The clinical strain of Clostridium tetani was obtained from Christian Medical College, Vellore, India. The strain exhibited 100% sequence identity with C. tetani strain E88 at 16S rDNA level. Clostridium perfringens ATCC13124 was obtained from Becton Dickinson India Pvt. Ltd., India. The clostridial isolates were cultivated anaerobically at 37°C in trypticase peptone yeast-extract glucose (TPYG) broth containing pancreatic digest of casein, 50 g; peptone, 5 g; yeast extract, 20 g; glucose, 4 g; sodium thioglycollate, 1 g; cycloserine, 250 mg; sulphamethoxazole, 76 mg and trimethoprim, 4 mg per litre.

Animal experiments were approved by the institutional Animal Ethical Committee at DRDE, Gwalior. Four-week-old female BALB/c mice were actively immunized against heat-killed vegetative cells of C. perfringens in a four week immunization schedule. Cells were grown in TPYG broth at 37°C, harvested in the exponential phase (OD_{600 nm} 0.8–1.0) and washed with phosphate buffer saline (PBS). The number of bacteria in the final suspension was determined by plating 10-fold serial dilutions onto SPS agar (Difco, USA) plates containing tryptone, 15 g; yeast extract, 10 g; ferric citrate, 0.5 g; sodium sulfite, 0.5 g; sodium thioglycollate, 0.1 g; polysorbate 80, 0.05 g; sulfadiazine, 0.12 g; polymyxin B sulfate, 0.01 g; agar, 15 g per litre. Heat inactivation was accomplished in a water bath at 60°C for 30 min. No live bacteria were detected after this suspension was plated onto agar plates. Cells were injected intraperitoneally using Freund's complete adjuvant (Sigma Aldrich, India) for the first immunization and Freund's incomplete adjuvant for booster immunizations. On day 1 and 7, 10² cfu (100 μl cell suspension in PBS and 100 μl adjuvant) was injected in each mouse while on day 14 and 27 the dose was increased to 10⁴ CFU. One week after administration of the last booster, 10 animals were anesthetized by halothane inhalation, and blood specimen (500 μl) was obtained from each by means of retroorbital puncture. Serum from these specimens was pooled and was used to verify specific antibody production by Western blot analysis. Sham-immunized animals received an equal volume of adjuvant alone in a parallel, same immunization schedule and serum was collected after 5 weeks.

For protection studies, four-week-old female BALB/c mice were similarly immunized with heat killed vegetative cells of C. perfringens in a four week immunization schedule as described above. On day 37, groups of immunized (with CPWC) and sham-immunized animals (n = 12) were challenged intra-peritonealy with different inocula of freshly grown C. tetani cells (1.2 × 10², 1.2 × 10⁴, 1.2 × 10⁶, and 1.2 × 10⁸ cfu). Death, as well as paralytic symptoms were recorded every 6 hr up to day 2 and every 12 hours for seven days. Animals that survived for the entire 7-days were considered survivors.

The culture supernatant from C. tetani was titrated for estimation of minimum lethal dose (MLD) by serial two-fold dilutions made in gelatin diluent. One half milliliter of each dilution was inoculated i.p. into each of six 20 gram mice. The mice were observed for four days and the flaccid paralysis and deaths were recorded. Mice immunized with heat killed C. perfringens, were challenged with 1, 3, and 5 MLD (n = 6) of crude tetanus toxin and observed for death and paralysis. Sham-immunised mice (n = 6) were also given equivalent doses of tetanus toxin i.p.

Twenty milliliter of culture was harvested in the exponential growth phase (OD_{600 nm}~0.8) and washed in 50 mM Tris/HCl, pH 7.5. The cells were resuspended in the same buffer supplemented with protease inhibitor (Protease inhibitor cocktail, Sigma). Cell lysis was performed by sonication and the un-disrupted cells were removed by centrifugation (6000 × g; 15 min; 4°C). In order to improve focusing of proteins the lysates (500 microgram) were purified using 2D-cleanup kit (Bio-Rad) and the protein pellet was finally resuspended in 250 μl of sample rehydration buffer (8 M urea, 2% w/v CHAPS, 15 mM DTT and 0.5% v/v IPG buffer pH 3–10).

Total protein concentration was determined according to the method of Bradford 9 using Quick Start Bradford Protein Assay kit (Bio-Rad, USA) as per manufacturer's instructions. The protein concentration was calculated using bovine serum albumin (BSA) as standard.

The isoelectric focusing was performed using immobilized pH gradient (IPG) strips (Bio-Rad, USA). IPG strips with a pH range from 5–8 were used for all the experiments. For the first dimension 250 μg of protein samples in 125 μl of rehydration solution was used to rehydrate IPG strip (7 cm, pH 5–8). The IPG strips were rehydrated overnight and then the proteins were focused for 8000 VHr at 20°C under mineral oil. After focusing, the strips were incubated for 10 min, in 2 ml of equilibrium buffer I (6 M urea, 30% w/v glycerol, 2% w/v SDS and 1% w/v DTT in 50 mM Tris/HCl buffer, pH 8.8) followed by equilibrium buffer II (6 M urea, 30% w/v glycerol, 2% w/v SDS and 4% w/v iodoacetamide in 50 mM Tris/HCl buffer, pH 8.8). After the equilibration steps the strips were transferred to 12% SDS-PAGE for the second dimension by the method of Blackshear 10. Protein spots were visualized by staining with Commassie Brilliant Blue G-250. Gel images were capture by GS800 densitometer (Bio-Rad, USA). Relative abundance of spots was determined by PD Quest software (Bio-Rad, USA).

Two independent cell preparations were pooled together for running the 2DE gel and obtaining the corresponding immunoblot. Replicate gels were generated from two such independent experiments, of which one representative gel has been shown.

For immunoblotting, the one dimensional or 2-DE separated proteins were transferred electrophoretically to nitrocellulose membrane (Bio-Rad, Hercules, CA) and then blocked with 5% skim milk in PBS (pH 7.2). Hyper-immune serum from mice raised against C. perfringens whole cell (CPWC) was used at 1:4000 dilutions in blocking buffer. Goat anti-mouse HRP conjugate was used as secondary antibody and blots were developed using the Immuno-Blot HRP assay kit (Bio-Rad, USA) as per manufacturer's instructions.

One milliliter of culture was harvested in the exponential growth phase (OD_{600 nm}~0.8), washed in phosphate buffer saline (PBS), pH 7.2, and resuspended in 1 ml of same buffer. Twenty microlitre of cells were air dried on 4 mm wells of printed slides (Flow Lab, USA) and fixed with methanol for 5 min. C. perfringens ATCC13124 and C. tetani cells were added to duplicate wells on two independent slides. Each spot was washed twice with PBS and blocked with 0.5% gelatin in PBS (PBSG) for 30 min at 37°C. To one slide, serum from sham-immunized mice (40 μl) was added at 1:40 dilution in PBSG and to the other slide mouse anti-C. perfringens serum was similarly added. Slides were incubated in humid chamber at 37°C for 1 hr and then washed 4 times with PBS. Forty microlitre of goat anti-mouse IgG fluorescein isothiocyanate (FITC) conjugate (Dako, Denmark) was added (1:20 diluted in PBSG) to each well and incubated in dark, moist chamber for 30 min at 37°C. Slides were washed with 4 changes of PBS and observed under a fluorescence microscope (Leica, Germany).

Protein spots were excised with the help of thin-walled PCR tubes (200 μl) appropriately cut at the bottom with the help of fresh surgical scalpel blade. Care was taken not to contaminate the spots from adjoining proteins or with skin keratin. The gel spots were washed with proteomic grade de-ionized water and identified by mass spectrometry by the commercial services provided by Dominion Pharmakine, Spain. The gel piece containing the protein was destained, reduced/alkylated and digested using the Montage In-Gel Digest Kit (Millipore) following the kit's instructions.

Analysis was performed using the Voyayer-DE PRO BioSpectrometry workstation from Applied Biosystems. Spectrum was obtained in the mass range of 500–4000 Da and calibrated using a calibration mixture containing angiotensin I, Substance P, ACTH (1–17), ACTH (18–39) and somatostain (28). Peptides masses of the unknown proteins were sent to two different peptide mass fingerprinting databases, Mascot from Matrix Science http://www.matrixscience.com and MS-Fit from Protein Prospector http://prospector.ucsf.edu and/or Aldente http://www.expasy.ch/tools/aldente. There were 3292813 entries in the Mascot database at the time of search. Search parameters were as follow: maximum allowed peptide mass error of 100 ppm, consideration of one incomplete cleavage per peptide and at least 4 peptides identified. Protein localization prediction was performed by the online tool PSORT at http://www.expasy.ch/.