. 5A). In
the case of M. pneumoniae, mutant missing 130-kDa protein is
avirulent (8). In view of the relationship between the lack
of MGC3 protein and avirulence, it was of interest to examine whether
M. gallisepticum F strain possesses MGC3
protein. For this purpose, the mouse polyclonal anti-MGC3 protein serum
was used to detect MGC3 protein by Western blotting. The 120-kDa
proteins were detected in all strains tested, including the F strain
(Fig. 5B), indicating that the F strain possesses MGC3 protein without
the epitope for MAb 35A6.
|
Expression of the mgc3 gene by using recombinant FPVs in CEF
cells.
Whereas the antigen can be affinity purified using MAb 35A6
from M. gallisepticum R strain lysate, only
a limited amount of the antigen was obtained by this method. Therefore,
an alternative strategy, which we have chosen, was the use of
recombinant DNA techniques to determine the gene for the protective
immunogen and to generate a recombinant FPV for analysis of the
expression. All 10 TGA codons in the mgc3 gene were replaced with TGG
codons by PCR using 15 primers. A recombinant FPV, recFPV-MGC3 encodes the full-length mgc3 gene under the control of a strong synthetic pox
promoter (35). Another recombinant FPV, recFPV-MGC3-S,
encodes the mgc3 gene fused to the MDV gB signal sequence in the place of its native signal sequence. The mgc3 gene products were synthesized in CEF cells infected with the recombinant FPVs and were characterized by immunoprecipitation with MAb 35A6 (Fig.
6). A 120-kDa protein was found in CEF
cells infected with recFPV-MGC3 (lane 2), which migrated to the same
position as native MGC3 protein of M. gallisepticum. In contrast, an approximately
50-fold-higher level of expression of a protein of 145 kDa was seen in
CEF cells infected with recFPV-MGC3-S (lane 5). Both 120- and 145-kDa
proteins were also recognized by MAb 34H1 with growth inhibition
activity (data not shown). No specific band was observed in the parent
FPV-infected CEF cells (lane 1). These results clearly demonstrated
that the mgc3 gene product possesses growth inhibition and
metabolic-inhibiting epitopes recognized by MAbs 35A6 and 34H1.
|
N-linked carbohydrate modification of MGC3 in recFPV-infected cells. To address the size differences between MGC3 proteins expressed by recFPV-MGC3 and recFPV-MGC-S, these immunoprecipitated proteins were treated with endoglycosidases. In recFPV-MGC3-infected cells, no mobility shifts was observed in MGC3 protein either after Endo H or PNGase F treatment (Fig. 6, lanes 3 and 4), whereas a mobility shift was observed at from 145- to 120 kDa after Endo H and PNGase F treatments in recFPV-MGC3-S-infected cells (Fig. 6, lanes 6 and 7). This result demonstrated that the size differences were due to the posttranslational modifications, and the 145-kDa protein expressed by recFPV-MGC3-S was the simple high-mannose type. There are 15 potential N-linked glycosylation sites in MGC3 protein. The altered mobility shift indicated that 10 to 13 glycosylation sites of MGC3 protein are N linked with high-mannose carbohydrates, assuming an increase in size of 1,000 to 2,000 Da per glycosylation. Thus, using FPV expression system, the protective epitopes on MGC3 protein recognized by the MAbs capable of inhibiting both growth and metabolism were unaffected by N-linked glycosylation.
Cell surface localization of MGC3 in recombinant FPV-infected
cells.
Expression of MGC3 protein on the cell surface might also
play an important role in humoral immunity because this protein elicits
growth-inhibiting antibodies. To assess whether MGC3 protein expressed
by recombinant FPV is transported to the cell surface, an
immunofluorescent analysis was performed with MAb 35A6. Strong cell
surface immunofluorescence was observed on the recFPV-MGC3-S-infected cells, whereas only a faint signal was detected on the
recFPV-MGC3-infected cells (Fig. 7). This
result showed that MGC3 protein was transported to the cell surface by
replacing with the MDV gB signal peptide.
|
| |
DISCUSSION |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
This study describes the identification of a gene encoding an epitope recognized by MAb 35A6 which is capable of inhibiting both the growth and metabolism of M. gallisepticum in vitro. The gene, designated the mgc3 gene, is a homologue of the ORF6 gene in the P1 operon of M. pneumoniae and is located downstream of the mgc1 gene. The two genes of the P1 operon of M. gallisepticum have been identified as the mgc1 and mgc2 genes homologous to the P1 and ORF4 genes, respectively (15, 11). MGC3 protein encoded by the mgc3 gene may function as a cytoadherence-associated molecule because the M. pneumoniae 130-kDa protein has been implicated in the cellular adhesion process (8).
A striking homology at the amino acid level was found in the C terminus among 130-kDa protein homologues, where the regions might function as a membrane spanning and anchoring. This result implies that there is a similarity in membrane structure among the mycoplasmas. On the other hand, the sequence diversity at N-terminal region might reflect differences in mycoplasma receptor proteins found on the surfaces of human and avian epithelial cells. We found a couple of differences with regard to gene expression and organization between M. gallisepticum and M. pneumoniae. The 130-kDa protein is co- or posttranslationally cleaved to 40- and 90-kDa proteins and is located on the cell surface as a membrane-associated protein (18). In addition, the ORF6 gene carries repetitive DNA sequences (RepMP5) which are dispersed as multiple copies on the chromosome, suggesting that gene conversion between the multiple-copy regions results in antigen variation (26). In contrast to the ORF6 gene, the mgc3 gene exists as a single chromosomal copy, and the gene product does not seem to be cleaved.
We have developed a recombinant FPV expression system to examine its potential to protect against avian diseases. For example, immunization with a recombinant FPV expressing the MDV gB gene elicited neutralizing antibodies in chickens, resulting in protection against a lethal MDV challenge (23). In addition, gB antigen expressed by the recombinant FPV was located on the cell surface (39). We therefore used not only this recombinant FPV expression system but also the gB signal sequence for cell surface expression. To assess the characteristics of MGC3 protein in its host cells, all of the TGA codons in the mgc3 gene, which encode a tryptophan in Mycoplasma species, were replaced with TGG codons. Additionally, recombinant FPVs harboring the altered mgc3 gene were constructed. Replacement of the natural signal sequence of MGC3 protein with the MDV gB signal sequence improved not only the transportation of MGC3 protein with a growth inhibiting and metabolic-inhibiting epitope to the cell surface but also the expression level of MGC3 protein. Although MGC3 protein expressed by recFPV-MGC3-S underwent N-linked glycosylation and would not be the native form in M. gallisepticum, the protective epitopes recognized by MAbs 35A6 and 34H1 were successfully expressed on the surface of its host cells. It is likely that surface-exposed epitopes which induce a neutralizing immune response should increase its immunogenicity. In addition, the MDV gB signal peptide could provide a good model system to express a gene derived from bacteria such as mycoplasma on the eukaryotic cell surface.
Our findings provide the first demonstration that MGC3 protein contains epitopes which can induce antibodies responsible for growth inhibition and metabolic-inhibition activities and is expressed on the cell surface in the recombinant FPV expression system. It is possible that the induction of antibodies to the epitopes recognized by the MAbs in chickens can result in protective immune responses against M. gallisepticum challenge. We are in the process of investigating recombinant FPV-based vaccines for the protection of chickens against M. gallisepticum infection.
| |
ACKNOWLEDGMENTS |
|---|
We thank A. Yasuda for DNA sequencing and B. Cowen for critical review of the manuscript. We especially thank K. Kamogawa and N. Yanagida for encouragement and support of this study.
| |
ADDENDUM |
|---|
The 5'-terminal regions of the mgc3 genes of M. gallisepticum F, S6, and KP13 strains were cloned by PCR and partially sequenced from the ATG start codon to nucleotide position 1,130 downstream of the start codon. An alignment of the mgc3 genes of the four strains revealed that the DNA sequences of M. gallisepticum R and KP13 were identical and that the DNA sequence homologies between strains R and S6 and between strains R and F are 93.1 and 89.7%, respectively. The partial nucleotide sequences of the mgc3 genes of M. gallisepticum F and S6 strains will appear in the DDBJ/EMBL/GenBank nucleotide sequence databases with the accession numbers AB033210 and AB033211, respectively.
| |
FOOTNOTES |
|---|
* Corresponding authors. Mailing address for A.F.: Life Science Laboratory, Research and Development Center, Nippon Zeon Co., Ltd, 1-2-1 Yako, Kawasaki-ku, Kawasaki 210-8507, Japan. Phone: 81-44-276-3744. Fax: 81-44-276-3766. E-mail: ayuchan{at}zeon.co.jp. Present address for S.Y.: Department of Medical Zoology, Jichi Medical School, 3311-1 Yakushiji Minamikawachimachi, Tochigi 329-0498, Japan. Phone: 81-285-58-7339. Fax: 81-285-44-6489. E-mail: shigeto{at}jichi.ac.jp.
Editor: W. A. Petri Jr.
| |
REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
| 1. | Abd-El-Motelib, T. Y., and S. H. Kleven. 1993. A comparative study of Mycoplasma gallisepticum vaccines in young chickens. Avian Dis. 37:981-987[CrossRef][Medline]. |
| 2. | Ausubel, F. A., R. Brent, R. E. Kingston, D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1986. Current protocols in molecular biology. Greene Publishing Associates and Wiley-Interscience, New York, N.Y. |
| 3. | Avakian, A. P., and D. H. Ley. 1993. Protective immune response to Mycoplasma gallisepticum demonstrated in respiratory-tract washings from M. gallisepticum-infected chickens. Avian Dis. 37:697-705[CrossRef][Medline]. |
| 4. | Carter, P. B., K. H. Beegle, and D. H. Gebhard. 1986. Monoclonal antibodies: clinical uses and potential. Vet. Med. Small Anim. Clin. 16:1171-1179. |
| 5. |
Chanock, R. M.,
L. Hayflick, and M. D. Barile.
1962.
Growth on artificial medium of an agent associated with atypical pneumonia and its identification as a PPLO.
Proc. Acad. Natl. Sci. USA
48:41 |
| 6. | Devereux, J., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395. |
| 7. | Evans, R. D., and Y. S. Hafez. 1992. Evaluation of a Mycoplasma gallisepticum strain exhibiting reduced virulence for prevention and control of poultry mycoplasmosis. Avian Dis. 36:197-201[CrossRef][Medline]. |
| 8. |
Franzoso, G.,
P. C. Hu,
G. A. Meloni, and M. F. Barile.
1993.
The immunodominant 90-kilodalton protein is localized on the terminal tip structure of Mycoplasma pneumoniae.
Infect. Immun.
61:1523-1530 |
| 9. |
Fraser, C. M.,
J. D. Gocayne,
O. White,
M. D. Adams,
R. A. Clayton,
R. D. Fleischmann,
C. J. Bult,
A. R. Kerlavage,
G. Sutton,
J. M. Kelley,
J. L. Fritchman,
J. F. Weidman,
K. V. Small,
M. Sandusky,
J. Fuhrmann,
D. Nguyen,
T. R. Utterback,
D. M. Saudek,
C. A. Phillips,
M. Merrick,
J. Tomb,
B. A. Dougherty,
K. F. Bott,
P. Hu,
T. S. Lucier,
S. N. Peterson,
H. O. Smith,
C. A. Hutchison III, and J. C. Venter.
1995.
The minimal gene complement of Mycoplasma genitalium.
Science
270:397-403 |
| 10. | Garcia, M., and S. H. Kleven. 1994. Expression of Mycoplasma gallisepticum F-strain surface epitope. Avian Dis. 38:494-500[CrossRef][Medline]. |
| 11. |
Hnatow, L. L.,
C. L. Keeler, Jr.,
L. L. Tessmer,
K. Czymmek, and J. E. Dohms.
1998.
Characterization of MGC2, a Mycoplasma gallisepticum cytadhesin with homology to the Mycoplasma pneumoniae 30-kilodalton protein P30 and Mycoplasma genitalium P32.
Infect. Immun.
66:3436-3442 |
| 12. | Inamine, J. M., S. Loechel, and P. C. Hu. 1988. Analysis of the nucleotide sequence of the P1 operon of Mycoplasma pneumoniae. Gene 73:175-183[CrossRef][Medline]. |
| 13. | Iritani, Y., S. Aoyama, S. Takigami, Y. Hayashi, R. Ogawa, N. Yanagida, S. Saeki, and K. Kamogawa. 1991. Antibody response to Newcastle disease virus (NDV) of recombinant fowlpox virus (FPV) expressing a hemagglutinin-neuraminidase of NDV into chickens in the presence of antibody to NDV or FPV. Avian Dis. 35:659-661[CrossRef][Medline]. |
| 14. | International Committee on Systematic Bacteriology and Subcommittee on the Taxonomy of Mollicutes. 1979. Proposal for minimal standards for description of new species of the class Mollicutes. Int. J. Syst. Bacteriol. 29:172-180. |
| 15. | Keeler, C. L., Jr., L. L. Hnatow, P. L. Whetzel, and J. E. Dohms. 1996. Cloning and characterization of a putative cytadhesin gene (mgc1) from Mycoplasma gallisepticum. Infect. Immun. 64:1541-1547[Abstract]. |
| 16. | Khan, M. I., K. M. Lam, and R. Yamamoto. 1987. Mycoplasma gallisepticum strain variations detected by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Avian Dis. 31:315-320[CrossRef][Medline]. |
| 17. | Layh-Schmitt, G., and M. Harkenthal. 1999. The 40- and 90-kDa membrane proteins (ORF6 gene product) of Mycoplasma pneumoniae are responsible for the tip structure formation and P1 (adhesin) association with the Triton shell. FEMS Microbiol. Lett. 174:143-149[CrossRef][Medline]. |
| 18. |
Layh-Schmitt, G., and R. Herrmann.
1992.
Localization and biochemical characterization of the ORF6 gene product of the Mycoplasma pneumoniae P1 operon.
Infect. Immun.
60:2906-2913 |
| 19. | Levisohn, S. 1984. Early stages in the interaction between Mycoplasma gallisepticum and the chick trachea, as related to pathogenicity and immunogenicity. Isr. J. Med. Sci. 20:982-984[Medline]. |
| 20. | Lin, M. Y., and S. H. Kleven. 1982. Pathogenicity of two strains of Mycoplasma gallisepticum in turkeys. Avian Dis. 26:360-364[CrossRef][Medline]. |
| 21. | Minion, F. C., C. Van Dyk, and B. K. Smiley. 1995. Use of an enhanced Escherichia coli opal suppressor strain to screen a Mycoplasma hyopneumoniae library. FEMS Microbiol. Lett. 131:81-85[CrossRef][Medline]. |
| 22. | Nazerian, K., S. Dhawale, and W. S. Payne. 1989. Structural proteins of two different plaque-size phenotypes of fowlpox virus. Avian Dis. 33:458-465[CrossRef][Medline]. |
| 23. |
Nazerian, K.,
L. F. Lee,
N. Yanagida, and R. Ogawa.
1992.
Protection against Marek's disease by a fowlpox virus recombinant expressing the glycoprotein B of Marek's disease virus.
J. Virol.
66:1409-1413 |
| 24. | Ogawa, R., N. Yanagida, S. Saeki, S. Saito, S. Ohkawa, H. Gotoh, K. Kodama, K. Kamogawa, K. Sawaguchi, and Y. Iritani. 1990. Recombinant fowlpox viruses inducing protective immunity against Newcastle disease and fowlpox viruses. Vaccine 8:486-490[CrossRef][Medline]. |
| 25. | Rodriguez, R., and S. H. Kleven. 1980. Pathogenicity of two strains of Mycoplasma gallisepticum in broilers. Avian Dis. 24:800-807[CrossRef][Medline]. |
| 26. |
Ruland, K.,
R. Himmelreich, and R. Herrmann.
1994.
Sequence divergence in the ORF6 gene of Mycoplasma pneumonia.
J. Bacteriol.
176:5202-5209 |
| 27. | Saito, S., A. Fujisawa, S. Ohkawa, N. Nishimura, T. Abe, K. Kodama, K. Kamogawa, S. Aoyama, Y. Iritani, and Y. Hayashi. 1993. Cloning and DNA sequence of a 29 kilodalton polypeptide gene of Mycoplasma gallisepticum as a possible protective antigen. Vaccine 11:1061-1066[CrossRef][Medline]. |
| 28. | Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. |
| 29. | Silva, R. F., and L. F. Lee. 1984. Monoclonal antibody-mediated immunoprecipitation of proteins from cells infected with Marek's disease virus or turkey herpesvirus. Virology 136:307-320[CrossRef][Medline]. |
| 30. | Sperker, B., P. Hu, and R. Herrmann. 1991. Identification of gene products of the P1 operon of Mycoplasma pneumoniae. Mol. Microbiol. 5:299-306[CrossRef][Medline]. |
| 31. | Sundquist, B. G., G. Czifra, and L. Stipkovits. 1996. Protective immunity induced in chicken by a single immunization with Mycoplasma gallisepticum immunostimulating complexes (ISCOMS). Vaccine 14:892-897[CrossRef][Medline]. |
| 32. | Taylor-Robinson, D., and D. M. Berry. 1969. The measurement of antibody to Mycoplasma gallisepticum by the metabolic-inhibition technique. J. Gen. Microbiol. 56:3[Medline]. |
| 33. | Tully, J. G. 1983. Cloning and filtration techniques for mycoplasmas, p. 173-177. In S. Razin, and J. G. Tully (ed.), Methods in mycoplasmology, vol. I. Academic Press, New York, N.Y. |
| 34. |
Yamao, F.,
A. Muto,
Y. Kawauchi,
M. Iwami,
S. Iwagami,
Y. Azumi, and S. Osawa.
1985.
UGA is read as tryptophan in Mycoplasma capricolum.
Proc. Natl. Acad. Sci. USA
82:2306-2309 |
| 35. |
Yanagida, N.,
R. Ogawa,
Y. Li,
L. F. Lee, and K. Nazerian.
1992.
Recombinant fowlpox viruses expressing the glycoprotein B homolog and the pp38 gene of Marek's disease virus.
J. Virol.
66:1402-1408 |
| 36. | Yoder, H. W., Jr. 1991. Mycoplasma gallisepticum infection, p. 198-212. In B. W. Calnek, H. J. Barnes, C. W. Beard, W. M. Reid, and H. W. Yoder, Jr. (ed.), Diseases of poultry, 9th ed. Iowa State University Press, Ames, Iowa. |
| 37. | Yoder, H. W., Jr., S. R. Hopkins, and B. W. Mitchell. 1984. Evaluation of inactivated Mycoplasma gallisepticum oil-emulsion bacterins for protection against airsacculitis in broilers. Avian Dis. 28:224-234[CrossRef][Medline]. |
| 38. | Yoshida, S., L. R. Lee, N. Yanagida, and K. Nazerian. 1994. The glycoprotein B genes of Marek's disease virus serotypes 2 and 3: identification and expression by recombinant fowlpox viruses. Virology 200:484-493[CrossRef][Medline]. |
| 39. | Yoshida, S., L. F. Lee, N. Yanagida, and K. Nazerian. 1994. Mutational analysis of the proteolytic cleavage site of glycoprotein B (gB) of Marek's disease virus. Gene 150:303-306[CrossRef][Medline]. |
| 40. | Whithear, K., G. Soeripto, K. E. Harrigan, and E. Ghiocas. 1990. Immunogenicity of a temperature-sensitive mutant Mycoplasma gallisepticum vaccine. Aust. Vet. J. 67:159-165[Medline]. |
Infection and Immunity, June 2000, p. 3186-3192, Vol. 68, No. 6
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
This article has been cited by other articles:
-
Brown, D. R., Whitcomb, R. F., Bradbury, J. M.
(2007). Revised minimal standards for description of new species of the class Mollicutes (division Tenericutes). Int. J. Syst. Evol. Microbiol.
57: 2703-2719
[Abstract] [Full Text] -
Mudahi-Orenstein, S., Levisohn, S., Geary, S. J., Yogev, D.
(2003). Cytadherence-Deficient Mutants of Mycoplasma gallisepticum Generated by Transposon Mutagenesis. Infect. Immun.
71: 3812-3820
[Abstract] [Full Text] -
Winner, F., Markova, I., Much, P., Lugmair, A., Siebert-Gulle, K., Vogl, G., Rosengarten, R., Citti, C.
(2003). Phenotypic Switching in Mycoplasma gallisepticum Hemadsorption Is Governed by a High-Frequency, Reversible Point Mutation. Infect. Immun.
71: 1265-1273
[Abstract] [Full Text] -
Malembic, S., Saillard, C., Bove, J. M., Garnier, M.
(2002). Effect of Polyclonal, Monoclonal, and Recombinant (Single-Chain Variable Fragment) Antibodies on In Vitro Morphology, Growth, and Metabolism of the Phytopathogenic Mollicute Spiroplasma citri. Appl. Environ. Microbiol.
68: 2113-2119
[Abstract] [Full Text]
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Copyright © 2009 by the American Society for Microbiology. For an alternate route to Journals.ASM.org, visit: http://intl-journals.asm.org | More Info»