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Oral Administration of a Salmonella enterica-Based Vaccine Expressing Bacillus anthracis Protective Antigen Confers Protection against Aerosolized B. anthracis

Defence Science and Technology Laboratory, Porton Down, Salisbury, Wiltshire SP4 0JQ, United Kingdom,¹ Department of Infectious and Tropical Diseases, London School of Hygiene and Tropical Medicine, Keppel Street, London WC1E 7HT, United Kingdom,² Center for Vaccine Development, School of Medicine, University of Maryland, Baltimore, Maryland 21201,³ University of Maryland Biotechnology Institute, University of Maryland, Baltimore, Maryland 21201⁴

Received 4 August 2006/ Returned for modification 20 October 2006/ Accepted 20 November 2006

	ABSTRACT

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Bacillus anthracis is the causative agent of anthrax, a disease that affects wildlife, livestock, and humans. Protection against anthrax is primarily afforded by immunity to the B. anthracis protective antigen (PA), particularly PA domains 4 and 1. To further the development of an orally delivered human vaccine for mass vaccination against anthrax, we produced Salmonella enterica serovar Typhimurium expressing full-length PA, PA domains 1 and 4, or PA domain 4 using codon-optimized PA DNA fused to the S. enterica serovar Typhi ClyA and under the control of the ompC promoter. Oral immunization of A/J mice with Salmonella expressing full-length PA protected five of six mice against a challenge with 10⁵ CFU of aerosolized B. anthracis STI spores, whereas Salmonella expressing PA domains 1 and 4 provided only 25% protection (two of eight mice), and Salmonella expressing PA domain 4 or a Salmonella-only control afforded no measurable protection. However, a purified recombinant fusion protein of domains 1 and 4 provided 100% protection, and purified recombinant 4 provided protection in three of eight immunized mice. Thus, we demonstrate for the first time the efficacy of an oral S. enterica-based vaccine against aerosolized B. anthracis spores.

	INTRODUCTION

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Bacillus anthracis is the causative agent of anthrax, a disease that affects wildlife, livestock, and humans. The ability of B. anthracis to cause disease is dependent on the production of a polyglutamic acid capsule, which provides resistance to phagocytosis and to the production of anthrax toxins. The toxins consist of three proteins—protective antigen (PA), edema factor (EF), and lethal factor (LF)—which act in binary combinations (20). PA and EF together produce the edema toxin, whereas PA and LF together produce the lethal toxin. Protection against anthrax is considered to be due mainly to the immune response to PA. Specifically, research into mechanisms associated with the efficacy of current anthrax vaccines has led to the conclusion that PA is essential and a dominant component of the vaccines since the protein can elicit effective protective immunity in the absence of LF and EF (19, 26).

The current licensed United Kingdom and U.S. anthrax vaccines for human use consist of cell-free filtrates of a nonencapsulated but toxigenic B. anthracis derivative, adsorbed to alum (U.S. vaccine) or aluminum hydroxide (United Kingdom vaccine). Although effective in animal studies, these vaccines must be administered by needle in multiple doses over several months, with annual boosters to maintain continuous protection (1). In addition to occasional cases of adverse local reactions, the vaccines are expensive to produce, have a limited shelf life as a consequence of their formulation, and are currently only available to military personnel. There is a need to develop vaccines capable of protecting both military and civilian populations, which poses challenges in terms of the general health of these populations, compliance, and the ability to mass vaccinate in the event of an attack. Therefore, improvements to increase the efficacy, longevity, and safety of the anthrax vaccine are warranted. A subunit vaccine consisting of purified recombinant PA protein adsorbed to aluminum hydroxide has been proposed (24) but will suffer from the drawbacks of limited ambient stability and the need to be administered by needle.

One approach to the development of an improved next-generation anthrax vaccine involves the use of live attenuated Salmonella vaccines to deliver PA. This approach offers a number of advantages (12). First, live Salmonella vaccines can be given orally (the natural route of infection), enabling a noninvasive route of vaccine administration. Second, both mucosal and systemic immune responses can be elicited, which may be important for protection against airborne infection. In addition, live attenuated Salmonella vaccines are able to simulate both humoral and cellular immune responses that may be important for protection against disease. Since the live attenuated Salmonella vaccine strain Ty21a (14) is licensed for human use and other next-generation attenuated Salmonella strains are in clinical trials (12), it should also be possible to develop safe recombinant Salmonella vaccines for licensure. Finally, since Salmonella is genetically tractable, recombinant Salmonella vaccines are relatively easy to develop and are also relatively cost-effective to produce.

Preliminary studies evaluating the use of attenuated Salmonella for delivery of PA have been reported (4, 13). Initially, PA was expressed in Salmonella from a high-copy-number plasmid, leading to high-levels of PA in vitro but plasmid instability in vivo and low colonization of the host tissues by the bacteria (4). More recently, a lower-copy-number plasmid was used to express PA as a fusion to the Escherichia coli hemolysin (Hly) export system in order to enable export of the expressed PA protein from the Salmonella (13). This plasmid was also found to be unstable, perhaps as a consequence of the high metabolic load placed upon the bacteria in continuously producing both the Hly export proteins and PA. However, when the Hly-PA fusion was integrated into the Salmonella chromosome, the resulting recombinant was able to provide protection against an injected anthrax spore challenge if administered via the intravenous route and not by the oral route.

We considered a number of approaches that would allow us to realize our goal of devising an orally delivered Salmonella vaccine which would provide protection against airborne B. anthracis. The use of an inducible promoter to selectively express PA in vivo coupled with a stabilized plasmid-based expression system would promote an enhanced immune response. In addition, we considered that expression only of the domains of PA which are associated with protective immunity (6) could allow the generation of a more stable recombinant. Recently, Galen et al. described the use of the S. enterica serovar Typhi cytolysin A (ClyA) export system for delivery of a domain of PA in Salmonella, improving the immunogenicity of PA compared to cytoplasmic expression (11). This ClyA export apparatus requires only the fusion of proteins to the 34-kDa ClyA protein, making it attractive and simple to use for the secretion of proteins from Salmonella.

In the present study, attenuated Salmonella strains expressing PA, domain 4 of PA, or a fusion protein of domains 1 and 4 of PA were produced and compared for immunogenicity and protective efficacy against aerosolized B. anthracis spores.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and growth conditions. S. enterica serovar Typhimurium SL3261 (aroA mutant), an attenuated amino acid-dependent strain, and S. enterica serovar Typhimurium LB5010, used for methylation of E. coli-derived plasmids prior to transformation of strain SL3261, were taken from laboratory stocks (Dstl Porton Down, United Kingdom). E. coli TOP10F' or E. coli DH5 cells (Invitrogen) were used for plasmid maintenance and E. coli BL21(DE3)/pLYsS cells were used for protein expression. Plasmid pVDL9.3PA83ec encoding an E. coli codon-optimized PA gene of B. anthracis (13) was used as a template DNA for PCR. The pCR2.1-TOPO plasmid vector (Invitrogen, United Kingdom) was used to clone PCR products. Plasmid pGEX-6-P3 (Amersham-Pharmacia) was used to express proteins as fusions to N-terminal glutathione S-transferase (GST). Bacterial strains were cultured aerobically on Luria agar or in Luria broth supplemented with ampicillin (100 µg/ml), kanamycin (10 µg/ml), or chloramphenicol (25 µg/ml), as appropriate, at 37°C and with agitation at 180 to 200 rpm or statically. Similarly, strain SL3261 was routinely supplemented with 1% (vol/vol) "aromix" comprising 4 mg of phenylalanine/ml, 4 mg of tryptophan/ml, 1 mg of para-aminobenzoic acid (PABA)/ml and 1 mg of dihydroxybenzoic acid/ml (adapted from Chatfield et al. [3]).

The growth rates of the recombinant Salmonella strains were determined by culturing the bacteria for 24 h in Luria broth containing antibiotic selection and enumerating them on Luria agar containing antibiotics. To establish the stability of the strains in vitro, the recombinant bacteria were cultured over 72 h, with passage every 24 h, in the absence of antibiotic (equivalent to culturing the bacteria for approximately 44 generations), and the stability of the plasmids within the Salmonella was calculated by enumeration of bacteria on Luria agar with or without antibiotic selection. Inocula were produced by culturing the recombinant Salmonella strains statically overnight at 37°C, harvesting the bacteria by centrifugation (7,000 x g for 20 min at 4°C), and then washing and resuspending the bacteria in sterile phosphate-buffered saline (PBS). The inoculum dose was verified by plating serial dilutions of each culture on Luria agar supplemented with antibiotic, where appropriate.

Mice. Female A/Jola (A/J) mice (supplied and used at 8 to 12 weeks of age; Harlan UK, Ltd.) were used for all studies since these mice provide a consistent mouse model for infection with a toxigenic nonencapsulated (Tox⁺ Cap^–) strain of B. anthracis (32). All animal procedures strictly adhered to the Animals (Scientific Procedures) Act of 1986.

Construction of recombinant Salmonella strains expressing PA domains. All methods for DNA manipulation were carried out according to the method of Sambrook et al. (29) unless otherwise stated. Taq DNA polymerase (Invitrogen) or Vent DNA polymerase (New England Biolabs) were used in the PCRs.

(i) Construction of expression plasmid pSEC10. A new expression plasmid was derived by using the origin of replication from pSC101 (2), which normally exists at five copies per chromosomal equivalent. The primers used are listed in Table 1, and the essential plasmids created from these primers are listed in Table 2. First, an ori101 replication cassette was synthesized by PCR using primers 1 and 2 with pSC101 as a template, generating a 1,949-bp BamHI-AvrII fragment. This fragment was inserted into the pBR322-derivative pGEN2, cleaved with BglII-AvrII to create pGEN4. The authenticity of this PCR product was confirmed by nucleotide sequencing the cloned DNA. Construction of pGEN132 was accomplished by removal of the ori101 cassette from pGEN4 as a 2,638-bp BamHI fragment and insertion into pJN5 digested with BglII and BamHI, thereby regenerating the gfpuv gene encoding the green fluorescent protein allele GFPuv (BD Biosciences/Clontech) under an osmotically controlled P_ompC promoter. Final assemblage of a pSC101-derived expression plasmid containing a complete plasmid maintenance system (9) was achieved by introduction of parA from pJN8. A 4,469-bp BamHI-SpeI cassette from pJN8 containing bla, hok-sok, and parA was ligated to the 2,649-bp BamHI-SpeI ori101 cassette from pGEN132 to regenerate gfpuv and create pGEN206. The ß-lactamase cassette of pGEN206 was replaced by partial cleavage with SpeI, complete digestion with XbaI, and replacement of the resulting 1,181-bp bla gene with a previously described 1,046-bp NheI fragment encoding resistance to kanamycin (11), creating pEXO5. Finally, the clyA cassette was cleaved from pSEC91 (11) as an XhoI-AvrII fragment and ligated into pEXO5 digested with XhoI-AvrII to generate pSEC10.

(iii) Transformation of Salmonella. The pSEC10 derivatives were transformed into E. coli, and individual transformants were screened for expression of the ClyA-PA proteins by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and Western blotting of colony lysates (see below) and one positive clone for each plasmid construct was electroporated into S. enterica serovar Typhimurium SL3261 via passage through S. enterica serovar Typhimurium LB5010, an intermediate host strain required for methylation of the plasmid DNA. In addition, plasmid pVDL9.3PA83ec, encoding full-length PA fused to the Hly export system and conferring resistance to chloramphenicol (13), was transformed into SL3261 for comparison.

Detection of PA expression. Recombinant Salmonella was cultured in L broth supplemented with antibiotic selection for 24 h with agitation. Samples (1 ml) were centrifuged at 13,000 x g for 10 min, and the resulting cell pellets or supernatants were diluted 1:1 in 2x Laemmli buffer then boiled for 5 min. The samples were normalized to 3 x 10⁸ CFU/ml for comparison. To evaluate PA expression, SDS-PAGE on 12.5% (wt/vol) polyacrylamide gels (PhastSystem; Amersham Pharmacia Biotech, Ltd.) and Western blotting on Immobilon-P nitrocellulose membrane (Millipore) was performed. After transfer of proteins from SDS-PAGE gels, membranes were blocked with PBS containing 2% (wt/vol) bovine serum albumin (PBS-BSA), and then probed by using mouse anti-PA4 antibody, 2D4J (produced at DSTL), and a rabbit anti-mouse horseradish peroxidase-conjugated secondary antibody (Sigma-Aldrich). Antibodies were used at 1:2,000 dilutions in PBS-BSA, and membranes were washed using PBS containing 0.05% (vol/vol) Tween 20. Proteins were visualized by using Sigma-Fast 3,3'-diaminobenzidine tablets (DAB peroxidase substrate; Sigma-Aldrich).

Determination of plasmid stability in vivo. Groups of eight female A/J mice were inoculated with approximately 1 x 10⁹ to 3.8 x 10⁹ CFU of SL3261 or SL3261 recombinants orally by intragastric gavage. On day 8 postinoculation, mice were culled by cervical dislocation and spleens and Peyer's patches (six/mouse) were harvested. The tissues were homogenized in 1 ml of sterile PBS using 50-µm-pore-size cell strainers (Becton Dickinson Labware) and subsequently inoculated onto agar plates with or without antibiotic selection to determine counts of recombinants or total bacteria, respectively, in order to calculate the stability of the plasmids in the Salmonella strains.

Production of PA1+4 protein. DNA encoding the PA1+4 fusion was PCR amplified from the recombinant the pCR2.1-TOPO vector using primers PA83/F4 and PA83/R4, containing XhoI and BamHI restriction sites (Table 1) and then cloned into the XhoI/BamHI sites of the expression vector pGEX-6-P3 (GE Healthcare) downstream and in frame of the lac promoter, as a fusion to GST. To produce purified recombinant GST-PA1+4 protein, the recombinant plasmid was transformed into E. coli BL21(DES)/pLysS, and transformants were cultured in Luria broth containing 50 µg of ampicillin/ml, 30 µg of chloramphenicol/ml, and 1% (wt/vol) glucose, followed by shaking at 37°C, to an A₆₀₀ of 0.4 prior to induction with 1 mM IPTG (isopropyl-ß-D-thiogalactopyranoside). Cultures were then incubated for a further 4 h, followed by harvesting by centrifugation at 10,000 rpm for 15 min. Cell pellets were resuspended in PBS and sonicated four times for 20 s each time in an ice water bath, and the suspension was centrifuged at 15,000 x g for 30 min. Subsequently, cell supernatants were loaded onto a 5-ml GSTrap 4B column (GE Healthcare) previously equilibrated with PBS. The column was washed with PBS, and the fusion protein was eluted with 20 mM reduced glutathione-50 mM Tris (pH 8). After analysis by SDS-PAGE, fractions containing PA1+4 were pooled and dialyzed into cleavage buffer (50 mM Tris, 150 mM NaCl, 1 mM EDTA, 1 mM dithiothreitol; pH 7). PreScission protease was added at a ratio of 2 U per 100 µg of fusion protein, followed by incubation overnight at room temperature. Cleaved PA1+4 protein was separated from the GST by reapplying to a 5-ml GSTrap 4B column pre-equilibrated with PBS. Unbound fractions containing protein were analyzed by SDS-PAGE, pooled, and dialyzed against PBS. The PA1+4 protein concentration was determined by using a BCA assay (Pierce). Purified recombinant (r) PA1, PA4, and PA1-4 were all produced using the same protocol as described previously (6). Purified proteins were visualized by SDS-PAGE alongside appropriate Bio-Rad molecular weight markers.

Immune response analysis. Groups of five to eight mice were inoculated orally by intragastric gavage with between 1 x 10⁸ and 5 x 10⁹ CFU of S. enterica serovar Typhimurium SL3261 or SL3261 recombinants on days 0, 14, and 28. Bacteria were centrifuged and resuspended in PBS before dosing. Alternatively, mice were injected via the intramuscular route with 10 µg of purified rPA proteins absorbed to a 20% (vol/vol) solution of 1.3% Alhydrogel (Superfos Biosector a/s, Vedback, Denmark). Subsequently, serum samples were evaluated for immune response analyses.

(i) ELISA. Serum samples were tested for specific antibody responses by enzyme-linked immunosorbent assay (ELISA) using standard procedures. Blood samples were collected from the tail veins of all immunized and control mice on days 13, 15, 46, and 73 after inoculations on days 0, 14, and 28 and serum was assayed for PA-specific immunoglobulin G (IgG) antibody responses. Ninety-six-well microtiter plates were coated with 5 µg of recombinant PA/ml (produced at Dstl [25]) overnight at 4°C and then washed. All washing steps were carried out with PBS containing 0.02% (vol/vol) Tween 20. Plates were then blocked with 2% (wt/vol) skimmed milk in PBS for 1 h, and each serum sample was serially diluted 1:2 in blocking solution across the plate, followed by a 1-h incubation. Bound antibody was detected by using horseradish peroxidase-conjugated polyclonal goat anti-mouse IgG (Harlan Sera-lab) diluted 1:2,000 in blocking buffer and incubated for 1 h. Plates were developed with 100 µl of ABTS [2,2' azinobis(3-ethylbenzthiazolinesulfonic acid)]; Sigma-Aldridge) substrate, and the A₄₁₄ of the plates were measured. All samples were assayed in duplicate. Endpoint antibody titers were expressed as the maximum dilution of sample giving an absorbance or more than 0.1 A₄₁₄ units, after subtraction of the absorbance due to nonspecific binding detected in control sera from mice immunized with the parent S. enterica serovar Typhimurium SL3261 strain. The results are presented as the reciprocal of the dilution, and the mean represented the average of duplicate values for each samples.

(ii) TNA. The titer of toxin-neutralizing antibody (TNA) in immune sera was determined based on the ability of the serum to inhibit the cytotoxicity of the combination of PA with LF as described previously (28). Briefly, J774A.1 murine macrophage cells (American Tissue Culture Collection) were harvested and plated out at approximately 3.5 x 10⁴ cells/well in a 96-well microtiter plate, and 40 to 60% confluent layers were allowed to form over a 17- to 19-h period at 37°C in 5% (vol/vol) CO₂ as viewed by microscopy. Antisera was prepared in a separate 96-well plates and serially diluted down the plate. A positive control reference sera with a known 50% effective dose was also included, and a nonspecific mouse antisera was used as a negative control. Then, 100 µl of anthrax lethal toxin was added (50 ng of PA/ml and 40 ng of LF/ml) per well, and the plates were incubated for 30 min. Medium was then removed from the J774A.1 cells, and the antiserum-toxin mix was added to the plates (100 µl/well). These were subsequently incubated for 4 h at 37°C in 5% (vol/vol) CO₂. Cell viability was determined by the addition of 25 µl of 5 mg of 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (Sigma)/ml dissolved in PBS (Gibco). Throughout the assay, wells containing positive and negative controls were randomly checked via microscopy to check cell viability visually; negative control wells contained small, rounded, dead cells, and positive control wells contained living, healthy cells, as expected. The incubation was continued for a further 2 h under the same conditions, and then the reaction was stopped by the addition of a 20% (wt/vol) SDS (Becton-Dickinson) dissolved in 50% (vol/vol) DMF (Becton-Dickinson) in water (Gibco). Plates were then incubated for 16 to 20 h at 37°C in 5% (vol/vol) CO₂. The optical density readings of the plates were taken by using MultisKan Ascent microplate photometer (Thermo Labsystems) at 570 and 690 nm as a reference filter. Endpoints were calculated by using SAS software (version 8.2), running an endpoint calculation algorithm developed by the Centers for Disease Control and Prevention. The TNA endpoint is defined as the reciprocal of the serum dilution that gives 50% neutralization of the anthrax lethal toxin, corresponding to the inflection point of a four-parameter logistic-log fit of the neutralization curve. All antisera were tested at least twice by two separate analysts; the results shown are the averages of each individual 50% effective dose from each separate assay performed by each analyst.

B. anthracis spore preparation. B. anthracis STI (Tox⁺ Cap^–) was cultured on the surface of Roux bottles containing New Sporulation medium (3.0 g of Difco Trypton, 6.0 g of Oxoid bacteriological peptone, 3.0 g Oxoid yeast extract, 1.5 g of Oxoid Lab Lemco, 1 ml of 0.1% MnCl₂·4H₂O, and 25 g of Difco Bacto agar in 1 liter of distilled H₂O) at 37°C until the cultures contained more than 95% phase bright spores, measured by phase-contrast microscopy; typically, incubation of between 7 to 10 days resulted in >95% phase bright spores. Spores were harvested by centrifugation at 10,000 x g for 10 min and then washed 10 times with ice-cold distilled water to remove any vegetative cells and cell debris. The spore preparation was heated at 70°C for 1 h to kill any remaining vegetative cells, and the final spore concentration was determined by serial dilution. Spore preparations were stored at –20°C until required.

Challenge with aerosolized B. anthracis spores. Aerosol exposure was carried out by using a Henderson-type apparatus (17) and Collison spray (22). Briefly, 10-ml aliquots of STI spores were suspended in sterile distilled water at a concentration of up to 10⁹ CFU/ml, and 3 drops of Antifoam 289 (Sigma) was added just before each preparation was placed in the Collison spray. Groups of mice (heads only) were exposed for 10 min to an air stream containing an aerosol of STI spores generated by the Collison spray and conditioned by the Henderson-type apparatus. The concentration of STI spores in the aerosol was determined by taking samples from the exposure chamber with an all-glass impinger (23) containing sterile distilled water and then plating diluted impinger samples onto nutrient agar to determine the number of spores per liter. The respiratory volume of the animals was calculated by the method of Guyton (15) and the actual dose inhaled and retained in the lungs was calculated by the method of Harper and Morton (16).

Initially, to identify a challenge dose with which to evaluate the Salmonella vaccine candidates, a small dose-finding study was carried out. Briefly, groups of four to five mice were exposed to B. anthracis STI, giving calculated retained doses of approximately 66 CFU, 4.7 x 10² CFU, 5.3 x 10³, or 6.3 x 10⁴ CFU. Subsequently, at 9 weeks after the final immunizing dose with Salmonella mice were challenged with B. anthracis STI spores via the aerosol route with a calculated retained dose of approximately 10⁵ CFU for all groups (ranging between 8.5 x 10⁴ and 1.4 x 10⁵ CFU). This is equivalent to approximately 200 median lethal doses by this route (6). The challenge experiment was carried out blinded. Animals were closely observed for 14 days after challenge to determine their protected status. Humane endpoints were strictly observed so that any animal that displayed a collection of clinical signs that indicated a lethal infection (piloerection, posture [hunching], and mobility problems) was culled.

Statistical analysis. One-way analysis of variance with Tukey's multiple comparison postanalysis test and statistical analysis of survival using the GraphPad Prism version 3.02 for Windows (GraphPad Software, San Diego, CA) were performed.

	RESULTS

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Construction of Salmonella expressing ClyA-PA fusion proteins. Proteins fused to the carboxyl terminus of the S. enterica serovar Typhi ClyA export apparatus can be expressed at a high level in Salmonella and could be transported out of the bacterial cell without causing lysis (10). Thus, in the present study we chose to evaluate ClyA as an export mechanism for known protective domains of PA expressed in Salmonella. Initially, a plasmid expression vector, pSEC10, was constructed that contained the gene encoding ClyA downstream of the P_ompC promoter. This plasmid is similar to those previously described by Galen et al. (11) and also included the hok-sok postsegregational killing locus and the parA gene encoding an active partitioning system. A fusion PCR protocol was followed to create a fusion between domain 1 of PA (PA1) and domain 4 of PA (PA4) and the resulting PA1+4 fusion was cloned into the expression plasmid pSEC10 as a fusion to ClyA, resulting in plasmid pSECPA1+4 (Fig. 1). Similar constructs producing ClyA fused to PA4 and full-length PA were also produced and termed pSECPA4 and pSECPA1-4, respectively. The recombinant plasmids containing the ClyA-PA fusions were subsequently transformed into S. enterica serovar Typhimurium SL3261 by electroporation (resulting in strains SL3261/pSECPA1+4, SL3261/pSECPA4, and SL3261/pSECPA1-4). In vitro expression of the ClyA-PA fusion proteins from the strains was detected by SDS-PAGE and Western blotting in whole-cell lysates with a PA4-specific antibody (Fig. 2). However, the ClyA-PA fusion proteins could not be detected in the culture supernatants using this method.

View larger version (18K): [in this window] [in a new window]   FIG. 1. PA expression plasmids. (A) Cloning of PA fragments into NheI sites of pSEC10 as fusions to the ClyA gene. (B) General structure of pSEC10-based plasmids encoding PA gene fragments: SL3261/PSECPA1-4 encoding domains 1 to 4 of PA, SL3261/pSECPA1+4 encoding domain 1 and domain 4 of PA, and SL3261/pSECPA4 encoding domain 4 of PA.

View larger version (11K): [in this window] [in a new window]   FIG. 2. Expression of PA as ClyA fusions from Salmonella. Normalized cell lysates (3 x 108 CFU/ml) and culture supernatants (either neat or diluted 1:10 as indicated) from S. enterica serovar Typhimurium SL3261 recombinants were subjected to SDS-PAGE and Western blotting with PA4-specific monoclonal antibody. Lane M, Bio-Rad broad-range biotinylated SDS marker; lane 1, SL3261/pSECPA1-4 1:10 cell pellet; lane 2, SL3261/pSECPA1-4 neat supernatant; lane 3, SL3261/pSECPA1+4 1:10 cell pellet; lane 4, SL3261/pSECPA1+4 neat supernatant; lane 5, SL3261/pSECPA4 1:10 cell pellet; lane 6, SL3261/pSECPA4 neat supernatant; lane 7, SL3261/pSEC10 1:10 cell pellet; lane 8, SL3261/pSEC10 neat supernatant; lane 9, 0.1 mg of rPA/ml.

Immunogenicity of Salmonella strains expressing PA. The immunogenicity of the SL3261 recombinants was assessed after intragastric dosing of A/J mice three times at 2-week intervals with approximately 10⁹ CFU of the bacteria. Serum samples were taken on day 13, 27, 45, or 73 and analyzed by ELISA for PA-specific IgG responses. A progressive increase in PA-specific IgG responses was detected over time in immunized mice (data not shown). After only one or two doses of the SL3261 recombinants, PA-specific IgG antibody responses were generally low. However, on day 73, and prior to challenge with B. anthracis spores, all of the mice immunized with Salmonella expressing PA or fragments of PA had developed PA-specific IgG responses (Fig. 3A). Furthermore, analysis of the sera by TNA demonstrated that antibodies capable of neutralizing anthrax toxin were present in the sera from mice immunized with the recombinant Salmonella (Fig. 3B). Differences in the magnitude of the anti-PA responses were observed in individual mice within the groups, and some individual mice failed to show measurable PA-specific responses. However, in mice showing responses, all groups showed statistically similar toxin-neutralizing activity.

View larger version (14K): [in this window] [in a new window]   FIG. 3. Serum immune responses to PA. Serum samples were taken from A/J mice orally immunized three times at 2-week intervals with 1 x 108 to 5 x 109 CFU of S. enterica serovar Typhimurium SL3261 or SL3261 recombinants (A and B) or intramuscularly immunized with 10 µg of PA protein adsorbed to a 20% (vol/vol) solution of Alhydrogel (C and D). Sera were used to determine the IgG (A or C) or TNA (B or D) responses to PA.

View larger version (61K): [in this window] [in a new window]   FIG. 4. SDS-PAGE analysis of purified recombinant PA proteins. Purified PA proteins (2 µg per 10-µl sample loaded) were subjected to SDS-PAGE. Lane 1, Bio-Rad Kaleidoscope-prestained standards; lane 2, rPA1; lane 3, rPA4; lane 4, rPA1+4; lane 5, rPA1-4; lane 6, Bio-Rad low-range prestained standards.

Mice inoculated with the SL3261 recombinants or the purified recombinant proteins were challenged with approximately 10⁵ CFU (equivalent to approximately 200 mean lethal doses) of aerosolized B. anthracis STI spores and monitored for survival. Naive mice and those given the SL3261 parental control strain succumbed to infection within 6 days, and all mice receiving SL3261/pSEC10, SL3261/pSECPA4, or SL3261/pVDL9.3PA83ec died by day 7 postchallenge (Table 3). However, two of eight mice immunized with SL3261/pSECPA1+4 were protected against the challenge, and five of six mice inoculated with SL3261/pSECPA1-4 also survived. Thus, SL3261/pSECPA1-4 expressing the full-length PA protein as a fusion with ClyA afforded significant protection against aerosolized B. anthracis spore challenge (P < 0.01 compared to SL3261/pSEC10). Mice immunized with rPA1-4, rPA1+4, or rPA4 were solidly protected against challenge, and immunization of mice with rPA1 protected two of six mice from challenge with B. anthracis STI (Table 3).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Although studies by Wai et al. (31) indicated that the ClyA protein accumulates in the periplasm and is subsequently exported from the bacterial cell via the release of outer membrane vesicles from the cell surface, we were unable to show that the ClyA-PA protein fusions were exported into the culture supernatants. However, PA expression was detected and the SL3261 recombinants containing pSEC10-based plasmids were found to be at least 80% stable in vitro and in vivo. The pVDL9.3PA83ec plasmid, previously shown to be unstable in S. enterica serovar Typhimurium strain Zoosaloral H (13), was stably maintained in SL3261. This finding perhaps reflects, generally, the relative stabilities of plasmids in different strains of Salmonella.

Mice orally inoculated with SL3261 recombinants expressing full-length PA, domain 4 only, or a fusion protein consisting of domains 1 and 4 generated anthrax toxin-neutralizing antibodies. The Western blot of the SL3261 recombinants probed with anti-PA was prepared using standardized CFU/ml samples (Fig. 2) indicated that full-length PA was not expressed at a higher level in Salmonella than PA1+4 or PA4. Thus, it is likely that the enhanced protective response induced after immunization with full-length PA is a result of the presence of domains 2 and 3. This is consistent with the previous finding that domain 2 is able to improve protection afforded by domain 1 (6). This could be due to the presence of additional protective epitopes or the role played by domains 2 and 3 in tertiary conformation or protein export (30).

Mice orally immunized with SL3261 expressing the full-length PA were protected (five of six mice) against a lethal exposure to aerosolized B. anthracis spores. In comparison, only two of eight mice given SL3261 expressing PA1+4 survived the exposure, whereas all of the mice given SL3261 expressing PA4 succumbed to infection. We believe that this is the first report of the protection of aerosolized anthrax after oral immunization with a Salmonella-based vaccine.

In the present study, we have also evaluated the ability of purified PA protein, the individual domains PA1 or PA4, or the PA1+4 fusion protein to protect mice against aerosolized B. anthracis spores. When administered with Alhydrogel, all of the proteins stimulated strong antigen-specific antibody responses. Although rPA4, rPA1+4, and rPA1-4 conferred complete protection, rPA1 was only able to protect three of eight animals. These data correspond with the finding that rPA1 provided a lower level of protection than rPA4 when challenged with B. anthracis by injection (6). It was not possible to determine whether the purified recombinant fusion protein, rPA1+4, offered a greater level of protection against anthrax than rPA4 only. A higher challenge level may have allowed this to be determined. However, the comparison of the Salmonella recombinants indicated that PA1+4 is more protective than PA1, supporting the evaluation of the fusion protein. Overall, the results from the in vitro and in vivo protection studies indicate that the optimum protective effect is obtained when the full-length PA protein is used to develop the Salmonella-based vaccine.

An important finding from the work reported here is the poor correlation of serum antibody levels to PA with the degree of protection against B. anthracis challenge. However, when sera was tested in a toxin-neutralizing assay, a good correlation was observed. Clearly, these findings suggest that only a proportion of the antibody generated after immunization is able to neutralize anthrax toxin, and immunogens that are able to induce high levels of antibody will not necessarily provide high levels of protection. Similar findings have recently been reported by Duc et al. (5).

The aim of this research is ultimately to develop an orally delivered vaccine for anthrax. In the present study, we have shown for the first time that orally administered Salmonella expressing PA is able to protect mice against infection caused by airborne B. anthracis. However, the development of a vaccine suitable for use in humans would be dependent on the expression of PA in S. enterica serovar Typhi. Depending on the immunogenicity of this recombinant, it may be more appropriate to use this vaccine to boost existing responses that have been primed at an earlier date. Such an orally delivered booster vaccine would be valuable when it is necessary to ensure that large populations rapidly develop protective immunity. Work to construct S. enterica serovar Typhi expressing PA, using the systems we have reported here, is currently under way.

	ACKNOWLEDGMENTS

 
This study was supported by NIH grant 5-U19-AI-56578-03.

We gratefully acknowledge the technical assistance provided by Helen Flick-Smith and the animal technicians at DSTL.

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Biomedical Sciences, Defence Science and Technology Laboratory, Porton Down, Salisbury, Wiltshire SP4 0JQ, United Kingdom. Phone: 44 (0)1980 614755. Fax: 44 (0)1980 614307. E-mail: hsatkins{at}dstl.gov.uk.

Published ahead of print on 4 December 2006.

Editor: J. B. Bliska

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