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Effect of Protein SV-IV on Experimental Salmonella enterica Serovar Typhimurium Infection in Mice

Institute of Microbiology,¹ Department of Biochemistry and Biophysics,² Department of Experimental Medicine, Medical School, 2nd University of Naples,³ CNR International Institute of Genetics and Biophysics, Naples, Italy⁴

Received 5 July 2001/ Returned for modification 18 September 2001/ Accepted 29 October 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

 
Seminal vesicle protein IV (SV-IV) is a secretory anti-inflammatory, procoagulant, and immunomodulatory protein produced in large amounts by the seminal vesicle epithelium of the rat under the strict transcriptional control of androgen. In particular, this protein was shown to possess the ability to markedly inhibit in vivo the humoral and cell-mediated immune responses of mice to nonbacterial cellular antigens (sheep erythrocytes and spermatozoa). We report data that demonstrate that in mice treated with SV-IV and infected with Salmonella enterica serovar Typhimurium, SV-IV is able to downregulate some important immunological and biochemical parameters that serovar Typhimurium normally upregulates in these animals. This event did not correlate with a lower bacterial burden but was associated with a markedly increased one (300%). Furthermore, the treatment of mice with SV-IV alone also produced a significant increase in the rate of mortality among serovar Typhimurium-infected animals. The mechanism underlying these phenomena was investigated, and the strong immunosuppression produced by SV-IV in serovar Typhimurium-infected mice was suggested to be the basis for the increased rate of mortality. The SV-IV-mediated immunosuppression was characterized by a decrease in the humoral and cell-mediated immune responses, altered lymphocyte-macrophage interaction, downregulation of cytokine and inducible nitric oxide synthase gene expression, inhibition of macrophage phagocytosis and intracellular killing activities, and absence of apoptosis in the splenocyte population of SV-IV- and serovar Typhimurium-treated mice. The immunosuppressive activity of SV-IV was specific and was not due to aspecific cytotoxic effects. SV-IV-specific receptors (K_d = 10^-8 M) occurring on the macrophage and lymphocyte plasma membranes may be involved in the molecular mechanism underlying the SV-IV-mediated immunosuppression. Some results obtained by the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide assay also revealed a functional impairment of mitochondria (a decrease in mitochondrial dehydrogenase activity), thus indicating the possible implication of these organelles in the immunosuppressive process.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

 
Seminal vesicle (SV) protein 4 (SV-IV; according to its mobility by sodium dodecyl sulfate [SDS]-polyacrylamide gel electrophoresis [PAGE]) is a small (M_r, 9,758), basic (pI 8.9), thermostable, secretory protein produced in large amounts by the SV epithelium of the adult rat under the strict transcriptional control of androgen (1, 15, 24). Proteins immunologically related to SV-IV have also been identified in several rat tissues (uterus, lung, liver, brain, etc.) as well as in human seminal fluid and SV secretions (2, 17, 18). The SV-IV protein has been purified to homogeneity and extensively characterized (1, 2, 15, 17, 18, 24, 25, 35). Its 90-amino-acid sequence is known, and the gene coding for it has been isolated, sequenced, and expressed in Escherichia coli (6, 12, 13, 16). SV-IV is a very flexible molecule that in aqueous solution behaves as a concentration-dependent self-associating system in which the degree of association (monomer dimer trimer equilibrium) appears to control the biological properties of the protein (35). The biological function of SV-IV is multifaceted. SV-IV is a remarkable bioactive protein due to its powerful non-species-specific anti-inflammatory, procoagulant, and immunomodulatory properties (3, 7, 8, 9, 11, 14, 19, 21, 28, 31, 37, 39). The anti-inflammatory activity of SV-IV is related to its ability to inhibit phospholipase A₂, the first enzyme of the arachidonate cascade (3, 19), while its procoagulant activity has been ascribed to its ability to inhibit antithrombin III (7–9). The modulatory effects of SV-IV on the humoral and cell-mediated immune responses are produced by its interference with macrophage-T cell cooperation (modulation of cytokine release and biological activity, inhibition of the macrophage antigen presentation activity, inhibition of the T-lymphocyte activation process) (19, 28, 31, 37). When it is transformed into a complex polymer by transglutaminase (EC 2. 3. 2. 13), the protein also has the ability to bind to the surfaces of epididymal spermatozoa, markedly decreasing their strong immunogenicity. It has been suggested that this biochemical event makes a critical contribution to immunoprotection of the spermatozoon during its perilous journey toward the egg in the immunologically competent female genital tract (20, 26, 28–30). The protein has also been found to possess a potent activating effect on the horseradish peroxidase and the selenium-dependent glutathione peroxidase (V. Metafora, F. Morelli, and S. Metafora, unpublished results), enzymes that are known to play important roles in the physiological maintenance of cell redox equilibrium. Furthermore, we have recently found that SV-IV has a marked ability to inhibit the apoptosis induced in vitro in Raji cells by serum withdrawal (Metafora et al., unpublished results). Another interesting biochemical property of SV-IV is defined by its ability to promote a lymphocyte cytotoxic activity against the lymphoblastoid Raji cell line in human peripheral blood mononuclear cells (PBMCs) (27). We have experimental evidence that the cytotoxic effectors of this activity are functionally activated natural killer cells (27).

On the basis of these data and considerations, experiments were planned to verify whether the SV-IV protein is able to exert its immunomodulatory activity in mice infected with sublethal doses of pathogenic microorganisms (Salmonella enterica serovar Typhimurium).

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

 
Mice. BALB/c male mice (weight, 20 to 25 g; diet, 70K Mignini [Petrignani, Perugia, Italy]) were maintained in a temperature-controlled animal house (20 ± 2°C) with automatic 12-h lighting cycles.

Microorganism. The microorganism used was S. enterica serovar Typhimurium NCTC 74 grown in nutrient broth (Difco Laboratories, Detroit, Mich.).

Purification of protein SV-IV. Milligram amounts (400 mg) of protein SV-IV were purified to homogeneity from SV secretions of adult Fisher-Wistar rats by a published procedure by using ion-exchange and gel filtration column chromatography (15). The purity of the protein was evaluated by SDS-PAGE under denaturing and nondenaturing conditions (17), amino acid composition analysis, the fingerprinting technique (1), and fast atom bombardment mass spectrometry (30). The SV-IV preparations were completely free of lipopolysaccharide (LPS) and tumor necrosis factor (TNF), as demonstrated by specific biological assays (32, 36). The concentration of the purified SV-IV was measured by its molar absorption at 276 nm (4,100 M^-1 · cm^-1), calculated on the basis of the numbers of tyrosine and phenylalanine residues present in the SV-IV polypeptide chain (8, 35).

Cell preparation. Splenocytes were prepared from aseptically removed mouse spleens by a conventional procedure. The cells were washed three times with RPMI 1640 medium and were resuspended in the same medium supplemented with 10% fetal calf serum, 2 mM glutamine, 20 mM HEPES buffer, 100 U of penicillin per ml, and 100 µg of streptomycin per ml (complete RPMI 1640 medium) at a final concentration of 3 x 10⁶ cells/ml. Appropriate aliquots of these cells were incubated in plastic culture flasks for 1 h at 37°C in an incubator with a humidified atmosphere consisting of 5% CO₂ and 95% air. The resulting adherent cells were cultured overnight in RPMI 1640 medium with 10% fetal calf serum. Cell viability was evaluated by the trypan blue exclusion test. At least 96% of the cells thus obtained were monocytes, as determined with a fluorescence-activated cell sorter (FACS) analyzer (Becton Dickinson, Mountain View, Calif.) with suitable fluorescent monoclonal antibodies (Becton Dickinson, San Jose, Calif.). Nonadherent cells (lymphocytes) were harvested, washed, and resuspended in complete RPMI 1640 medium at a final concentration of 3 x 10⁶ cells/ml; flow cytometry analysis of stained cells with anti-CD3, anti-CD14, anti-CD19, or anti-CD56 monoclonal antibodies (Ortho, Raritan, N.J.; Becton Dickinson, San Jose, Calif.; Serotec, Milan, Italy) demonstrated that more than 94% of the isolated cells were lymphocytes.

For both the control and the experimental groups of animals, peritoneal macrophages were isolated from a pool of cells drawn from the peritoneal cavities of eight mice. Briefly, adherent cells were removed as follows: 10⁷ cells suspended in 3 ml of complete RPMI 1640 medium were incubated for 3 h at 37°C in plastic sterile petri dishes. Nonadherent cells were gently sucked off with a Pasteur pipette. Adherent cells were collected after 15 min of incubation in the presence of 1 mM EDTA in calcium- and magnesium-free phosphate-buffered saline (PBS), washed twice in the same medium, and resuspended in Hank’s medium at a final concentration of 2 x 10⁶ cells/ml.

Standard and alternative mouse treatment protocols with SV-IV and Salmonella. Different groups of 50 mice each were treated for 14 days with a daily subcutaneous injection of either PBS alone (group A) or SV-IV in PBS (5 nmol/mouse; group B).

In the standard protocol, each mouse in a group of 50 mice that had been subcutaneously injected with PBS alone for 14 days was infected with three sublethal doses (4 x 10⁵ CFU/mouse) of S. enterica serovar Typhimurium, each of which was administered intraperitoneally (i.p.) on days 1, 7, and 14 of the PBS treatment (group C), respectively. Each mouse in another group of 50 mice that had been subcutaneously injected with SV-IV in PBS (5 nmol/mouse) for 14 days was infected with three sublethal doses (4 x 10⁵ CFU/mouse) of serovar Typhimurium, each of which was administered i.p. on days 1, 7, and 14 of the SV-IV treatment (group D), respectively. Blood, splenocytes, and peritoneal macrophages obtained from the four groups of animals (groups A, B, C, and D) at different times (3, 7, 15, and 21 days) after the end of the 14 days of treatment with PBS alone, SV-IV alone, PBS and serovar Typhimurium, or SV-IV and serovar Typhimurium were used to perform the majority of the experiments whose results are reported in the Results section.

In the alternative protocol, groups of mice belonging to group A or B were inoculated i.p. with either PBS (control) or a 50% lethal dose (LD₅₀) dose (8 x 10⁵ CFU/mouse) of serovar Typhimurium on day 3, 7, 14, or 21 after the end of the PBS or the PBS and SV-IV treatment. Forty-eight hours after the i.p. inoculation the percent mortality and intracellular bacterial clearance abilities of control or serovar Typhimurium-infected animals were evaluated by the procedures described below.

In preliminary experiments we have found that the optimal in vivo immunosuppressive effect of SV-IV in our murine model was detectable in the range of 2 to 8 nmol of SV-IV/mouse. On this basis, we decided to use in all the experiments reported in this paper an SV-IV concentration of 5 nmol/mouse. Higher or lower concentrations of SV-IV always produced significantly lower immunosuppressive effects, with the decrease in the biological effect of SV-IV at higher concentrations probably being related to the self-associative concentration-dependent properties of this protein in aqueous solutions (formation of biologically inactive SV-IV trimers).

Evaluation of anti-serovar Typhimurium antibody titer. A conventional agglutination test (10) was used to evaluate the anti-serovar Typhimurium antibody titer in sera obtained from groups (groups A, C, and D) of mice treated by the standard protocol described above. Briefly, serum samples serially diluted twofold in PBS were prepared in final volumes of 0.1 ml in glass test tubes (10 by 75 mm). A serovar Typhimurium suspension (0.05 ml; optical density at 550 nm, 0.600/ml) was added to each tube, the contents of the tubes were mixed, the tubes were covered with Parafilm and incubated at 37°C, and the results were read after 24 h. The FACS analysis demonstrated that the immunoglobulins occurring in the analyzed antisera were mainly immunoglobulin G (IgG). Similar anti-serovar Typhimurium antibody titers for comparison were obtained by calculating these titers either as an average of the various titers obtained for the single animals belonging to each group or as the titers for the pooled sera obtained from the different groups of mice.

FACS analysis. Splenocytes obtained from groups of mice treated by the standard protocol (groups A, C, and D) were stained for immunofluorescence analysis by an indirect labeling procedure. Unconjugated antibodies (anti-CD3 and anti-surface IgG [anti-sIgG] from Becton Dickinson [Mountain View, Calif.]; anti-Ia and anti-Mac1 from Serotec) were used as the first staining reagents, whereas fluorescein isothiocyanate-labeled xenogeneic polyspecific or IgG class-specific antibodies were used as the second staining reagents. Control indirect staining procedures that included only the second staining reagent were routinely carried out. Following immunostaining, the cells were counterstained with propidium iodide to allow exclusion of dead cells (brightly stained with propidium iodide) from the immunofluorescence analysis. In particular, before testing for Ia the CD3⁺ cells were separated from other splenocytes by affinity chromatography on an R & D Systems column. Cell fluorescence was analyzed with a cytofluorograph (FACScan; Becton Dickinson, Mountain View, Calif.) by using the 488-mm emission line of an argon laser. Macrophages were identified and separately analyzed on the basis of their characteristic combination of forward, right-angle scatter and their positive fluorescence staining with the specific monoclonal antibodies. The percentage of fluorescence-positive live cells, the mean fluorescence, and the scatter values of fluorescence-positive cells were determined with a Hewlett-Packard computer system. In sandwich staining procedures, the percentage of specifically stained cells was determined by subtracting the percentage of positive cells present in the stained control (the layer stained only with the second staining reagents) from that obtained after staining with both the first and the second reagent antibodies.

Mitogen-induced T- and B-cell proliferation. One hundred microliters of splenocyte suspensions (3 x 10⁵ cells) prepared from groups of mice treated by the standard protocol (groups A, C, and D) was added to the wells of 96-well, round-bottom, sterile microtiter tissue culture plates containing 100 µl of mitogen solution (24 µg of concanavalin A [ConA; Sigma, Milan, Italy] per ml or 20 µg of LPS from E. coli O128:B12 [Sigma] per ml) in complete RPMI 1640 medium. The plates were incubated at 37°C in an incubator with a humidified atmosphere consisting of 5% CO₂ and 95% air for 72 h. Six hours before harvesting of the cells, 0.5µCi of [methyl-³H]thymidine (5 Ci/mmol; Amersham, Little Chalfont, United Kingdom) was added to each well and the culture was continued for another 6 h. All cultures were harvested with a 12-well automated cell harvester and placed onto glass fiber filters. The filters were dried, and their radioactivities were measured with a Beckman liquid scintillation counter. All the determinations were carried out in triplicate.

Evaluation of animal mortality and enumeration of numbers of Salmonella CFU in serovar Typhimurium-infected mice. The effect of SV-IV treatment (5 nmol/mouse for 14 days) on the mortality of S. enterica serovar Typhimurium-infected mice was evaluated in animals inoculated i.p. with 8 x 10⁵ serovar Typhimurium cells (LD₅₀) in PBS at different times (3, 7, 15, and 21 days) after the end of SV-IV treatment (alternative protocol). The mean mortality rates for control mice (PBS-treated mice; group A) and experimental mice (SV-IV-treated mice; group B) were recorded 48 h after infection, and the data are expressed in percent.

Groups of three serovar Typhimurium-infected mice that survived infection with the LD₅₀ were killed by cervical dislocation, and their spleens and livers were aseptically removed and homogenized separately in 2 ml of cold PBS with a sterile glass-Teflon Potter-Elvehjem motor-driven homogenizer. Serial dilutions of the homogenates in sterile PBS were plated on nutrient agar. The numbers of CFU were carefully counted after overnight incubation at 37°C, and the counting results were expressed as the log₁₀ number of bacteria (CFU) per organ.

Phagocytosis assay and killing index determination. The phagocytic activities of the peritoneal macrophages obtained from mice treated by the standard protocol were expressed by the phagocytic index determined with suspended cells by a previously published procedure (38). Briefly, the cells, suspended in complete RPMI 1640 medium (2 x 10⁶/ml), were incubated at 37°C with Staphylococcus epidermidis (10⁶ cells/ml) as target cells. Following 60 min of incubation, 0.5 ml of the sample was added to 1.5 ml of ice-cold complete RPMI 1640 medium to stop the phagocytosis, and the sample was centrifuged at 110 x g for 4 min. Two aliquots (0.1 ml) of three consecutive dilutions of the supernatant were plated. Plates with 10 to 500 colonies were counted, the number of bacteria in the supernatant was calculated, and the phagocytic index was determined. After 60 min of incubation at 37°C to allow phagocytosis, the noningested bacteria were separated from the macrophages by centrifugation (at 110 x g for 4 min) and the macrophages were washed twice at 4°C with ice-cold PBS. The sedimented macrophages were lysed by freezing and thawing, and the numbers of viable intracellular bacteria in the lysates were determined. The level of intracellular killing at 60 min was expressed as the number of viable intracellular bacteria (killing index) by the formula log N₀ - log N_t, in which N₀ is the number of viable intracellular bacteria at time zero and N_t is the number of viable intracellular bacteria at 60 min. Controls were prepared with macrophages not incubated with Staphylococcus to account for the possible occurrence of viable S.enterica serovar Typhimurium or other contaminating bacteria in the different lysates analyzed.

DNA fragmentation analysis: electrophoresis and TUNEL. In order to evaluate by agarose gel electrophoresis internucleosomal DNA fragmentation, a typical biochemical apoptotic event, 10⁶ PBS-washed splenocytes purified from mice treated with PBS alone, SV-IV in PBS alone, PBS-serovar Typhimurium, or SV-IV-serovar Typhimurium by the standard protocol were first sedimented by centrifugation and were then separately suspended in 100µl of TNE buffer (150 mM sodium chloride, 10 mM EDTA, 10 mM Tris-HCl [pH 8]). The cell suspensions were lysed by the addition of 3 volumes of lysis buffer (0.2% SDS, 50 µg of RNase in TNE buffer per ml), and the lysates were incubated at 37°C for 1 h. After incubation, 100 µg of proteinase K per ml was added to the lysate and the mixture was incubated for a further 2.5 h at 56°C. The high-molecular-weight genomic DNA, extracted from the proteinase K-treated lysates by a previously published procedure (33), was analyzed by electrophoresis (2 h, 80 V) in an ethidium bromide-containing 1% agarose gel in TBE (0.045 M Tris-borate, 0.001 M EDTA [pH 8.0]). DNA fragmentation in mouse splenocytes was also detected by the technique of terminal deoxytransferase-mediated dUTP-biotin nick end labeling (TUNEL) of DNA strand breaks (Apoptosis Detection System, Fluorescein; Promega). Splenocytes obtained from control or treated mice and adherent to glass slides were rinsed with PBS and fixed in 4% methanol (20 min, 4°C). The slides were washed with PBS and then covered with equilibration buffer. Terminal deoxynucleotidyltransferase dissolved in a reaction buffer containing fluorescein-dUTP was then added to the cells, and the mixture was incubated (37°C, 1 h) in a humidified chamber. The reaction was first stopped by immersion in 2x SSC (1x SSC is 0.15 M NaCl plus 0.015 M sodium citrate; 15 min), and then the cells were washed and stained with propidium iodide (1 µg/ml; 15 min). The slides were observed by fluorescence microscopy by using a standard fluorescein excitation wavelength. Normal cells were stained red throughout the cytoplasm. Apoptotic cells were identified by their yellow-orange and green fluorescence within the nucleus due to the fluorescein-12-dUTP incorporated at the 3'-OH ends of the fragmented DNAs. Splenocytes partially digested with DNase were used as positive controls. The negative controls were splenocytes treated by the same TUNEL protocol but without the addition of terminal deoxynucleotidyltransferase. Finally, a positive control for apoptosis was prepared by using splenocytes cultured for 6 h at 37°C in standard culture medium in the presence of 250 µM H₂O₂.

MTT test. The 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) test is a colorimetric assay that measures the reduction of the soluble yellow salt MTT (Sigma) with mitochondrial succinate dehydrogenase, an important enzyme of the citrate cycle pathway active in the mitochondrial matrix. The MTT enters the cells and passes into the mitochondria, where it is reduced to a water-insoluble purple formazan product (23). The cells are then solubilized with an organic solvent (isopropanol, dimethyl sulfoxide, etc.), and the released, solubilized formazan is measured spectrophotometrically. Since reduction of MTT can occur only in metabolically active cells, the level of activity is a measure of the viability of the cells and, in particular, of their mitochondrial function. Briefly, at the end of each experimental treatment, 10⁶ purified washed splenocytes obtained from mice subjected to the standard treatment protocol and suspended in 200 µl of PBS were introduced into the wells of 96-well, round-bottom microtiter tissue culture plates; 20µl of MTT reagent (5 mg/ml in PBS) was added to each well, and the plate was incubated at 37°C for 1 h. At the end of the incubation time, the medium was removed by centrifugation (200 xg for 5 min) and the cells were solubilized in dimethyl sulfoxide (200 µl). The extent of MTT reduction to formazan within the living cells was quantitated by measuring the optical density of the solubilized material at 550 nm with a microplate reader (Molecular Devices, Richmond, Calif.).

Nitrite determination. The nitrite concentrations of supernatants from 24-h cultures of peritoneal macrophages (10⁷) isolated from different groups of mice treated by the standard treatment protocol were evaluated by the standard Griess reaction (4) and were compared with those of supernatants from cultures of peritoneal macrophages obtained from control mice. Briefly, 0.1 ml of supernatant was mixed with 0.1 ml of Griess reagent (0.5% sulfanilamide, 0.05%N-1-naphthylethylenediamine dihydrochloride in 2.5% phosphoric acid), and the mixture was incubated for 10 min at room temperature; the absorbance of the reaction mixture was read at 570 nm with a spectrophotometer. The data, expressed as micromoles of NO₂^- per 10⁷ cells, represent the means ± standard errors of the means (SEMs) of triplicate determinations.

RT-PCR analysis. Two micrograms of total RNA prepared by the procedure of Chomczynski and Sacchi (5) from 10⁷ adherent or nonadherent splenocytes obtained from mice subjected to the standard treatment protocol was reverse transcribed with random nanomers and Superscript II reverse transcriptase (GIBCO-BRL) at 37°C for 1.5 h according to the manufacturer’s protocol. The reaction was terminated by heating the reverse transcriptase incubation mixture at 95°C for 5 min, followed by quick chilling on ice. Negative controls for the amplification reactions were obtained by performing RNA transcription in the absence of reverse transcriptase. Two microliters of the synthesized cDNA was amplified in a reaction mixture containing, in a final volume of 50µl, 10 mM Tris-HCl (pH 8.3), 1.5 mM MgCl₂, 50 mM KCl, 200 µM concentration of each of the deoxynucleoside triphosphates, 0.5 U of Taq DNA polymerase Gold (Perkin-Elmer), and 100 ng of both sense and antisense murine primers for gamma interferon (IFN-; sense primer, 5' -TGCATCTTGGCTTTGCAGCTCTTCCTCATGGC-3'; antisense primer, 5' -TGGACCTGTGGGTTGTTGACCTCAAACTTGGC-3'), interleukin-10 (IL-10; sense primer, 5'-CTGGAAGACCAAGGTGTCTAC-3'; antisense primer, 5' -GAGCTGCTGCAGGAATGATGA-3'), IL-5 (sense primer, 5' -GACAAGCAATGACAGACGATGAGG-3'; antisense primer, 5' -CCTGGATTACCTGCAAGAGAGTTC-3'), IL-4 (sense primer, 5' -ATGGGTCTCAACCCCCAGCTAGT-3'; antisense primer, 5' -GCTCTTTAGGCTTTCCAGGAAGTC-3'); transforming growth factorß (TGF-ß; sense primer, 5'-TGGACCGCAACAACGCCATCTATGAGAAAACC-3'; antisense primer, 5'-TGGAGCTGAAGCAATAGTTGGTATCCAGGGCT-3'), TNF alpha (TNF-; sense primer, 5'-TTCTGTCTACTGAACTTCGGGGTGATCGGTCC-3'; antisense primer, 5'-GTATGAGATAGCAAATCGGCTGACGGTGTGGG-3'), IL-1 (sense primer, 5'-AAGATGTCCAACTTCACCTTCAAGGAGAGCCG-3'; antisense primer, 5'-AGGTCGGTCTCACTACCTGTGATGAGTTTTGG-3'), and inducible nitric oxide synthase (iNOS; sense primer, 5' -AACTACTGCTGGTGGTGACAA-3'; antisense primer, 5' -TGCGGCTGGCTTTTCACTCT-3'). The PCR products expected for IFN-, IL-10, IL-5, IL-4, TGF-ß, TNF-, IL-1, and iNOS are 380, 600, 500, 456, 502, 354, 491, and 500 bp, respectively. As internal controls for the IL-10, IL-5, IL-4, TGF-ß, IL-1, and iNOS analyses, sense and antisense primers for the mouse hypoxanthine phosphoribosyltransferase (HPRT) gene were added to the PCR assay mixtures. In contrast, as internal controls for the IFN- and TNF- analyses, sense and antisense primers for the mouse ß-actin gene were added to the PCR assay mixtures. The PCR products synthesized by using the HPRT-specific primers (sense primer, 5' -CCTGCTGGATTACATTAAAGCACTG-3'; antisense primer, 5' -CCTGAAGTACTCATTATAGTCAAGG-3') and the ß-actin-specific primers (sense primer, 5'-GACTACCTCATGAAGATCCT-3'; antisense primer, 5' -GCTTGCTGATCCACATCTGC-3') are expected to be 362 and 520 bp, respectively. The PCRs were performed in a DNA thermal cycler (GeneAmp PCR system 9700; Perkin-Elmer-Applied Biosystems). The HPRT reverse transcription-PCR (RT-PCR) coamplification protocol for iNOS, IL-5, IL-1, IL-10, and TGF-ß was as follows. PCR was started with 10 min of denaturation at 95°C, followed by 38 cycles of 1 min at 95°C, 1 min at 56°C, and 1 min at 72°C, with a final 7 min at 72°C. The ß-actin RT-PCR coamplification protocol for IFN-, IL-4, and TNF- was similar to the HPRT RT-PCR coamplification protocol, except that an annealing temperature of 58°C was substituted for one of 56°C. Coamplification of the different cDNA sequences was performed by adding the primers for HPRT and ß-actin into the amplification reaction mixture 8 cycles later than the time of addition of the other interleukin- or iNOS-specific primers, according to the"primer-dropping" method (40), so that the amplification remained in the exponential phase. The PCR products were analyzed by electrophoresis on an ethidium bromide-containing 1.2% agarose gel in TBE. The identities of these products were confirmed by comparing their sizes with the size expected from the known gene sequence and by direct nucleotide DNA sequencing. Quantitation of each PCR product was achieved by integrating the peak area obtained by densitometry of the ethidium bromide-stained agarose gels (with NIH image software, version 16). The ratio between the yield of each amplified product and that of the coamplified HPRT or ß-actin allowed a relative estimate of mRNA levels in the samples analyzed.

IL-1 and IL-1ß quantitation by immunoassay. The concentrations of IL-1 and IL-1ß in the culture medium of peritoneal macrophages stimulated or not stimulated with LPS (20µg/ml) in the presence or absence of SV-IV (15 µM) were evaluated with two specific competitive enzyme immunoassay kits (ACCUCYTE; Technogenetics, Milan, Italy) according to the manufacturer’s protocol.

Statistical analysis. The data are reported as means ± SEMs obtained from three separate experiments, in which each point was determined from assays performed in triplicate. The means were compared by analysis of variance plus Bonferroni’s t test, and a P value of less than 0.05 was considered significant.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

 
SV-IV pretreatment of S. enterica serovar Typhimurium-infected mice increases the animal mortality rate and produces a marked decrease in intracellular bacterial clearance in spleen and liver macrophages. The effect of SV-IV (5 nmol/mouse for 14 days) on the mortality rate and the in vivo intracellular bacterial clearance for mice injected with a single LD₅₀ of serovar Typhimurium (8 x 10⁵ cells) at different times (3, 7, 15, or 21 days) after the end of SV-IV treatment by the alternative treatment protocol (see Materials and Methods) was evaluated, and the relevant data are reported in Tables 1 and 2, respectively. At this point, it is noteworthy that as a consequence of the large doses of serovar Typhimurium used in this protocol, the death of the infected animals was rapid (few days) and was caused by a severe endotoxic shock. From these data it appears that the percent mortality of the infected mice progressively increased with time, reaching a maximum of 85% 21 days after the end of SV-IV treatment (Table 1). Concurrent with the increase in the animal mortality rate, a marked increase (about 65%) in the number of intracellular living bacteria in serovar Typhimurium-infected spleen and liver macrophages was already detectable by day 3 after the end of SV-IV treatment. The bacterial burden in these cells increased progressively with time, reaching a maximum (about 320%) 21 days after the SV-IV treatment. It is interesting that the increase in the organism burden was about the same (300%) when the experiment was repeated with the standard treatment protocol.

View larger version (34K): [in this window] [in a new window]   FIG. 1. (A) Suppressive effect of SV-IV on the mouse humoral immune response to sublethal serovar Typhimurium infection (standard protocol). (B) Nitric oxide production by splenic macrophages (107) obtained from mice injected with PBS or SV-IV for 14 days and concurrently infected with sublethal doses of serovar Typhimurium by the standard protocol. (C) Mitochondrial dehydrogenase activity (MTT test) of splenocytes obtained from animals infected with sublethal doses of serovar Typhimurium in the presence or absence of SV-IV (standard protocol). The extent of MTT reduction to formazan within the living cells, which is proportional to the mitochondrial dehydrogenase activity, was quantitated by measuring the optical density at 550 nm of the solubilized material with a Molecular Devices microplate reader. Open bars, mice injected with PBS only (control); bars with diagonal stripes, serovar Typhimurium-infected mice injected with PBS only; solid bars, serovar Typhimurium-infected mice injected with SV-IV. Experimental details are reported in Materials and Methods. The data represent the means ± SEMs of triplicate determinations.*, P < 0.05 versus the serovar Typhimurium-infected mice injected with PBS; **, P < 0.01 versus the serovar Typhimurium-infected mice injected with PBS.

View larger version (73K): [in this window] [in a new window]   FIG. 2. Semiquantitative RT-PCR analysis of cytokine (A to G) or iNOS (H) mRNA expression in lymphocytes (A to D) or macrophages (E to H) obtained from the spleens of mice 3 and 7 days after the end of the standard treatment with SV-IV and serovar Typhimurium, alone or in combination. Total RNA was isolated from 107 splenocytes obtained from untreated mice (control mice injected with PBS only) or treated mice (serovar Typhimurium-infected mice injected with PBS [STM]; mice injected with PBS and SV-IV [SV4]; serovar Typhimurium-infected mice injected with SV-IV [STM + SV4]) and amplified by RT-PCR with specific primer pairs. Experimental details are reported in Materials and Methods. No products were detectable in control amplifications performed in the absence of cDNA [negative control; control (-)]. The semiquantitative evaluation of each PCR product was achieved by integrating the peak area obtained by densitometry of the ethidium bromide-stained agarose gels (with NIH image software, version 16). The ratio between the yield of each amplified product and that of the coamplified internal control allows a relative estimate of mRNAs levels in the samples analyzed. The ratios were as follows, from left to right: IFN-/ß-actin mRNA ratio, 3.22, 3.16, 2.65, 0.20, 1.64, 1.00, 0.63, and 0.005; IL-10/HPRT mRNA ratio, 0.17, 6.71, 4.47, 3.15, 4.26, 4.28, 3.35, and 1.02; IL-5/HPRT mRNA ratio, 0.08, 1.04, 0.15, 0.10, 0.13, 0.15, 0.06, and 0.05; IL-4/HPRT mRNA ratio, 0.13, 1.03, 0.12, 0.10, 0.10, 0.07, 0.06, and 0.06; TGF-ß/HPRT mRNA ratio, 0.03, 1.98, 0.50, and 0.02; TNF-/ß-actin mRNA ratio, 0.59, 1.9, 1.29, and 1.54; IL-1/HPRT mRNA ratio, 0.08, 2.33, 0.08, and 0.28; iNOS/HPRT mRNA ratio, 0.01, 1.67, 0.02, and 0.01.

Release of IL-1 and IL-1ß from LPS-stimulated peritoneal macrophages is markedly inhibited by SV-IV in vitro.

Mitochondrial damage not associated with classic apoptotic signs is detectable in the splenocytes of mice treated with SV-IV and serovar Typhimurium-. In the previous paragraphs we have reported data that strongly suggest the possibility that an SV-IV-mediated immunosuppressive mechanism could be the basis for the marked increase in the rate of mortality that occurs in mice treated with the combination of SV-IV and serovar Typhimurium. To explore the involvement of apoptosis in this mechanism, we evaluated by TUNEL analysis and a DNA fragmentation electrophoretic assay the occurrence of apoptotic death in the splenocyte population obtained from mice treated with either PBS alone, SV-IV in PBS, PBS and serovar Typhimurium, or SV-IV and serovar Typhimurium by the standard protocol. The results obtained demonstrated that the number of apoptotic events in all splenocyte populations analyzed (data not shown) was not significant, whereas in the apoptosis-positive control evaluation performed with splenocytes treated with 250 µM H₂O₂ at 37°C for 6 h, more than 50% of the cell population was clearly apoptotic (data not shown).

In contrast to these findings, the data from the MTT assay reported in Fig. 1C show that a progressive decrease with time of the mitochondrial dehydrogenase activity (expression of a functional mitochondrial damage) in splenocytes of mice treated with SV-IV and serovar Typhimurium was especially evident (about 70%) 21 days after the end of the standard experimental treatment. It is noteworthy that a similar but smaller reduction of the activity of the same enzyme (about 25%) was also detectable in splenocytes prepared from mice treated with serovar Typhimurium alone 21 days after the last serovar Typhimurium inoculation (Fig. 1C).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

 
The infection of SV-IV-treated mice with a single LD₅₀ of S. enterica serovar Typhimurium on day 3, 7, 15, or 21 after the end of the SV-IV treatment (alternative protocol) produced a significant increase in the rate of mortality among these animals that was associated with a marked reduction of the intracellular bacterial clearance abilities of their spleen and liver macrophages. The SV-IV treatment of mice concurrently infected with sublethal doses of serovar Typhimurium (standard protocol) produced a decrease in the in vitro phagocytosis and intracellular killing activities of their peritoneal macrophages. The reduction in the level of clearance of the bacteria from the spleens and livers and the decrease in the level of intracellular killing of the bacteria in the peritoneal macrophages of mice treated with SV-IV and serovar Typhimurium were probably related to a marked downregulation in the abilities of these macrophages to produce NO (a free radical involved in the intracellular killing of bacteria) and iNOS. The inhibitory effect of SV-IV on iNOS gene expression could be related, in turn, to the binding of SV-IV to SV-IV-specific tyrosine kinase-associated receptors (K_d = 10^-8 M; 80,000 to 100,000 SV-IV-specific binding sites/cell) 11, 19, 21, 35; Metafora et al., unpublished data), with the subsequent production of a protein phosphorylation cascade following the plasma membrane signal transduction process. In addition, as a result of the known ability of anti-inflammatory drugs to control the inflammatory process through the downregulation of the NF-B gene expression pathway, the possible inhibition of NF-B (41) by SV-IV (an anti-inflammatory protein) could reasonably be involved in the process. The SV-IV-mediated reduction of phagocytosis observed in serovar Typhimurium-infected mice confirms previous data from our laboratory that have demonstrated the in vitro inhibitory effects of SV-IV on human macrophage and polymorphonucler leukocyte phagocytosis activities (11, 21).

The higher rate of mortality observed among serovar Typhimurium-infected mice treated with SV-IV in comparison with that observed among the PBS-treated animals could be related not only to the decrease in the level of macrophage phagocytosis and intracellular killing activity but also to the marked inhibition of the humoral and cell-mediated immune responses to the serovar Typhimurium infection. The mechanism of this SV-IV-mediated effect was investigated. The data reported in this paper show that in the spleens of mice treated with SV-IV and serovar Typhimurium a significant decrease in the total number of splenocytes and their main cell subsets (T and B cells, macrophages) was associated with a marked decrease in the total number of Ia⁺ splenic T cells and a strong inhibition of the ability of the splenocytes to respond in vitro to polyclonal mitogen stimuli (this may be the possible expression of SV-IV-mediated anergy). In addition, classic signs of apoptosis were not detected in these cells, although their mitochondria were found to be functionally damaged (MTT assay; see below). These findings may reasonably be related to a decrease in the level of cell proliferation resulting from both a marked reduction of the serovar Typhimurium-mediated macrophage and lymphocyte activation process and the establishment in these cells of a certain degree of SV-IV-mediated anergy instead of to an increase in the level of cell death. Taken together, these data strongly suggest that the inhibitory effect of SV-IV on the humoral immune response is the consequence of altered cooperation between macrophages and lymphocytes (inhibition of macrophage antigen presentation activity, inhibition of macrophage and lymphocyte cytokine synthesis and release, inhibition of lymphocyte activation and proliferation [19, 28, 31, 37]).

It is interesting that the in vivo immunosuppressive effects of SV-IV on serovar Typhimurium-infected mice correlate very well not only with the in vivo inhibitory action of SV-IV on the mouse humoral immune response to other cell antigens (sheep red blood cells and mouse epididymal spermatozoa) but also with the in vitro immunosuppressive action of SV-IV on LPS-, ConA-, or antigen-stimulated rat, mouse, or human PBMCs (19, 28, 31, 37).

The possibility that the immunosuppressive activity of SV-IV could be due to aspecific cytotoxic properties of this protein can be ruled out by the following observations. (i) The immunosuppressive activity of SV-IV is detectable in vitro on activated PBMCs only at a relatively low range of concentrations (5 to 30 µM); higher concentrations become progressively ineffective (biphasic effect) as a consequence of the SV-IV concentration-dependent self-association equilibrium (at higher concentrations there is a shift from the active monomeric form to the biologically inactive, nontoxic dimeric or trimeric configuration) (35). (ii) The same protein at similar concentrations does not inhibit but, rather, stimulates in vitro quiescent macrophages and lymphocytes to produce and release specific cytokines (37). (iii) We have demonstrated that the inhibitory effect of SV-IV on cell proliferation is specific for immunocompetent cells; the growth characteristics and morphologies of a variety of normal or transformed cell lines, in fact, do not change in the presence of concentrations of SV-IV (5 µM) unequivocally immunosuppressive for PBMCs (19). (iv) Finally, the nontoxicity of SV-IV is strongly supported by the data reported in this paper, which show that in the splenocytes of mice treated with either SV-IV-PBS or SV-IV-serovar Typhimurium the rate of death from apoptosis was insignificant. In addition, the intrinsic antiapoptotic activity of SV-IV recently discovered in our laboratory (see the introduction) could also contribute to an explanation of the absence of classic signs of apoptosis in the splenocytes of SV-IV-treated mice. Apoptosis was also absent in the splenocytes of serovar Typhimurium-infected mice. In contrast to this finding, the literature reports data that show that a variety of invasive strains of Salmonella serovar Typhimurium indeed possess the ability to promote in vitro the apoptotic death of human and murine macrophages after cell invasion (22, 34). Such a discrepancy may be related to both the in vivo conditions and the particular strain of serovar Typhimurium (NCTC 74) used in our murine model of experimental serovar Typhimurium infection.

Although the SV-IV protein is not cytotoxic per se and classic signs of apoptosis have not been detected in the splenocytes of mice treated with SV-IV and serovar Typhimurium, the metabolic activities of these cells seem to be somehow impaired, as shown by the significant reduction of their mitochondrial dehydrogenase activity (as determined by the MTT assay). This finding suggests that mitochondria could play an important role (perhaps an involvement in the induction of anergy) in the molecular mechanism at the basis of the marked immunosuppression induced in mice by long-term (14 days) treatment with SV-IV. Experiments are in progress to verify this hypothesis.

The immunosuppressive effect of SV-IV in our murine model of experimental serovar Typhimurium infection can be related either to the direct inhibitory effect of SV-IV on the strong immunogenicity of some important components of the serovar Typhimurium outer membrane (LPS, porins, etc.) or to the negative interference of this protein with the signal transduction biochemical machinery of the macrophage and/or the lymphocyte plasma membrane. Against the first hypothesis there is the finding that SV-IV is unable to form in vitro a stable molecular complex with LPS (39). On the contrary, the second possibility is supported by the finding that SV-IV has the ability to interact with its target cells (lymphocytes, macrophages, polymorphonuclear lymphocytes, spermatozoa, and platelets) (35) by binding to SV-IV-specific tyrosine kinase-associated plasma membrane receptors (see above). This hypothesis is also consistent with our previously published data that have demonstrated the ability of SV-IV to inhibit in vitro the processes of macrophage antigen presentation and lymphocyte activation following its binding to the plasma membranes of these cells (19, 28).

The cytokine mRNA profiles of lymphocytes and macrophages isolated from the splenocyte populations of mice treated with serovar Typhimurium and SV-IV indicate that SV-IV does not inhibit cytokines (IFN-, Il-10, IL-4, IL-5, IL-1, TNF-, and TGF-ß) but, rather, inhibits the serovar Typhimurium-induced rise in cytokine levels. The molecular mechanism underlying the downregulation effect of SV-IV on cytokine gene expression is probably defined by the same mechanism, suggested above, that explains the inhibitory effect of SV-IV on iNOS gene expression.

As we have already mentioned in the introduction, SV-IV is an immunomodulatory protein that activates lymphocytes and macrophages when they are resting, inhibiting them, on the contrary, when they are activated (37). This finding suggests the possibility that SV-IV could play an important role in the maintenance of the homeostasis of the immune system. To play such a role, a molecule is expected to be produced in the right amount only when it is needed, i.e., when the activity of the system being controlled is significantly shifted from the equilibrium point. The production of abnormal levels of this substance for a long time could alter the homeostasis of the system being controlled in such a way as to bring about devastating consequences for the survival of the organism in which this event occurs. In our murine model of experimental serovar Typhimurium infection, an SV-IV-induced inhibitory adjustment of the mouse immune system stimulated by the bacterial invasion is useful if it is appropriate (in terms of time and level) to maintain the balance of the immune response, but if it is not appropriate, it can lead the organism to succumb to the bacterial invasion.

	ACKNOWLEDGMENTS

 
We are very grateful to Salvatore Baiano and Francesco Moscatiello for skillful, excellent technical assistance.

	FOOTNOTES

 
* Corresponding author. Mailing address: Istituto di Microbiologia, Larghetto Santaniello a Caponapoli, 80138, Naples, Italy. Phone: (39) 081-5665663. Fax: (39) 081-5665663. E-mail: caterina.romano{at}unina2.it.

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