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Original Article |
Is Required for Macrophage Activation and Defense Against Bacterial Infection
Address correspondence to Lisardo Boscá, Instituto de Bioquímica, Facultad de Farmacia, 28040 Madrid, Spain. Phone: 34-91394-1853; Fax: 34-91544-7254; E-mail: boscal{at}eucmax.sim.ucm.es
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Abstract |
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in the immune system, we generated mice that carried a homozygous disruption of the PKC locus. PKC-/- animals appeared normal and were generally healthy, although female mice frequently developed a bacterial infection of the uterus. Macrophages from PKC-/- animals demonstrated a severely attenuated response to lipopolysaccharide (LPS) and interferon (IFN)
, characterized by a dramatic reduction in the generation of NO, tumor necrosis factor (TNF)-
, and interleukin (IL)-1ß. Further analysis revealed that LPS-stimulated macrophages from PKC-/- mice were deficient in the induction of nitric oxide synthase (NOS)-2, demonstrating a decrease in the activation of I
B kinase, a reduction in IB degradation, and a decrease in nuclear factor (NF)B nuclear translocation. After intravenous administration of Gram-negative or Gram-positive bacteria, PKC-/- mice demonstrated a significantly decreased period of survival. This study provides direct evidence that PKC is critically involved at an early stage of LPS-mediated signaling in activated macrophages. Furthermore, we demonstrate that in the absence of PKC, host defense against bacterial infection is severely compromised, resulting in an increased incidence of mortality.
Key Words: nitric oxide • protein kinase C • nitric oxide synthase • macrophage activation • bacterial infection
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Introduction |
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, PKCßI and ßII, and PKC. The novel isotypes are also diacylglycerol dependent, but are calcium independent. These include PKC
, PKC, PKC
, and PKC
(2). The atypical isotypes, comprising of PKC
and PKC
/
, are nonresponsive to diacylglycerol. In any one tissue several isoenzymes can be expressed, and redundancy of function has often hampered the identification of definitive roles for individual family members. Nevertheless, in recent years, mice deficient for PKCß (both ßI and ßII), PKC, PKC, and PKC have all been generated, and the analysis of these animals has increasingly highlighted the essential nonredundant roles for PKC isoenzymes in many systems (3–6).
Several of the reported phenotypes for PKC mutant mice have identified a role for a specific isoenzyme in the cells of the immune system. For example, mice deficient for PKC ßI and ßII have a marked immunodeficiency that is characterized by an attenuated humoral immune response specifically associated with an impairment of signaling through the B cell receptor (4). In contrast, mice deficient for PKC have a defect in T cell receptor signaling, which results in a severe decrease in nuclear factor (NF)B activation and mature T cell proliferation (6).
A number of in vitro and ex vivo studies have also implicated a role for PKC in the regulation of the immune system. In immature thymocytes, it was suggested that PKC was involved in glucocorticoid-induced apoptosis (7), while in mature T cell lines, PKC activation was implicated in signaling through the high-affinity IL-2 receptor (8). Much evidence also exists to suggest that PKC could be an important mediator of macrophage function. For example, it was demonstrated using several complementary experimental approaches that the macrophage-specific inhibition of PKC was partly responsible for the antiinflammatory action of IL-4 (9). In addition, the expression of PKC was shown to be sufficient for NO production in the RAW 264.7 macrophage cell line (10), while a number of studies have suggested that the activation of PKC is a critical event in the signaling response of primary macrophages to either LPS (11, 12), or GM-CSF (13). Furthermore, it was recently demonstrated that PKC is required for the induction of mitogen-activated protein kinase phosphatase-1 in LPS-stimulated macrophages (14), and that macrophage phagocytosis is dependent on the activation of a nPKC, specifically PKC (15).
To address directly whether PKC has a role in the function of the various cell types of the immune system, we generated and characterized mice with a targeted disruption of the PKC gene. Thymocyte apoptosis, T cell proliferation, and B cell function were all comparable to that observed in control littermates. However, even though circulating monocytes were present at wild-type levels, and maturation and homing of these cells appeared normal, elicited peritoneal macrophages generated significantly lower levels of NO, TNF, and IL-1ß in response to LPS and IFN stimulation. We demonstrate that LPS-treated macrophages from PKC-/- mice failed to induce nitric oxide synthase-2 (NOS-2) expression and showed a significant reduction in the activation of both IB kinase (IKK) and NFB. The p44 and p42 extracellular signal–regulated kinase (ERK) kinases and the p38 mitogen-activated protein (MAP) kinases were also activated to a considerably lesser extent in PKC-/- cells. In addition, we demonstrate that PKC-/- mice displayed a significant increase in sensitivity and mortality in response to either an intravenous Gram-negative or Gram-positive bacterial infection. Taken together, these data implicate PKC as a critical component of the LPS signaling cascade in activated macrophages, and highlights the importance of this gene in mounting an effective immune response to various bacterial pathogens.
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Materials and Methods |
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Generation of PKC-/- Mice
A 9.3-kb EcoRI fragment containing the first exon of the PKC gene was isolated from a murine 129/Sv genomic DNA library (gift from T. Rabbitts, Laboratory of Molecular Biology, Cambridge). A targeting vector was generated by introducing a positive selectable cassette into the PstI site of exon 1. This cassette contains stop codons in all three frames, an independent ribosomal entry site (IRES) followed by the LacZ gene with an SV40 polyadenylation sequence, and a neomycin phosphotransferase gene (MC1Neo poly(A); gift from A. Smith, Centre for Genome Research, Edinburgh, UK). Correctly targeted GK129 ES cells (see Fig. 1
for Southern blot details) were injected into C57BL/6 blastocysts. Chimeric mice were bred to C57BL/6 mice in specific pathogen-free (SPF) conditions to generate PKC homozygous mutant animals. PKC-/- and PKC+/- mice were maintained on a mixed C57Bl/6 x 129/Sv genetic background and were genotyped by Southern blot (Fig. 1, A and B) or PCR analysis of tail DNA (data not shown). Mice were fed ad libitum with a standard diet (Panlab) and kept under a light and dark cycle of 12 h (lights on at 8 a.m.).
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Flow Cytometric Analysis
Cells were stained with PE-labeled antimurine CD11b (clone M1/70) and FITC-labeled anti-CD14 (clone rmC5–3) from BD PharMingen and analyzed on a FACScanTM cytometer (Becton Dickinson) equipped with a 25-mW argon laser. Analysis of apoptotic cells was performed by propidium iodide staining, following a previous protocol (19, 20). The quantification of the percentage of apoptotic cells was done using a dot plot of the forward scatter against the phosphatidylinositol fluorescence. Cell sorting and analysis of viable and apoptotic populations was performed to confirm the criteria of gating (20).
Preparation of Blood Samples for Cytokine and PGE2 Assay
Blood was collected from the tail vein or by cardiac puncture at the indicated times and the levels of TNF, IL-1ß, and PGE2 were assayed using an enzyme immunoassay kit, following the suppliers recommendations (Biotrak; Amersham Pharmacia Biotech).
Determination of NO Synthesis
NO release was determined spectrophotometrically by the accumulation of nitrite and nitrate in the medium (phenol red-free). Nitrate was reduced to nitrite as described (16). Nitrite levels were determined with Griess reagent. Results are expressed as the amount of nitrite and nitrate released per mg of cell protein.
Preparation of Cell Extracts
Adhered macrophages were washed twice with ice-cold PBS and the plates (6-cm diameter) were filled with 0.4 ml of buffer A (20 mM Tris-HCl, pH 7.8; 5 mM MgCl2, 10 mM KCl, 0.5 mM EGTA, 1 mM phenylmethylsulfonyl fluoride, 0.5 mM dithiothreitol, and 10 µM leupeptin). The cells were scraped off the dishes using a rubber policeman and mixed with one volume of a 1% Nonidet P-40 solution. The tubes were gently vortexed for 15 s and nuclei were sedimented by centrifugation at 8,000 g for 15 s. Aliquots of the supernatant were stored at -80°C (cytosolic extracts), and the nuclear pellets were resuspended in 100 µl of buffer A supplemented with 0.4 M KCl. Nuclear proteins were extracted by centrifugation at 13,000 g for 15 min and aliquots of the supernatant were stored at -80°C (16). Proteins were measured using the Bio-Rad Laboratories detergent-compatible protein reagent. All steps of cell fractionation were performed at 4°C.
Measurement of IKK2 Activity
Cells (107) were homogenized in buffer A and centrifuged at maximal speed for 10 min in a microcentrifuge. The supernatant (1 ml) was precleared and IKK2 was immunoprecipitated with 1 µg of anti-IKK2 Ab (21). After five washes of the immunoprecipitate with buffer A, the pellet was resuspended in kinase buffer (20 mM HEPES, pH 7.4; 0.1 mM EDTA, 100 mM NaCl, 1 mM DTT, 0.5 mM PMSF, 2 µg/ml aprotinin, 10 µg/ml leupeptin, 2 µg/ml TLCK, 5 mM NaF, 1 mM NaVO4, 10 mM Na2MoO4 and 10 nM okadaic acid). Kinase activity was assayed in 100 µl of buffer A containing 100 ng of immunoprecipitation, 50 µM [-32P]ATP (0.5 µCi), and using as substrate 100 ng of GST-IB (amino acids 1–54). Controls with the corresponding S32A and S36A mutated protein were unable to be phosphorylated under these conditions (data not shown). Aliquots of the reaction were stopped at various time points with 1 ml of ice-cold buffer A supplemented with 5 mM EDTA. The linearity of the kinase reaction was confirmed over a period of 30 min.
Electrophoretic Mobility Shift Assays
An oligonucleotide corresponding to the proximal B motif of the murine NOS-2 promoter (22, 23) 5'-CCAACTGGGGACTCTCCCTTTGGGAACA-3', and one corresponding to the PPAR binding site of the promoter of acyl-CoA oxidase (24) 5'-CGAACGTGACCTTTGTCCTCCCCTTTTGCTCGATC-3', were annealed with complementary sequence (50 ng) and labeled with Klenow enzyme in the presence of 50 µCi of [-32P]dCTP plus unlabeled dNTPs to a final volume of 50 µl. The probes were precipitated with ethanol and extracted with phenol/chloroform. DNA binding assays of nuclear extracts were performed by incubating for 30 min at 4°C, 5 x 104 dpm of the DNA probe with 5 µg of nuclear protein, 1 µg/ml of poly(dI·dC), 5% glycerol, 1 mM EDTA, 100 mM KCl, 5 mM MgCl2, 1 mM dithiothreitol, and 10 mM Tris-HCl, pH 7.8, in a final volume of 20 µl. The incubation mixture was applied to a 6% polyacrylamide gel that had been electrophoresed previously for 30 min at 100 V. Gels were electrophoresed at 0.8 volts/cm2 in 45 mM Tris-borate, followed by vacuum-transference to 3MM Whatman paper and quantification of the band intensities in an autoradiograph (Fuji Bas 1000). Analysis of competition with unlabeled oligonucleotides was performed using a 20-fold excess of double stranded DNA in the binding reaction, and adding the nuclear extracts as the last step in the binding assay. Supershift assays were performed after addition of antibodies (0.5 µg) to the binding reaction and incubation for 1 h at 4°C (22).
Western Blot Analysis
Cytosolic and nuclear extracts were obtained as described previously (22). Samples containing equal amounts of protein (30 µg and 10 µg per lane of cytosolic and nuclear extracts, respectively) were boiled in 250 mM Tris-HCl, pH 6.8, 2% SDS, 10% glycerol, 2% ß-mercaptoethanol, and size-separated in 10% SDS-PAGE. The gels were processed as recommended by the supplier of the antibodies against various murine antigens (NOS-2, IB, phospho(S32)IB, p38 and p42/p44 MAP kinases, p50, and p65; from Santa Cruz Laboratories or New England Biolabs, Inc.) and after blotting onto a polyvinylidine difluoride (PVDF) membrane, proteins were revealed following the enhanced chemoluminescence (ECL) technique (Amersham Pharmacia Biotech). Different exposure times of the films were used to ensure that bands were not saturated. Quantification of the films was performed by laser densitometry (Molecular Dynamics). Westerns for PKC were as described previously (see reference 10).
RNA Extraction and Analysis
Total RNA (2–4 x 106 cells) was extracted following the guanidinium thiocyanate method (Trizol; GIBCO BRL). For Northern blot analysis equal amounts of RNA were denatured and size-separated by electrophoresis in a 0.9% agarose gel containing 2% formaldehyde and MOPS buffering system as described previously (22). The RNA was transferred to Nytran membranes (NY 13-N; Schleicher & Schuell) with 10x SSC (1.5 mM NaCl, 0.3 mM sodium citrate, pH 7.4). An 817-bp fragment (nucleotides 1 to 817) from the cDNA of murine NOS-2 was labeled as a probe with the Rediprime kit (Amersham Pharmacia Biotech). The intensity of the bands was quantified in a Fuji BAS1000 autoradiograph using hybridization with a ribosomal 18S probe as an internal control. For reverse transcription (RT)-PCR, cDNA was generated from 10 µg of total RNA using the SMART cDNA synthesis technique (CLONTECH Laboratories, Inc.). A standard 30 cycle PCR was then performed on one hundredth of the starting sample using the following primers; PKC(F) 5'-GCCAAAGTGCTGGCTGACCTTGG-3', PKC(R) 5'-CGGCATAGAACCGAGAACGAGGC-3', ß-act(F) 5'-TGCCTGACGGCCAGGTCATCA-3', ß-act(R) 5'-CGGACTCGTCATACTCCTGC-3'. An annealing temperature of 62°C was used for both PCRs (Advantage 2; CLONTECH Laboratories, Inc.).
Statistical Analysis
The data shown are the means ± SEM of the number of experiments or animals indicated. The product limit of the cumulative survival (Kaplan-Meier) was calculated with the Log-rank test for all survival data using the SPSS 10.0 software. Statistical significance was estimated with analysis of variance (ANOVA) and Student's t test for unpaired observations, using commercially available software (SPSS). A P value of less than 0.05 was considered significant.
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, in various aspects of the maturation and function of the immune system. To address these issues directly, mice deficient for PKC were generated by inserting a LacZ/Neo sequence into the first exon of the PKC gene (Fig. 1 A). ES cells (data not shown) and mice heterozygous or homozygous for the PKC mutation were assessed by Southern blot analysis for a correct targeting event (Fig. 1, A and B). RT-PCR (Fig. 1 C), Northern blot analysis (data not shown), and Western blot analysis confirmed that PKC mRNA and protein were absent at this level of detection, whereas protein levels for other PKC isoenzymes remained unaltered (Fig. 1 D).
After heterozygous mating, PKC-/- mice were born at the expected Mendelian frequency, with life expectancy no different to wild-type littermates. PKC-deficient animals were, however, 10–15% smaller than controls, and did not lay down a large amount of adipose tissue with increasing age.
Various aspects of the immune system were investigated in PKC-/- mice. Thymocytes and T cells developed normally, had an unchanged surface phenotype, and were present at expected numbers. Thymocyte apoptosis to a range of stimuli, including dexamethasone, was comparable to wild type. T cell proliferation to anti-CD3 antibody or anti-TCRß antibody was marginally reduced to 
80% of controls, although the T cell response to antigen after a prior immunization was comparable to wild-type littermates (data not shown). B cells were present at expected numbers with a normal surface phenotype, and serum Ig levels were similar to controls. Basic blood histology and biochemistry revealed no differences between PKC-/- mice and wild-type littermates (data not shown).
A problem was observed when breeding with homozygous PKC-/- animals. On average, only one in four female PKC-/- mice produced a litter, with a second litter from these animals being very rare. On closer examination there was no evidence of a pregnancy of any length in non-litter bearing mothers after a plugging event. On autopsy, 30% of non-litter bearing female mice presented with distended fluid-filled uteri. Furthermore, even though autoclaved bedding, water, and food were used, a granulocyte/macrophage infiltrate and the presence of copious Gram-negative bacteria such as E. coli and various strains of Proteus were detected in the uterine fluid. No obvious deformity in uterus structure was observed in healthy PKC-/- animals (data not shown).
Macrophages from PKC-/- Mice Generate Reduced NO and Express Lower Levels of NOS-2 mRNA and Protein in Response to In Vitro Challenge with LPS
As PKC-/- mice were succumbing to E. coli–related bacterial infection, it was hypothesized that their response to Gram-negative bacteria was somehow compromised. To test this, macrophages were elicited via intraperitoneal thioglycollate injection and their response to in vitro administration of LPS was assessed measuring nitrite generation as a functional end point. The number of macrophages obtained from PKC-/- mice were comparable to littermate controls, and the percentage of cells expressing cell-surface levels of both CD14, an integral component of the LPS receptor, and CD11b was similar (Fig. 2
A). At lower doses of LPS, below 200 ng/ml, macrophages from PKC-/- mice generated significantly lower amounts of NO than macrophages from control animals (Fig. 2 B). However, at substantially higher concentrations of LPS, above 500 ng/ml, a comparable production of NO was detected from both groups. Macrophages can be activated to a greater degree if IFN is allowed to act synergistically with LPS. Using a set concentration of both LPS and IFN, the generation of NO over a 36-h period was also demonstrated to be significantly reduced in macrophages from PKC-/- mice when compared with macrophages from wild-type controls (Fig. 2 C). It should be noted that IFN treatment alone can result in the generation of NO from macrophages, although this response is lower and delayed with respect to the response observed with LPS (16). In PKC-/- animals the generation of NO after in vitro IFN treatment of elicited macrophages was also reduced in comparison to wild-type littermates (data not shown). The basis of this reduced response to IFN in the PKC-/- mice is presently unclear. However, studies are underway to assess the extent of this defect and to characterize the cellular components involved.
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. Fig. 3
A demonstrates that cultured macrophages from PKC-/- mice displayed a severely reduced level of NOS-2 protein expression after both 18 and 24 h of stimulation when compared with wild-type cells. To verify this decrease in LPS-induced NOS-2 expression, LPS was administered in vivo via an intraperitoneal injection. After 24 h, macrophages were isolated from the peritoneal cavity and again assayed for NOS-2 protein expression. As shown in Fig. 3 B, the extent of induction of NOS-2 protein in response to LPS is severely attenuated in macrophages from PKC-deficient animals. As NOS-2 activity is mainly controlled at the level of transcription (23), the in vitro expression of NOS-2 RNA in response to LPS plus IFN challenge was determined. Fig. 3 C demonstrates that after such a challenge NOS-2 RNA levels were significantly decreased in macrophages from PKC-/- mice when compared with controls. These data suggest that the reduction in LPS-induced NO generation in macrophages from PKC-/- mice is a result of the failure to upregulate the expression of both NOS-2 RNA and protein.
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-/- Mice Release Reduced Levels of Proinflammatory Mediators in Response to LPS, and Fail to Undergo Activation-induced Apoptosis, IL-1ß, and prostaglandin E2 (PGE2) were therefore analyzed after in vitro LPS and IFN stimulation of thioglycollate-elicited macrophages. Fig. 4, A–C , clearly demonstrates that macrophages from PKC-/- mice generated severely attenuated levels of TNF, IL-1ß, and PGE2 compared with macrophages from wild-type animals. The release of these proinflammatory mediators was also assessed in vivo after the intraperitoneal administration of LPS after sensitization with D-galactosamine (17). Serum levels of TNF and IL-1ß were both significantly reduced in PKC-/- mice when compared with the levels observed in littermate controls (Fig. 4, D and E).
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, or LPS, IFN, and 15dPGJ2, apoptotic conditions that have been characterized previously (20). As shown in Fig. 4 F, <15% of elicited macrophages from PKC-/- mice undergo apoptosis in response to any of the three treatments. In contrast, wild-type macrophages show a level of apoptosis of over 20% for each stimulation, with over 50% of the cells undergoing apoptosis in response to the combined action of LPS, IFN, and 15dPGJ2. Taken together these results indicate that many mediators of macrophage function in response to LPS are severely disrupted in mice deficient for PKC.
LPS-activated Macrophages from PKC-/- Mice Show Significant Impairment of NFB Activation, and IB Kinase Activity
Much evidence exists to suggest that the upregulation of NOS-2 requires the transcription factor NFB (23, 25). Macrophages are known to express NFB constitutively, but in resting cells NFB forms an inactive cytoplasmic complex with IB. On activation, IB is phosphorylated and degraded, leading to the release of NFB, which translocates to the nucleus as an active transcription factor. To assess whether the reduction of NOS-2 expression in PKC-/- mice was due to a decrease in NFB activation, the presence of active NFB in macrophage nuclear extracts was analyzed by electrophoretic mobility shift assay (EMSA) after increasing length of LPS stimulation of thioglycollate-elicited cells. The distal B sequences from the NOS-2 promoter were used to bind the nuclear extracts. In comparison to the clear binding of NFB (p50.p65) in wild-type lysates, NFB levels in nuclear extracts from PKC-/- mice were greatly reduced at all time points analyzed (Fig. 5
A). Supershift assays were performed to verify the nature of the observed bands (data not shown). These results suggest that the failure to activate NFB in PKC-/- macrophages could be responsible for the low levels of NOS-2 expression observed in response to LPS stimulation.
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B results from the phosphorylation and subsequent degradation of IB. Macrophages from PKC-/- mice demonstrate an impaired degradation of IB in response to LPS (Fig. 5 B). Consistent with this observation, a reduction in the phosphorylation of IB was detected with a specific anti-P(S32)IB Ab in PKC-deficient macrophages treated with MG 132 to inhibit proteasome function (21) and hence IB degradation (Fig. 5 B). Phosphorylation of IB is mediated in part by IB kinase-2 (IKK-2). Therefore, the activity of IKK-2 in LPS-activated thioglycollate-elicited macrophages was assessed after immunoprecipitation of IKK-2 from cytosolic extracts, using a kinase assay with GST-IB and [-32P]ATP as substrates. Phosphorylation of the GST-IB substrate by IKK-2 was significantly decreased in macrophages from PKC-/- mice when compared with that of controls (Fig. 5 C). Thus, a failure to activate IKK-2 in LPS-stimulated macrophages could be responsible for the impaired degradation of IB and the reduction in active NFB observed in nuclear extracts from PKC-/- mice.
LPS-activated Macrophages from PKC-/- Mice Display Defects in a Number of Cellular Signaling Pathways
Previous work has implicated several signaling pathways in the upregulation of expression of genes such as NOS-2, TNF, and IL-1ß after the LPS stimulation of macrophages. Two such pathways are those involving the ERK1/2 MAP kinases and the family of p38 MAP kinases. The activation of these kinases was therefore assessed by detection of the phosphorylated forms of p44ERK, p42ERK, and p38 in LPS-stimulated macrophage cytosolic extracts. The amount of phosphorylated p44, p42, and p38 is clearly reduced in extracts from LPS-stimulated macrophages from PKC-/- mice, particularly at early time points after stimulation (Fig. 6, A and B)
. The relevance of this reduction in LPS-induced p44/p42ERK and p38 activation with respect to NO synthesis was evaluated. Whereas PD 98059, an inhibitor of ERK, was unable to modify NO synthesis in response to LPS in macrophages from wild-type animals, SB 203580 and SB 202190, two inhibitors of p38 MAPK, significantly inhibited NO synthesis in activated macrophages from PKC+/+ mice (Fig. 6 C), confirming previous data (26). However, neither SB 203580 nor SB 202190 affected the already lowered synthesis of NO in PKC-/- mice (Fig. 6 C). These results suggest that although both the ERK and p38 MAP kinase signaling cascades are attenuated in PKC-/- mice in response to LPS, only the p38 MAP kinase pathway is directly involved in NO production in a PKC-dependent manner.
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-/- Mice Are Less Resistant to Gram-negative and Gram-positive Bacterial Challenge-/- mice displayed an unexpected incidence of uterine Gram-negative bacterial infection, and macrophages from PKC-/- mice were demonstrated to have a severely attenuated response to LPS stimulation, it was hypothesized that PKC-deficient animals would be more sensitive to Gram-negative bacteria than wild-type controls. To assess this possibility directly, a controlled E. coli bacterial infection was administered intravenously to both PKC-/- and wild-type mice. At a bacterial dose of 3 x 105 pathogens per gram, 40% of the control animals survived for at least 20 d after infection. In contrast, all PKC-/- mice had died by day 8 (median; 4.6 and 25.3 d for PKC-/- and wild-type, respectively; Fig. 7
A). At the higher bacterial dose of 3 x 106 pathogens per gram, all animals from the wild-type group had died by day 3. However again, the PKC-/- mice showed a decreased resistance to infection, as no animal survived beyond the first day (Fig. 7 B). Interestingly, when animals were injected with 3 x 105 Gram-positive S. aureus per gram of body weight, a difference in survival was also observed between PKC-/- and wild-type animals (median; 6.8 and 21 d, respectively; Fig. 7 C). These results clearly demonstrate that mice deficient for PKC are more sensitive to both Gram-negative and Gram-positive bacterial infection than wild-type controls, and that this increased sensitivity to infection can significantly decrease the likelihood of bacterial clearance and survival.
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plays a major role in macrophage biology. Although the absence of PKC did not seem to influence the differentiation of monocytes and macrophages from bone marrow precursors, or affect extravasation of macrophages in response to proinflammatory stimuli, a major defect in the ability of extravased macrophages to respond to LPS was observed. At low concentrations of LPS (ca. 200 ng/ml) the generation of NO from PKC-/- macrophages was severely reduced. The generation of NO, TNF, and IL-1ß was also decreased after the synergistic activation of PKC-/- macrophages with LPS and IFN (23, 27). Furthermore, several LPS-activated signaling pathways, involving IKK-2, IB, NFB, the ERK MAP kinases, and p38 MAP kinase were attenuated in PKC-deficient cells. Taken together, these results suggest that PKC has a critical function in the regulation of a number of signaling pathways that mediate various aspects of macrophage activation.
Macrophages constitute a key component of the innate immune system, having the ability to recognize relatively invariant pathogen-associated molecular patterns from a range of bacteria and fungi (28–31). As a defensive response to these microbial structures, macrophages can release a diverse array of bioactive molecules at sites of infection. These effector molecules include reactive oxygen and nitrogen species, prostaglandins, and matrix metalloproteinases (32–36). Macrophages can also contribute to the initiation of the adaptive immune response by presenting antigen to T cells and by expressing costimulatory molecules, such as B7, and a range of cytokines, such as IL-1ß, IL-6, IL-10, and TNF, that instruct the adaptive immune system about the general nature of the invading pathogen (28, 35).
LPS is a component of the outer membrane of Gram-negative bacteria that is recognized as a pathogen-associated molecular pattern by macrophages (35). The major LPS receptor complex has been demonstrated to consist of a serum protein known as LPS-binding protein, a GPI-linked surface protein known as CD14, and the toll-like receptor-4 (TLR-4) transmembrane protein in association with the product of the MD-2 gene (28, 37–40). The percentage of macrophages expressing CD14 (and mouse embryonic fibroblasts, data not shown) from PKC-/- mice is comparable to that observed in wild-type controls. Furthermore, the apparent affinity for LPS and anti-CD14 mAbs was also unaltered on macrophages from PKC-deficient animals (data not shown). This would imply that PKC has a role downstream of the CD14/TLR-4 complex. However, the defect in LPS-induced macrophage activation in PKC-/- mice is not as severe as that observed in TLR-4-/- animals, as some NO generation is observed at low concentrations of LPS and NO production is comparable to wild-type levels at much higher concentrations of LPS. This would suggest that PKC is not absolutely essential for LPS-mediated signaling, but instead could have a modulatory role, amplifying the signaling cascade when levels of LPS are limiting.
The full complement of downstream signaling events that are initiated by LPS receptor binding are still not fully understood. However, evidence exists to suggest the involvement of Src-kinases (41), G proteins (42), phospholipase C (43–45), and protein kinase A (46). Several studies have also implicated MAP kinase activation as a critical event in LPS-mediated signaling (47–51). We have demonstrated that the extent of both p38 MAP kinase activation and ERK-1/ERK-2 MAP kinase activation is significantly decreased after LPS-stimulation of PKC-/- macrophages. Furthermore, our results suggest that the PKC-dependent activation of the p38 MAP kinase pathway partially induces NO production (26). This would suggest that the role of PKC is upstream of phosphorylation events that activate these kinases, and implicates PKC in the activation of a number of diverse signaling cascades. In this regard, the PKC-mediated activation of the MAP kinase pathway, leading to the nuclear translocation of NFB, has recently been demonstrated in adult rabbit cardiomyocytes (52).
The synthesis of NO has been extensively studied in macrophages. It is known that NO generation is dependent on the cellular levels of NOS-2, and that the upregulation of NOS-2 expression is in turn dependent on NFB binding at B sites located in the NOS-2 promoter (25, 53). In resting cells, NFB forms an inactive complex with the inhibitor IB in the cytosol. On activation, the phosphorylation and degradation of IB by an IB kinase (IKK) results in the nuclear translocation of NFB and the activation of target genes (54–57). In RAW 264.7 cells, PKC expression was demonstrated to be sufficient for NFB activation and NOS-2 induction (16). Consistent with these observations, our data demonstrate that LPS-induced NFB translocation and induction of NOS-2 expression are both severely disrupted in macrophages from PKC-/- mice. Furthermore, IB phosphorylation and degradation is reduced, and IKK-2 activity is significantly decreased in the absence of PKC.
At present, the signaling events upstream of IKK are not fully understood, although the involvement of several kinases has been implicated, including NFB-activating kinase (NAK) (58) and TGFß-activated kinase (TAK-1) possibly via the activation of NFB-inducing kinase (NIK) (59). Interestingly, the expression of a catalytically inactive NAK protein was shown to specifically inhibit activation of NFB by PKC, but not by PKC or PKC (58). In addition, this NAK mutant blocked NFB activation by PDGF, which has been reported to signal through PKC (60). However, the authors also reported that although a dominant negative IKK-2 mutant blocked activation of NFB by LPS, the catalytically inactive NAK had little effect. This would suggest that the activation of IKK-2 is probably mediated by a number of signaling pathways that may not all be influenced by PKC.
TAK-1 has recently been implicated in a complex signaling cascade from the LPS receptor TLR-4 which involves MyD88, IRAK, TRAF-6, ECSIT, and TAB2 (61–66). It is presently unclear exactly how PKC could interact with this pathway. However, it is worth noting that the TLR-2 receptor-induced signaling cascade has been shown to share many of these intermediary molecules (67). As the TLR-2 complex is known to mediate potent macrophage responses to pathogens such as Gram-positive bacteria and mycoplasma (68–70), and as PKC-/- mice displayed an increased sensitivity to Gram-positive bacterial challenge, it is tempting to speculate that PKC could function at a point common to both the TLR-4 and TLR-2 cascades. Further work is underway to establish the basis of the increased sensitivity to Gram-positive bacteria observed in this study.
The synthesis of LPS-induced proinflammatory mediators such as NO, TNF, and IL-1ß are required for the full activation of macrophage function and the correct initiation of an appropriate immune response to a Gram-negative bacterial infection (28, 35, 71–73). Our results clearly demonstrate that in mice lacking PKC the generation of LPS-induced proinflammatory mediators is notably diminished. This would predict that PKC-/- mice would be sensitive to infection by Gram-negative bacteria such as E. coli. Consistent with this hypothesis, we observed a frequent incidence of E. coli infection in the uteri of PKC-/- animals, a type of infection that was never observed in control animals over a similar period. Furthermore, in a controlled intravenous infection of animals with E. coli, survival times were markedly reduced in the absence of PKC. However, we also observed a decreased macrophage response to IFN challenge, and an increased sensitivity to Gram-positive bacteria in PKC-deficient animals. Taken together, these data conclude that PKC is a critical mediator of several signaling cascades in activated macrophages, and that in the absence of PKC, the successful initiation of an effective immune response against a range of bacterial pathogen is severely compromised.
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Acknowledgments |
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This work was supported by the Imperial Cancer Research Fund, and grants FEDER 2FD-1997-1432 from Comisión Interministerial de Ciencia y Tecnología (CICYT) and PM98-0120 from Dirección General de Enseñanza Superior e Investigación Científica, Spain. F. Otto was supported by Deutsche Forschungsgemeinschaft grant Ot 134/1-1.
Submitted: February 26, 2001
Revised: September 4, 2001
Accepted: September 21, 2001
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Footnotes |
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* Abbreviations used in this paper: ERK, extracellular signal–regulated kinase; IKK, I
B kinase; MAP, mitogen-activated protein; NAK, NFB-activating kinase; NF, nuclear factor; NOS, nitric oxide synthase; PKC, protein kinase C; TLR, Toll-like receptor. 
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References |
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1
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