B-Cell Receptor- and Phorbol Ester-Induced NF-{kappa}B and c-Jun N-Terminal Kinase Activation in B Cells Requires Novel Protein Kinase C's

doi:10.1128/MCB.21.19.6640-6650.2001

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Molecular and Cellular Biology, October 2001, p. 6640-6650, Vol. 21, No. 19
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.19.6640-6650.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

B-Cell Receptor- and Phorbol Ester-Induced NF- $kappa$ B and c-Jun N-Terminal Kinase Activation in B Cells Requires Novel Protein Kinase C's

Daniel Krappmann,^* Alina Patke, Vigo Heissmeyer, and Claus Scheidereit

Max-Delbrück-Centrum for Molecular Medicine, 13125 Berlin, Germany

Received 23 March 2001/Returned for modification 30 May 2001/Accepted 2 July 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Antigen receptor signaling is known to activate NF- $kappa$ B in lymphocytes. While T-cell-receptor-induced NF- $kappa$ B activation criticallydepends on novel protein kinase C $theta$ (PKC $theta$ ), the role of novelPKCs in B-cell stimulation has not been elucidated. In primarymurine splenic B cells, we found high expression of the novelPKCs $delta$ and $varepsilon$ but only weak expression of the $theta$ isoform. Rottlerinblocks phorbol ester (phorbol myristate acetate [PMA])- or B-cellreceptor (BCR)-mediated NF- $kappa$ B and c-Jun N-terminal kinase (JNK)activation in primary B and T cells to a similar extent, suggestingthat novel PKCs are positive regulators of signaling in hematopoieticcells. Mouse 70Z/3 pre-B cells have been widely used as a modelfor NF- $kappa$ B activation in B cells. Similar to the situation in splenicB cells, rottlerin inhibits BCR and PMA stimulation of NF- $kappa$ B in70Z/3 cells. A derivative of 70Z/3 cells, 1.3E2 cells, are defectivein NF- $kappa$ B activation due to the lack of the I $kappa$ B kinase (IKK $gamma$ ) protein.Ectopic expression of IKK $gamma$ can rescue NF- $kappa$ B activation in responseto lipopolysaccharides (LPS) and interleukin-1 $beta$ (IL-1 $beta$ ), but notto PMA. In addition, PMA-induced activation of the mitogen-activatedprotein kinase JNK is blocked in 1.3E2 cells, suggesting thatan upstream component common to both pathways is either missingor mutated. Analysis of various PKC isoforms revealed that exclusivelyPKC $theta$ was absent in 1.3E2 cells while it was expressed in 70Z/3cells. Stable expression of either novel PKC $theta$ or - $delta$ but not classicalPKC $beta$ II in 1.3E2 IKK $gamma$ -expressing cells rescues PMA activation ofNF- $kappa$ B and JNK signaling, demonstrating a critical role of novelPKCs for B-cellactivation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Transcription factor NF- $kappa$ B is critically involved in many cellular processes such as inflammation, immune response, proliferation,and apoptosis. In most cells, NF- $kappa$ B resides in the cytoplasm andactivation is triggered in response to multiple stimuli, e.g.,proinflammatory cytokines (tumor necrosis factor alpha [TNF- $alpha$ ]or interleukin-1 $beta$ [IL-1 $beta$ ]), bacterial lipopolysaccharides (LPS),mitogenic signals (i.e., phorbol myristate acetate [PMA]), orantigen receptor signaling. The signal transduction pathways whichare initiated by all these signals converge at the I $kappa$ B kinase(IKK) complex, which upon activation phosphorylates NF- $kappa$ B-inhibitorymolecules (I $kappa$ Bs). Phosphorylated I $kappa$ Bs are prone to rapid ubiquitinationand proteasomal degradation, liberating NF- $kappa$ B, which subsequentlytranslocates to the nucleus and activates gene transcription (23).In addition, most NF- $kappa$ B-inducing agents also stimulate mitogen-activatedprotein kinase (MAPK) signaling cascades, leading to the activationof the transcription factor AP-1 (8). NF- $kappa$ B and AP-1 cooperateat the level of transcription, and the induction of certain promoters(e.g., IL-2 promoter) depends on the activation of both transcriptionfactors (1, 22).

Intensive work has focused on the signaling cascades upstream of the IKK complex. Especially the events leading to NF- $kappa$ B activationin response to pro-inflammatory cytokines and LPS have been analyzedin great detail. Ligand binding induces the association of effectormolecules (e.g., TRAFs, RIP) into the respective receptor complexes.Nevertheless, the exact mechanism by which activation of the IKKcomplex is accomplished remains to be determined, but there isgood evidence that MAPK kinase kinases play a role (16, 23).

More recently it was shown that signaling events downstream of the T-cell receptor (TCR), TCR/CD3, are distinct from cytokine-mediatedsignaling in that they require Vav and the novel protein kinaseC $theta$ (PKC $theta$ ) for the activation of the IKK complex (9, 11,29). In mature T cells from PKC $theta$ -deficient mice, NF- $kappa$ B activationwas blocked in response to T-cell stimulation, proving the essentialand selective role of PKC $theta$ (40). TCR/CD28 costimulation canbe mimicked by PMA plus Ca²⁺ ionophore (39). Yet, it is not clear how PKC $theta$ activates theIKK complex in response to TCR/CD28 or PMA stimulation. EndogenousPKC $theta$ associates with the activated IKK complex, and TCR/CD28 signalinginduces recruitment of PKC $theta$ and IKK into membrane lipid rafts(24). Furthermore, Bcl10 is required for NF- $kappa$ B activation inresponse to TCR signaling and PMA treatment, but not LPS, IL-1,or TNF- $alpha$ , and Bcl10 probably acts either at the level of or downstreamof PKC $theta$ (38). However, due to the absence of well-defined substratesfor PKCs, the exact mechanism by which PKC $theta$ triggers NF- $kappa$ B activationremains to be identified. Recently, the IKK-related NF- $kappa$ B-activatingkinase has been proposed to act as a direct target of PKCs andto function as an intermediate for IKK activation in responseto PMA (41). It was also reported that different PKC isoenzymescan activate IKK $beta$ directly (27). Still, the relevance of bothfindings for T-cell activation is notclear.

Using Jurkat T cells, several studies have demonstrated that PKC $theta$ , but not other PKC isoforms, also mediate c-Jun N-terminalkinase (JNK) activation in a T-cell specific manner (2, 14,39, 43). However, peripheral T cells from PKC $theta$ -deficient micedisplay no defect in TCR/CD28-induced activation of JNK, eventhough AP-1 activation was reduced, questioning the physiologicalrelevance of MAPK signaling for T-cell activation (1, 40).

In primary B cells, immunoglobulin M (IgM) cross-linking of the B-cell receptor (BCR) as well as CD40 ligation have been shownto activate NF- $kappa$ B (12, 13, 30, 35). CD40 receptor is amember of the TNF receptor superfamily, and signal transductionthrough the receptor involves association of TRAFs and subsequentIKK activation (19-21). Considerably less is known about BCR-triggeredNF- $kappa$ B activation. Recently, it was demonstrated that Bruton'styrosine kinase activates phospholipase C- $gamma$ 2, which couples theBCR to the IKK complex and subsequently activates NF- $kappa$ B (3,33, 34). Furthermore, antigen receptor-induced NF- $kappa$ B activationin B cells and T cells is abrogated in Bcl10-deficient mice, suggestingthat Bcl10 is a common constituent of both pathways (38). Still,nothing is known about other signaling intermediates, especiallyabout the role of PKCs for BCR-induced NF- $kappa$ Bactivation.

In this study we provide evidence that novel PKCs are necessary for BCR- and PMA-induced NF- $kappa$ B and JNK activation in B cells.Pharmacological inhibitors indicate that novel PKCs transmit PMAand BCR signaling in primary splenic B cells as well as in 70Z/3pre-B cells. 1.3E2 cells, a derivative of 70Z/3 pre-B cells, carrya defect in PMA signaling that is independent of a functionalIKK complex. Novel PKC $theta$ was found to be weakly expressed in 70Z/3cells but was absent in 1.2E3 cells. Stable expression of eithernovel PKC $theta$ or - $delta$ but not classical PKC $beta$ II could rescue PMA-mediatedNF- $kappa$ B and JNK activation in 1.3E2 cells, suggesting that novelPKCs are critically involved in B-cellactivation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and treatment. 70Z/3 and 1.3E2 cells were grown in RPMI medium supplemented with 7.5% fetal calf serum, 2 mM L-glutamine, 100 U of penicillinand streptomycin per ml, and $beta$ -mercaptoethanol. Jurkat T cellswere grown in RPMI supplemented with 10% fetal calf serum, 2 mML-glutamine, and 100 U of penicillin and streptomycin per ml.The stable 1.3E2 IKK $gamma$ clone was cultured using 1 µg of G418/ml,and stable 1.3E2 IKK $gamma$ /PKC $theta$ clones were grown using 1 µg of G418/mland 1 µg of hygromycin/ml. Cells were treated with the followingagents and concentrations: 200 ng of PMA (Calbiochem) per ml,10 µg of LPS (Sigma) per ml or 10 ng of IL-1 $beta$ (Promega) per ml,20 ng of TNF- $alpha$ (Biomol) per ml, 12 µg of anti-mouse IgM F(ab')₂fragment (Jackson Laboratories) per ml, and 10 ng of gamma interferon(IFN $gamma$ ; Endogene) per ml. PKC inhibitors Gö6976 and rottlerinwere purchased from Calbiochem. For UV irradiation, cells wereexposed to 150 J/m² at 254 nm (UV-C) in a Stratagene UV cross-linker.

Stable and transient transfection. 1.3E2 cells were transfected by electroporation. Generation of 1.3E2 IKK $gamma$ -expressing clones was described previously (17).For stable transfections of PKC isoenzymes, cells were electroporatedusing 28 µg of either PEF-PKC $theta$ , PEF-PKC $delta$ , or MTH-PKC $beta$ II togetherwith 2 µg of pTK-hygromycin (Clontech) in a Bio-Rad gene pulserat 950 µF and 220 V. After 2 days, selection was started using2.5 µg of hygromycin/ml. For transient transfections, cells wereelectroporated using 1 µg of pTK-luciferase (Clontech), 2 µg of6xNF- $kappa$ B-luciferase (6), and 27 µg of pcDNA3. Thirty-six hoursposttransfection, the cells were stimulated for 6 h as indicatedand luciferase activity was determined using a dual luciferaseassay kit(Promega).

Antibodies. The following antibodies were used: I $kappa$ B $alpha$ (C-21), I $kappa$ B $beta$ (N-20), IKK $alpha$ (H744), IKK $gamma$ (FL419), PKC $beta$ I (C-16), PKC $beta$ II (C-18), PKC $delta$ (C-17), and PKC $varepsilon$ (C-15) were obtained from Santa Cruz; monoclonalPKC $alpha$ , PKC $gamma$ , and PKC $theta$ antibodies were purchased from TransductionLaboratories. Further antibodies used were monoclonal JNK1 (Pharmingen),phospho-SAPK/JNK (Cell Signaling), ERK1/2 (Calbiochem), and phospho-ERK1/2(Biomol).

Extracts, EMSA, Western blotting, and kinase assay. Whole cell extracts were prepared and analyzed by electrophoretic mobility shift assay (EMSA) and Western blotting essentiallyas described previously (26). Preparation of nuclear and cytoplasmicextracts was performed using low-salt lysis with 0.1% NP-40 andsubsequent high-salt lysis essentially as described previously(25).

For the IKK and JNK1 kinase assays, lysis of cells, immunoprecipitation using specific antibodies (see above), and kinasereactions were performed as described previously (18). For IKKactivity, GSTI $kappa$ B $alpha$ 1-53 was used as substrate, and for JNK1 activityGSTJun1-79 was used as substrate. PKC kinase assays were performedwith purified rat brain PKC (Promega) and 1 µg of myelin basicprotein as a substrate in 30 mM Tris-HCl (pH 7.5), 100 mM KCl,6 mM MgCl₂, 0.5 mM CaCl₂, 10 µg of phospatidylserine/ml, 1 µgof diolein/ml, 10 µM ATP, and 5 µCi of [ $gamma$ -³²P]ATP for 15 min at 30°C.

Purification of splenic B and T cells and flow cytometry. Either BALB/c wild-type or BALB/c nude mice were used for the preparation of splenic B and T cells. Spleens were homogenizedusing a 70-µm cell strainer (Falcon), and erythrocytes were removedby ACK lysis buffer (150 mM NH₄Cl [pH 7.3], 1 mM KHCO₃, 0.1 mMEDTA). Magnetic-activated cell sorting (MACS) was performed accordingto the manufacturer's protocol using B220 or Thy1.2 microbeadsand VS+ columns (Miltenyi Biotech.). In order to get maximal purificationof B220-positive B cells, splenocytes from BALB/c wild-type micewere first sorted for Thy1.2-positive cells and then the Thy1.2-negativecells were subsequently sorted using B220 microbeads. B220-positivecells from BALB/c nude mice were obtained in a single round ofpurification. Purification efficiency was determined by fluorescence-activatedcell sorter flow cytometry using fluorescein isothiocyanate (FITC)-labeledThy1.2 (Caltag Laboratories) and phycoerythrin-labeled B220 (SouthernBiotech) antibodies. IgM surface expression was analyzed withFITC-labeled anti-mouse IgM antibody (R6-60.2; Pharmingen). Analysisand quantification were done usingWinMDI.

Indirect immunofluorescence. 70Z/3 and 1.3E2 cells were grown on chamber slides in the absence of serum. After 16 h the cells completely attached to thesurface of the chamber slide. Cells were fixed for 15 min in 4%paraformaldehyde and permeabilized for 5 min with 0.1% TritonX-100. For the detection of monoclonal PKC $theta$ antibody, a donkeyanti-mouse tetramethyl rhodamine isocyanate-conjugated antibodyfor the detection of the polyclonal IKK $gamma$ antibody and a donkeyanti-rabbit FITC-conjugated antibody (both Jackson Laboratories)were used. Chamber slides were analyzed and photographed by indirectimmunofluorescence microscopy using an Axioplan 2 microscope(Zeiss).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Novel PKCs are involved in PMA- and BCR-induced NF- $kappa$ B and JNK activation in splenic B cells. In lymphocytes, stimulation with PMA, a pleiotropic PKC activator, induces activation of NF- $kappa$ B and MAPK signaling pathways.To assess the expression and the function of novel PKCs in primarylymphocytes, splenic B and T cells were obtained from wild-typeand nude mice (Fig. 1). Splenic B and T cells were purified byMACS using Thy1.2 (CD90) and B220 (CD45R) microbeads. The purificationled to almost homogenous B-cell and T-cell populations with minimalcross-contamination (Fig. 1A). Expression of PKC isoforms wasanalyzed by Western blotting (Fig. 1B). In agreement with previouslypublished results (32), we found high expression of PKC $delta$ andPKC $varepsilon$ in primary B220-positive B cells compared to Thy1.2-positiveT cells. In contrast, there was only a weak signal for PKC $theta$ inthe B220-positive B cells and strong expression of PKC $theta$ in Thy1.2-positiveT cells. After 24 h in culture, the B and T cells were stimulatedwith PMA in the absence or presence of the PKC inhibitors rottlerinand Gö6976 and analyzed for NF- $kappa$ B and JNK kinase activation (Fig.1C and D). Rottlerin, an inhibitor with high specificity towardsCa²⁺-independent (novel) PKCs (15, 42), interfered with NF- $kappa$ Band JNK activation in B and T cells at a concentration of 30 µM,whereas the PKC inhibitor Gö6976, which inhibits Ca²⁺-dependent (classical) PKCs, had no effect on either signalingpathway. The specificity was confirmed in a kinase reaction onpurified rat brain PKC, which consists primarily of the $alpha$ , $beta$ ,and $gamma$ isoforms, with lesser amounts of $delta$ and $zeta$ isoforms (Fig.1E). Whereas 200 nM Gö6976 strongly inhibited the activity ofrat brain PKCs, rottlerin exerted no effect at concentrationsup to 30 µM. Loss of NF- $kappa$ B signaling was most likely due to impairedupstream signaling events because I $kappa$ B $alpha$ was significantly stabilizedin the presence of rottlerin (Fig. 1D, upper panel). These resultsindicate that similar signaling pathways which involve novel PKCscontribute to NF- $kappa$ B and JNK1 activation in primary B and T cells.

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FIG. 1. Novel PKCs are involved in NF- $kappa$ B and JNK activation in response to PMA in primary murine splenic B and T cells. (A) Splenocytes, MACS-separated Thy1.2-positive cells (Thy1.2+), or MACS-separated B220-positive cells (B220+) from either wild-type (BALB/c) or nude mice were analyzed for Thy1.2 and B220 expression by flow cytometry. (B) Whole cell extracts of B220- or Thy1.2-positive cells were analyzed for the expression of different PKC isoenzymes, as indicated. A nonspecific band that migrates slightly faster than PKC $theta$ is indicated by a circle. (C and D) T cells from BALB/c mice and B cells from nude mice were pretreated for 30 min with the indicated concentrations of PKC inhibitors Gö6976 or rottlerin and subsequently stimulated with PMA. NF- $kappa$ B activity was determined by EMSA (C) and I $kappa$ B $alpha$ degradation and JNK phosphorylation were determined by Western blotting (D). (E) Specificities of Gö6976 and rottlerin were confirmed in an in vitro kinase reaction using purified rat brain PKCs and myelin basic protein as a substrate.

It has been shown that NF- $kappa$ B is activated in response to stimulation of the BCR (3, 34). To elucidate the role of novelPKCs for BCR-mediated NF- $kappa$ B activation we treated primary B cellsfrom nude mice with anti-IgM antibody. We checked expression ofsurface IgM (sIgM) in splenocytes and B220-positive cells fromnude mice (Fig. 2A). Nearly all B220-positive cells were alsosIgM positive. NF- $kappa$ B was activated in B220-positive B cells inresponse to IgM cross-linking (Fig. 2B). Activation of NF- $kappa$ B correlatedwith reduced I $kappa$ B $alpha$ protein levels, and the process was inhibitedby rottlerin but not by Gö6976. We did not detect MAPK activationin response to IgM ligation (data not shown). These data demonstratethat novel PKCs are involved in BCR-induced activation of NF- $kappa$ Band provide evidence that a conserved pathway links antigen receptorsfrom B and T cells to their downstream targets.

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FIG. 2. BCR-directed activation of NF- $kappa$ B requires novel PKCs. (A) Splenocytes from nude mice and B220-positive cells obtained after MACS (Fig. 1) were analyzed for B220 and IgM surface expression by flow cytometry. Left and middle panels represent single stains; right panels represent double stains. (B) NF- $kappa$ B activation and I $kappa$ B $alpha$ degradation of B220 cells in response to anti-IgM or PMA stimulation was analyzed by EMSA or Western blotting, respectively. Rottlerin or Gö6976 was added at the indicated concentrations 30 min prior to stimulation.

Novel PKCs are involved in NF- $kappa$ B and JNK activation in 70Z/3 pre-B cells. We analyzed the requirement of individual PKCs for the activation of NF- $kappa$ B in mouse 70Z/3 pre-B cells as a model system. Thiswell-characterized cell line can be activated to express surfaceIgM in response to LPS or IFN- $gamma$ (36). We first investigatedby pharmacological inhibition which PKC subfamilies are responsiblefor NF- $kappa$ B and JNK activation in 70Z/3 cells (Fig. 3). Rottlerinwas a potent inhibitor of PMA-induced NF- $kappa$ B activation with aneffective concentration of 5 to 10 µM (Fig. 3A). In Jurkat T cells,where PKC $theta$ has been implicated in PMA-mediated NF- $kappa$ B activation(42), complete inhibition was exerted with 30 µM rottlerin.These concentrations had no effect on NF- $kappa$ B activation in responseto either LPS (70Z/3; Fig. 3A, lanes 9 to 11) or TNF- $alpha$ (Jurkat;Fig. 3A, lanes 20 to 22), showing that rottlerin specificallyinhibited PMA-induced activation of NF- $kappa$ B. Furthermore, administrationof rottlerin inhibited PMA-induced degradation of I $kappa$ B $alpha$ (Fig. 3B),demonstrating that PKC inhibition affected upstream signalingevents. Gö6976 did not elicit an effect on NF- $kappa$ B activation ata concentration of 200 nM in 70Z/3 and Jurkat T cells. Similarto NF- $kappa$ B activation, JNK1 phosphorylation in 70Z/3 cells was inhibitedat a rottlerin concentration of 5 µM and Gö6976 had no effect(Fig. 3B).

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FIG. 3. Inhibition of novel PKCs blocks NF- $kappa$ B and JNK kinase activation in 70Z/3 cells. (A) 70Z/3 pre-B or Jurkat T cells were pretreated for 30 min with the indicated amounts of Gö6976 or rottlerin and subsequently stimulated with PMA, TNF- $alpha$ , or LPS for 15 min. Whole cell extracts were analyzed for NF- $kappa$ B activation by EMSA. (B) 70Z/3 cells were treated as for panel A, and JNK1 as well as I $kappa$ B $alpha$ were analyzed by Western blotting. The star indicates the position of the hyperphosphorylated 46-kDa JNK1 isoform. (C) 70Z/3 cells were stimulated for 24 h with 10 ng of IFN- $gamma$ /ml, and IgM surface expression was determined by flow cytometry (untreated and stimulated cells, left and right panels, respectively). (D) IFN- $gamma$ -stimulated cells were pretreated with the indicated concentrations of rottlerin for 30 min and stimulated with mouse anti-IgM antibody (30 min), PMA (10 min), or LPS (30 min). NF- $kappa$ B DNA binding activity was determined by EMSA.

We treated 70Z/3 pre-B cells for 24 h with IFN- $gamma$ to induce expression of sIgM (Fig. 3C). IFN- $gamma$ pretreatment induced sIgM expressionwithout any effect on NF- $kappa$ B (Fig. 3 and data not shown). Incubationof the IgM-positive cells with an anti-IgM antibody led to a weakNF- $kappa$ B activation in 70Z/3 cells (Fig. 3D). NF- $kappa$ B activation wasstrictly dependent on sIgM expression, because in 70Z/3 cellsthat had not been pretreated with IFN- $gamma$ , IgM ligation did notactivate NF- $kappa$ B (data not shown). NF- $kappa$ B activation in responseto IgM cross-linking or PMA was inhibited by rottlerin to a similarextent. Again, LPS induction of NF- $kappa$ B was not affected by rottlerin.As in primary B cells, we did not observe activation of JNK inresponse to IgM ligation (data not shown). We conclude that NF- $kappa$ Bactivation in 70Z/3 pre-B cells and in primary B cells by PMAor IgM cross-linking involves the same signaling pathways thatdepend on novel PKCs. Therefore, 70Z/3 pre-B cells are a suitablemodel system to investigate the contribution of novel PKCs inresponse to B-cellactivation.

Defective activation of NF- $kappa$ B and JNK by PMA in the mutant pre-B-cell line 1.3E2. 1.3E2 cells, derivatives of 70Z/3 cells, are unable to activate NF- $kappa$ B in response to either LPS, IL-1, PMA, Taxol, or double-strandedRNA (10). This deficiency is due to the lack of IKK $gamma$ (44).In order to analyze the pathway for NF- $kappa$ B activation by PMA, wereintroduced IKK $gamma$ into the 1.3E2 cells. Stable expression of IKK $gamma$ HArescued NF- $kappa$ B activation after stimulation with either LPS orIL-1 $beta$ but, surprisingly, IKK $gamma$ failed to rescue NF- $kappa$ B activationin response to PMA in three different IKK $gamma$ -expressing clones (Fig.4A). Also, in transient transfections N-terminally Flag-taggedIKK $gamma$ could rescue LPS- but not PMA-induced activation of an NF- $kappa$ Breporter, ruling out that the position or sequence of the epitopetag has an effect on NF- $kappa$ B activation (S. Tegethoff, unpublishedresults). NF- $kappa$ B activation in 1.3E2 IKK $gamma$ clones by LPS or IL-1 $beta$ was slightly reduced in comparison to 70Z/3 cells, which was mostlikely due to the increased amounts of IKK $gamma$ (Fig. 4A; lower panel).Overexpression of IKK $gamma$ alone has been shown to inhibit IKK andNF- $kappa$ B activation, probably through competition for upstream activatorsof the IKK complex (25, 28). Next, we tested whether PMA ledto the activation of IKKs by performing in vitro kinase reactionsafter immunoprecipitation of the IKK complex (Fig. 4B). PMA efficientlyactivated the IKK complex in 70Z/3 cells but failed to do so ineither 1.3E2 or 1.3E2 IKK $gamma$ cells. Therefore, the loss of NF- $kappa$ Bactivation must be due to an upstream defect that is independentof IKK $gamma$ deficiency.

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FIG. 4. (A) IKK $gamma$ expression rescues LPS- and IL-1 $beta$ - but not PMA-induced NF- $kappa$ B activation of 1.3E2 cells. 70Z/3 cells, three 1.3E2 IKK $gamma$ -expressing clones, and 1.3E2 cells were treated with PMA, LPS, or IL-1 $beta$ for 30 min and NF- $kappa$ B DNA-binding activity was determined by EMSA. IKK $gamma$ protein was determined by Western blotting (lower panel). (B and C) Activation of IKK and JNK1 in response to PMA is defective in 1.3E2 and 1.3E2 IKK $gamma$ cells. (B) 70Z/3, 1.3E2, and 1.3E2 IKK $gamma$ 2 cells were stimulated with PMA (10 min), and extracts were analyzed for IKK $alpha$ protein expression. IKK activity was determined in an in vitro kinase reaction after IKK immunoprecipitation with an anti-IKK $alpha$ antibody. GstI $kappa$ B $alpha$ 1-53 was used as a substrate. (C) 70Z/3, 1.3E2, and 1.3E2 IKK $gamma$ 2 cells were stimulated with PMA (10 min), LPS (20 min), or UV light (20 min) and cellular extracts were analyzed for JNK1 expression (upper panel). The hyperphosphorylated 46-kDa JNK1 isoform is indicated by a star. JNK1 kinase activity was determined in an in vitro kinase reaction after immunoprecipitation of JNK1. Kinase activity was determined with recombinant GstJun1-79 as substrate. (D) Activation of ERK1/2 is not defective in 1.3E2 cells. Cells were stimulated with PMA for 10 min and cellular extracts were analyzed by Western blotting using JNK1, phospho-ERK1/2, or ERK1/2 antibodies (as indicated). Migration of the hyperphosphorylated 46-kDa JNK1 is indicated by a star.

Since PMA is a potent inducer of MAPK signaling pathways, we tested its ability to activate JNK1 in the different cell lines(Fig. 4C). JNK1 kinase assays using GstJun1-79 as a substratewere performed after immunoprecipitation with JNK1 antibody. PMAor UV light led to an activation of JNK1 in 70Z/3 cells, whereasLPS only weakly activated JNK1. In contrast, in neither 1.3E2nor 1.3E2 IKK $gamma$ cells could JNK1 kinase activity be stimulatedby PMA. Since JNK1 could still be activated by UV light, JNK signalingis not generally defective in 1.3E2 cells. To further test MAPKsignaling in 1.3E2 cells, we analyzed activation of ERK1/2 usinga phospho-specific antibody (Fig. 4D). Phosphorylation of ERK1/2in response to PMA did not differ in 70Z/3, 1.3E2, and 1.3E2 IKK $gamma$ cells. We did not observe activation of p38 in either 70Z/3 or1.3E2 cells when a phospho-specific antibody was used (data notshown). These results suggest that the loss of PMA-mediated NF- $kappa$ Band JNK activation in 1.3E2 cells is caused by a common defectupstream of the IKK complex that does not affect activation ofERKs.

Novel PKC $theta$ is absent in 1.3E2 cells. Classical and novel PKC isoforms are directly activated by phorbol ester. We compared the protein amounts of various PKC familymembers in 70Z/3, 1.3E2, 1.3E2 IKK $gamma$ , and Jurkat cells by Westernblotting (Fig. 5A). As expected, compared to Jurkat T cells thepre-B cell line 70Z/3 as well as its 1.3E2 derivative containedhigh amounts of the Ca²⁺-independent PKC $delta$ and PKC $varepsilon$ , both of which have been shown to beexpressed in the B-cell lineage (32). Nevertheless, novel PKCs $delta$ and $varepsilon$ and the classical Ca²⁺-dependent PKCs $alpha$ , $beta$ I, $beta$ II, and $gamma$ (Fig. 5A) as well as the atypicalphorbol ester-independent PKC isoforms $iota$ and $lambda$ (data not shown)were all equally expressed in 70Z/3 cells compared to 1.3E2 cells.In contrast, PKC $theta$ was only weakly expressed in 70Z/3 cells versusJurkat T cells, and it was absent in 1.3E2 and 1.3E2 IKK $gamma$ cells.We confirmed this result by nuclear-cytoplasmic fractionationof 70Z/3, 1.3E2, and Jurkat cells (Fig. 5; lower panel). As expected,PKC $theta$ was predominantly localized in the cytoplasmic compartmentand only weakly in the nucleus. Again, PKC $theta$ expression was observedin Jurkat and, albeit more weakly, in 70Z/3 cells, but it waslacking in 1.3E2 cells. Due to the weak expression of PKC $theta$ in70Z/3 cells, a nonspecific band appears that migrates slightlyfaster than the specific signal.

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FIG. 5. PKC $theta$ is absent in 1.3E2 and 1.3E2 IKK $gamma$ cells. (A) Whole cell extracts were prepared from 70Z/3, 1.3E2, 1.3E2 IKK $gamma$ 2, and Jurkat T cells and the expression of various PKC family members was determined by Western blotting. Lower panel, nuclear (N) and cytoplasmic (C) extracts of 70Z/3, 1.3E2, and Jurkat cells were analyzed for PKC $theta$ expression. A nonspecific band migrating faster than PKC $theta$ is indicated by a dot. (B) In response to PMA, PKC $theta$ translocates to the membrane but does not quantitatively associate with IKK $gamma$ . Cells were attached to the surface of the chamber slides by culturing in the absence of serum for 16 h. 70Z/3, 1.3E2, 1.3E2 IKK $gamma$ /PKC $theta$ , or 1.3E2 IKK $gamma$ cells were left untreated or stimulated with PMA for 20 min. After fixation and permeabilization, cells were costained with polyclonal IKK $gamma$ and monoclonal PKC $theta$ primary antibodies. For the detection, FITC-conjugated donkey anti-rabbit and tetramethyl rhodamine isocyanate-conjugated donkey anti-mouse secondary antibodies were used.

Previous studies have suggested that the function of PKC $theta$ in the hematopoietic lineage is restricted to T cells (32, 40).Therefore, by performing indirect immunofluorescence in 70Z/3pre-B cells, we tested if PKC $theta$ translocates to the membrane inresponse to PMA (Fig. 5B). In unstimulated 70Z/3 cells, PKC $theta$ residedpredominantly in the cytoplasm, but upon activation the majoritywas localized to the cytosolic membrane. In parallel, we costainedIKK $gamma$ in the same cells and found that IKK $gamma$ resided in the cytoplasmand to a small degree also in the nuclear compartment, with nochange upon stimulation. Congruent with the Western blotting data,no staining of either PKC $theta$ or IKK $gamma$ was observed in 1.3E2 cells,which confirms the specificity of the staining in 70Z/3 cells.PKC $theta$ deficiency in 1.3E2 cells together with defective PMA signalingsuggested that this isoform could be engaged in NF- $kappa$ B and JNKactivation in 70Z/3 pre-B cells and encouraged us to rescue PMAsignaling by ectopic expression of PKC $theta$ .

Stably expressed novel PKC $theta$ or PKC $delta$ , but not classical PKC $beta$ II, rescues NF- $kappa$ B and JNK activation in 1.3E2 IKK $gamma$ -expressing cells. We decided to introduce different PKC isoenzymes into 1.3E2 IKK $gamma$ -expressing cells to see if defective PMA signaling can berescued. Novel PKC $theta$ and PKC $delta$ as well as classical PKC $beta$ II werestably transfected in 1.3E2 IKK $gamma$ cells and PKC-positive cloneswere selected (Fig. 6A). In some cases IKK $gamma$ protein expressionwas lost during the process of selection (clones 1, 4 and 9),making it possible to determine the role of PKCs in the absenceof a functional IKK complex.

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FIG. 6. Stable expression of PKC $theta$ or PKC $delta$ , but not PKC $beta$ II, rescues PMA activation of NF- $kappa$ B and JNK in 1.3E2 IKK $gamma$ cells. (A) Expression of the different PKC isoforms and IKK $gamma$ in the stable transfectants was analyzed by Western blotting. Note that some clones (1, 4, and 9) lost IKK $gamma$ expression during the process of selection. (B) Activation of NF- $kappa$ B in 70Z/3, 1.3E2, and 1.3E2 IKK $gamma$ cells and various PKC-expressing clones in response to PMA (10 and 30 min) or LPS (45 min), as determined by EMSA. (C) NF- $kappa$ B activation in response to LPS and PMA was determined by NF- $kappa$ B reporter assays in 1.3E2 IKK $gamma$ cells and either PKC $theta$ - or PKC $delta$ -expressing clones. Each bar represents the average of three independent experiments, with standard deviations indicated. (D) PMA-induced JNK activation in 70Z/3 cells and in various 1.3E2 clones was determined in a Western blot using phospho-JNK and anti-JNK1 antibodies. Migration of transiently phosphorylated JNK is marked by a star.

NF- $kappa$ B activation by PMA (10 and 30 min) or LPS (45 min) was determined by EMSA (Fig. 6B). Stable expression of either PKC $theta$ or PKC $delta$ in 1.3E2 IKK $gamma$ cells (clones 2, 3, 5, and 6) rescued NF- $kappa$ Bactivation in response to PMA. In contrast, ectopic PKC $beta$ II failedto reinstate PMA responsiveness in 1.3E2 IKK $gamma$ cells. NF- $kappa$ B activationwas abrogated in response to LPS only in 1.3E2 cells and in thePKC $theta$ -expressing clone 4, which had lost any detectable IKK $gamma$ protein.Thus, LPS responsiveness was unaffected as long as a functionalIKK complex was present. NF- $kappa$ B activation was functional, as observedin a luciferase reporter assay (Fig. 6C). Whereas LPS activatedthe NF- $kappa$ B reporter independent of ectopic PKC $theta$ or PKC $delta$ , PMA couldonly activate the reporter in the presence of either kinase. Wealso tested NF- $kappa$ B activation by IgM ligation in 1.3E2 cells orin the IKK $gamma$ - or IKK $gamma$ /PKC-expressing clones. No activation wasdetectable; however, only about 50% of the IFN $gamma$ -treated 1.3E2cells were sIgM positive. In addition, the overall level of sIgMin positive cells was decreased compared to IFN $gamma$ -induced 70Z/3cells (data not shown). Therefore, given the relatively weak activationof NF- $kappa$ B in 70Z/3 cells (see Fig. 3D), the lack of activationin 1.3E2 cells is probably due to the limiting amount of the BCRon the cellsurface.

Besides NF- $kappa$ B activation, stable expression of novel PKC $theta$ and PKC $delta$ also rescued JNK activation in 1.3E2 cells (Fig. 6D). Westernanalysis using anti-phospho-JNK and anti-JNK1 antibodies showedthat JNK was transiently phosphorylated in response to PMA in70Z/3 cells as well as in all 1.3E2 cell clones, which were expressingeither PKC $theta$ or PKC $delta$ . JNK kinase activation was independent ofa functional IKK complex, since JNK phosphorylation was also obtainedin the clones which had lost IKK $gamma$ expression. Since several clones(two PKC $theta$ - and one PKC $delta$ -expressing clone; Fig. 6D and data notshown) displayed JNK activation in the absence of IKK $gamma$ , clonaldifferences cannot account for the maintenance of JNK signaling.Again, ectopic expression of PKC $beta$ II did not rescue JNK signalingin 1.3E2cells.

We conclude that a defect in NF- $kappa$ B and JNK activation in response to PMA in the 70Z/3-derived 1.3E2 cell line can be overcomeby the ectopic expression of novel PKC $theta$ or - $delta$ . Expression of classicalPKC $beta$ II cannot promote NF- $kappa$ B and JNK activation. Taken together,the results present evidence for a specific role of novel PKCsfor PMA- or BCR-specific activation of NF- $kappa$ B in Bcells.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

During the last years much attention has been focused on the role of novel PKCs and especially of PKC $theta$ for TCR/CD3, and CD28costimulation with PMA-ionomycin is thought to mimic this stimulationin T cells (2, 9, 11, 14, 24, 29, 40, 42). Usingthe PKC inhibitor rottlerin, we showed that novel PKCs are alsoinvolved in PMA-induced NF- $kappa$ B activation in primary B220-positiveB cells derived from spleens of wild-type and nude mice. It wasdemonstrated that stimulation of the BCR leads to activation ofNF- $kappa$ B (5, 35), a process which involves Bruton's tyrosinekinase, phospholipase C- $gamma$ 2, and the IKK complex (3, 33, 34).We now demonstrate that BCR activation of NF- $kappa$ B requires novelPKCs in 70Z/3 pre-B cells as well as in primary B cells. In contrastto peripheral T cells, which are characterized by high expressionof novel PKC $theta$ , B cells express high amounts of PKC $delta$ and - $varepsilon$ . Congruentwith this observation, BCR signaling was shown to activate PKC $delta$ (4). We did not observe MAPK activation after BCR cross-linkingin 70Z/3 cells or primary B cells (data not shown). Interestingly,Ruland et al. (38) have now shown that Bcl10^/ mice are defective in NF- $kappa$ B activation in response to both antigenreceptors (TCR and BCR). Our data suggest that the upstream signalingevents leading to IKK activation in response to antigen receptorsignaling in B and T cells are distinct from those of pathwaysinitiated by TNF- $alpha$ , IL-1, or LPS. Signal transduction in bothcases involves novel PKCs, Bcl10, the IKK complex, and subsequentlyNF- $kappa$ B, which shows that signaling initiated by TCR and BCR ishighlyconserved.

We looked for a cellular model to study NF- $kappa$ B activation in a well-characterized cell line of the B-lymphocytic lineage. 70Z/3pre-B cells were chosen because expression of sIgM can be inducedand it was previously shown that cross-linking of sIgM leads toNF- $kappa$ B activation (35). We found that, just like in primary Bcells, IgM ligation activated NF- $kappa$ B in 70Z/3 cells, demonstratingthat these cells express a functional BCR and contain all componentsnecessary for downstream signaling. Importantly, both BCR- andPMA-induced signaling required novel PKCs. The 1.3E2 cell linehas been isolated by immunoselection as a variant of 70Z/3 cellsthat is unable to express surface IgM in response to LPS (31).Subsequently, it was shown that the cells are defective in NF- $kappa$ Band Oct-2 activation (7, 10, 36). 1.3E2 cells do not functionallyexpress the NF- $kappa$ B essential modulator (NEMO) or IKK $gamma$ , which isessential for activation of the IKK complex (37, 44). NF- $kappa$ Bactivation in response to multiple stimuli can be recovered byNEMO/IKK $gamma$ expression. In contrast to previous results by Yamaokaet al. (44), we found that defective NF- $kappa$ B activation by PMAwas not complemented by the stable expression of IKK $gamma$ , even thoughLPS and IL-1 responses could be recovered. Possibly, clonal differencesdepending on the lots of the 1.3E2 cells used may explain thisdiscrepancy. Nevertheless, all other molecular and cellular parameterswhich we determined for 1.3E2 cells (i.e., lack of NEMO/IKK $gamma$ protein,reduced Oct-2 DNA binding, active ERK1/2 kinases, sIgM expressionin response to IFN $gamma$ but not to LPS) are congruent with previouslypublished observations. We have used the human NEMO/IKK $gamma$ cDNAfor complementation, but the fact that LPS and IL-1 responsesas well as PMA stimulation in the presence of novel PKCs couldbe rescued in 1.3E2 cells strongly argues against species-specificfunctional differences of IKK $gamma$ . The reproducible finding of defectivePMA responses of NF- $kappa$ B and JNK (see also below) in 1.3E2 cellsas well as in 1.3E2 IKK $gamma$ clones made it possible to specificallyinvestigate the requirements for PKC-mediated antigen receptorsignaling in pre-Bcells.

The observation that 1.3E2 cells are not only defective in NF- $kappa$ B activation but also fail to activate the MAPK JNK providesfurther evidence that loss of PMA responsiveness is caused bya defect in a component common to both pathways. Defective JNKactivation was shown with antibodies recognizing the hyperphosphorylatedform of JNK as well as in vitro kinase reactions using GSTJun1-79as a substrate. Importantly, UV light-induced JNK signaling wasstill intact, providing evidence that the defect resides in PMA-inducedsignal cascades and is not a consequence of a mutation in JNKitself. NF- $kappa$ B and JNK signaling pathways diverge somewhere upstreamof the IKK complex, making it very likely that either the lossof or a mutation at the level of PKCs is responsible for the signalingdefect. Interestingly, MAPK signaling is not generally affectedbecause ERK1 and -2 are still active in 1.3E2 cells (Fig. 4D)(10), showing that distinct pathways activate individual MAPKs(also reviewed in reference 8). Also, in Jurkat T cells ithas been demonstrated that PKC $theta$ contributes to JNK but not toERK activation (14; see alsobelow).

Since PMA directly activates PKCs, we determined the expression of a panel of PKC family members. Just like in primary B cells,strong expression of PKC $delta$ and - $varepsilon$ could be observed in the pre-Bcell lines. However, of all PKC isoenzymes tested in Western blotting,only PKC $theta$ was differentially expressed in 70Z/3 versus 1.3E2 cells.This result was confirmed by indirect immunofluorescence, showingthat PKC $theta$ is not only expressed in 70Z/3 cells but also translocatesto the membrane in response to PMA. In T cells it has been shownthat upon stimulation with PMA-ionomycin or CD3/CD28, PKC $theta$ associateswith IKK $alpha$ or - $beta$ and colocalizes at the membrane (24). Therefore,we investigated if endogenous IKK $gamma$ is at least partially shiftedto the membrane in response to stimulation, but we found thatIKK $gamma$ resides in the cytoplasm and maybe partially in the nucleus(see also reference 28). Since IKK $gamma$ quantitatively associateswith IKK $beta$ and IKK $alpha$ in 70Z/3 cells (25), we find no evidencethat membrane translocation of the IKK complex precedes its activationby PMA. Nevertheless, a transient translocation of the IKK complexto the membrane might precede itsactivation.

The finding that PKC $theta$ was differentially expressed in the pre-B cell lines was quite surprising, because an analysis of PKCsin hematopoietic cells reveals that PKC $theta$ is predominantly expressedin T cells (Fig. 1B) (32). However, the differential expressionof PKC $theta$ in 70Z/3 and 1.3E2 cells clearly suggests that this isoenzymeshould have a key function for NF- $kappa$ B and JNK activation. Due tothe extremely poor transfection efficiency in 70Z/3 cells, wefailed to block NF- $kappa$ B activation using kinase-inactive mutantsof either PKC $theta$ , PKC $delta$ , or PKC $varepsilon$ (data not shown), and we thereforeattempted to rescue PMA signaling by stable expression of PKCsin 1.3E2 IKK $gamma$ cells. In line with the hypothesis that PKC $theta$ isessential for NF- $kappa$ B and MAPK activation by PMA in the pre-B-celllines, we could rescue both signaling pathways by ectopic expressionof PKC $theta$ (Fig. 6). Surprisingly, PKC $delta$ , another novel PKC isoform,could also rescue NF- $kappa$ B and JNK activation. In contrast, PMA activationwas not restored by expression of the Ca²⁺-dependent classical PKC isoform $beta$ II. Therefore, in agreementwith the data obtained using the pharmacological inhibitor rottlerin,a rescue was observed only when novel PKCs were transfected. Thequestion remains why PKC function could be rescued with eitherPKC $theta$ or - $delta$ , even though PKC $delta$ , in contrast to PKC $theta$ , was expressedin considerable amounts in 70Z/3 as well as in 1.3E2 cells. Asa likely explanation, strong overexpression of one novel PKC isoformmight suffice to compensate for the loss of the other. In fact,among the novel PKCs, PKC $delta$ is the closest relative of PKC $theta$ , withan overall extended identity of 59% suggesting that both isoformscould be functionally redundant. The similarity between PKC $theta$ andother novel PKC isoforms is considerably lower, with 38% identityfor PKC $varepsilon$ as the next relative. Significant homologies to classicalPKCs are restricted to the kinase and PMA binding domains. Furthermore,NF- $kappa$ B and JNK activation in 1.3E2 cells was strictly dependenton PKC activation by PMA, and PKC overexpression alone did notsuffice to activate signaling nonspecifically. Moreover, in themutant 1.3E2 cells, ectopically expressed PKC $theta$ translocates tothe membrane in response to PMA, indicating that all other componentsnecessary for PMA signaling are intact. It was shown recentlythat Bcl10 is necessary for NF- $kappa$ B activation in response to TCRstimulation and acts downstream or at the level of PKC $theta$ (38).We found no change in Bcl10 protein expression between 70Z/3 and1.3E2 cells (data not shown). Furthermore, Bcl10 deficiency doesnot affect MAPK activation (38), indicating that the point whereNF- $kappa$ B and MAPK pathways diverge is upstream of Bcl10 at the levelof PKC activation. Therefore, it is most likely that PKC $theta$ deficiencyin 1.3E2 cells is responsible for the PMA signaling defect, butthis defect can be overcome either by reintroduction of PKC $theta$ orby increasing the levels of the related $delta$ isoform.

The data thus suggest that besides the specific function of PKC $theta$ in T-cell lines, mature primary T cells, and the 70Z/3 and1.3E2 pre-B cell lines, PKC $theta$ plays a key role in NF- $kappa$ B signalingin primary B cells. The analysis of PKC isoenzyme expression inprimary B and T cells revealed that PKC $theta$ levels are highest inT cells. Nevertheless, we did observe expression of PKC $theta$ , albeitweaker, also in primary B cells. A detailed analysis of B cellsfrom PKC $theta$ - and/or PKC $delta$ -deficient mice needs to be performed toanswer the question of which PKC isoform plays a crucial rolefor pre-B cells or at any other stage of B-cell differentiation.In this respect, it is interesting that PKC $theta$ is essential forTCR-mediated NF- $kappa$ B activation in mature but not immature T lymphocytes(40). The PKC isoform responsible for NF- $kappa$ B activation in immatureT lymphocytes remains to be identified. In addition, in mice,MAPK signaling in T cells was not influenced by PKC $theta$ deficiency,even though PKC $theta$ is an upstream regulator for JNK in Jurkat Tcells (2, 14). The data indicate that each individual PKCisoform carries out specific functions which are not only dependenton the cell type but which also differ in the downstream signalingpathway that theyactivate.

In this study we established a role for novel PKCs in BCR signaling to NF- $kappa$ B, and thereby we underscored a striking conservationfor antigen receptor signaling in T and B cells. Future studieswill need to address the mechanism by which novel PKCs are linkingthe antigen receptor activation to the IKKcomplex.

	ACKNOWLEDGMENTS

We thank Gottfried Baier for providing us with PKC $theta$ and PKC $delta$ , Harald Mischak for the gift of PKC $beta$ II, and Robert Newton forthe 6xNF- $kappa$ Bluc constructs. We thank Carol Sibley for the giftof the 70Z/3 and 1.3E2 cells. Furthermore, we thank Erika Scharschmidtfor excellent technical assistance, Benjamin Mordmüller for purificationof GstJun1-79, and Susanne Preiss for the help with the lymphocytepurification.

	FOOTNOTES

^* Corresponding author. Mailing address: Max-Delbrück-Centrum for Molecular Medicine, Robert-Rössle Str. 10, 13125 Berlin,Germany. Phone: 49-30-9406-3751. Fax: 49-30-9406-3866. E-mail:dkrapp{at}mdc-berlin.de.

Present address: Center for Blood Research, Harvard Medical School, Boston, MA02115.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Altman, A., N. Isakov, and G. Baier. 2000. Protein kinase C $theta$ : a new essential superstar on the T-cell stage. Immunol. Today 21:567-573[CrossRef][Medline].
2.	Avraham, A., S. Jung, Y. Samuels, R. Seger, and Y. Ben-Neriah. 1998. Co-stimulation-dependent activation of a JNK-kinase in T lymphocytes. Eur. J. Immunol. 28:2320-2330[CrossRef][Medline].
3.	Bajpai, U. D., K. Zhang, M. Teutsch, R. Sen, and H. H. Wortis. 2000. Bruton's tyrosine kinase links the B cell receptor to nuclear factor kappaB activation. J. Exp. Med. 191:1735-1744[Abstract/Free Full Text].
4.	Barbazuk, S. M., and M. R. Gold. 1999. Protein kinase C-delta is a target of B-cell antigen receptor signaling. Immunol. Lett. 69:259-267[CrossRef][Medline].
5.	Bendall, H. H., M. L. Sikes, D. W. Ballard, and E. M. Oltz. 1999. An intact NF-kappa B signaling pathway is required for maintenance of mature B cell subsets. Mol. Immunol. 36:187-195[CrossRef][Medline].
6.	Bergmann, M., L. Hart, M. Lindsay, P. J. Barnes, and R. Newton. 1998. I $kappa$ B $alpha$ degradation and nuclear factor- $kappa$ B DNA binding are insufficient for interleukin-1 $beta$ and tumor necrosis factor-alpha-induced $kappa$ B-dependent transcription. Requirement for an additional activation pathway. J. Biol. Chem. 273:6607-6610[Abstract/Free Full Text].
7.	Briskin, M., M. Damore, R. Law, G. Lee, P. W. Kincade, C. H. Sibley, M. Kuehl, and R. Wall. 1990. Lipopolysaccharide-unresponsive mutant pre-B-cell lines blocked in NF-kappa B activation. Mol. Cell. Biol. 10:422-425[Abstract/Free Full Text].
8.	Chang, L., and M. Karin. 2001. Mammalian MAP kinase signalling cascades. Nature 410:37-40[CrossRef][Medline].
9.	Coudronniere, N., M. Villalba, N. Englund, and A. Altman. 2000. NF-kappa B activation induced by T cell receptor/CD28 costimulation is mediated by protein kinase C-theta. Proc. Natl. Acad. Sci. USA 97:3394-3399[Abstract/Free Full Text].
10.	Courtois, G., S. T. Whiteside, C. H. Sibley, and A. Israel. 1997. Characterization of a mutant cell line that does not activate NF-kappaB in response to multiple stimuli. Mol. Cell. Biol. 17:1441-1449[Abstract].
11.	Dienz, O., S. P. Hehner, W. Droge, and M. L. Schmitz. 2000. Synergistic activation of NF-kappa B by functional cooperation between vav and PKCtheta in T lymphocytes. J. Biol. Chem. 275:24547-24551[Abstract/Free Full Text].
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B-Cell Receptor- and Phorbol Ester-Induced NF-B and c-Jun N-Terminal Kinase Activation in B Cells Requires Novel Protein Kinase C's

B-Cell Receptor- and Phorbol Ester-Induced NF- $kappa$ B and c-Jun N-Terminal Kinase Activation in B Cells Requires Novel Protein Kinase C's