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Previous Article | Next Article 
Infection and Immunity, October 2001, p. 6030-6037, Vol. 69, No. 10
Veterinary Infectious Disease Organization,
Saskatoon, Saskatchewan,1 and
Canadian Bacterial Diseases Network,
Calgary,2 Canada
Received 4 May 2001/Returned for modification 20 June
2001/Accepted 12 July 2001
The mig gene of Streptococcus
dysgalactiae, a major bovine mastitis pathogen,
encodes two plasma protein-binding receptors, The Lancefield serological group C
bacterium Streptococcus dysgalactiae is one of the most
common pathogens of bovine mastitis and causes large economic losses in
the dairy industry. It is capable of survival in the mouth, vagina, and
skin of healthy animals as well as bedding and pastures
(32). Because of its environmental location, normal
hygiene methods and antibiotic therapy are less effective in preventing
S. dysgalactiae infections than infections with other
contagious pathogens. Therefore, an effective way to prevent
S. dysgalactiae mastitis might be to identify conserved
potential virulence factors expressed on the cell surface as targets
for vaccines.
S. dysgalactiae expresses various receptors on its cell
surface that bind to host-derived proteins such as immunoglobulin G
(IgG), The other receptor present in the Mig protein binds to the universal
protease inhibitor In this study, the degree of conservation of DNA regions encoding the
Bacterial strains and media.
The Lancefield group C
S. dysgalactiae isolates ATCC 43078, renamed SDG8 in
this study, and ATCC 27957 were obtained from the American Type Culture
Collection. Other S. dysgalactiae strains isolated from
milk of cows with mastitis were kindly provided by M. Chirino-Trejo,
University of Saskatchewan, and by Agriculture Development and
Marketing, Winnipeg, Manitoba, Canada. The clinical isolates were
identified by the API 20 Strep diagnostic kit (BioMérieux, Quebec, Canada) and analyzed by APILAB Plus software provided by the
same supplier. Escherichia coli strain DH5
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.10.6030-6037.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Surface-Expressed Mig Protein Protects
Streptococcus dysgalactiae against Phagocytosis by
Bovine Neutrophils
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
2-macroglobulin (2-M) and immunoglobulin
G (IgG). In this study, the mig gene from one
S. dysgalactiae isolate was cloned and expressed in
Escherichia coli. The IgG receptor region encoded by
mig was conserved in 16 S.
dysgalactiae strains. An isogenic mig mutant was
constructed by allele replacement mutagenesis of the wild-type gene in
S. dysgalactiae. The IgG-binding activity was lost
in the mig mutant strain, whereas the 2-M
receptor activity was still expressed but was detected only in the
culture supernatant. In flow cytometry phagocytosis and
bacterial-colony-counting bactericidal assays, the wild-type strain was
found to be significantly more resistant to phagocytosis and killing by
bovine neutrophils (PMNs) than the mig mutant strain
when bacteria were preincubated with bovine serum. We therefore
speculate that the Mig protein of S. dysgalactiae
plays a role in virulence of the bacteria by binding to the plasma
protein 2-M or IgG and thus preventing phagocytosis by
bovine PMNs.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
2-macroglobulin
(2-M), albumin, fibronectin, fibrinogen, collagen, vitronectin, and plasminogen (5, 23, 30). These receptors mediate the interaction between the host and the bacterium, and therefore they might be involved in the adhesion or invasion to the
host cells or in resistance to the host defense system. Two of these
receptors, IgG and 2-M, have been identified
in a surface-expressed protein, designated Mig (12). The
IgG receptor expressed by Mig belongs to the type III IgG-binding
receptor family, and its sequence shares homology with other type III
IgG receptors. However, in contrast to the two or three repeated
domains in the extensively studied protein G in the human group C and G
streptococci (2, 25, 27), the IgG-binding region of Mig contains five repeats and it binds goat IgG via both the Fc and Fab
domains (31). Although the role of the IgG receptor of Mig in S. dysgalactiae virulence is unclear, the IgG
receptor of the group A streptococcus (GAS) strains has been found to
be involved in virulence in a mouse skin infection model
(21).
2-M, but only to the
complex form (fast form) of 2-M, the
2-M-trypsin complex (2-M-T). This is in
contrast to the 2-M receptor in GAS, which
binds only to the native form (slow form) of
2-M (1, 16). The DNA sequence encoding the 2-M receptor portion of the
mig gene is different from other streptococcus
surface-expressed 2-M receptors, such as Mag
in S. dysgalactiae (10), Zag in
Streptococcus zooepidemicus (11), and protein G
from human group G streptococci (17, 28). Recently, a
novel 2-M receptor, carried by the protein
G-related 2-M-binding protein (Grab) from
human GAS strains was found to be more virulent than the
Grab
mutant in a mouse infection model
(24). Furthermore, the 2-M bound
to the bacterial surface via Grab was still capable of inhibiting the
activity of proteases, thereby protecting important virulence factors
from proteolytic degradation (24). Another role for the
2-M receptor was found in S. dysgalactiae, where the binding of 2-M-T
to S. dysgalactiae cells interferes with
phagocytosis by bovine neutrophils (PMNs), but the specific
2-M receptor was not identified in that study
(29).
2-M- and IgG-binding regions of Mig was
assessed by Southern blot analyses of genomic DNA from several
S. dysgalactiae isolates. In addition, a mig
mutant strain was constructed by allele replacement mutagenesis in
S. dysgalactiae, and its ability to resist phagocytosis
and killing by bovine PMNs was investigated in a parallel analysis with
the wild-type strain. We report here that the IgG receptor region
encoded by mig was conserved in 16 S. dysgalactiae strains, while the mig
2-M region was present in 5 strains only.
Furthermore, we found that the wild-type strain was more resistant to
the phagocytosis and killing by bovine PMNs than the mig
mutant strain in the presence of serum. This mechanism of resistance to
phagocytosis is probably mediated by the binding of
2-M-T to the 2-M
receptor and not to binding of IgG to the IgG receptor of Mig.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
[
80dlacZ
M15 recA1 endA1
gyrA96 thi-1 hsdR17 supE44
relA1 deoR
(lacZYA-argF)U169] and cloning vectors
pBluescript II KS, pPCR-Script, and pAA505 were from laboratory
collections. The temperature-sensitive shuttle vector pEU904 was
a generous gift from June R. Scott, Emory University, Atlanta, Ga.
DNA preparations. Plasmid DNA was prepared with the Qiagen plasmid kit (Qiagen GmbH, Hilden, Germany). S. dysgalactiae genomic DNA was prepared by a modification of the method provided by Qiagen (Qiagen genomic DNA handbook). Briefly, bacteria grown in 50 ml of THY were harvested by centrifugation and then washed once in 0.1 M phosphate-buffered saline buffer (PBS), pH 7.2. The bacterial pellets were suspended in 11 ml of buffer B1 (50 mM Tris HCl, pH 8.0; 50 mM EDTA, pH 8.0; 0.5% Tween-20; 0.5% Triton X-100), and the following enzymes (Sigma) were added to the pellet suspensions: 20 µl of RNase A (100 mg/ml), 50 µl of hyaluronidase (34 mg/ml), 150 µl of lysozyme (100 mg/ml), 150 µl of proteinase K (50 mg/ml), and 30 µl of mutanolysin (10,000 U/ml). The suspension was incubated overnight at 37°C until it became clear. Four milliliters of buffer B2 (3 M guanidine HCl, 20% Tween-20) was added and mixed by vortex prior to another incubation for 30 min at 50°C. The genomic DNA was precipitated with 0.7 volume of isopropanol, spooled with a glass rod, washed three times with 70% ethanol, and dissolved in 2 ml of 10 mM Tris-HCl (pH 8.0).
Transformation. Transformation and electroporation of E. coli strains were performed with standard methods by using either RbCl-treated (Qiagen) or CaCl2-treated (26) competent cells. Alternatively, plasmid DNA was transformed into polyethylene glycol-treated E. coli as described previously (14). Preparation of competent cells of S. dysgalactiae and electroporation were carried out as described previously (19).
PCR.
Oligonucleotides (Table
1; Fig. 1)
used for cloning and sequencing of the mig gene from the
S. dysgalactiae strain SDG8 were basically selected
from the published mig sequence from the S. dysgalactiae strain SC1 (12) and synthesized either
at the Veterinary Infectious Disease Organization or by Gibco Life
Technologies (Burlington, Ontario, Canada). Taq DNA
polymerase and deoxynucleoside triphosphates were obtained from
Amersham Pharmacia Biotech (Piscataway, N.J.). PCR amplification was
performed for 35 cycles of 45 s at 94°C, 45 s at 55°C,
and 1 min at 72°C with an initial denaturation step of 3 min at
95°C and a final extension of 5 min at 72°C.
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Plasmids and strain constructions. Restriction endonucleases and T4 DNA ligase were obtained from Amersham Pharmacia Biotech, and the molecular weight standard was from MBI Fermentas (Vilnius, Lithuania). Plasmid DNA bands were purified from agarose gels by using a Geneclean spin kit (Bio101, Vista, Calif.). To isolate the mig gene from S. dysgalactiae strain SDG8, PCR fragments were amplified from chromosomal DNA and cloned into different vectors. The inserts present in each construct are shown in Fig. 1. The vectors used were pAA505 (p5Me and p5Me-Sp), pBluescript II KS (pKSMig-3 and pMC-5e), pPCR-Script (pPMig2-8), and pEU904 (pMig-1).
pMig-1 was transformed into S. dysgalactiae strain SDG8 by electroporation; clones in which a double crossover took place were selected by varying the incubation temperatures and examining the resistance to antibiotics (19).Southern blots.
Briefly, 5 µg of genomic DNA was cleaved
with HindIII, separated in a 1.0% agarose gel,
transferred to nylon membranes (Zeta-Probe GT; Bio-Rad) by capillary
blotting, and fixed by baking the blot at 80°C for 30 min. The DNA
probe 2-M-1, specific to the
2-M-binding region of mig, was a
330-bp PCR fragment amplified from the SDG8 genomic DNA with Mig-3 and
Mig-4 primers and digested with XmnI, which cleaves within
the 2-M coding region (Fig. 1). This probe was
used to check the allele replacement of the mig gene in the Mig8-Mt strain. The SP resistance (Sp)- and EM resistance (Em)-specific probes were a 1.2-kb ClaI-EcoRI fragment and a
0.9-kb EcoRI-SacI fragment of pEU904,
respectively. Approximately 25 ng of the above gel-purified DNA
fragments were randomly labeled with [32P]dCTP
by using a rediprimeII labeling kit (Amersham Pharmacia Biotech). The prehybridizations and hybridizations were done in a
buffer containing 0.25 M sodium phosphate (pH 7.2)-7% sodium dodecyl
sulfate (SDS) at 65°C for 30 min and 16 h, respectively. The
membranes were washed twice with 20 mM sodium phosphate (pH 7.2)-5%
SDS for 30 min at 65°C, followed by two washes with 20 mM sodium
phosphate, pH 7.2, and 1% SDS for 30 min at 65°C prior to exposure
to X-films.
2-M-2 probe, specific to and comprising all of
the 2-M-binding region, was labeled with
DIG-dUTP in a PCR with the Mig-11 and Mig-12 primers by using the
2.4-kb Mig-7 and Mig-4 PCR product as the template (Fig. 1). Similarly,
the 1.1-kb IgG probe, specific to the IgG-binding region, was labeled
with Mig-9 and Mig-8 primers in the presence of DIG-dUTP, by using the
same 2.4-kb PCR product as the template (Fig. 1). Prehybridization and
hybridization were carried out with DIG Easy Hyb (Roche Boehringer
Mannheim) at 42°C for 2 and 16 h, respectively. Prior to
autoradiography, the membrane was incubated with alkaline phosphatase
(AP)-conjugated anti-DIG antibodies and the chemiluminescent substrate
as recommended by the manufacturer. For reprobing, the previous probe
on the membrane was stripped by washing twice with 0.2 M NaOH and 0.1%
SDS at 37°C for 15 min, and washed again with 2× SSC (1× SSC is
0.15 M NaCl plus 0.015 M sodium citrate).
SDS-PAGE and Western blots.
Proteins were analyzed by
SDS-polyacrylamide gel electrophoresis (PAGE) as described previously
(15). The purified IgG samples were analyzed on gels with
-mercaptoethanol excluded from the gel-loading buffer. Gels were
either stained with Coomassie brilliant blue or transferred onto
nitrocellulose membranes (Bio-Rad). After blocking with PBS-T buffer
(PBS-0.05% Tween 20), the membranes were either incubated with rabbit
anti-Mig polyclonal antibodies at a dilution of 1:1,000 and followed
with AP-conjugated goat anti-rabbit IgG (heavy plus light chains; Zymed
Laboratories, South San Francisco, Calif.) at a dilution of 1:5,000 in
PBS-T or incubated with AP-conjugated goat anti-rabbit IgG at a
dilution of 1:500 directly. When purified IgG samples were examined, an AP-conjugated goat anti-bovine IgG (heavy plus light chains; Kirkegaard & Perry Laboratories, Gaithersburg, Md.) diluted at 1:2,000 was used.
The membranes were developed in AP buffer (100 mM NaCl; 5 mM
MgCl2; 100 mM Tris · HCl, pH 9.5)
supplemented with nitroblue tetrazolium and
5-bromo-4-chloro-3-indolylphosphate. The concentration of the protein
samples was determined on a microtiter plate with a DC protein assay
kit and Microplate Manager software (Bio-Rad) with bovine serum albumin
or IgG (Pierce, Rockford, Ill.) as standards.
Preparation and purification of proteins.
Subcellular
fractionation of S. dysgalactiae was carried out
according to the method of Kling et al. (13). Protease
inhibitor cocktail tablets (Roche Diagnostic GmbH, Mannheim, Germany)
were used during the preparation. Prior to analysis, the culture
supernatant fractions were concentrated 10-fold by centrifugation
through an Ultrafree-15 filter Biomax-5 K protein concentrator
(Millipore). For preparation of the purified Mig protein, E. coli DH5 carrying p5Me was grown in 50 ml of Luria-Bertani
medium to logarithmic phase and induced with 1 mM
isopropyl--D-thiogalactopyranoside (Sigma) for
5 h at 37°C with shaking. The cell pellet was washed once in
PBS, and the cells were disrupted by sonication. Cell debris was
removed by centrifugation at 15,000 × g for 20 min, and the supernatant was loaded onto a column packed with 5 ml of bovine
IgG agarose (Sigma). After extensive washing and elution of the column
according to the supplier's recommendations, the column eluate was
washed three times with PBS and concentrated approximately 10-fold
using an Ultrafree-15 filter Biomax-30 K protein concentrator
(Millipore) prior to SDS-PAGE analysis.
Preparation of antibodies. To prepare polyclonal antibodies against Mig of S. dysgalactiae strain SDG8, two New Zealand White rabbits were immunized by subcutaneous injection of approximately 100 µg of the affinity-purified Mig protein with incomplete Freund's adjuvant. Three weeks later, a second injection with same amount of Mig with incomplete Freund's adjuvant was administered. The rabbits were humanely euthanized at 14 days after the boost injection, and serum samples were collected.
Determination of DNA sequences. The nucleotide sequences of both strands of the mig gene in S. dysgalactiae strain SDG8 were determined on an ABI 373 DNA automatic sequencer (Applied Biosystems) at the Plant Biotechnology Institute (National Research Council, Saskatoon, Canada) by using multiple primers (Table 1). The sequence data were analyzed with the Genetics Computer Group software provided by The Canadian Bioinformatics Resource.
Preparation of bovine PMNs. Whole blood from clinically normal 5- to 7-year-old dairy cows was collected in EDTA tubes. PMNs were prepared according to the method provided by Becton Dickinson Immunocytometry Systems (Mountain View, Calif.). Erythrocytes were lysed with a lysis solution (168 mM NH4Cl, 10 mM KHCO3, 0.1 mM tetrasodium EDTA), and the PMNs were washed twice with 1× Hanks' balanced salt solution before being suspended in 1× minimum essential medium without antibiotics. Prior to the assay, the viability and the number of PMNs were determined in a hemocytometer under a light microscope by the trypan blue dye (Gibco BRL, Life Technologies, Grand Island, N.Y.) exclusion test.
Fluorescence labeling and opsonization of bacteria. PKH2 fluorescence dye (Sigma) was used to label S. dysgalactiae strains for the phagocytosis assays, modified from a previous report (8). Briefly, 6 ml of logarithmic-phase bacterial culture was washed once in PBS and suspended in 0.5 ml of labeling buffer (Sigma) in a polypropylene centrifuge tube. An aliquot of this suspension (0.2 ml) was diluted in 1 ml of labeling buffer and mixed with 1 ml of the same buffer containing 10 µl of the PKH2 dye. The reaction mixture (total volume, 2.210 ml) was incubated for 10 min at room temperature protected from the light. After two washes with PBS-0.5% bovine serum albumin (BSA) (fraction V; Boehringer Mannheim, Mannheim, Germany), the labeled bacteria were suspended in 0.15 ml of PBS-0.5% BSA.
The bacterial opsonization or serum treatment was performed by incubating mixtures of 100 µl of labeled bacteria and either 50 µl of a pool of heat-inactivated bovine sera (obtained from cows that had recovered from S. dysgalactiae mastitis) or 50 µl of purified IgG from the same bovine serum pool at various concentrations for 15 min at 37°C. The bacteria were then washed twice with 10 ml of PBS and suspended in 0.45 ml of Ca2+- and Mg2+-free Dulbecco's PBS containing 5 mM glucose and 0.1% gelatin (PBSg). The viability of bacteria in each labeling samples was determined by plating 10-fold dilutions on THY.Flow cytometry (FC)-based phagocytosis. Equal volumes (100 µl) of serum-treated or nontreated bacteria were mixed with bovine PMNs in a 96-well U-bottom microtiter plate (Nunclon surface; Nunc, Roskilde, Denmark) and incubated at 37°C for 45 min with gentle shaking in the dark. The reaction was stopped by the addition of 20 µl of 0.3 M EDTA. After two washes with 150 µl of PBSg containing 10 µg of gentamicin per ml (Gibco BRL), the PMNs were suspended in the same solution and incubated for 30 min at 37°C. Finally, the PMNs were washed twice with 150 µl of PBSg and suspended in 100 µl of ice-cold PBSg containing 2% formalin before the analysis. A FC assay was performed on a FACScan flow cytometer (Becton Dickinson, Mississauga, Ontario, Canada) with a 15-MW argon laser light source. Five thousand PMNs were counted for each sample, and cell populations were selected by gating according to their granularity and fluorescence.
Bactericidal assay. Killing of bacteria by bovine PMNs was measured by a viability assay modified from a previously report (20). Exponential-phase bacteria were washed once in PBS, suspended in Hanks' balanced salt solution, and incubated in the presence or absence of bovine serum. Equal volumes (100 µl) of bacteria and bovine PMNs were mixed in an Eppendorf tube, and the mixtures were incubated at 37°C with end-to-end mixing. At the required incubation time points (0, 1, and 4 h), 50 µl of the reaction mixtures was transferred to a 96-well microtiter plate well containing 25 µl of 2% saponin (Sigma) in PBS. After incubation at room temperature for 10 min, the samples were diluted up to 1,000-fold in PBS, and three serial dilutions (50 µl of each sample) were plated on THY plates in duplicate. Prior to the counting of CFU, the agar plates were incubated for 16 h at 37°C with 5% CO2. The CFU count at time zero was used to calculate the initial ratio of bacteria to PMNs. The killing of bacteria by PMNs was calculated as the bacterial survival rate, measured as the CFU at 1 and 4 h relative to the CFU at time zero.
Statistical analysis. The P values of the phagocytosis and bactericidal analyses were obtained from paired t-test analysis (two tailed) with Excel (Microsoft) and Prism (GraphPad Software) software.
Nucleotide sequence accession number. The nucleotide sequence of the mig gene in S. dysgalactiae strain SDG8 has been deposited in GenBank under the accession number AF354651.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Molecular cloning and sequencing of the mig gene. The mig coding sequence was obtained from the plasmid p5Me, from which a mature Mig protein was expressed. The upstream sequence was determined from the plasmids pKSMig-3 and pPMig2-8, both carrying the same PCR product but in different vectors, while the 3'-end sequence was obtained from pMC-5e, carrying a DNA region spanning the mig stop codon (Fig. 1). Assembled, the sequence revealed an open reading frame of 2,007 bp and 669 deduced amino acids with a molecular mass of 72,681 Da and a pI of 4.49. Except for a 15-bp extra sequence at the cell wall-spanning region, the sequence of the mig coding region of SDG8 was highly homologous to the mig gene of S. dysgalactiae SC1 (12), sharing 99 and 98% identity at the nucleotide and amino acid levels, respectively (data not shown).
A BLAST search revealed four proteins sharing overall sequence homology to the SDG8 Mig protein. They were protein G from human group G streptococcus (61% identity [27]), Mag from S. dysgalactiae (54% identity [10]), Zag from S. zooepidemicus (48% identity [11]), and Grab from Streptococcus pyogenes (31% identity [24]). Except for Grab, which has only one2-M receptor related to protein G, all the
other proteins express multiple receptors binding to
2-M, IgG, or albumin. When analyzed by
regions, the homology between Mig and the other proteins was higher in the IgG-binding region (sequence identity with Mag, protein G, and Zag,
99, 83, and 71%, respectively). In contrast, the sequence encoding the
2-M-binding domain of Mig was less conserved,
with identities between 25 and 30%.
Construction and characterization of the mig-mutant
strain.
Recent work suggests a role in virulence for the
2-M-binding region of the GAS and group C
streptococcus surface proteins (see Discussion). We attempted the
construction of an isogenic mutant lacking only the Mig
2-M-binding region with no success. However,
we were able to obtain a mutant in which an antibiotic-resistant cassette replaced sequences downstream of the
2-M region. Briefly, the
mig-internal 420-bp ClaI fragment present in p5Me
was replaced with a blunted EcoRI-ClaI fragment
containing an Sp cassette to generate p5Me-Sp (Fig. 1). The
mig-Sp insert was cloned into a temperature-sensitive
suicide vector, and this construct was named pMig-1 (Fig. 1). For
allele replacement mutagenesis, pMig-1 was transformed into
S. dysgalactiae and selected for single crossover in
the presence of EM at 30°C. The strain carrying the plasmid was
incubated at 37°C and plated on SP. Bacteria in which the double
crossover between homologous plasmid and chromosomal sequences had
occurred were selected from colonies resistant to SP but sensitive to
EM. One such isolate, Mig8-Mt, was selected for further analysis.
2-M-1
probe was used, 2.5- and 2.4-kb HindIII fragments were
detected in the SDG8 and Mig8-Mt genomic DNAs, respectively
(Fig. 2A). The smaller fragment in the mutant results from the
introduction of an extra HindIII site close to the 3'
end of the Sp cassette (Fig. 1). The HindIII bands of
2.5 kb in SDG8 and 2.4 kb in Mig8-Mt were also present when the IgG probe was employed (Fig. 2C). As expected from the restriction map of
the mutant strain, an extra 1.2-kb HindIII band was also detected in Mig8-Mt, since the IgG probe spanned the ClaI
site used to construct the mutant (Fig. 1). These results indicate that
the Mig8-Mt strain carries a mutation on the mig gene. The restriction map of the mutant strain suggests that this strain could
export the 2-M receptor alone, since the
export signal and the 2-M receptor sequences
are still intact, but stop codons were added by the Sp cassette,
resulting in a truncated peptide lacking the IgG-binding and
carboxy-terminal regions of Mig. However, if exported, this peptide
cannot be attached to the cell wall, since the conserved LPTTGE region
(7) is missing from its sequence, and the gene product
should be found in the culture supernatant.
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2-M and IgG
receptors in the Mig8-Mt strain was examined by Western blotting using
AP-conjugated goat IgG and/or rabbit polyclonal antibodies
against Mig (Fig. 3). Protein
preparations from the wild-type strain exhibited one band at about 80 kDa reacting to goat IgG (Fig. 3A). The relative mass of this band was
larger than the expected 69 kDa of the mature Mig protein, a phenomenon
similar to the gel patterns of the protein G in the group C and G
streptococci which is probably due to the low content of hydrophobic
residues resulting in poor binding to SDS (27). No signal
was detected from the Mig8-Mt protein preparations with the
AP-conjugated IgG (Fig. 3A). This suggested that the mig
mutant has lost the IgG-binding ability, although half of the first
IgG-binding repeat could still be expressed with the upstream regions
(Fig. 1). When detected with the antibodies against Mig, a band at
about 28 kDa was found in concentrated culture supernatants of Mig8-Mt
but not in the cell wall preparations (Fig. 3B), indicating that
Mig8-Mt still expressed the 2-M receptor but
it was lost into the medium. Concentrated culture supernatants and
whole-cell extracts of the wild-type strain exhibited the ca. 80-kDa
bands reacting to the goat IgG (Fig. 3B). The presence of the Mig
protein in the concentrated culture supernatant of the wild-type strain
could be due to either bacterial cell wall or membrane turnover or
release of the Mig protein from the cell wall by a cysteine protease,
as is the case for the M protein of GAS (24).
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Distribution of the mig gene in S.
dysgalactiae strains.
A total of 16 S. dysgalactiae isolates, including two strains from the American
Type Culture Collection, were examined for the presence of sequences
homologous to the mig gene by using DNA probes containing
the mig-specific 2-M and IgG
receptor coding regions. Southern blot analysis of
HindIII digested-genomic DNA revealed that five
strains possessed sequences homologous to the 2-M-2 probe (Fig. 1), but the sizes of those
bands varied between 2.1 and 2.7 kb (Fig.
4A). The same five strains were also
positive in PCR amplifications of the mig
2-M coding region with the Mig-11 and Mig-12
primers (Fig. 1), but they exhibited bands of the same size at 0.5 kb
(data not shown). Further PCR analysis of these strains with primers
Mig-9 and Mig-8 (Fig. 1), amplifying the IgG receptor-encoding regions,
indicated that the 0.6-kb size difference found with the
2-M-2 probe was located on this region (data
not shown). In the mig gene, one IgG-binding repeat is
encoded by a ca. 200-bp DNA fragment. Taking into account the size
differences of the IgG receptor-coding regions, the five
2-M positive strains therefore might carry
three to six IgG-binding repeats instead of only five repeats, as are
present in the mig genes of the SDG8 and SC1 strains. In
contrast to the 2-M-2 probe, the IgG probe (Fig. 1) detected homologous sequences in all the tested strains with a
total of seven different hybridization patterns (Fig. 4B). As expected,
in the five isolates possessing the specific mig 2-M sequences, the IgG probe hybridized to
HindIII fragments of the same size (numbered bands in
Fig. 4), suggesting that both regions were part of the same genetic
unit.
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Phagocytosis.
To determine the role of the Mig protein in
resistance to phagocytosis, SDG8 and Mig8-Mt were labeled with the
fluorescent dye PKH2, and the percentage of intracellular
microorganisms was measured by FC after ingestion of the bacteria by
bovine PMNs. No deleterious effects on the bacterial cell viability
were observed after labeling with PKH2 (data not shown). Optimal
conditions for phagocytosis were obtained with a ratio of bacteria to
PMNs of about 10:1. The results from four individual experiments
indicated that the wild-type strain SDG8 (66%) and the mutant Mig8-Mt
(66%) were phagocytosed at the same rate (P > 0.05)
in the absence of bovine serum (Fig. 5A).
When bovine serum was included in the assay, SDG8 was more
resistant to phagocytosis than Mig8-Mt (54 versus 69% ingested
bacteria, respectively; P < 0.05) (Fig. 5B). This
result indicated that the Mig protein in SDG8 is capable of protecting
the bacterium from phagocytosis in the presence of antiserum.
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2-M in the serum to the Mig
2-M receptor but not to the binding of IgG to
the Mig IgG receptor.
The role of complement receptors was excluded by analyzing the
phagocytosis of strain SDG8 incubated with either a heat-inactivated or
an unheated bovine serum pool. Similar bacterial internalization rates
were observed in two groups (data not shown). To rule out the influence
of other serum proteins, we incubated SDG8 with purified IgG prepared
from the same serum pool prior to the phagocytosis assay. Similar
ingestion rates of the wild-type strain were observed for the control
and with 0.2 to 0.8 mg of IgG (P values between 0.7919 and
0.9319, n = 4), suggesting that IgG does not influence phagocytosis by PMNs of S. dysgalactiae. To confirm
this observation, we performed several complementary experiments on
SDG8. First, we did not observe any differences in phagocytosis of
control and SDG8 cells preincubated with a different serum pool
obtained from four cows challenged with SDG8 (P = 0.566, n = 2). Second, another S. dysgalactiae strain, ATCC 27957, was analyzed in the same
way by using a serum pool containing specific antibodies against this strain. As in the case with SDG8, we did not see a
significant enhancement of phagocytosis (P = 0.5896, n = 2). Third, an S. agalactiae strain
was incubated with bovine serum containing antibodies against
S. agalactiae, and its resistance to phagocytosis was
analyzed by the same method. A significantly higher ingestion rate was
observed with the opsonized sample than the nonopsonized one
(P < 0.0001, n = 4), suggesting that
the methodology used for S. dysgalactiae was appropriate.
Bactericidal assay. To investigate the roles of serum proteins in the intracellular bacterial survival rate, bacteria were incubated with bovine PMNs in the absence or presence of bovine serum for different time points. The internalized bacteria were released by lysis of the cells with saponin, and viable counts were determined by plating on THY. The lysis of PMNs by saponin was confirmed by microscopic examination, and no deleterious influence of the detergent on the bacterial viability was observed (data not shown). The optimal ratio of bacteria and PMNs in this assay was between 1:1 and 6:1. From six individual experiments, we found that the serum-free SDG8 and Mig8-Mt strains survived at similar rates after incubation with PMNs for 1 h (27% for both) and 4 h (46% for SDG8 and 40% for Mig8-Mt) (P > 0.05). When the bacteria were incubated with bovine serum, a significant difference in the survival rate was observed between the two strains after incubation with PMNs for 4 h (93% for SDG8 and 35% for Mig8-Mt; P < 0.01) but not for 1 h (25% for SDG8 and 27% for Mig8-Mt; P > 0.05). These data suggest that in the presence of serum proteins, the wild-type strain is more resistant to the killing by PMNs after being phagocytosed than the mig mutant strain.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The mig gene of the S. dysgalactiae
strain SC1 contains 2-M- and IgG-binding
regions with five repeat units (12). We sequenced the
mig gene from another S. dysgalactiae
strain, SDG8, and its sequence exhibited high homology to the
mig gene of SC1. However, among the five
mig-positive strains in our collection, the size of the DNA
encoding the IgG-binding region varied, with a difference of up to 0.6 kb. Based on the restriction map of the mig gene and the
size of the IgG-binding repeat units (ca. 0.2 kb) in SDG8, we speculate
that three to six IgG-binding repeats might exist in the Mig proteins
of these other strains. The number of IgG-binding repeats correlates
with the capacities for binding to IgG, since protein G (two or three
IgG-binding repeats) binds to the IgG-Fc part (9, 27) and
the Mig protein (five IgG-binding repeats) simultaneously binds to both
IgG Fc and Fab regions. An 11-residue peptide derived from a single
protein G repeat was shown to inhibit the binding of protein G to human
IgG Fc fragments. Despite the amino acid differences (4 out of 11), a
similar peptide from the first repeat of the Mig protein inhibited the
binding of protein G to human IgG Fc (31). This suggests
that the remaining conserved amino acids or the secondary structure of
the peptide might play a role in the binding to the Fc portion of IgG.
The distribution of the mig gene in a total of 16 S. dysgalactiae isolates was investigated in this
study. All of them possessed DNA fragments that hybridized to the IgG
probe (Fig. 4B), suggesting that the IgG-binding sequence of
mig is highly conserved in these strains. Only five strains
(31%) were found to carry the mig
2-M-homologous sequences linked to the
IgG-binding domains (Fig. 4A). This suggests that genes other than
mig encode the IgG receptors in the rest of the
S. dysgalactiae strains. The mag gene of
S. dysgalactiae encodes a surface protein capable of
binding to IgG, albumin, and 2-M
(10). While the IgG-binding domains of mig and
mag are highly related (99% identity [this work]), the
2-M receptors are not (25% identity). Only
three strains (19%) were found to carry sequences homologous to the
mag 2-M-binding region (data not
shown) and none of them were the previously identified five mig-positive strains. Among the total 16 strains, the
percentage of isolates carrying 2-M receptors
was only 50% (31% mig and 19% mag), which was
much lower than the 73% found in a direct binding assay using labeled
2-M-T (23). This suggests that other types of 2-M receptors with unique
sequences might exist in S. dysgalactiae, especially in
the mig- and mag-negative strains.
Besides Mig and Mag in S. dysgalactiae,
2-M receptors were also identified in several
other proteins in streptococci, such as Zag in S. zooepidemicus (11), protein G in human group G streptococcus strain 148 (17, 28), and the protein
G-related 2-M receptor Grab in human group A
S. pyogenes (24). As the binding of
2-M to the bacterial
2-M receptors is highly dependent upon
conformation, the sequences encoding
2-M-binding receptors are unique among these
proteins. Furthermore, the pattern of binding of streptococcus cells to
the 2-M protein of the infected hosts was
divergent. The 2-M receptors from human group
A and G streptococci bind only to the native form of
2-M, whereas the 2-M
receptors from bovine and equine group C streptococci bind only to
2-M-T (16, 17). The effects on
phagocytosis of these two kinds of binding are also different. The
binding of native 2-M to S. pyogenes enhanced phagocytosis by PMNs (29). It is
possible that in GAS, binding of 2-M provides
protection against virulence factor degradation by interfering with
intracellular host cell proteases following phagocytosis of the
bacterium. Recent findings support this hypothesis. The
2-M receptor expressed by the protein
Grab of human group A S. pyogenes strains has been
shown to be involved in virulence in a mouse infection model via
binding to 2-M, thereby inhibiting activities
of both bacterial and host proteases and thus protecting important
virulence determinants from proteolytic degradation (24). The binding of 2-M-T to
S. dysgalactiae inhibited phagocytosis (29), perhaps by protecting other virulence factors
against host protease degradation.
In bovine mastitis, the PMN-mediated phagocytosis is the most important
host defense system in the mammary gland (3). The concentration of immunoglobulins (3) and
2-M (22) also increases dramatically following infections of the gland. This suggests that
binding of 2-M and IgG to the Mig protein of
S. dysgalactiae could mask the surface of the bacterium
and interfere with phagocytosis by PMNs. To test this hypothesis, we
constructed an isogenic mig mutant strain and analyzed its
resistance to phagocytic ingestion and killing by bovine PMNs. Although
the 2-M receptor portion of Mig was still
expressed in the mig mutant strain, it was not cell
associated and it could not be detected in the supernatants of the
phagocytosis reactions by Western blotting (data not shown). S. dysgalactiae SDG8 was more resistant to phagocytosis
in the presence (54%) than in the absence (66%) of serum-ingested
bacteria, while no differences were observed with Mig8-Mt (69 versus
66%) (Fig. 5), suggesting that binding of 2-M
and/or IgG to the Mig protein of the wild-type strain influenced
phagocytosis by bovine PMNs. Control experiments performed with
purified bovine IgG, serum samples from different cows, and a different
S. dysgalactiae strain indicated that the phagocytosis
of S. dysgalactiae cells by bovine PMNs is probably due
to a nonopsonic mechanism. This kind of phagocytosis is usually
influenced by some factors that mediate interactions between bacteria
and phagocytes, such as carbohydrate-protein, protein-protein, and
hydrophobic interactions (18). Hydrophobic interactions of
S. dysgalactiae have been shown to play a role in
bacterial ingestion by phagocytic cells (4), but more
experiments are needed to confirm our observations of nonopsonic
phagocytosis of S. dysgalactiae by bovine PMNs.
We speculate that the higher resistance to phagocytosis of the
wild-type strain is probably mediated by the binding of
2-M-T to the 2-M
receptor of Mig and not to binding of IgG to the IgG receptor. Since
2-M is a large molecule, ca. 720 kDa
(17), the 2-M-T bound to
bacteria probably protects it from phagocytosis directly or indirectly
by masking other receptors that mediate phagocytosis, thereby
inhibiting bacterial ingestion. In our phagocytic killing study, a very
significant survival rate of the serum-incubated wild-type strain
compared to the mig mutant strain correlates with a previous
observation that the binding of 2-M-T to
S. dysgalactiae whole cells inhibited phagocytic
killing (29) and thus played a role in virulence of
S. dysgalactiae. The 2-M
protein bound to the bacterial surface via the Grab protein of
S. pyogenes inhibits the activities of bacterial and
host proteases, thereby preventing bacteria or some other virulence
factors from proteolytic degradation (24). In the case of
S. dysgalactiae, the mechanism of resistance to
phagocytosis mediated by the 2-M receptor in
Mig remains undetermined, since Mig binds only to the trypsin complex
form of 2-M. It is unclear if
2-M-T bound to the bacterial surface via the
2-M receptor still traps and inhibits the
activities of proteases, since the enzymatic activity of
2-M-T against low-molecular-mass substrates
was unimpaired while its activity against high-molecular-mass substrates was severely affected (22).
In human group A S. pyogenes strains, the M protein has been shown to protect the bacteria against phagocytosis by PMNs (6). Recently, an M-like protein was also isolated from a strain of S. dysgalactiae (30). A comparison of the amino acid sequence of this protein to that of Mig indicated a low degree of homology (data not shown). Although Mig and the M proteins do not share extensive amino acid homology, Mig possesses structural features similar to the M family of proteins, namely, an alpha coiled-coil structure, repeated amino acid sequences, a carboxy-terminal region embedded in the cell wall, and the conserved sequence LPTTEG essential for anchoring to the cell membrane. A functional classification of the M proteins is their ability to confer resistance to phagocytosis (6). The mechanism by which the M protein protects the bacteria appears to be binding to the serum protein factor H, which regulates the activity of complement deposited on the cell surface (6). Although some of the proteins that bind Mig and M are different, it is tempting to include Mig as a member of the M-protein family, since they exert the same biological function, i.e., protection of the bacterium against the immunological surveillance of the host.
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ACKNOWLEDGMENTS |
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We thank Susantha Gomis, Dale Godson, and Michael Fontaine for valuable discussions, Terry Beskorwayne for performing FACS analysis, The Animal Care Unit at the Veterinary Infectious Disease Organization for collecting animal blood samples, and Philip Willson for help with the statistical analyses.
This work was supported by The Natural Sciences and Engineering Research Council of Canada, Canadian Bacterial Diseases Network, Saskatchewan Agriculture Development Fund, and The Dairy Farms of Canada.
| |
FOOTNOTES |
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* Corresponding author. Mailing address: Veterinary Infectious Disease Organization (VIDO), University of Saskatchewan, 120 Veterinary Rd., Saskatoon, Saskatchewan, Canada S7N 5E3. Phone: (306) 966-7484. Fax: (306) 966-7478. E-mail: Potter{at}sask.usask.ca.
Published with permission of the director of the Veterinary
Infectious Disease Organization as journal series no. 292.
Editor: E. I. Tuomanen
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Materials and Methods
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Discussion
References
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