A p90rsk Mutant Constitutively Interacting with MAP Kinase Uncouples MAP Kinase from p34cdc2/Cyclin B Activation in Xenopus Oocytes

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Vol. 10, Issue 9, 2971-2986, September 1999

A p90^rsk Mutant Constitutively Interacting with MAP Kinase Uncouples MAP Kinase from p34^cdc2/Cyclin B Activation in Xenopus Oocytes

Anne-Claude Gavin, Aine Ni Ainle, Emanuele Chierici, Margaret Jones, and Angel R. Nebreda^*

European Molecular Biology Laboratory, 69117 Heidelberg, Germany

Submitted April 21, 1999; Accepted July 7, 1999
Monitoring Editor: Marc W. Kirschner

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

The efficient activation of p90^rsk by MAP kinase requires their interaction through a docking site located at the C-terminalend of p90^rsk. The MAP kinase p42^mpk1 can associate with p90^rsk in G₂-arrested but not in mature Xenopus oocytes. In contrast,an N-terminally truncated p90^rsk mutant named D2 constitutively interacts with p42^mpk1. In this report we show that expression of D2 inhibits Xenopusoocyte maturation. The inhibition requires the p42^mpk1 docking site. D2 expression uncouples the activation of p42^mpk1 and p34^cdc2/cyclin B in response to progesterone but does not prevent signalingthrough p90^rsk. Instead, D2 interferes with a p42^mpk1-triggered pathway, which regulates the phosphorylation and activationof Plx1, a potential activator of the Cdc25 phosphatase. Thisnew pathway that links the activation of p42^mpk1 and Plx1 during oocyte maturation is independent of p34^cdc2/cyclin B activity but requires protein synthesis. Using D2, wealso provide evidence that the sustained activation of p42^mpk1 can trigger nuclear migration in oocytes. Our results indicatethat D2 is a useful tool to study MAP kinase function(s) duringoocyte maturation. Truncated substrates such as D2, which constitutivelyinteract with MAP kinases, may also be helpful to study signaltransduction by MAP kinases in other cellularprocesses.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Xenopus oocytes are naturally arrested in prophase (late G₂) of the first meiotic division and are induced to reinitiate meiosisand enter M-phase by progesterone stimulation. This process iscalled meiotic maturation and is associated with dramatic structuralchanges in the oocyte. During maturation the nucleus migratesto the cortex of the oocyte, and the nuclear membrane disappears(this is known as germinal vesicle breakdown [GVBD]) concomitantwith the appearance of a white spot at the animal pole of theoocyte. The chromosomes also condense and a metaphase spindleassembles. The meiotic maturation is associated with the activationof the ubiquitous M-phase- or maturation-promoting factor (MPF)(Masui and Markert, 1971; Masui and Clarke, 1979), which is requiredfor the initiation of mitosis and is also likely to be responsiblefor most of the structural changes associated with the progressionthrough M-phase. MPF is a heterodimer of a B-type cyclin and thep34^cdc2 protein kinase (reviewed by Nurse, 1990).

An essential requirement for progesterone-induced meiotic reinitiation is the translation of dormant maternal mRNAs storedin the oocyte. De novo synthesis of several proteins takes placeduring oocyte maturation (Sagata et al., 1988; Nebreda et al.,1995; Barkoff et al., 1998), one of them being the Mos proteinkinase (Sagata et al., 1988, 1989; Freeman et al., 1990; Sheetset al., 1995). Mos is an efficient activator of the MAP kinasepathway (Nebreda et al., 1993a; Nebreda and Hunt, 1993; Posadaet al., 1993; Shibuya and Ruderman, 1993), and several lines ofevidence indicate that the activation of the Xenopus MAP kinasep42^mpk1 (which is most similar to the mammalian ERK1/ERK2 MAP kinases)is required for meiotic reinitiation and p34^cdc2/cyclin B activation (reviewed by Kosako et al., 1994a; Gotohand Nishida, 1995). For example, injection of inhibitory anti-MAPkinase kinase antibodies (Kosako et al., 1994b, 1996) or a specificMAP kinase phosphatase (Gotoh et al., 1995) inhibits meiotic reinitiation.On the other hand, injection of constitutively active MAP kinasekinase or thio-phosphorylated p42^mpk1 induces meiotic reinitiation in the absence of progesterone (Matsudaet al., 1992; Haccard et al., 1995; Huang et al., 1995). It hasalso been reported that MPF can trigger p42^mpk1 activation, suggesting the existence of a positive feedback loopthat links the activation of p42^mpk1 and MPF (Gotoh et al., 1991; Matsuda et al., 1992). This mayexplain why the activation of p42^mpk1 and MPF is coupled in progesterone-treated oocytes (Ferrell andMachleder, 1998). A positive feedback loop has also been describedbetween p42^mpk1 and the synthesis and/or stability of Mos (Matten et al., 1996;Roy et al., 1996; Howard et al., 1999).

G₂-arrested oocytes contain a stockpile of p34^cdc2/cyclin B complexes, which are inactivated by the phosphorylation of p34^cdc2 on Thr-14 and Tyr-15 (Cyert and Kirschner, 1988; Gautier andMaller, 1991; Kobayashi et al., 1991). The kinase responsiblefor these inhibitory phosphorylations in oocytes is most likelyto be Myt1, a membrane-associated member of the Wee1 protein kinasefamily (Atherton-Fessler et al., 1994; Kornbluth et al., 1994;Mueller et al., 1995; Palmer et al., 1998). The dephosphorylationof p34^cdc2 at the onset of M-phase is triggered by the activation of thephosphatase Cdc25 (Dunphy and Kumagai, 1991; Gautier et al., 1991;Kumagai and Dunphy, 1991; Strausfeld et al., 1991). In G₂-arrestedoocytes, Cdc25 is maintained inactive by Chk1 phosphorylationand association with 14-3-3 proteins (Nakajo et al., 1999). Theactivation of the p34^cdc2/cyclin B complexes in progesterone-treated oocytes may be broughtabout by Myt1 inhibition and/or Cdc25 activation. Myt1 and Cdc25are both hyperphosphorylated in mature oocytes as in M-phase-arrestedextracts, and this correlates with the inhibition of Myt1 andthe activation of Cdc25 (Izumi et al., 1992; Kumagai and Dunphy,1992; Mueller et al., 1995; Booher et al., 1997; Palmer et al.,1998). Both proteins can be phosphorylated by p34^cdc2/cyclin B complexes in vitro (Hoffmann et al., 1993; Izumi andMaller, 1993; Strausfeld et al., 1994; Booher et al., 1997; Palmeret al., 1998), and in the case of Cdc25 this phosphorylation up-regulatesits phosphatase activity (Hoffmann et al., 1993; Izumi and Maller,1993; Strausfeld et al., 1994). The ability of MPF to regulateCdc25 (and potentially Myt1) constitutes a positive feedback loop,the so-called MPF autoamplification process, by which a smallamount of active p34^cdc2/cyclin B would be able to trigger the activation of more p34^cdc2/cyclin B from the stored pre-MPF complexes (Masui and Markert,1971). However, p34^cdc2/cyclin B is unlikely to be the triggering kinase that phosphorylatesMyt1 and Cdc25 during oocyte maturation. We have recently foundthat the C-terminal regulatory domain of Myt1 can be efficientlyphosphorylated by the p42^mpk1-activated protein kinase p90^rsk. Moreover, phosphorylation by p90^rsk decreases the inhibitory activity of Myt1 on p34^cdc2/cyclin B complexes in vitro, thereby providing a potential linkbetween p42^mpk1 and MPF activation at the onset of meiotic maturation (Palmeret al., 1998). On the other hand, p90^rsk does not phosphorylate the N-terminal regulatory domain of Cdc25(Palmer et al., 1998), but this is efficiently phosphorylatedby the Polo-like kinase of Xenopus Plx1 (Kumagai and Dunphy, 1996).Plx1 phosphorylation can activate Cdc25 in vitro, suggesting thatPlx1 may be one of the triggering kinases responsible for thephosphorylation and activation of Cdc25 at the onset of M-phase(Kumagai and Dunphy, 1996; Qian et al., 1998a). A protein kinasethat can phosphorylate and activate Plx1 has been recently purifiedand cloned from Xenopus eggs and named xPlkk1 (Qian et al., 1998b).

p90^rsk contains two protein kinase domains (Jones et al., 1988): the N-terminal domain (D1) is required for the phosphorylationof exogenous substrates, and the C-terminal domain (D2) is involvedin p90^rsk autophosphorylation (Bjørbaek et al., 1995; Leighton et al.,1995; Fischer and Blenis, 1996). Association between p90^rsk family members and ERK MAP kinases has been detected in variouscell types, including Xenopus oocytes, mammalian fibroblasts,and PC12 cells (Scimeca et al., 1992; Hsiao et al., 1994; Zhaoet al., 1996). In G₂-arrested Xenopus oocytes the unphosphorylatedand inactive p90^rsk is complexed with inactive p42^mpk1, but the complex dissociates during oocyte maturation concomitantwith the phosphorylation and activation of both protein kinases(Hsiao et al., 1994).

There is growing evidence that the efficient phosphorylation of some substrates requires specific sequences, which facilitatethe kinase-substrate interaction and are distinct from the phosphoacceptorsites_. These sequences, usually referred to as docking sites,were first described to be important for the phosphorylation ofthe transcription factor c-jun by JNK/MAP kinases (Kallunki etal., 1994). Docking sites have been later identified on Smadsphosphorylated by transforming growth factor- $beta$ receptors (Chenet al., 1998; Lo et al., 1998), on some cdk2/cyclin A substrates(Adams et al., 1996; Schulman et al., 1998), and on the transcriptionfactor Elk-1 (Yang et al., 1998a,b; Jacobs et al., 1999). Theinteraction between Elk-1 and activating ERK, JNK, and p38 MAPkinases appears to involve several distinct and overlapping interactionmotifs, which have been suggested to work either synergisticallyor competitively (Jacobs et al., 1999). We and others have alsorecently characterized a novel MAP kinase docking site locatedat the C terminus of p90^rsk, which is required for the efficient phosphorylation and activationof p90^rsk both in vitro and in vivo (Gavin and Nebreda, 1999; Smith etal., 1999). This docking site is specific for ERK MAP kinasesand shows no amino acid sequence similarity with other MAP kinasedocking sites, suggesting that it may represent the prototypeof a novel ERK MAP kinase interactionmotif.

In this report we use an N-terminally truncated form of p90^rsk named D2, which constitutively interacts with p42^mpk1, to investigate the function(s) of p42^mpk1 during oocyte maturation. Our results indicate that activationof p42^mpk1 normally precedes the activation of pre-MPF in progesterone-treatedoocytes. We also found that p42^mpk1 can trigger an MPF-independent pathway that leads to the activationof Plx1 and that the activation of p42^mpk1 in the absence of pre-MPF activation can trigger nuclear migrationin Xenopusoocytes.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

cDNA Cloning and Site-directed Mutagenesis

Full-length Xenopus p90^rsk $alpha$ and the N-terminal (D1, amino acids 1-308) and C-terminal (D2, amino acids 309-733) domains alonewere cloned in the FTX5 expression vector as described (Palmeret al., 1998). The mutants D2/KR (Lys-445 changed to Arg), D2 $Delta$ 43(stop codon following amino acid 690), and p90^rsk 6xAla (phosphorylation sites at positions Ser-221, Thr-359, Ser-363,Ser-380, Thr-571, and Ser-730 changed to Ala) were prepared usingthe QuikChange site-directed mutagenesis kit (Stratagene, La Jolla,CA) according to the manufacturer's instructions. To prepare D1+43Ct,the C-terminal 43 amino acids of p90^rsk were amplified using a 5' oligonucleotide that introduced anNcoI site at position 2069 of p90^rsk (Lys-691 was changed to Met) and a 3' oligonucleotide that introduceda BamHI site downstream of the stop codon. The PCR product wasdigested with NcoI and BamHI and subcloned into the correspondingsites of the plasmid FTX5. The resulting plasmid FTX5-43Ct waslinearized with NcoI and ligated to the NcoI-NcoI D1 fragmentfrom FXT5-D1.

FTX5-p42^mpk1 was prepared by subcloning a PCR fragment containing the p42^mpk1 coding sequence from pMalcRI-p42^mpk1 (Rouse et al., 1994) into FTX5 previously digested with BamHIand XhoI. The mutant p42^mpk1 AEF (Thr-187 and Tyr-189 changed to Ala and Phe, respectively)was prepared using the QuikChange site directed mutagenesis kit.FTX5-Mos was prepared by subcloning a 1.2-kb NcoI-XhoI DNA fragmentcontaining the full-length Xenopus c-mos protooncogene from MLV-Mos(Nebreda et al., 1993a) into NcoI-XhoI digestedFTX5.

Xp9 was amplified from a Xenopus oocyte cDNA library using oligonucleotides that created EcoRI sites both upstream of thefirst ATG and downstream of the stop codon. A PCR product withthe same sequence as the cDNA described by Patra and Dunphy (1996)was cloned into EcoRI-digestedFTX5.

Oocyte Maturation and Expression of myc-tagged Proteins

In vitro-transcribed mRNAs were obtained from FTX5 constructs linearized with either XbaI (p90^rsk, D1, D2, Mos, and Xp9) or XmnI (p42^mpk1) using the MEGAscript kit (Ambion, Austin, TX) according to themanufacturer's instructions. The mRNAs were resuspended in 25µl of diethylpyrocarbonate-treated water and further diluted 1:5in diethylpyrocarbonate-treated water beforemicroinjection.

Fully grown oocytes were sorted either manually or after collagenase B treatment (Boehringer Mannheim, Indianapolis, IN; 0.5mg/ml, 30-60 min) and left at 18°C in mBarth for at least 2 hbefore injection. Meiotic maturation was induced by incubationwith 5 µg/ml progesterone (Sigma, St. Louis, MO) or by injectionwith 50 nl of either malE-mos protein (40 ng, Nebreda and Hunt,1993) or Mos mRNA. Maturation was scored by the appearance ofa white spot at the animal pole of the oocyte, and GVBD was confirmedafter either fixation in 5% trichloroacetic acid or by boilingfor 90 s inPBS.

The oocytes were lysed in 10 µl per oocyte histone H1 kinase (H1K) buffer (80 mM $beta$ -glycerophosphate, 20 mM EGTA, 15 mM MgCl₂,2 µg/ml leupeptin, 2 µg/ml aprotinin, 2.5 mM benzamidine, 1 mM4-(2-aminoethyl)-benzenesulfonyl fluoride, and 1 mM DTT, pH 7.4)and centrifuged at 14,000 rpm (Eppendorf centrifuge), and thesupernatant (oocyte lysate) was stored at $-$ 70°C. To prepare concentratedextracts, oocytes were lysed in 1-2 µl per oocyte H1K buffer orlysis buffer (80 mM $beta$ -glycerophosphate, pH 7.4, 10 mM EDTA, 1mM sodium orthovanadate, 2 mM PMSF, 2 µM microcystin, 10 mM p-nitrophenylphosphate,100 µg/ml leupeptin, and 100 µg/ml aprotinin) and clarified bycentrifugation at 14,000 rpm for 90 s. The clear cytoplasm wasremoved from between the overlying lipid layer and the yolk proteinand was further clarified by a second centrifugation at 14,000rpm for 10 min. Concentrated oocyte extracts were stored in aliquotsat $-$ 70°C.

Immunoblotting and Immunoprecipitation

Immunoblotting was performed as previously described (Palmer et al., 1998) using the following antibodies: the monoclonalantibody 3E1 (provided by J. Gannon and T. Hunt, Imperial CancerResearch Fund, South Mimms, United Kingdom) for p34^cdc2 (Nebreda et al., 1995); the rabbit antiserum 3297.1 for p42^mpk1 (Palmer et al., 1998); a mixture of purified anti-Rsk1 and anti-Rsk2goat antibodies (Santa Cruz Biotechnology, Santa Cruz, CA) forp90^rsk; a rabbit anti-Pl×1 antiserum (provided by A. Tavares, C. Avides,and D. Glover, University of Dundee, Dundee, United Kingdom) forPlx1; and the 9E10 monoclonal antibody for myc-taggedproteins.

For the immunoprecipitation of myc-tagged proteins, 10 µl of anti-myc agarose conjugate (Santa Cruz; sc-40 AC) was incubatedwith 70 µl of oocyte lysate for 2 h at 4°C. The beads were thenwashed three times in immunoprecipitation buffer (50 mM Tris,pH 7.5, 150 mM NaCl, 0.5% NP-40, 5 mM EGTA, 5 mM EDTA, 20 mM NaF,100 µM NaVO₄, 1 mM PMSF, 2.5 mM benzamidine, 10 µg/ml leupeptin,10 µg/ml aprotinin, and 2 µM microcystin) and once in S6 kinasebuffer (see below) and immediately used for an in vitro kinaseassay. Coimmunoprecipitation experiments were performed essentiallyas described above, except that 40-70 µl of concentrated oocyteextracts wereused.

For the immunoprecipitation of p42^mpk1, we used an anti-ERK2 antibody conjugated to agarose (Santa Cruz). As a control, we usedpurified rabbit immunoglobulin G (IgG; Sigma) covalently boundto protein A beads using dimethylpimelimidate. Concentrated oocyteextracts (50-100 µl) were precleared with 20 µl of protein A beadsfor 30 min at 4°C and incubated for 2 h at 4°C with the bead-boundantibody. The beads were then washed three times in either H1Kbuffer supplemented with 2 µg/ml microcystin, 4 mM p-nitrophenylphosphate,1 mM PMSF, 10 µg/ml aprotinin, and 10 µg/ml leupeptin or lysisbuffer and then used forimmunoblotting.

For the immunoprecipitation of Plx1, 7 µl of oocyte lysate were diluted to 200 µl in buffer B (50 mM Tris, pH 8.0, 0.5% NP-40,120 mM NaCl, 20 mM EDTA, and 1 mM DTT) and mixed with 5 µl ofanti-Plx1 antiserum and 20 µl of protein A-Sepharose beads. After2 h, the beads were washed twice in 10 mM Tris, pH 7.0, 0.1% NP-40,1 M NaCl, and 1 mM DTT, twice in buffer B, and twice in kinasebuffer (20 mM HEPES, pH 7.2, 2 mM DTT, 10 mM MgCl₂, 0.1 mM EGTA,and 0.01% Brij35).

The immunoprecipitation of endogenous p90^rsk was performed as described by Palmer et al. (1998) but using a mixture of both anti-Rsk1and anti-Rsk2 antibodies (SantaCruz).

In Vitro Kinase Assays

Myc-tagged and endogenous p90^rsk immunoprecipitates were assayed for 40 min at room temperature in a final volume of 15 µl ofS6 kinase buffer (50 mM 3-morpholinepropanesulfonic acid, pH 7.2,1 mM DTT, 10 mM MgCl₂, 20 mM p-nitrophenylphosphate, 0.1% TritonX-100, 1 mM NaVO₃, 10 µg/ml leupeptin, 10 µg/ml aprotinin, and1 mM PMSF or 4-(2-aminoethyl)-benzenesulfonyl fluoride) containing100 µM ATP, 5 µCi of [ $gamma$ -³²P]ATP (3000 Ci/mmol) and 0.4 µg of GST-Myt1 Ct (Palmer et al.,1998).

Plx1 immunoprecipitates were incubated for 30 min at 30°C in 15 µl of kinase buffer containing 67 µM ATP, 5 µCi [ $gamma$ -³²P]ATP, and 1 µg/µl dephosphorylated casein(Sigma).

Phosphorylation reactions were analyzed by SDS-PAGE followed by Coomassie staining andautoradiography.

Gel Filtration

Concentrated oocyte extracts were further clarified by centrifugation at 50,000 rpm in a Beckman Instruments (Palo Alto, CA)TLA 100 rotor at 4°C for 1 h. Samples (100 µl) from 100 oocyteswere chromatographed on a Superose 12 column (Pharmacia, Piscataway,NJ; flow rate 0.4 ml/min) equilibrated with lysis buffer containing80 mM $beta$ -glycerophosphate, pH 7.4, 10 mM EDTA, 1 mM sodium orthovanadate,0.1 mM PMSF, 0.2 µM microcystin, 0.5 mM p-nitrophenylphosphate,1 µg/ml leupeptin, and 1 µg/ml aprotinin. Fractions of 100 µlwere collected and analyzed by immunoblotting. The molecular massstandards were aldolase (158 kDa), BSA (67 kDa), ovalbumin (43kDa), chymotrypsinogen A (25 kDa), and ribonuclease (13.7kDa).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

A N-Terminally Truncated Form of p90^rsk Constitutively Interacts with p42^mpk1

In G₂-arrested Xenopus oocytes, p90^rsk and p42^mpk1 are associated in a complex that dissociates upon activation of both kinases (Hsiaoet al., 1994), suggesting that the interaction may be regulatedby the phosphorylation state of either p90^rsk or p42^mpk1 or both. To investigate this possibility, we prepared a p90^rsk mutant with the amino acids that are known to be phosphorylatedupon activation (Dalby et al., 1998), being replaced by nonphosphorylatableAla residues (p90^rsk/6xA). As expected, this mutated p90^rsk was neither hyperphosphorylated nor activated when expressedin progesterone-treated oocytes (Figure 1A, compare lanes 2 and4 in the upper and middle panels). We also prepared a p42^mpk1 mutant in which the sequence TEY in the activation loop was changedto AEF to prevent phosphorylation. The wild-type and mutant formsof both p90^rsk and p42^mpk1 were coexpressed in oocytes, which were either left untreatedor treated with progesterone to induce the activation of the p42^mpk1 pathway and meiotic reinitiation (Figure 1B). The associationbetween p90^rsk and p42^mpk1 was determined by anti-p42^mpk1 immunoprecipitation followed by immunoblotting using an anti-p90^rsk antibody (Figure 1B). The wild-type p42^mpk1 associated with the wild-type p90^rsk only in G₂-arrested oocytes (Figure 1B, lanes 9 and 10). Similarly,p42^mpk1/AEF interacted much more efficiently with the unphosphorylatedthan with the phosphorylated p90^rsk (Figure 1B, lanes 13 and 14), suggesting that the interactionbetween p42^mpk1 and p90^rsk might be regulated by the phosphorylation of p90^rsk. Consistent with this possibility, the nonphosphorylatable mutantp90^rsk/6xA was able to interact with p42^mpk1 both in prophase- and progesterone-treated oocytes (Figure 1B,lanes 11, 12, 15, and 16), indicating that the phosphorylationof p90^rsk is responsible for the dissociation of the p42^mpk1/p90^rsk complex.

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Figure 1. Mutation to alanine of six phosphorylatable residues in p90^rsk impairs its activation by progesterone and its ability to dissociate from p42^mpk1. (A) Lysates were prepared from untreated or progesterone-treated oocytes expressing either myc-tagged p90^rsk or p90^rsk (6xA) and were analyzed by immunoblotting using anti-myc and anti-p42^mpk1, as indicated. Anti-myc immunoprecipitates were prepared from the same oocyte lysates, and their associated kinase activity was assayed using GST-Myt1 as an in vitro substrate. (B) Lysates were prepared from either untreated or progesterone-treated oocytes expressing the indicated p90^rsk and p42^mpk1 proteins and were immunoprecipitated with anti-p42^mpk1 antibodies. The total lysates (lanes 1-8) and the anti-p42^mpk1 immunoprecipitates (lanes 9-16) were analyzed by immunoblotting with anti-p90^rsk and anti-myc antibodies.

We have previously shown that a truncated form of p90^rsk named D2, which lacks the N-terminal kinase domain (Figure 2A), wasable to bind to p42^mpk1. This interaction was mediated by a p42^mpk1 docking site, which was located at the C-terminal 25 amino acidsof p90^rsk (Gavin and Nebreda, 1999). Moreover, both nonphosphorylated andphosphorylated GST-D2 were able to bind p42^mpk1 with similar affinity in pulldown experiments (Gavin and Nebreda,1999). To further characterize the ability of this truncated p90^rsk to interact with p42^mpk1, myc-tagged D2 was expressed in Xenopus oocytes, which were theneither treated with progesterone or left untreated. The associationbetween p42^mpk1 and either p90^rsk or D2 was determined by anti-p42^mpk1 immunoprecipitation followed by immunoblotting using either anti-p90^rsk or anti-myc antibodies (Figure 2B). As expected, p90^rsk was found to coimmunoprecipitate with p42^mpk1 in control oocytes (Figure 2B, lanes 1 and 3) but not in progesterone-treatedoocytes, in which p90^rsk is phosphorylated (Figure 2B, lanes 2 and 4). In contrast, D2associated with p42^mpk1 both in control and in progesterone-treated oocytes (Figure 2B,lanes 3 and 4, anti-myc blot). Moreover, the electrophoretic mobilityof D2 was significantly reduced upon progesterone treatment (Figure2B, lanes 3 and 4), suggesting that it became hyperphosphorylated.This is consistent with previous reports showing that the majorphosphorylation sites for p42^mpk1 map in the C-terminal half of p90^rsk (Dalby et al., 1998).

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Figure 2. The C-terminal D2 domain of p90^rsk constitutively interacts with endogenous p42^mpk1 in oocytes. (A) Schematic representation of full-length p90^rsk indicating the two kinase domains, D1 and D2, the p42^mpk1 docking site located in the last 25 amino acids (25 aa) and the three p42^mpk1 phosphorylation sites (asterisks). The N-terminally truncated p90^rsk protein D2 is also shown. (B) Oocytes injected with water (lanes 1 and 2) or expressing myc-tagged D2 (lanes 3 and 4) were induced to mature by progesterone or not as indicated. Anti-p42^mpk1 immunoprecipitates prepared from the oocyte lysates were analyzed by immunoblotting with anti-p90^rsk, anti-myc and anti-p42^mpk1 antibodies. The unphosphorylated and hyperphosphorylated D2 are indicated as D2 and D2-P, respectively.

We further tested the ability of D2 to interact with p42^mpk1 by gel filtration chromatography. Oocyte lysates were chromatographedon a Superose 12 column, and the fractions were analyzed by immunoblotting(Figure 3). In lysates prepared from G₂-arrested oocytes, p42^mpk1 exhibited a broad size distribution, which, as described by others(Hsiao et al., 1994), may correspond to two overlapping peaksof ~40 and 110 kDa (Figure 3, control/water). After progesteronetreatment, the high-molecular-weight peak of p42^mpk1 disappeared (Figure 3, progesterone/water), consistent with p42^mpk1 being mainly present in its monomeric form (Hsiao et al., 1994).Interestingly, in lysates prepared from D2-expressing oocytes,a significant amount of p42^mpk1 was shifted toward a higher-molecular-weight form, which coelutedwith D2 (Figure 3, control/D2). Moreover, the pattern of elutionof p42^mpk1 (and D2) was not changed by progesterone treatment of the oocytes,despite the hyperphosphorylation of D2 (Figure 3, progesterone/D2).These results confirm that D2 interacts with p42^mpk1 in the oocytes and that, in contrast to full-length p90^rsk, the association between D2 and p42^mpk1 does not appear to be regulated by the phosphorylation stateof D2.

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Figure 3. D2 expressed in oocytes comigrates with endogenous p42^mpk1 in a high-molecular-weight complex upon gel filtration chromatography. Oocytes injected with water or expressing myc-tagged D2 were induced to mature by progesterone or not as indicated. The oocyte lysates were separated by gel filtration chromatography on Superose 12, and the fractions were analyzed by immunoblot using anti-myc and anti-p42^mpk1 antibodies. The elution of the molecular weight markers is indicated at the bottom. The unphosphorylated and hyperphosphorylated D2 are indicated as D2 and D2-P, respectively.

Overexpression of the p42^mpk1 Docking Site Negatively Regulates Oocyte Maturation

The overexpression of the p42^mpk1 docking site located at the C terminus of p90^rsk interferes with the phosphorylation of p90^rsk by p42^mpk1 in reticulocyte lysates (Gavin and Nebreda, 1999). We wantedto investigate whether D2, which contains the p42^mpk1 docking site and constitutively interacted with p42^mpk1, could also inhibit signaling by p42^mpk1 in oocytes. We observed that expression of D2 in oocytes significantlydelayed the kinetics of progesterone-induced maturation (Figure4A). As a control, expression of similar levels of the D1 catalyticdomain alone (Figure 4B) did not affect meiotic reinitiation (Figure4A). Moreover, a catalytically inactive mutant of D2 (D2/KR) wasas efficient as D2 in delaying oocyte maturation (Figure 4A),indicating that the autophosphorylation activity of D2 (Fischerand Blenis, 1996; our unpublished data) was not required for theinhibition of oocyte maturation. The inhibitory effect of D2 wasalso observed when oocyte maturation was induced by the injectionof either Mos mRNA or bacterially produced Mos protein (Figure4C; also see Figure 7A).

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Figure 4. Expression of D2 inhibits oocyte maturation. (A) Groups of 25-30 oocytes were injected with water or mRNAs encoding the indicated proteins and after overnight incubation were treated with progesterone and scored for GVBD. D2 was found to inhibit or delay progesterone-induced maturation in 27 of 34 experiments. (B) Lysates were prepared from the same oocytes as in A after overnight incubation and analyzed by immunoblotting using anti-myc antibodies. (C) Groups of 25-30 oocytes were injected with water or D2 mRNA, incubated overnight, and then either injected with Mos mRNA or incubated with progesterone. GVBD was scored 8 h later.

To investigate whether the inhibitory effect of D2 required the p42^mpk1 docking site, we used a truncated form of D2, which lacks thelast 43 amino acids (Figure 5A, D2 $Delta$ 43) and does not interact withp42^mpk1 (Gavin and Nebreda, 1999). We also used a chimera in which thelast 43 amino acids of p90^rsk have been added to the C terminus of D1 (Figure 5A, D1+43Ct)resulting in a fusion protein that can interact with p42^mpk1 in oocytes (Gavin and Nebreda, 1999). Oocytes were injected witheither water or the mRNAs encoding these proteins and then weretreated with progesterone. We found that truncation of the C-terminal43 amino acids abrogated the inhibitory effect of D2 (Figure 5B,D2 $Delta$ 43). Furthermore, in contrast to D1 alone, which had no effecton progesterone-induced maturation, D1+43Ct also delayed the kineticsof maturation to the same extent as D2 (Figure 5B). These resultsindicate that overexpression of the p42^mpk1 docking site is able to inhibit the meiotic reinitiation in oocytes.

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Figure 5. Expression of the p42^mpk1 docking site is necessary and sufficient to inhibit oocyte maturation. (A) Schematic representation of the recombinant proteins expressed in oocytes. (B) Groups of 25-30 oocytes were injected with water or mRNAs encoding the indicated proteins and after overnight incubation were treated with progesterone and scored for GVBD.

D2 Uncouples the Activation of p42^mpk1 and MPF in Response to Progesterone

The observation that D2 can also interfere with oocyte maturation induced by Mos (Figures 4C) suggested that it might inhibitdownstream of p42^mpk1. To test this possibility, oocytes were injected with eitherwater or the D1 or D2 mRNAs and then treated with progesterone.When the oocytes started to mature (as determined by the appearanceof a white spot), single oocytes were taken and analyzed by immunoblottingwith anti-p42^mpk1 and anti-p34^cdc2 antibodies. The activation of p42^mpk1 was scored based on the upward mobility shift of the p42^mpk1 protein in SDS-PAGE, which correlates with its phosphorylationand the activation of pre-MPF for the disappearance of the slow-migratingp34^cdc2 band, which corresponds to tyrosine-phosphorylated and cyclinB-bound p34^cdc2 (Figure 6). We found that in every progesterone-treated oocytethat had a white spot there was activation of both p42^mpk1 and pre-MPF, independently of whether they had been injectedwith water or the D1 or the D2 mRNAs (Figure 6, A, white spot,and B, ws, show a representative example). When progesterone-treatedoocytes without a white spot were analyzed, we found two categoriesof oocytes from each injection with either water or the D1 mRNA(Figure 6, A, No white spot, and B, No ws): oocytes with neitherp42^mpk1 nor pre-MPF activation, which looked like G2-arrested oocytes(Figure 6, A, control, and B and C) or oocytes with both kinasesin an active state as in oocytes with a white spot (these oocyteswere probably about to undergo maturation when they were collected).This confirmed previous work showing that the activation of p42^mpk1 is always coupled to the activation of preformed p34^cdc2/cyclin B complexes (pre-MPF) in response to progesterone stimulation(Ferrell and Machleder, 1998). Interestingly, when we analyzedsingle progesterone-treated oocytes expressing D2, we found thatabout half of the oocytes without a white spot fell into a thirdcategory in which p42^mpk1 was partially activated (>40% of the p42^mpk1 protein showed reduced electrophoretic mobility), but p34^cdc2 was tyrosine phosphorylated, and thus preMPF was still inactive(Figure 6, A and B, D2).

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Figure 6. Expression of D2 uncouples the activation of p42^mpk1 and pre-MPF in response to progesterone. (A) Groups of 30 oocytes were injected with water or mRNAs encoding either D1 or D2 and after overnight incubation were treated with progesterone. Every hour, starting 3 h after the addition of progesterone, two or three progesterone-treated oocytes without a white spot were transferred to dry ice. Untreated oocytes (control) and progesterone-treated oocytes that had a white spot were also taken for comparison. Oocyte lysates were prepared from single oocytes and analyzed by immunoblotting with anti-p42^mpk1 and anti-p34^cdc2 antibodies. Each bar represents a single oocyte. A total of 30 oocytes were analyzed in three independent experiments. The activation of p42^mpk1 was scored by the phosphorylation of the protein, which causes its upward mobility shift in the blots. The activation of pre-MPF was scored for the disappearance in the blots of the slow migrating p34^cdc2 form, which corresponds to Tyr-phosphorylated cyclin B-bound p34^cdc2. (B) Representative examples of the p42^mpk1 and p34^cdc2 immunoblots from single oocytes described in A.

The uncoupling between the activation of p42^mpk1 and MPF in response to progesterone suggested that D2 interferes with p42^mpk1 signaling in oocytes. These results also indicate that p42^mpk1 activation normally precedes the activation of pre-MPF duringprogesterone-induced oocyte maturation. The partial activationof p42^mpk1 is probably a consequence of the lack of an MPF-activated positivefeedback loop, which has been proposed to be required for fullp42^mpk1 activation in response to progesterone (Gotoh et al., 1991; Matsudaet al., 1992). Consistent with this possibility, we observed thatD2 expression in Mos-injected oocytes delayed GVBD (Figure 7A)and the activation of pre-MPF (Figure 7B, lower panel) but didnot interfere with the activation of p42^mpk1 (Figure 7B, middle panel). This suggested that D2 does not directlyprevent p42^mpk1 activation and is more likely to act downstream of p42^mpk1, uncoupling the activation of p34^cdc2/cyclin B from the activation of p42^mpk1.

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Figure 7. Expression of D2 does not affect the Mos-induced activation of p42^mpk1 and p90^rsk. (A) Groups of 25-30 oocytes were injected with water or mRNAs encoding either D2 or D2 $Delta$ 43 and after overnight incubation were injected with malE-mos protein and scored for GVBD. (B) Lysates were prepared from the same oocytes as in A and analyzed by immunoblotting with anti-p90^rsk, anti-p42^mpk1, and anti-p34^cdc2 antibodies. (C) Groups of 100 oocytes were injected with either water or D2 mRNA, incubated overnight, and then treated or not treated with progesterone for 12 h. Oocyte lysates were subjected to two sequential rounds of immunoprecipitation using either anti-p42^mpk1 or control rabbit IgG. The immunoprecipitates and the final supernatant (after the second round of immunoprecipitation) were analyzed by immunoblotting with anti-p90^rsk and anti-p42^mpk1 antibodies. The asterisk indicates a nonspecific band that probably corresponds to control IgG leaking from the beads.

D2 Does Not Prevent p90^rsk Activation

We have recently shown that after activation by p42^mpk1, p90^rsk associates with and phosphorylates the p34^cdc2 inhibitory kinase Myt1 (Palmer et al., 1998). Thus, one possibilityis that D2 uncouples p42^mpk1 from p34^cdc2/cyclin B activation by interfering with p42^mpk1 signaling through p90^rsk.

We observed, however, that overexpression of D2 inhibits neither the phosphorylation nor the activation of p90^rsk when p42^mpk1 was activated by Mos injection (Figure 7B, upper panel; see Figure9D). Furthermore, we could detect approximately the same amountof p90^rsk in the anti-p42^mpk1 immunoprecipitates prepared from either control or D2-expressingoocytes (Figure 2B), suggesting that D2 did not disrupt the endogenousp42^mpk1/p90^rsk complexes in G₂-arrested oocytes. These results were confirmedwhen two consecutive rounds of anti-p42^mpk1 immunoprecipitation were performed (Figure 7C).

A Possible Role for p42^mpk1 Upstream of Plx1

Because D2 did not interfere with p42^mpk1 signaling through p90^rsk, we investigated alternative pathways that could potentially beregulated by p42^mpk1. One obvious candidate was the Plx1/Cdc25 pathway (Kumagai andDunphy, 1996; Abrieu et al., 1998; Qian et al., 1998a). To investigatethe possible role of p42^mpk1 upstream of Plx1, oocytes were injected with Mos to activatep42^mpk1. We then analyzed by immunoblotting the phosphorylation stateof p42^mpk1, p34^cdc2, and Plx1 in single oocytes. As expected, the appearance of thewhite spot always correlated with the activation of pre-MPF (tyrosinedephosphorylation of p34^cdc2) and with the phosphorylation of both p42^mpk1 and Plx1 (Figure 8A, GVBD). When Mos-injected oocytes not showinga white spot were analyzed, we observed some Plx1 phosphorylationoccurring before any detectable tyrosine dephosphorylation ofp34^cdc2 (Figure 8A, Mos). This result was observed in three experimentsof five; in the other two experiments Plx1 phosphorylation wascoupled to the activation of preMPF (see example in Figure 9A).To confirm that Plx1 could be phosphorylated independently ofpre-MPF activation, we injected the small p34^cdc2-binding protein Xp9, which can interfere with p34^cdc2/cyclin B activation and delay M-phase entry in Xenopus egg extracts(Patra and Dunphy, 1996). We found that expression of Xp9 inhibitedMos-induced (Figure 8B) as well as progesterone-induced (our unpublishedresults) oocyte maturation, as measured by the absence of GVBD.These Xp9-injected oocytes, however, had a less pigmented area,which resembled an irregular white spot (see below and Figure10A), although the nucleus was still detected upon dissection offixed oocytes. The activation of p42^mpk1 by Mos was not affected in Xp9-expressing oocytes, whereas p34^cdc2/cyclin B activation was either blocked or severely delayed dependingon the batch of oocytes (Figure 8A). However, Plx1 phosphorylationwas still observed in the absence of pre-MPF activation in oocytescoinjected with Mos and Xp9 (Figure 8A).

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Figure 8. Mos induces partial phosphorylation and activation of Plx1 independently of pre-MPF activation. (A) Groups of 35 oocytes were injected with either Xp9 mRNA or water and after overnight incubation were injected again with malE-mos protein. At the indicated times injected oocytes that did not have a normal white spot were transferred to dry ice. Uninjected oocytes (control) and malE-mos matured oocytes (GVBD) were also taken for comparison. Lysates were prepared from single oocytes, and half of this lysate was analyzed by immunoblotting with anti-Plx1, anti-p42^mpk1, and anti-p34^cdc2 antibodies. (B) Kinetics of maturation of the same oocytes as in A. (C) Lysates corresponding to half an oocyte (the second half of the lysates prepared from single oocytes that in A were used for immunblotting) were immunoprecipitated with anti-Plx1 antibodies, and their associated kinase activity was assayed using casein as an in vitro substrate. Each bar represents single oocytes that were uninjected (control), malE-mos injected and matured (GVBD), or injected with malE-mos either alone or plus Xp9 but had no GVBD (these corresponded to the oocytes that in A showed partial Plx1 phosphorylation but had no preMPF activation). The Plx1 activity taken as 100% in mature oocytes (GVBD) was usually 30- to 40-fold higher than in control oocytes.

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Figure 9. Activation of Plx1 by Mos requires protein synthesis and is inhibited by expression of D2. (A) Groups of 30 oocytes that had been either preincubated for 45 min or not with cycloheximide (CHX, 50 µg/ml) were injected with malE-mos protein. At the indicated times oocytes were individually transferred to dry ice. Uninjected oocytes (C) were also taken for comparison. Oocyte lysates were prepared from single oocytes and analyzed by immunoblotting with anti-Plx1, anti-p42^mpk1, and anti-p34^cdc2 antibodies. (B) Groups of 25 oocytes were injected first with mRNAs encoding either D2 or D2 $Delta$ 43 and 2 h later with Xp9 mRNA. After overnight incubation the oocytes were injected again with malE-mos protein and incubated for 12 h. Lysates prepared from three oocytes were analyzed by immunoblotting with anti-Plx1, anti-p42^mpk1, and anti-p34^cdc2 antibodies. Uninjected oocytes (control) and Mos-matured oocytes (GVBD) were also analyzed in parallel. (C) Groups of 35 oocytes were injected first with mRNAs encoding either D2 or D2 $Delta$ 43 and 2 h later with Xp9 mRNA. After overnight incubation the oocytes were injected again with malE-mos protein, and 4 h later oocytes that did not have a normal white spot were individually taken every hour and stored on dry ice. Lysates were prepared from single oocytes and immunoprecipitated with anti-Plx1 antibodies to assay their associated kinase activity using casein as an in vitro substrate. Each bar represents single oocytes that were uninjected (control), malE-mos injected and matured (GVBD), or injected with malE-mos plus Xp9 and either D2 or D2 $Delta$ 43. The Plx1 activity taken as 100% in mature oocytes (GVBD) was usually 30- to 40-fold higher than in control oocytes. (D) Groups of 25 oocytes were injected first with mRNAs encoding Xp9 and either D2 or D2 $Delta$ 43 and later with malE-mos protein as in A. After 12 h, lysates were prepared from three oocytes, immunoprecipitated with anti-p90^rsk antibodies, and assayed for kinase activity using GST-Myt1 Ct as an in vitro substrate. Uninjected oocytes (control) were also analyzed in parallel.

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Figure 10. The sustained activation of p42^mpk1 in the absence of pre-MPF activation produces morphological changes in the oocytes. (A) Oocytes were injected with Xp9 mRNA alone or together with either D2 or D2 $Delta$ 43 mRNAs, incubated overnight, and then injected again with malE-mos protein. Pictures were taken 10 h after malE-mos injection. (B) Oocytes were injected as in A and 8-24 h later were fixed by boiling for 90 s in PBS. After dissection, the oocytes were monitored for the presence of the nucleus (control), GVBD (white spot), or nuclear migration (pseudomatured). The results represent four independent experiments with ~40 oocytes being dissected for each treatment.

The early Plx1 phosphorylation in Mos-injected oocytes was associated with a partial increase in the kinase activity of Plx1immunoprecipitates (usually 20-50% of the activity measured inGVBD oocytes) (Figure 8C), in agreement with previous reportsshowing that the phosphorylation of Plx1 correlates with its activation(Qian et al., 1998a; Karaiskou et al., 1998). These results suggestedthat the activation of p42^mpk1 could lead to partial Plx1 activation. However, full Plx1 activationapparently required the activation of MPF, which is consistentwith the existence of a positive feedback loop linking p34^cdc2/cyclin B and Plx1 (Abrieu et al., 1998; Karaiskou et al., 1998).Interestingly, although p42^mpk1 can be activated as early as 1 h after Mos injection, the phosphorylationand activation of Plx1 was detected only 3-5 h later (Figure 8A).This suggested that the link between p42^mpk1 and Plx1 was not direct. To determine whether Plx1 activationby p42^mpk1 might require protein synthesis, oocytes were preincubated withcycloheximide before injection of the recombinant Mos protein.We observed that the phosphorylation of Plx1 induced by Mos injectionwas completely inhibited in the presence of cycloheximide (Figure9A). The same results were obtained when Xp9 was overexpressedbefore Mos injection to uncouple Plx1 phosphorylation from theactivation of pre-MPF. Altogether these results suggested thatp42^mpk1 can induce partial phosphorylation and activation of Plx1 viaa pathway that requires protein synthesis but is independent ofMPF activity. We then investigated whether D2 expression couldinterfere with the p42^mpk1-dependent phosphorylation of Plx1. For this experiment, we coexpressedin oocytes Xp9 with either D2 or D2 $Delta$ 43 and then injected Mos proteinto activate p42^mpk1. We observed that expression of D2 but not D2 $Delta$ 43 inhibited Plx1phosphorylation in Mos/Xp9-injected oocytes, whereas p90^rsk activation was not significantly affected (Figure 9, B and D).This also correlated with a reduction in the extent of Plx1 activationin D2 versus D2 $Delta$ 43-expressing oocytes (Figure 9C). The resultssuggested that D2 interfered with this pathway and further supportsthat the early Plx1 phosphorylation observed after Mos injectionis mediated by p42^mpk1.

We also found that in oocytes coinjected with Mos and Xp9 the animal pole tends to become either mottled or opaque, suggestingthat sustained p42^mpk1 activation in the absence of MPF activity may have some unexpectedeffects. These oocytes also had a less pigmented area, which resembleda kind of irregular white spot (Figure 10A, Mos+Xp9). However whenthe oocytes were fixed and dissected, ~50% of them still containeda nucleus, which was usually located closer to the cortex thanin uninjected oocytes and sometimes was also flatter in shape(we refer to these oocytes as pseudomatured; Figure 10B). In thesame experiment, the majority of Mos-injected oocytes showed anormal white spot, and the nucleus was not detected inside (Figure10, A and B, Mos). This suggested that some of the morphologicalchanges associated with meiotic maturation, such as the germinalvesicle migration, can occur independently of pre-MPF activation.A role for p42^mpk1 in this process was confirmed by the observation that when D2was expressed together with Mos and Xp9, the pseudomaturationwas blocked, and both the oocytes and their nucleus had the appearanceof normal uninjected oocytes (Figure 10, A and B, Mos+Xp9+D2).In contrast, the expression of D2 $Delta$ 43 did not block oocyte pseudomaturation(Figure 10, A and B, Mos+Xp9+D2 $Delta$ 43), consistent with the inabilityof this truncated form to associate with p42^mpk1. These results suggest that nuclear migration may be regulatedby the activation of p42^mpk1; however, GVBD appears to require MPFactivation.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

In this report we show that expression of D2, an N-terminally truncated p90^rsk that contains a MAP kinase docking site, interferes with Xenopusoocyte maturation. D2 inhibition is mediated by the p42^mpk1 docking site and uncouples the activation of p42^mpk1 and p34^cdc2/cyclin B in response to progesterone. The uncoupling does notcorrelate with the inhibition of p90^rsk, suggesting that p42^mpk1 can target pre-MPF activation through alternative pathways. Consistentwith this hypothesis, we found that in Mos-injected oocytes theactivation of p42^mpk1 is followed by the partial phosphorylation and activation ofPlx1 via a pathway that requires protein synthesis. Plx1 activationtriggered by p42^mpk1 was independent of pre-MPF activation and was decreased by D2expression in the oocytes. We also provide evidence that D2 interfereswith nuclear migration triggered by the sustained activation ofp42^mpk1 in the absence of MPF activity (Figure 11).

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Figure 11. A summary of possible p42^mpk1 functions during Xenopus oocyte maturation. Progesterone stimulates the translation of maternal mRNAs and triggers the synthesis of the protein kinase Mos, which activates p42^mpk1 via MAP kinase kinase. p42^mpk1 activates p90^rsk, which in turn down-regulates the p34^cdc2 inhibitory kinase Myt1. Our results indicate that D2 interferes with p42^mpk1 signaling in oocytes but does not affect the activation of p42^mpk1 and p90^rsk. Instead, D2 interferes with the phosphorylation and activation of Plx1. This pathway, which may lead to Cdc25 up-regulation, is triggered by p42^mpk1 independently of pre-MPF activation but requires protein synthesis. Expression of D2 also inhibits the nuclear migration and pseudomaturation, which appears to be triggered by the sustained activation of p42^mpk1 in the absence of MPF activation.

A Regulated Interaction between p42^mpk1 and p90^rsk Is Essential for Signal Transduction by p42^mpk1

The efficient activation of p90^rsk requires binding to the Xenopus ERK MAPK p42^mpk1 through a specific docking site located in the last 25 aminoacids of p90^rsk. In G₂-arrested oocytes, this interaction is regulated, and thep90^rsk/p42^mpk1 complex dissociates during maturation (Hsiao et al., 1994). Wefound that in contrast to wild-type p90^rsk, a mutant with Ala substitutions in the six residues that areknown to be phosphorylated upon p90^rsk activation (p90^rsk/6xA) was able to interact with both the inactive and the activep42^mpk1. This suggests that the phosphorylation state of p90^rsk regulates the interaction between the full-length p90^rsk and p42^mpk1. However, D2, which lacks the N-terminal kinase domain but isefficiently phosphorylated by p42^mpk1 (Fischer and Blenis, 1996; Dalby et al., 1998; Gavin and Nebreda,1999), can still constitutively interact with p42^mpk1. This suggests that upon p90^rsk phosphorylation, the D1 kinase domain is somehow required forthe dissociation of the p90^rsk/p42^mpk1 complex. D1 has been reported to phosphorylate Ser-730 of p90^rsk, which is located in the p42^mpk1 docking site (Dalby et al., 1998), but this is unlikely to preventthe binding to p42^mpk1, because Ser-730 is apparently phosphorylated both in activeand inactive p90^rsk (Dalby et al., 1998). An alternative possibility is that thephosphorylation of p90^rsk induces some conformational change, so that D1 will then stericallyprevent p42^mpk1 from accessing its docking site in p90^rsk. Finally, it is also possible that the D1 kinase domain is requiredfor the interaction of phosphorylated p90^rsk with other proteins, which in turn might prevent p42^mpk1 binding. Interestingly, the C-terminal regulatory domain of Myt1can specifically bind to the phosphorylated form of p90^rsk and this association requires the full-length p90^rsk (Palmer et al., 1998). It is thus possible that p90^rsk interaction with Myt1 prevents p42^mpk1binding.

The observation that a truncated form of p90^rsk, which constitutively binds to p42^mpk1 can inhibit signaling by p42^mpk1, suggests an important role for the regulated interaction betweenp42^mpk1 and p90^rsk. The association between these two kinases in G₂-arrested oocytes,in which p42^mpk1 is inactive, would ensure the preferential phosphorylation ofthe bound p90^rsk. However, upon progesterone stimulation, dissociation of thecomplex is probably necessary for the accessibility of p42^mpk1 and p90^rsk to other substrates. Expression of peptides based on the sequenceof an ERK MAP kinase docking site from Elk-1 has been also reportedto inhibit Xenopus oocyte maturation (Jacobs et al., 1999). Thus,truncated substrates and docking site peptides may be helpfulinhibitory tools to study signal transduction by MAP kinases.They might also allow the differential inhibition of specificMAP kinase pathways, because some docking sites appear to targetspecific MAP kinase family members. Furthermore, these tools mightpreferentially inhibit particular subsets of substrates, becausetheir ability to compete with endogenous substrates may dependon the relative affinities of the different docking sites forthe MAPkinases.

The Inhibitory Effect of D2 Requires Binding to p42^mpk1

The inhibitory effect of D2 on meiotic reinitiation does not depend on its kinase activity, suggesting that D2 inhibits byinteraction with endogenous proteins and not catalytically. Fragmentsof monomeric enzymes can sometimes work in a dominant negativeway by interfering with the folding of the wild-type endogenousprotein (Michaels et al., 1996). However, it appears unlikelythat D2 works by targeting p90^rsk in a similar way. We have not detected interactions between D2and either p90^rsk or the D1 or D2 kinase domain alone in a yeast two-hybrid system(our unpublished results). Furthermore, we showed that D2 associateswith endogenous p42^mpk1 in the oocytes (which is recruited to higher-molecular-weightcomplexes), whereas the elution pattern of p90^rsk in gel filtration was unchanged upon D2 expression (our unpublishedresults). These results together with the observation that D2inhibition is mediated by the p42^mpk1 docking site suggest that the inhibitory effect of D2 is broughtabout by binding to p42^mpk1.

A New Pathway That Links the Activation of p42^mpk1 and p34^cdc2/Cyclin B during Oocyte Maturation

We have taken advantage of the inhibitory effect of D2 to investigate the function of p42^mpk1 during Xenopus oocyte maturation. We found that D2 expressionuncouples the activation of p42^mpk1 and p34^cdc2/cyclin B. This confirms previous results showing that the interferencewith p42^mpk1 activation prevents meiotic reinitiation and p34^cdc2/cyclin B activation (Kosako et al., 1994b, 1996; Gotoh et al.,1995). However, in contrast to previous studies in which the activationof p42^mpk1 was also prevented, we use a tool that does not block p42^mpk1 activation but inhibits downstream of p42^mpk1 and prevents the activation of p34^cdc2/cyclin B. Thus, our work indicates that p42^mpk1 activation normally precedes the activation of pre-MPF duringprogesterone-induced meioticmaturation.

We found that D2 did not disrupt the preformed p90^rsk/p42^mpk1 complexes present in G₂-arrested oocytes. This observation is surprisingbecause we have not detected significant differences in the affinitiesof either D2 or p90^rsk for p42^mpk1. One possible explanation is that in G₂-arrested oocytes theinteraction between p42^mpk1 and p90^rsk might not be dynamic. In support of this possibility, when eitherp42^mpk1 or full-length p90^rsk is overexpressed, it does not bind to the endogenous partners(our unpublished results); however, the overexpressed p42^mpk1 and p90^rsk are able to interact with each other (Figure 1B). These observationssuggest that there may be mechanisms to stablilise the preformedp90^rsk/p42^mpk1 complexes in oocytes. Whether this is due to the binding of additionalproteins that stabilize the complex or to the localization ofthe complexes in particular subcellular compartments where theyare not accessible to the exogenous, overexpressed proteins remainsto be investigated. Consistent with the observation that D2 didnot disrupt the preformed p90^rsk/p42^mpk1 complex, D2 did not delay the kinetics of phosphorylation andactivation of p90^rsk by p42^mpk1, suggesting that D2 does not interfere with the p90^rsk/Myt1 pathway. Thus, p42^mpk1 might target pre-MPF activation through alternative pathways.In G₂-arrested oocytes only part of the p42^mpk1 is found associated with p90^rsk, and our gel-filtration experiments suggest that D2 interactswith the p42^mpk1 subpopulation, which is not associated with p90^rsk. This p42^mpk1 subpopulation is likely to target substrates other than p90^rsk, which might also participate in the regulation of p34^cdc2/cyclin B activity (and hence the activation of pre-MPF) duringoocyte maturation. We cannot rule out, however, that upon progesteronestimulation D2 might also interact with the active p42^mpk1 released from the p42^mpk1/p90^rskcomplex.

The Cdc25 activating kinase Plx1 can be phosphorylated and activated by the protein kinase xPlkk1, which itself is also regulatedby phosphorylation by one or more protein kinases (Qian et al.,1998b). Several reports indicate that Plx1 activation may be triggeredby p34^cdc2/cyclin B as part of the MPF autoamplification loop (Abrieu etal., 1998; Karaiskou et al., 1998). Here we provide evidence fora p42^mpk1-triggered pathway, which also regulates Plx1 phosphorylationand activation. We observed that in Mos-injected oocytes, theactivation of p42^mpk1 is followed by partial phosphorylation of Plx1 before any detectablepre-MPF activation. In some batches of oocytes, however, the phosphorylationof Plx1 induced by Mos injection coincides with pre-MPF activation.One interpretation is that Plx1 phosphorylation normally precedesthe activation of pre-MPF, although in some oocytes the two eventsmay take place too close in time to be separated experimentally.To rule out an implication of p34^cdc2/cyclin B in the phosphorylation of Plx1 induced by Mos, we coexpressedthe Xenopus Suc1/Cks protein Xp9 together with Mos. Xp9 is a p34^cdc2-binding protein that appears to be important for targeting p34^cdc2/cyclin complexes to some substrates (Kusubata et al., 1992; Patraand Dunphy, 1998). For example, Xp9 can enhance the phosphorylationof the Cdc27 component of the anaphase-promoting complex by p34^cdc2/cyclin B and affect cyclin B stability (Patra and Dunphy, 1998).When overexpressed in Xenopus egg extracts, Xp9-like proteinscan delay entry into mitosis by interfering with p34^cdc2 tyrosine dephosphorylation (Dunphy and Newport, 1989; Patra andDunphy, 1996). Consistent with this, we found that injection ofXp9 into oocytes prevented Mos-induced meiotic reinitiation byinterfering with the activation of p34^cdc2/cyclin B. In these oocytes, however, ectopic Mos was still ableto activate p42^mpk1, and we could confirm that Plx1 phosphorylation and activationoccurred independently of pre-MPF activation. Importantly, thephosphorylation and partial activation of Plx1 induced by Moswas inhibited by the expression of D2, indicating that it involvesp42^mpk1. A link between p42^mpk1 and Plx1 has not been found in extracts prepared from G₂-arrestedoocytes (Karaiskou et al., 1998). In these extracts, however,the activation of p42^mpk1 and p34^cdc2/cyclin B appear to be independent events (Huang and Ferrell,1996) probably attributable to the impaired ability of the oocyteextracts to translate mRNAs (our unpublished results). In agreementwith this, we show that the p42^mpk1-dependent phosphorylation of Plx1 is abolished by cycloheximideand thus requires protein synthesis. This observation togetherwith the 3- to 5-h delay observed between the activation of p42^mpk1 and Plx1 argue against a direct link between p42^mpk1 and either Plx1 or xPlkk1 and rather suggest that p42^mpk1 triggers the accumulation of a protein or proteins that are requiredfor the activation of Plx1. Whether this link between p42^mpk1 and Plx1 activation is related to the triggering pathway thatleads to Plx1 activation at the onset of M-phase remains to bedetermined. In any case, the delayed kinetics observed betweenp42^mpk1 and Plx1 activation suggest that Plx1 activation is probablynot an early p42^mpk1-dependent step in maturation and may be the basis of a positivefeedback loop ensuring the coordinated activation of both p42^mpk1 and MPF.

During oocyte maturation p42^mpk1 can participate in p34^cdc2/cyclin B activation via several pathways (Figure 11). One pathway may involvephosphorylation and inhibition of Myt1 by p90^rsk (Palmer et al., 1998). Accumulation of Mos is also stimulatedby p42^mpk1 through a positive feedback loop (Matten et al., 1996; Roy etal., 1996), and it has recently been shown that p42^mpk1 can up-regulate cytoplasmic polyadenylation of the Mos mRNA (Howardet al., 1999). However, the initial progesterone-induced synthesisof Mos is probably independent of p42^mpk1, because it occurs before any detectable p42^mpk1 activation. Our results suggest a new connection between p42^mpk1 and a protein or proteins that are required for the phosphorylationand partial activation of Plx1. p42^mpk1 could stimulate synthesis of these proteins and/or post-translationallyregulate their activity, for example, at the level of proteinstability. As in the case of Mos, synthesis of these proteinsmight be also initiated during progesterone-induced maturationbefore the activation of p42^mpk1. This suggests the possibility that the susceptibility of theoocytes to inhibition by D2 may depend on the initial rate ofprotein synthesis induced byprogesterone.

A Possible Role for p42^mpk1 in Nuclear Migration

MPF is a key regulator of M-phase progression during the cell cycle and is likely to be responsible for most of the structuralchanges associated with M-phase. ERK MAP kinases and p34^cdc2/cyclin B, however, have some overlapping substrate specificity.For example, both can phosphorylate nuclear lamins at the sitesthat are involved in lamin disassembly before nuclear envelopebreakdown (Peter et al., 1992). In mouse oocytes and embryos ERKMAP kinases have also been implicated in some M-phase events (Gavinet al., 1994; Moos et al., 1996; Verlhac et al., 1996). However,a possible role for p42^mpk1 in controlling M-phase structural changes in Xenopus oocyteshas been difficult to address, because p42^mpk1 is usually activated at the same time as MPF during meiotic maturation.Here we show that activation of p42^mpk1 by Mos in the absence of p34^cdc2/cyclin B activation may induce some of the morphological changesassociated with meiotic maturation such as nuclear migration tothe cortex of the oocyte. This is likely to be triggered by p42^mpk1 activation, because it can be inhibited by the overexpressionof D2, but not of a truncated version of D2, which lacks the p42^mpk1 docking site. However, the sustained activation of p42^mpk1 in the absence of MPF activation appears to lead to an abnormalmaturation as indicated by the morphological appearance of theoocytes. Similar effects (including germinal vesicle migrationwithout breakdown) have also been described when maturation isinduced by the injection of oncogenic Ras in the presence of eitherdrugs that increase cAMP levels (Birchmeier et al., 1985) or proteinsynthesis inhibitors (Nebreda et al., 1993b). Our results alsoshow that activation of p42^mpk1 alone is not enough to trigger GVBD in Xenopus oocytes, indicatingthat nuclear envelope breakdown during M-phase is likely to requirethe activation of MPF.

In summary, we have found that overexpression of the p42^mpk1 docking site located at the C-terminal end of p90^rsk can inhibit Xenopus oocyte maturation, and we have used thisas a tool to elucidate the role(s) of p42^mpk1 in the process. Our main conclusions are that activation of p42^mpk1 normally precedes the activation of pre-MPF and that there isan MPF-independent pathway that links the activation of p42^mpk1 and the Cdc25-activating kinase Plx1 during oocyte maturation.We also show that p42^mpk1 may have a role in nuclear migration during Xenopus oocyte maturation.Finally, our results indicate that the regulated interaction withsubstrates is essential for signal transduction by MAPkinases.

	ACKNOWLEDGMENTS

We are grateful to A. Tavares, C. Avides, and D. Glover for the anti-Plx1 antiserum, to A. Björnson for preparation of FTX5-Mos,and to D. Barila, K. Dorey, A. Palmer, and G. Superti-Furga forcritically reading the manuscript. A.-C.G. was supported by theSwiss National Science Foundation and the European Molecular BiologyLaboratory.

	FOOTNOTES

^* Corresponding author. E-mail address: nebreda{at}EMBLheidelberg.de.

ABBREVIATIONS

Abbreviations used: GVBD, germinal vesicle breakdown; H1K, histone H1 kinase; IgG, immunoglobulin G; MPF, M-phase- or maturation-promoting factor.

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				E. Kiss-Toth, S. M. Bagstaff, H. Y. Sung, V. Jozsa, C. Dempsey, J. C. Caunt, K. M. Oxley, D. H. Wyllie, T. Polgar, M. Harte, et al. Human Tribbles, a Protein Family Controlling Mitogen-activated Protein Kinase Cascades J. Biol. Chem., October 8, 2004; 279(41): 42703 - 42708. [Abstract] [Full Text] [PDF]

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