Tempeh

Dehulled yellow-seeded soyabeans (Glycine max) were soaked overnight for about 16 h in tap-water while undergoing accelerated lactic acid fermentation using naturally acidified soaking water as an inoculumReference Nout, de Dreu, Zuurbier and Bonants van Laarhoven¹⁷. Subsequently, the beans were washed with tap-water and cooked (100°C) in fresh tap-water at a ratio of 1:3 for 20 min, and cooled to room temperature within 20 min by evaporation of adhering water by spreading them on perforated trays. Sporangiospore suspension was obtained by scraping off the sporangia from pure slant cultures of Rhizopus microsporus var. microsporus LU 573 grown on malt extract agar (Oxoid, CM 59) for 7 d at 30°C and suspending them in sterile distilled water with 0·85 % NaCl and 0·1 % peptone. After inoculation of the cooked soyabeans with the sporangiospore suspension (1 %, v/w), the beans (450 g) were packed in hard-PVC, perforated boxes (205 × 90 × 45 mm) and incubated at 30°C for 72 h. The resulting fresh tempeh was cut into 1 cm dice and dehydrated for 6 h at 60°C, ground using a 1·0 mm screen and stored at − 20°C until use.

Tempeh was pre-digested as described earlierReference Kiers, Nout and Rombouts¹⁸. It was suspended in distilled water (5 g/30 ml) and incubated while stirring with 2 ml α-amylase solution consisting of 125 000 units/l α-amylase (A-1031; Sigma Chemical Co., St Louis, MO, USA), 1·5 g/l NaCl, 1·5 g/l K₂HPO₄, 0·5 g/l Na₂CO₃ (pH 7·0) for 30 min at 37°C. Next, the pH was adjusted to 4·0 using 5 m-HCl and the suspensions were incubated with 8 ml stomach-medium (0·1 g/l lipase (Rhizopus F-AP15; Amano Pharmaceuticals, Nagoyy, Japan), 0·125 g/l pepsin (P-6887; Sigma), 3·1 g/l NaCl, 1·1 g/l KCl, 0·6 g/l Na₂CO₃, 0·11 g/l CaCl₂, pH 4·0) for 1 h at 37°C. The pH was then adjusted to 6·0 using solid NaHCO₃. Finally, 10 ml of a 2 % pancreatic solution (20·0 g/l pancreatin (P-1750; Sigma), 5·0 g/l bile (B-3883; Sigma), 5·0 g/l NaCl, 0·68 g/l KH₂PO₄, 0·3 g/l Na₂HPO₄, 0·84 g/l NaHCO₃) was added and the suspensions were incubated for 30 min at 37°C. After pre-digestion the slurry was diluted using distilled water to 6·5 % DM.

Part of the suspension was centrifuged at 3000 g for 15 min at 4°C. The supernatant was filtered through a filter aid (Celite^®545, 22 140; Fluka, Buchs, Switzerland) to remove residual coarse particles and finally filtered through a 0·22 μm filter (Steritop SCGPT05RE; Millipore, Billerica, MA, USA).

Supernatant of pre-digested tempeh was fractionated into permeate and retentate using ultra-filtration through a spiral wound membrane with molecular weight cut-off of 5 kDa (S2K328; Koch, Wilmington, MA, USA) against distilled water. In order to obtain fractions having the same volume as that of the original supernatant, permeate and retentate volumes were adjusted using rotary vacuum evaporation at 40°C.

Analysis

DM content of pre-digested supernatant, permeate and retentate was determined by drying aliquots until constant weight and nitrogen content was measured using a NA2100 nitrogen analyser (Interscience, Breda, The Netherlands). After centrifugation (10 min, 1300 g), sodium, potassium and chloride concentrations were determined using an Electrolyte 4+ analyser (Nova Biomedical, Waltham, MA, USA) and osmolality was determined using a cryoscopic osmometer (Osmomat; Gonotec, Berlin, Germany).

Gel permeation chromatography was performed on a LC-10Ai HPLC (Shimadzu Benelux, 's-Hertogenbosch, The Netherlands) equipped with a Superdex Peptide column (17-5003-01; Pharmacia Biotech, Piscataway, NJ, USA) and elution at 30°C with 0·1 % (v/v) trifluoroacetic acid and 30 % (v/v) acetonitrile at 0·5 ml/min. The eluate was monitored using a UV detector at 200 nm. Calibration was performed using proteins and peptides ranging from 200 to 7000 Da.

High-performance size-exclusion chromatography was performed on a SP8800 HPLC (Spectra Physics, Mountain View, CA, USA) equipped with three columns (each 300 × 75 mm) of Bio-Gel TSK in series (40XL, 30XL and 20XL; Bio-Rad Labs, Hercules, CA, USA) in combination with a TSK guard column (40 × 6 mm) and elution at 30°C with 0·2 m-NaNO₃ at 0·8 ml/min. The eluate was monitored using a refractive index detector. Calibration was performed using dextrans ranging from 180 Da to 500 kDa.

Net intestinal absorption

All procedures involving animal handling and testing were reviewed and approved by the Animal Care and Ethics Committee of the Animal Sciences Group Lelystad, The Netherlands.

Piglets (crossbred Yorkshire × (Large White × Landrace)) were weaned at 3 weeks of age. About 2 weeks after weaning biopsies from the duodenal mucosa were taken using a fiberscope (Olympus GIF XP10; Olympus, Hamburg, Germany) and receptor status was determinedReference Sellwood, Gibbons, Jones and Rutter¹⁹. Sixteen piglets that expressed the receptor (K88/F4) involved in binding of the ETEC strain were used in the experiments 3 weeks after weaning.

The small intestinal segment perfusion test was carried out essentially as described beforeReference Nabuur, Hoogendoorn, van Zijderveld and van der Klis²⁰. Up to ten segments, with a cranial inflow and a caudal outflow tube and 20 cm long, were situated between 35 and 65 % of the total length of the small intestine.

At 15 min before the perfusion started, the odd-numbered segments were injected with 5 ml ETEC (5 × 10⁹ colony forming units, O149:K91:K88^ac, producing LT and STb) and the even-numbered segments with 5 ml PBS. In each piglet, pairs of segments (a non-infected and an adjacent ETEC-infected) were perfused with either saline (supplemented with 0·1 % glucose and 0·1 % casamino acids and serving as an internal control to determine the maximum response to the infection) or any of the tempeh products, using a Latin-square design. Each segment was perfused with 64 ml product over 8 h, by injecting 2 ml product every 15 min.

Three consecutive experiments were carried out. In experiment 1 the total pre-digested tempeh, its supernatant, saline (and another not relevant soyabean product) were tested in four piglets in a 4 × 4 Latin-square design. In experiment 2 saline, the supernatant of the pre-digested tempeh, the permeate and the retentate obtained after ultra-filtration were tested in eight piglets in a replicated 4 × 4 Latin-square design. In experiment 3 with four piglets saline, the supernatant of pre-digested tempeh, the supernatant of undigested tempeh (and another not relevant soyabean product) were tested in a 4 × 4 Latin-square design.

At the end of the small intestinal segment perfusion test the product remaining in the segments was blown out into the drainage bottles. The piglets were killed by injection of sodium pentobarbital (200 mg/kg body weight) and the segments were cut from the mesenterium and their length was measured.

Net fluid, sodium, chloride and solute absorption were calculated from the difference between the volume and concentration of inflow and outflow divided by the surface area (length × circumference) of each segment. Reduction in net fluid absorption upon ETEC infection was determined by subtracting net fluid absorption in ETEC-infected segments from net fluid absorption in non-infected segments perfused with the same perfusion fluid.

Statistics

Results of non-infected and ETEC-infected segments perfused with the same product were compared using the Student's paired t test. The effect of the perfusion fluid on net fluid absorption upon ETEC infection was analysed with ANOVA for a Latin-square design with piglet, pair of segment and treatment as model effects. Results on net fluid absorption and osmolality in experiment 2 were analysed using linear regression analysis. All statistics were performed with GraphPad Prism version 4.00 for Windows (GraphPad Software, San Diego, CA, USA). Net absorption of fluid, DM, sodium, chloride and solutes are presented as means and their standard errors.