Membrane Translocation of Novel Protein Kinase Cs Is Regulated by Phosphorylation of the C2 Domain*

Antonio M. PepioDagger and Wayne S. Sossin§

From the Department of Neurology and Neurosurgery, McGill University, Montreal Neurological Institute, Montreal, Quebec H3A 2B4, Canada

Received for publication, July 18, 2000, and in revised form, November 7, 2000



    ABSTRACT
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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Ca2+-independent or novel protein kinase Cs (nPKCs) contain an N-terminal C2 domain of unknown function. Removal of the C2 domain of the Aplysia nPKC Apl II allows activation of the enzyme at lower concentrations of phosphatidylserine, suggesting an inhibitory role for the C2 domain in enzyme activation. However, the mechanism for C2 domain-mediated inhibition is not known. Mapping of the autophosphorylation sites for protein kinase C (PKC) Apl II reveals four phosphopeptides in the regulatory domain of PKC Apl II, two of which are in the C2 domain at serine 2 and serine 36. Unlike most PKC autophosphorylation sites, these serines could be phosphorylated in trans. Interestingly, phosphorylation of serine 36 increased binding of the C2 domain to phosphatidylserine membranes in vitro. In cells, PKC Apl II phosphorylation at serine 36 was increased by PKC activators, and PKC phosphorylated at this position translocated more efficiently to membranes. Moreover, mutation of serine 36 to alanine significantly reduced membrane translocation of PKC Apl II. We suggest that translocation of nPKCs is regulated by phosphorylation of the C2 domain.



    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Protein kinase Cs (PKCs)1 are a family of lipid-activated enzymes that play important roles in many cellular processes including regulation of synaptic strength in the nervous system (1). We have studied the regulation of PKC in Aplysia, an important model system for synaptic plasticity, where PKC plays several important roles in regulating synaptic strength (2-6). The structure of PKCs is conserved in Aplysia. Ca2+-activated PKCs (cPKCs) in vertebrates (alpha , beta , gamma ) and invertebrates (PKC Apl I in Aplysia) have two C1 domains and a C2 domain. Ca2+-independent or novel PKCs (nPKCs) in vertebrates (delta , epsilon , eta , and theta ) and invertebrates (PKC Apl II in Aplysia) also have two C1 domains and a C2 domain. However, the C2 domain in these kinases is N-terminal to the C1 domains and lacks several of the critical aspartic acids necessary for the coordination of Ca2+ ions (7).

In cPKCs, the C2 domain mediates Ca2+-dependent binding to the membrane lipid phosphatidylserine (PS) (8, 9). This binding is believed to be the primary step in kinase activation. First, it transiently recruits the enzyme to the membrane where its physiological activator, diacylglycerol (DAG), resides. Second, in conjunction with the C1 domain interacting with DAG, binding of the C2 domain to PS induces a conformational change that activates the enzyme (10, 11). Finally, the C2 domain binds to the receptor for activated protein kinase C (RACK), and this binding is important for the location of PKC translocation and for cellular functions of PKC (12).

In contrast to cPKCs, a detailed model for the role of the N-terminal C2 domain in nPKC activation is not available. C2 domains of nPKCs do not bind constitutively to lipids and are not regulated by calcium (13). However, similar to cPKCs, C2 domain-derived peptides from nPKCs act as isoform-specific inhibitors and activators in cells, implicating the C2 domain in the regulation of enzymatic activity (14-16). Removal of the C2 domain of PKCeta does not perturb the substrate specificity or response of the enzyme to phosphatidylinositol 3-kinase activity (17, 18). However, removal of the C2 domain of PKC Apl II decreases the amount of PS necessary for kinase activity, implicating the C2 domain in kinase regulation (19).

In vitro, PKC Apl II is activated more poorly than PKC Apl I, even when calcium is removed from PKC Apl I, suggesting a requirement of additional activators for stimulation of PKC Apl II in vivo (13, 19). Comparisons between PKCepsilon and PKCalpha also indicate that nPKCs require additional factors to bind efficiently to lipid membranes (20). PKC Apl II can be activated under a number of physiological conditions in cells, usually after prolonged activation of signal transduction pathways (6, 21). Prolonged activation also induces autonomous activity of PKC Apl II (22). This activation is specific, as PKC Apl I does not become autonomous under these conditions. The autonomous activity does not result from proteolysis to form a protein kinase M but probably results from post-translational modifications in the regulatory domain of PKC Apl II (22).

PKCs are regulated by phosphorylation. Phosphorylation in the activation loop by phosphoinositide-dependent protein kinase I (PDK-1) is required for subsequent PKC "maturation" by autophosphorylation at two residues critical for enzyme stability and activity (8, 23, 24). Phosphorylation of PKCdelta on tyrosine residues is thought to be important for activation of the kinase (25-27). Upon activation, PKCs additionally phosphorylate themselves on several residues. The roles for these phosphorylations are still unknown. Autophosphorylation at a conserved site in the C-terminal domain has been associated with persistent activation of PKC and may be involved in removal of the enzyme from the membrane (28, 29). A phosphorylation site has also been identified in the C2 domain of vertebrate PKCalpha that is correlated with PKC activation (30). Autophosphorylation of the epsilon -eta family of novel PKCs, which includes the invertebrate kinases PKC Apl II in Aplysia, Drosophila PKC98F, and Caenorhabditis elegans PKCIB, has not been investigated.

In this paper we identify two autophosphorylation sites, serine 2 and serine 36, in the C2 domain of the nPKC Apl II. Phosphorylation at serine 36 increases lipid binding to the C2 domain and increases translocation of PKCs in cells. We suggest that phosphorylation of C2 domains in novel PKCs is important for regulating their translocation.


    EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Reagents-- 4-beta -Phorbol 12,13-dibutyrate was from LC Services; dioleoyl phosphatidylserine (PS) and dioleoyl phosphatidylcholine (PC) were from Avanti Polar Lipids Inc., Alabaster, AL; Triton X-100 was from Avanti; prestained molecular weight markers were from Amersham Pharmacia Biotech; and N-tosyl-L-phenylalanine chloromethyl ketone-treated trypsin (TPCK) was from Worthington. All other reagents were of the highest grade available.

Plasmid Construction of PKCs, Fusion Proteins, and Mutants-- Full-length clones of PKC Apl II were present in Bluescript SK and the baculovirus vector BB3 (19). Initially, PKC Apl II was excised from baculovirus BB3 using SacI/SalI and inserted into the new vector BB4 (Invitrogen) at SacI/SalI. The C2 domain S36A and S36E mutations were generated with a two-step mutagenic procedure using the polymerase chain reaction (PCR). First round PCR used the C2 domain of PKC Apl II in the pMALC-C2 plasmid (New England Biolabs) as a template and either the outside 5' primer (O5) and the inside 3' primer (I3) or the inside 5' primer (I5) and the outside 3' primer (O3) (see Table I for primers). The products from the first round synthesis were combined and used as the template for second round synthesis using O5 and O3. The resultant product was cut with appropriate enzymes (Table I) and inserted into PKC Apl II in the BB4 vector. A new site was formed by the mutagenesis (Table I) and was used to confirm the cloning. The mutations were also made in the pMAL-C2 vector encoding the MBP-C2 fusion protein using a similar procedure. The final product was cut with appropriate enzymes (Table I) and inserted into the MBP-C2 domain at the indicated cloning sites (Table I). Ser-68 right-arrow Ala and Ser-2 right-arrow Ala were made with a similar strategy using different inside primers and the same outside primers (Table I). A clone of human PKCepsilon was a kind gift of A. Toker (Harvard Medical School). The construct was amplified with PCR using VENT DNA polymerase (New England Biolabs, Beverly, MA) and inserted into BB4 at KpnI and BamHI. The construct lacking the C2 domain used an alternative 5' primer containing the initiating methionine of PKCepsilon followed by amino acid 145. GST and MBP-C2 fusion proteins and MBP-C2 deletion constructs were made previously (13, 21).


                              
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Table I
Wild type and mutant PKC primers and cloning sites

Baculovirus Construction-- Spodoptera frugiperda (Sf9, Sf21; Invitrogen) cells were grown in suspension cultures with supplemented Grace's media (Life Technologies, Inc.) and 10% fetal bovine serum (Life Technologies, Inc.). The baculovirus transfer vectors were cotransfected with linearized baculovirus (Invitrogen), and the resultant blue colonies were plaque-purified. Positive colonies were confirmed by PCR and by immunoblotting with anti-PKC Apl II or anti-PKCepsilon antibodies ((31) Calbiochem). High titer viral stocks (108-1010 plaque-forming units (pfu)/ml) were generated as described (19).

PKC Purification from Baculovirus-- Biochemical purification of all Aplysia PKCs, human PKCepsilon , and mutants was performed as described previously (19) with the following modifications. Briefly, 250 ml of Sf21 cells (2 × 106 cells/ml) were infected with 1 × 109 pfus of baculovirus and incubated for 64 h for optimal PKC expression. Cells were pelleted, resuspended, sonicated, and centrifuged as described. The supernatant solution was passed through a 0.22-µm filter, diluted to 50 ml with buffer A (20 mM Tris-HCl, pH 8.0, 0.5 mM EGTA, 0.5 mM EDTA, 10 mM 2-mercaptoethanol, 10% glycerol), and loaded onto a Mono-Q column (Bio-Rad) previously equilibrated in buffer A. The remaining steps were performed following previous protocols (19). All baculovirus expressed enzymes were aliquoted and stored frozen at -70 °C until needed.

Fusion Protein Synthesis-- Both a maltose-binding protein (MBP) and a glutathione S-transferase (GST) fusion protein were expressed in bacterial DH5alpha cells from either a pMAL-C2 plasmid (New England Biolabs) or a pGEX 5x.1 plasmid (Amersham Pharmacia Biotech). These plasmids contained an insert of PKC Apl II amino acids 1-155 corresponding to the C2 domain (13, 21). The MBP-C2 domain and GST-C2 domain fusion proteins were purified by affinity chromatography on amylose (New England Biolabs) or GST resin columns (Amersham Pharmacia Biotech), respectively.

Antibody Production and Immunoblotting-- We synthesized a peptide (CRLQKG(pS)TKEK; where pS is phosphoserine) corresponding to amino acids 30-40 of the C2 domain of PKC Apl II with Ser-36 converted to phosphoserine (Quality Controlled Biochemicals, MA) to generate a phosphopeptide antibody. The peptide was conjugated to bovine serum albumin maleimide (Pierce) via the cysteine and was injected intramuscularly into rabbits along with TitreMax Gold (Cytrx, Norcross, GA) three times at 4-week intervals. Serum was affinity purified and used in Western blots as described (32) with the phosphorylated peptide antibody at 1 µg/ml dilution and goat anti-rabbit, horseradish peroxidase-conjugated secondary antibody at 1 µg/ml. The phosphopeptide antibody was preabsorbed using the nonphosphorylated form of the peptide at 1 µg/µl for 30 min prior to its addition to the immunoblot. Results were visualized by enhanced chemiluminescence (PerkinElmer Life Sciences).

Lipid Preparation-- Sucrose-loaded large unilamellar vesicles containing trace [3H]PC were prepared. Briefly, lipid mixtures in chloroform were dried under a stream of nitrogen and resuspended in buffer (20 mM HEPES, pH 7.5, 170 mM sucrose). They were then subjected to 5 freeze-thaw cycles in liquid nitrogen and extruded through two stacked 0.1-µm polycarbonate filters using a Liposofast microextruder (Avestin, Inc., Ontario, Canada) as described (33). Phosphatidylserine liposomes were prepared by resuspending dried lipids in buffer and vortexing (19).

PKC Assays-- Protein kinase C (5 nM) activity was assayed using phorbol esters or the mixed micelle assay as described (19, 34).

PKC and Fusion Protein in Vitro Phosphorylation-- PKCs (200-500 nM) or PKC-derived C2 domain fusion proteins (2 µM) were incubated in reaction buffer (50 mM Tris-HCl, pH 7.5, 10 mM MgCl2, 5 mM EGTA) with 50 µg/ml dioleoyl phosphatidylserine, 20 nM PMA, and [gamma -32P]ATP (4 µCi in 50 µM ATP) for 30 min at room temperature. Phosphorylation was quenched by the addition of 5× Laemmli sample buffer and boiled.

C2 Domain Membrane-binding Assay-- Membrane binding of C2 domain constructs was determined by measuring the binding to sucrose-loaded vesicles (19, 33, 35). MBP fusion proteins on amylose beads were phosphorylated by PKC as described above. PKC, ATP, and lipids were removed by sedimenting the beads at low speeds (3000 × g for 1 min) followed by three washes with sedimentation buffer (0.3 mg ml-1 ovalbumin, 100 mM KCl, 1 mM dithiothreitol, 5 mM MgCl2, 20 mM HEPES, pH 7.5). Fusion proteins were eluted from the beads with sedimentation buffer containing 10 µM maltose. The purified fusion proteins were prespun to pellet aggregates for 30 min at 100,000 × g and 15 °C in a TLA-100 ultracentrifuge (Beckman Instruments, Palo Alto, CA). Soluble fusion proteins (1-2 µM) were incubated with sucrose-loaded vesicles (20 µM lipid) for 10 min at 15 °C. The proteins associated with the sucrose-loaded vesicles were then separated from free protein by ultracentrifugation at 100,000 × g for 30 min at 15 °C. Pelleting of lipids was confirmed using scintillation counting of [3H]PC which was included as a tracer in the sucrose-loaded vesicles or liposomes. Membrane-bound (pellet fraction) and free (supernatant fraction) C2 domain fusion protein was separated by SDS-PAGE and transferred to nitrocellulose membranes. Total protein was visualized by Ponceau-S staining and phosphorylated protein by autoradiography using Kodak BioMax MS film on the membrane. In some cases quantitation of the Ponceau-S staining was confirmed by immunoblotting using an antibody to the maltose-binding protein. In some experiments, the fusion protein was excised from the gels, and the amount of radioactivity incorporated was calculated by scintillation counting with correction for quenching. This experiment demonstrated that less than 5% of the total fusion protein was phosphorylated under these conditions.

Cell Fractionation-- Recombinant baculovirus encoding wild type, S36A, or S36E PKC Apl II was incubated with Sf-21 cells in media at 27 °C. After 72 h of infection, cells were incubated with vehicle (control) or 4-beta -PDBu (experimental) for 1 h at 27 °C. Cells were then harvested and lysed in homogenization buffer (50 mM Tris, pH 7.5, 1 mM EGTA, 10 mM MgCl2, 2.6 mM 2-mercaptoethanol, 20 mg/ml aprotinin, 5 mM benzamadine, 0.1 mM leupeptin, 50 mM NaF, 5 mM sodium pyrophosphate, pH 8.5, and 1 µM microcystin). The lysate was centrifuged at 100,000 × g for 30 min at 4 °C to separate the cytoplasmic fraction (supernatant) from the membrane/cytoskeleton fraction (pellet). Equal fractions of the supernatant and pellet fractions were analyzed by SDS-PAGE (9% acrylamide gels), transferred to nitrocellulose membranes, and immunoblotted with the PKC Apl II antibody and the phospho-Ser-36 antibody.

Phosphorylation and Partial Tryptic Digestion-- Purified PKC Apl II or PKC Apl IIDelta C2 was autophosphorylated as described (19). The phosphorylation reaction contained 10 pmol of PKC Apl II or PKC Apl IIDelta C2, 50 µM ATP, reaction buffer (80 mM Tris, pH 7.5, 10 mM EGTA, 20 mM MgCl2, 40 nM PMA, and 150 µg/ml dioleoyl phosphatidylserine) and proceeded for 30 min at room temperature in the presence of [gamma -32P]ATP. Phosphorylation was quenched by the addition of 5 µM inhibitory peptide. The 75-µl proteolysis reaction contained 10 pmol of either phosphorylated PKC Apl II or PKC Apl IIDelta C2 and 0.1% Triton X-100. The phosphorylated kinase component was incubated for 3 min at 30 °C, and proteolysis was initiated by addition of 2 µg/ml of N-tosyl-L-phenylalanine chloromethyl ketone-treated trypsin and incubated for an additional 5 min at 30 °C. Reactions were quenched by addition of 20 µl of Laemmli sample buffer and boiled. Proteins were separated by SDS-PAGE on 7% gels and electrophoretically transferred to nitrocellulose. Membranes were subjected to autoradiography to visualize phosphate incorporation into proteins and immunoblot with the anti-C2 domain antibody for identification of C2 domain containing protein fragments (13).

Analysis of Tryptic Peptides by Two-dimensional Thin Layer Chromatography-- Analysis was performed as described with several modifications (32, 36). Membrane fragments containing protein bands were preblocked in 0.5% PVP-360 in 100 mM acetic acid, washed, and subsequently digested overnight with 10 µg of TPCK-treated trypsin in 10 mM Tris, pH 7.5, and 5% acetonitrile. An additional 10 µg of trypsin was added to each band for 3 h the following day, and the supernatant solution containing desired peptides was lyophilized to completion. Peptides were resuspended in pH 1.9 buffer (0.6 M formic and 1.4 M acetic acid) and analyzed by two-dimensional TLC using a Hunter-3000 HTLC. Labeled peptides were visualized by autoradiography using Kodak BioMax MS film on the plate. Predicted migrations of phosphopeptides were calculated as described (36).

Phosphoamino Acid Analysis-- After tryptic digestion and lyophilization, PKC Apl II or C2 fusion protein peptides derived from in vitro phosphorylations were hydrolyzed to constituent amino acids using constant boiling N HCl for 2.5 h at 110 °C. Sample amino acids were mixed with phosphoserine, phosphothreonine, and phosphotyrosine standards prior to running the mixture in the primary TLC dimension using standard buffers (36). Phosphoamino acid standards were stained with 0.25% ninhydrin in acetone, and autoradiography was performed on the completed plate.

Data Analysis-- Immunoblots and autoradiograms were scanned, and analysis was performed using the public domain NIH Image program (developed at the National Institutes of Health and available on the Internet). We calibrated the program with the uncalibrated OD feature of NIH Image, which transforms the data using the formula y = log10 (255/(255 - x)), where x is the pixel value (0-254). Control experiments demonstrated that after this calibration, values were linear with respect to the amount of protein over a wide range of values (37). To measure translocation, the relative percentage was calculated by first determining the percentage on the pellet in control and experimental (PDBu-treated) conditions. The percentage change between these two conditions (experimental - control/control)·100 was determined.


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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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The C2 Domain of PKC Apl II Contains Two Autophosphorylation Sites-- To determine whether the C2 domain of PKC Apl II is regulated by autophosphorylation, we compared tryptic phosphopeptide maps generated after autophosphorylation of purified PKC Apl II or a purified mutant lacking the C2 domain (PKC Apl IIDelta C2). PKC Apl II had 5 reproducible phosphopeptides (Fig. 1A). Two of these phosphopeptides (2 and 3) were not found in the enzyme lacking the C2 domain (Fig. 1B). Removing the C2 domain generated no additional or modified sites (Fig. 1C). The absence of phosphopeptides 2 and 3 could be due to their location in the C2 domain or conformational changes due to the loss of the C2 domain. To obtain further evidence these sites were actually located in the C2 domain, we obtained tryptic phosphopeptide maps of C2 domain-containing regions of PKC Apl II after partial tryptic digests of autophosphorylated PKC Apl II and PKC Apl IIDelta C2 (Fig. 2A). The C2 domain containing fragments were identified based on immunoreactivity to a C2 domain-specific antibody (Fig. 2B) and by their absence in partial tryptic digests of PKC Apl IIDelta C2 (Fig. 2B, lane 2). Three bands were isolated from the gel and completely digested with trypsin for phosphopeptide mapping analysis (Fig. 2C). The largest C2 domain fragment, corresponding to the size of the intact regulatory domain contained phosphopeptides 2-5 suggesting that all four of these sites are present in the regulatory domain (Fig. 2C, upper panel). Phosphopeptide 1 was not further investigated but based on predicted mobility it may correspond to the C-terminal fragment that contains two predicted phosphorylated sites (28). The C2 domain core itself is quite resistant to tryptic digestion (13). Phosphopeptide mapping of the smallest C2 domain fragment corresponding to the size of the core exhibited only phosphopeptide 3 (Fig. 2C, lower panel). Thus, phosphopeptide 3 is contained in the C2 domain, whereas phosphopeptide 2 is either near the end of the C2 domain and is sensitive to tryptic digestion or is outside the C2 domain, and its phosphorylation is decreased by C2 domain removal.



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Fig. 1.   PKC Apl II autophosphorylates on five primary peptides (peptides 1-5), two of which are in the C2 domain. Proteins were phosphorylated, digested, and analyzed as described under "Experimental Procedures." A, phosphopeptide map of wild type PKC Apl II. B, phosphopeptide map of the mutant PKC Apl II lacking its C2 domain (PKC Apl IIDelta C2) illustrating that it does not phosphorylate peptides 2 and 3. C, phosphopeptide map of coapplied PKC Apl II wild type and PKC Apl IIDelta C2 illustrating that the spots from wild type PKC Apl II are the same as those from PKC Apl IIDelta C2 with the exception of peptides 2 and 3. + and - refer to the polarity of the primary electrophoresis dimension in buffer pH 1.9; vertical arrows indicate direction of liquid chromatography; S signifies origin of sample application or coapplication.



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Fig. 2.   Phosphopeptide 3 originates in the core of the C2 domain. Proteins were phosphorylated, digested, and analyzed as described under "Experimental Procedures." A, PKC Apl II wild type (lane 1) and PKC Apl IIDelta C2 (lane 2) were phosphorylated in vitro for 30 min in the presence of [gamma -32P]ATP. The samples were partially digested with 2 µg/ml trypsin for 5 min at 30 °C, separated by SDS-PAGE, transferred to nitrocellulose, and exposed to x-ray film (Autoradiogram). B, Western blot of the membrane in A using an antibody (Ab) directed to the C2 domain of PKC Apl II (13) confirming that the bands positive for 32P incorporation in A are C2 domain-containing fragments. C, phosphopeptide maps of C2 domain containing bands from B, lane 1 (upper to lower), illustrating that peptide 3 is isolated as the C2 domain core is isolated. + and - refer to the polarity of the primary electrophoresis dimension in buffer pH 1.9; vertical arrows indicate direction of liquid chromatography; S signifies origin of sample application.

The Autonomous PKC Apl II Is Not Autophosphorylated at Site 4-- Purified PKC Apl II contains both regulated and autonomous activities (22). The autonomous activity generated by purification is similar to the autonomous form of PKC Apl II that is found in the nervous system (22). To determine differences between autonomous and regulated kinase activities, we compared tryptic phosphopeptide maps of PKC Apl II that were autophosphorylated in the absence of activators (autonomous activity) or after activation by phorbol esters (Fig. 3A). Autophosphorylation of peptide 4 was greatly decreased in the autonomous kinase (Fig. 3B). Quantitation of the relative phosphorylation of site 4 in three separate experiments from two different purified preparations confirmed this result (Fig. 3C). This could be due to existing phosphorylation of the site corresponding to peptide 4 in this kinase or to a conformational change in the regulatory domain that reduces phosphorylation of this site.



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Fig. 3.   Autophosphorylation of peptide 4 is absent in the autonomous kinase. Proteins were phosphorylated, digested, and analyzed as described under "Experimental Procedures." A, wild type PKC Apl II was in vitro autophosphorylated in the presence of [gamma -32P]ATP and either no activators, PS/TPA, or oleic acid for stimulation. The samples were separated by SDS-PAGE, transferred to nitrocellulose, and exposed to x-ray film (Autoradiogram). B, phosphopeptide mapping analysis of bands from A. + and - refer to the polarity of the primary electrophoresis dimension in buffer, pH 1.9; vertical arrows indicate direction of liquid chromatography; S signifies origin of sample application. C, quantitation of NIH image analyzed data. Values are means ± S.E. (n = 3).

Fatty Acids Do Not Preferentially Autophosphorylate the C2 Domain-- PKC Apl II also can be stimulated by fatty acids. Autophosphorylation induced by fatty acids can be distinguished from that induced by phorbol esters since removal of the C2 domain greatly decreases fatty acid-induced autophosphorylation without affecting phosphorylation induced by phorbol esters (19). To determine whether this difference is due to selective fatty acid-induced phosphorylation of the C2 domain, we compared PKC that was autophosphorylated in the presence of oleic acid or in the presence of phorbol esters (Fig. 3A). Phosphorylation of phosphopeptides 2 and 3 by oleic acid and PS-PMA was comparable (Fig. 3B). Quantitation of the relative phosphorylation in three separate experiments showed no significant difference between oleic acid and phorbol ester stimulation (Fig. 3C). Thus, the selective requirement of the C2 domain for fatty acid-induced phosphorylation is not due to preferential autophosphorylation of this domain.

Sites in the C2 Domain Can Be Trans-phosphorylated-- Incubation of PKC Apl II or PKC Apl I (data not shown) with fusion proteins containing the C2 domain led to trans-phosphorylation of the C2 domain (Fig. 4A). Phosphopeptide mapping results of both trans-phosphorylated GST- and MBP-C2 domain fusion proteins indicated two major C2 domain phosphorylation sites (Fig. 4, B and C). In contrast, phosphorylation of GST or MBP alone did not generate these sites (data not shown). Coapplication of phosphopeptides derived from autophosphorylated PKC Apl II and the trans-phosphorylated GST-C2 domain fusion protein demonstrated that phosphopeptide 3 was identical in the autophosphorylated kinase and in the trans-phosphorylated C2 domain (Fig. 4D). An additional phosphopeptide (2') was also observed in both fusion proteins, whose migration was slightly altered from phosphopeptide 2 in autophosphorylated PKC Apl II.



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Fig. 4.   C2 domain fusion proteins are transphosphorylated on phosphopeptides 2' and 3. Proteins were phosphorylated, digested, and analyzed as described under "Experimental Procedures." A, GST-C2 and MBP-C2 domain fusion proteins were transphosphorylated by PKC Apl II in the presence of [gamma -32P]ATP. The samples were separated by SDS-PAGE, transferred to nitrocellulose, and exposed to x-ray film (Autoradiogram). B, phosphopeptide mapping analysis of the GST-C2 domain fusion protein in A illustrating that the GST-C2 domain fusion protein yields phosphopeptides 2' and 3 as well another phosphopeptide (see A in panel B) which is also seen after phosphorylation of GST alone (data not shown). C, phosphopeptide mapping analysis of the MBP-C2 domain fusion protein in A indicating that the MBP-C2 domain fusion protein also yields phosphopeptides 2' and 3. D, phosphopeptide analysis of coapplied wild type PKC Apl II and the GST-C2 domain fusion protein illustrating that phosphopeptide 3 is identical in the autophosphorylated kinase and the fusion protein. + and - refer to the polarity of the primary electrophoresis dimension in buffer pH 1.9; vertical arrows indicate direction of liquid chromatography; S signifies origin of sample application.

Site 2 Is Serine 2-- We used a series of C2 domain deletion constructs (19) to attempt to delineate the sites of trans-phosphorylation that corresponded to the various phosphopeptides. However, deleting any area of the C2 domain prevented phosphorylation of peptide 3 suggesting that phosphorylation of this site is sensitive to conformation of the C2 domain (data not shown). In contrast, the site that produced phosphopeptide 2' was removed by an N-terminal deletion but not a C-terminal deletion (data not shown). If site 2 was at the N terminus of the C2 domain, the tryptic peptide is predicted to be altered by addition of two amino acids from the linker region of the fusion protein (MSR right-arrow ASMSR) consistent with the change from site 2 to the new site 2'. An N-terminal location would also be consistent with the loss of phosphopeptide 2' from the C2 domain by the partial tryptic digestion (Fig. 2C, lower panel). Indeed, site 2 was not observed when serine 2 was mutated to alanine in the MBP-C2 domain fusion protein (data not shown).

The Major Autophosphorylation Site of PKC Apl II Is Serine 36-- Phosphoamino acid analysis of phosphopeptides 2, 3, and 5 revealed them all to be serines (data not shown). By using a hypothetical phosphopeptide map of regulatory domain tryptic peptides, and assuming phosphopeptide 2 is M(pS)R, there were only two possible serines (serine 36 and serine 68) that were consistent with the migration of phosphopeptide 3 (Fig. 5A). Conversion of serine 68 to alanine did not affect peptide 3 phosphorylation (data not shown). In contrast conversion of serine 36 to alanine prevented peptide 3 phosphorylation in both the trans-phosphorylated fusion protein (Fig. 5, B-D) and the intact kinase (Fig. 5, E-G).



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Fig. 5.   Serine 36 is the primary phosphorylated residue in the C2 domain of PKC Apl II. A, hypothetical phosphopeptide mapping of the regulatory domain of PKC Apl II identifies probable peptide 3. The regulatory region of PKC Apl II was divided into constituent tryptic peptides and their mass/charge ratio calculated based on singular phosphorylations. The relative hydrophobicity of each peptide was then calculated in the phospho-chromatography buffer (36). The resulting values for regulatory domain peptides (black circles), C2 domain-specific peptides (gray circles), and C2 domain peptide TTTK (white circle) were plotted against each other to generate a phosphopeptide "map" where the location of each peptide is relative. B-D, the residue within peptide 3 responsible for its heavy phosphorylation is serine 36. Proteins were phosphorylated, digested, and analyzed as described under "Experimental Procedures." B, phosphopeptide analysis of the wild type (wt) MBP-C2 domain. C, phosphopeptide analysis of the MBP-C2 domain fusion protein with a Ser-36 right-arrow Ala mutation (MBP-C2 S36A). D, phosphopeptide analysis of coapplied wild type MBP-C2 domain and MBP-C2 S36A. E-G, PKC Apl II autophosphorylates at serine 36. E, phosphopeptide analysis of wild type PKC Apl II. F, phosphopeptide map of the mutant PKC Apl II containing the Ser-36 right-arrow Ala mutation (PKC Apl II S36A). G, phosphopeptide map of coapplied PKC Apl II wild type and PKC Apl II S36A. + and - refer to the polarity of the primary electrophoresis dimension in buffer pH 1.9; vertical arrows indicate direction of liquid chromatography; S signifies origin of sample application or coapplication.

C2 Domain Phosphorylation at Serine 36 Promotes Lipid Binding-- The C2 domain of PKC Apl II does not bind to phosphatidylserine membrane preparations using vesicles (19), lipid micelles (13), or extruded sucrose-loaded vesicles (Fig. 6A; quantitated in Fig. 6B). In contrast, the C2 domain showed significant binding to extruded sucrose-loaded vesicles (60% PS, 40% PC) after trans-phosphorylation by PKC Apl II (Fig. 6A; quantitated in Fig. 6B). This result was also observed using PS vesicles (data not shown). In these experiments less than 5% of the fusion protein was phosphorylated (see "Experimental Procedures"), and thus phosphorylated protein did not contribute significantly to the measured translocation of total fusion protein. The binding was reduced if the vesicles contained only PC (Fig. 6A; quantitated in Fig. 6B). Conversion of serine 36 to alanine significantly decreased binding of the phosphorylated fusion protein to the lipid vesicles (Fig. 6A; quantitated in Fig. 6B), whereas conversion of serine 68 to alanine did not decrease binding (data not shown). In contrast, conversion of serine 36 to glutamic acid significantly increased binding of the fusion protein to lipids, even in the absence of phosphorylation. These results suggest that phosphorylation of serine 36 increased lipid binding. Phosphorylation of serine 2 may also be involved in binding since the phosphorylated form of both the S36E and S36A fusion proteins bound lipids better than did their nonphosphorylated form (Fig. 6A, quantitated in Fig. 6B).



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Fig. 6.   Sucrose-loaded lipid vesicle assay for C2 domain membrane binding. Proteins were phosphorylated on beads, washed, eluted, precentrifuged to remove aggregates, and then incubated with sucrose-loaded vesicles as described under "Experimental Procedures." A, purified MBP-Apl II C2 (WT), MBP-Apl II C2 with serine 36 converted to alanine (S36-A), or MBP-Apl II C2 with serine 36 converted to glutamic acid (S36-E) were incubated with sucrose-loaded vesicles (20 µM lipid) consisting of either 60% PS, 40% PC (PS/PC) or 100% PC (PC) for 10 min at 15 °C. The sucrose vesicles were subsequently sedimented in a Beckman TLA-100 ultracentrifuge at 100,000 × g for 30 min, and the supernatant (S) and pellet (P) fractions were separated and analyzed by PAGE and membrane transfer. Total protein was visualized by Ponceau-S staining (bottom gel), whereas phosphorylated protein was measured by autoradiography (top gel). Although very little of the nonphosphorylated wild type fusion protein domain is sedimented, a considerable amount of the phosphorylated protein does sediment. The serine 36 to alanine mutation reduced sedimentation of the phosphorylated protein significantly, whereas converting serine 36 to glutamic acid increased sedimentation of the nonphosphorylated protein. B, graphic illustration of quantitated results from experiments similar to those in A. Data are displayed as the percentage of total protein found in the bound (P) fraction for both total protein (T, white bars) and phosphorylated protein (black bars). Values are means ± S.E. (n = 6).

The conversion of serine 36 to glutamic acid caused a small shift in the position of the protein on SDS-PAGE gels (Fig. 6A). This band comigrated with a phosphorylated form of the wild type fusion protein (Fig. 6A). The form of the fusion protein migrating at this position bound better to the lipid vesicles than did the lower band (Fig. 6A). These results suggest that phosphorylation caused a conformational change involved in lipid binding. However, phosphorylation was neither necessary nor sufficient to cause the shift, since (i) phosphorylated wild type protein incubated with PC vesicles alone rarely exhibited the shift in molecular weight (Fig. 6A) and (ii) in experiments using higher concentrations of fusion proteins and sucrose-loaded vesicles, the shifted band was seen in the nonphosphorylated wild type protein and even in the nonphosphorylated S36A fusion protein (data not shown). These results are consistent with a model whereby a conformational shift is required for lipid binding, and phosphorylation of the fusion protein enhances the stability of this conformation.

Conversion of Serine 36 to Alanine or Glutamic Acid Does Not Affect Enzyme Activation-- Removal of the C2 domain allows kinase activation at lower concentrations of PS using the mixed micelle assay. To determine whether mutations at serine 36 could mimic this effect, we assayed PKC Apl II S36A and S36E and wild type PKC Apl II in the mixed micelle assay. No difference was seen in the concentration of PS required for activation of PKC Apl II S36A or S36E compared with the wild type control (Fig. 7). The lack of an effect of S36E suggests that phosphorylation of this site is not important for removing C2 domain inhibition or that the glutamic acid does not mimic phosphorylation of serine 36. Whereas the conversion to glutamic acid does allow for lipid binding of the isolated C2 domain, there may be differences between the phosphorylated residue and the glutamic acid in the context of the whole protein.



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Fig. 7.   Substrate phosphorylation is unaffected by the S36A or S36E mutations. Protein kinase C activity assays were performed as described under "Experimental Procedures." PKC assays were performed for wild type (wt) PKC Apl II (white circles), PKC Apl II S36A (black circles), and PKC Apl II S36E (white squares) illustrating no significant change in phosphatidylserine-dependent substrate phosphorylation in the mutant kinases.

Characterization of a Phosphospecific Antibody to Serine 36-- To examine phosphorylation of serine 36 in cells, we generated a phosphopeptide antibody to serine 36 (phospho-Ser-36). We tested the specificity of the antibody using autophosphorylated, purified PKC Apl II and PKC Apl II S36A (Fig. 8A). Purified PKC Apl II showed some reactivity with the phosphopeptide antibody, and stimulation of PKC Apl II by either PS-PMA or oleic acid resulted in a large increase in immunoreactivity with the antibody (Fig. 8A, upper panel). In contrast, no immunoreactivity was seen with Apl II S36A either before or after stimulation despite the ability of this enzyme to autophosphorylate itself as measured using incorporation of [gamma -32P]ATP (Fig. 8A, middle panel). Thus, this antibody was specific for phosphorylation of serine 36. 



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Fig. 8.   Serine 36 is phosphorylated in vivo and is necessary for PKC membrane translocation. Proteins were phosphorylated and kinase assays performed as described under "Experimental Procedures." A, purified wild type (wt) PKC Apl II and PKC Apl II S36A were autophosphorylated in vitro. Enzymes were stimulated by no activators (BL), 50 µg/ml dioleoyl phosphatidylserine and 20 nM PMA (PS/TPA), or 20 µM oleic acid (Oleic) in the absence (-) or presence (+) of 50 µM ATP and [gamma -32P]ATP. A, upper panel, immunoblot using the phospho-Ser-36 antibody illustrating the increase in immunoreactivity with PS/PMA and oleic acid stimulation of the wild type PKC that is absent in the mutant, PKC Apl II S36A. A, middle panel, autoradiogram of the upper panel illustrating an increase in 32P incorporation for the stimulated wild type PKC that parallels that seen in the anti-phospho-Ser-36 Western blot. A, lower panel, immunoblot of the upper panel using the PKC Apl II antibody indicating that approximately equal protein is loaded in each lane and between PKC constructs. B, cells were fractionated as described under "Experimental Procedures." Anti-PKC Apl II immunoblot of fractionated Sf-21 cells infected with baculovirus coding for wild type PKC Apl II (1st to 4th lanes) and PKC Apl II S36A (5th to 8th lanes) after treatment in the absence (-) or presence (+) of 4-beta -PDBu. C, anti-phospho-Ser-36 immunoblot of the experiment in B illustrating serine 36 phosphorylation in vivo of only wild type PKC Apl II and the preferential PDBu-induced membrane translocation of serine 36-phosphorylated PKC.

Phosphorylation of Serine 36 in Cells-- The phosphopeptide antibody to serine 36 recognized PKC Apl II overexpressed in Sf21 cells (Fig. 8B). Immunoreactivity was specific for phosphorylated proteins as no immunoreactivity is seen when PKC Apl II S36A was expressed to the same levels (Fig. 8, B and C). Immunoreactivity increased after addition of PDBu to the cells (150 ± 30%, n = 3, S.E.), consistent with serine 36 being autophosphorylated in cells (Fig. 8B). PDBu also translocated serine 36-phosphorylated PKC (Fig. 8B). The relative percent translocation of serine 36-phosphorylated PKC was increased compared with total PKC Apl II (690 ± 300% compared with 90 ± 30%, n = 3, S.E.), consistent with a role for phosphorylation in translocation. However, this large increase in percentage translocation is probably also related to a pool of misfolded PKC after overexpression in SF21 cells. Misfolded PKC would neither translocate nor be autophosphorylated at serine 36, thus decreasing the relative translocation of the nonphosphorylated pool of PKC Apl II. Phosphorylation was not sufficient for translocation, since in the absence of PDBu phosphorylated protein was found mainly in the supernatant. Similarly, the distribution of Apl II S36E was not different than that of the wild type enzyme (data not shown), and translocation of Apl II S36E was similar to wild type PKC Apl II (60 ± 18%, n = 3, S.E.). In contrast, the relative percent translocation of PKC Apl II S36A was impaired compared with wild type PKC Apl II (20 ± 20% compared with 90 ± 30%, n = 3, S.E.), suggesting that phosphorylation of the wild type protein is required for proper translocation of PKC. Thus, even though only a small percentage of wild type enzyme is phosphorylated at any one point in time, a larger percentage of the translocated wild type protein may have been assisted in translocation by transient phosphorylation, and this would lead to an increased translocation of wild type protein compared with the Ser right-arrow Ala mutation.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Autophosphorylation of PKC Apl II-- A major site for autophosphorylation in PKC Apl II is serine 36 in the C2 domain, and PKC Apl II is probably also autophosphorylated at serine 2 in the C2 domain. Although these autophosphorylations are likely due to cis-autophosphorylation (initial studies suggest single order kinetics), unlike many PKC phosphorylations, serines 2 and 36 can be phosphorylated in trans. Furthermore, serine 36 is contained in a consensus PKC phosphorylation site (Fig. 9A). At this time, we do not know whether serine 2 and serine 36 are cis- or trans-phosphorylated in cells. The site was trans-phosphorylated by PKC Apl I in vitro; however, we did not see phosphorylation of a kinase-dead mutant of PKC Apl II when coexpressed in Sf21 cells with PKC Apl I (data not shown).



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Fig. 9.   Sequence alignment of novel C2 domains and model of phosphorylation-induced lipid binding. A, comparison of the C2 domains of PKC Apl II and novel vertebrate PKCs. Loop positions are based on those described previously (7, 41). Shaded residues are conserved in all isoforms. Darkly shaded residues represent known phosphorylation sites in PKC Apl II (serine 2 and 36) and phosphorylatable residues in loop 1 of C2 domains of other novel PKCs. Sites of the Rack inhibitory peptide and pseudo-Rack peptide are from Ref. 16. B, model of phosphorylation-induced lipid binding. B, left panel, a hypothetical representation of the C2 domain of PKC Apl II with a positively charged lipid binding surface on loop 1 whose access is restricted by the position of loop 3. B, right panel, phosphorylation of serine 36 in the putative alpha -helix of loop 1 shifts the position of loop three to expose the lipid binding surface on loop 1. C2 domain structure adapted from Ref. 41.

The autonomous kinase was not autophosphorylated at peptide 4. We have not directly determined the sequence of peptide 4, but based on partial tryptic digests it is likely to be in the regulatory domain. Furthermore, based on predicted tryptic phosphopeptide mobilities, both peptides 4 and 5 are in the hinge domain (Fig. 5A). It seems unlikely that phosphorylation in the hinge domain would be sufficient to produce an autonomous kinase, and thus we favor a model for autonomous kinase formation where a conformational change in the regulatory region no longer presents the site in peptide 4 for autophosphorylation. This is consistent with experiments using proteolysis as an assay for hinge domain conformation that found discrete constraints on sensitivity of proteolytic sites in the hinge domain. These constraints changed with conformational changes of the whole enzyme (38). We could consider this as additional evidence that autonomous enzyme formation is a result of conformational changes in PKC Apl II.

Mechanistic Model for C2 Domain Phosphorylation-- The C2 domains of nPKCs contain an extended region in what would be the calcium binding region loop 1 as defined in cPKCs. In PKCdelta this region forms an alpha -helix (40), but there is little sequence conservation in this region in the epsilon /eta family (7), and without a crystal structure of an epsilon -like C2 domain the organization of the loops is still speculative. Serine 36 is contained in the extended C-terminal region of loop 1 (Fig. 9A). Phosphorylation of serine 36 increases in vitro lipid binding and cellular translocation of PKC Apl II. However, since phosphorylation increases negative charge, it would not be expected to increase binding to acidic lipids by electrostatic interactions directly. We propose a model (Fig. 9B) where phosphorylation of this residue leads to a conformational shift in the loops of the C2 domain that expose a cryptic lipid-binding site. The N-terminal portion of loop 1 is highly conserved in PKCepsilon -like PKCs and contains a peptide used as a specific inhibitor of PKCepsilon binding to RACK (14-16; Fig. 9A). This region might act as the cryptic lipid binding/RACK-binding domain for these nPKCs. In contrast, the extended region of the loop that contains serine 36 is not as well conserved. However, all isoforms contain a phosphorylatable site in this region (Fig. 9A), and PKCepsilon contains at least one autophosphorylation site in the C2 domain.2

This hypothesis is consistent with earlier results measuring lipid binding to C2 domain deletion constructs of PKC Apl II. In these studies, removal of the C terminus of the C2 domain allows for lipid binding, whereas removal of the N terminus of the C2 domain (containing the phosphorylation site and proposed lipid-binding site) does not (19). This suggests that the N-terminal region of the C2 domain contains a site for lipid binding that is normally inhibited by the C-terminal of the C2 domain. A model for the actions of the PKCepsilon -activating peptide also predicts intra-C2 domain interactions (16). This peptide leads to increased isoform-specific membrane translocation of PKCepsilon (16). The peptide is made from a conserved sequence around loop 3 (Fig. 9A) and is believed to interact with loop 1 to increase access of PKCepsilon to RACKS (16). We suggest that phosphorylation of the C2 domain serves the same purpose as the peptide, inhibiting intra-loop interactions to expose a cryptic lipid or RACK-binding site. Indeed loop 3 is negatively charged suggesting that introducing a negative charge in loop 1 would inhibit loop 1-loop 3 interactions. Intra-C2 domain interactions have also been shown to be important in regulating the C2-B domain of synaptotagmin (39). Different synaptotagmin isoforms show distinct abilities to bind to inositol polyphosphates through a region in the C2 domain. However, differences in binding are not due to the actual inositol polyphosphate binding sequence, which is well conserved in all isoforms. Instead isoform-specific differences map to the C terminus of the C2 domain where some isoforms have residues that interact with the inositol polyphosphate binding domain and inhibit binding, whereas other isoforms lack these residues and exhibit binding (39). Deletion of the C terminus of the C2 domain of synaptotagmin allows inositol polyphosphate binding to all the isoforms (39).

Role of C2 Domain Phosphorylation in Translocation by PDBu-- Phorbol esters translocate PKC Apl II to the membrane in cells, and this translocation may be partially dependent on C2 domain phosphorylation at serine 36. Although one might expect PDBu-mediated translocation to depend only on the C1 domain, mutations in the C2 domain of cPKCs can decrease PDBu-mediated translocation, suggesting that both domains are required for translocation (11, 42). Moreover, the C2 domain is required for translocation of cPKCs by natural stimuli (43). Since there are few differences in lipid and/or phorbol ester-binding between the C1 domains of cPKCs and nPKCs (13), it is likely that the C2 domain is also required for nPKC translocation in vivo. Deletions in the C2 domain can block PDBu binding, and the presence of the C2 domain decreases the affinity of the C1 domain for PDBu in a PS-dependent fashion (44, 45). The phosphorylation at serine 36 may not only increase lipid binding to the C2 domain but decrease C2 domain-mediated inhibition of the C1 domain. However, whereas conversion of serine 36 to glutamic acid was sufficient to increase binding of the C2 domain to lipids, it did not appear to decrease C2 domain-mediated inhibition of the C1 domain in kinase assays and did not have a dramatic effect in the translocation of PKC. The conformational change in C2 domain that allows binding to lipid may not affect the C2-C1 domain interaction. Alternatively, the conformations may not be identical in the phosphorylated protein and the S36E fusion protein. Thus, whereas S36E is sufficient to induce a lipid binding conformation, it is not sufficient to remove the C2-C1 domain interaction. Future work will be needed to address this issue.

It has also been demonstrated that the C1 and C2 domains work in a concerted fashion to facilitate prolonged activation of cPKCs (10, 11, 20, 42). The transient translocation of PKC is mediated by the binding of the C2 domain of the soluble kinase to the membrane in the presence of Ca2+ ions (11). However, a more stable and prolonged translocation was associated with the DAG binding to the C1 domain in the presence of C2 domain binding. Thus, there exist two distinct states of cPKC membrane association as follows: a low affinity state mediated by the C2 domain alone and a high affinity state mediated by both the C1 and C2 domains acting together. We propose that where calcium recruits the aid of conventional C2 domains to translocate cPKCs, phosphorylation may recruit the aid of novel C2 domains to bind lipids and perpetuate PKC membrane association (Fig. 10). This requirement of the C2 domain to perpetuate PKC membrane association would act to help rather than hinder kinase activity and may indeed be a mechanism for persistent kinase activation.



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Fig. 10.   Model of the role for C2 domain phosphorylation in novel PKC membrane translocation and activation. A, fully mature PKC Apl II (phosphorylated on its activation loop Thr-561 by PDK1 and autophosphorylated on its two C-terminal residues resides in the cytosol awaiting activation. The pseudosubstrate (PS) is occupying the catalytic pocket, and the C2 domain restricts activator binding to the C1 domain. B, PKC Apl II can become activated through production of DAG by PLCgamma or PLCbeta and high levels of phosphatidylserine binding to its C1 domain. Solely the C1 domain of PKC Apl II mediates this membrane translocation and as a result its membrane affinity would be low and lead to only transient kinase activation. C, alternatively, PKC Apl II can become autophosphorylated (in cis or perhaps in trans) on serine 36 in loop 1 of its C2 domain. D, this phosphorylation may expose a cryptic C2 domain lipid binding site allowing phosphatidylserine binding, and now both the C1 and C2 domains are responsible for recruiting the kinase to the membrane. This C1- and C2-mediated activation produces a high membrane affinity and may be responsible for persistent activation of novel PKCs like PKC Apl II.



    ACKNOWLEDGEMENT

We thank Dr. Peter McPherson for helpful comments on the manuscript.


    FOOTNOTES

* This work was supported in part by Grant MT-12046 from the Medical Research Council of Canada.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Dagger Recipient of a Medical Research Council of Canada Studentship.

§ Recipient of a Chercheur-Boursier from the Fonds de la Recherche en Santé du Québec. To whom correspondence be addressed: Dept. of Neurology and Neurosurgery, McGill University, Montreal Neurological Institute, Rm. 776, 3801 Rue University, Montreal, Quebec H3A 2B4, Canada. Tel.: 1-514-398-1486; Fax: 1-514-398-8106; E-mail: mdws@musica.mcgill.ca.

Published, JBC Papers in Press, November 9, 2000, DOI 10.1074/jbc.M006339200

2 A. M. Pepio and W. Sossin, unpublished data.


    ABBREVIATIONS

The abbreviations used are: PKC, protein kinase C; cPKC, classical PKCs; nPKC, novel PKC; PS, phosphatidylserine, PC, phosphatidylcholine; pfu, plaque-forming units; MBP, maltose-binding protein; GST, glutathione S-transferase; TPCK, N-tosyl-L-phenylalanine chloromethyl ketone-treated trypsin; PDBu, phorbol dibutyrate; PMA, phorbol 12-myristate 13-acetate; RACK, receptor for activated protein kinase C; PCR, polymerase chain reaction; O5, outside 5' primer; I3, inside 3' primer; I5, inside 5' primer; O3, outside 3' primer; DAG, diacylglycerol.


    REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES


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