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RESEARCH |
Department of Cell and Developmental Biology, Sackler Faculty of Medicine, Tel Aviv University, Ramat-Aviv 69978 Tel-Aviv, Israel and 1 Department of Anatomy and Cell Biology, University of Kansas Medical Center, Kansas City, Kansas 66160, USA
Correspondence should be addressed to R Shalgi; Email: shalgir{at}post.tau.ac.il
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Abstract |
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We suggested that SFKs mediate significant functions during the organization of the MII spindle. In view of CAF injection experiments, and of the pronounced concentration of Fyn kinase at the spindle, we propose that Fyn may play an important role in some aspects of the spindle functions, possibly those involving the MTs.
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Introduction |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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Src family protein tyrosine kinases (SFKs) are implicated in a variety of cellular processes. SFKs are cytoplasmic enzymes, linked to the cell membrane via amino-terminal fatty acids. They are composed of one src homology 2 (SH2) domain, one src homology 3 (SH3) domain, a catalytic domain and a carboxy-terminal regulatory sequence (Superti-Furga & Courtneidge 1995). Their function at fertilization is currently under investigation. There is increasing evidence that SFKs play an important role in regulating mitotic events. Fyn, c-Src and c-Yes are activated in response to various growth factors during the transition from the G0 to the G1 phase of the cell cycle (Kypta et al. 1990, Courtneidge et al. 1993, Rongish & Kinsey 2000). The three SFKs are also activated in fibroblasts during the late G2 phase and during the entry into mitosis (Roche et al. 1995a). Furthermore, microinjection of antibodies which neutralize c-Src, c-Yes and Fyn in NIH3T3 cells, inhibits entry into mitosis, suggesting that the catalytic activity of SFKs is necessary for initiation of mitosis (Roche et al. 1995b). Progression of the cell cycle is blocked by inhibition of SFKs (Moasser et al. 1999). These studies demonstrate the requirement of SFKs for entry into mitosis, suggesting that interactions among the SH2 domain of the SFKs, the signaling-tyrosine-phosphorylating (STP) proteins and the cytoskeletal proteins, are necessary for mitotic cell division in fibroblasts.
Changes in activity and localization of c-Src during mitosis, suggest a mitotic function (David-Pfeuty & Nouvian-Dooghe 1990, 1995, Bagrodia et al. 1991, Zhao et al. 1992, Taylor & Shalloway 1993, David-Pfeuty et al. 1993). An increase in the tyrosine phosphorylation of a 68 kDa protein is observed during mitosis, concomitant with an increase in c-Src activity (Fumagalli et al. 1994, Taylor & Shalloway 1994). Localization of c-Src to fibroblastic endosomes and to MT structures, implies c-Src involvement in protein trafficking and in mitotic centriol organization (David-Pfeuty & Nouvian-Dooghe 1990, Kaplan et al. 1992). Fyn kinase was found to be associated (Katagiri et al. 1993, Marie-Cardine et al. 1995) or co-localized (Ley et al. 1994, Yasunaga et al. 1996) with the spindle MTs during the M-phase of various cells.
Although the function of the specific SFKs is unclear at present, their subcellular localization has provided some clues. Localization of c-Src, c-Yes and Fyn to different compartments in the rat egg indicates that these proteins may have different functions within the egg (Talmor et al. 1998, Talmor-Cohen et al. 2004). The localization of Fyn (but not of c-Src or c-Yes) to the MTs suggests that Fyn may have a role in directing the MTs’ action. The use of SFK inhibitors enabled us to inhibit the completion of the cell cycle (Talmor-Cohen et al. 2004). We may infer that SFKs in general and Fyn in particular, could control MT organization. The objective of the present study is to analyze the association of SFKs with the spindle.
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Materials and Methods |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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Antibodies and drugs
Anti-Fyn-3 peptide polyclonal antibody (pAb; Santa Cruz Biotechnology, Santa Cruz, CA, USA), was chemically coupled to protein A-sepharose to prepare an immobilized antibody affinity reagent for immunoprecipitation (Talmor et al. 1998). Anti-ßtubulin monoclonal antibody (mAb) and nocodazole were purchased from Sigma. Stock solution of 2 mg/ml of nocodazole was prepared in DMSO and diluted in TH medium before use to a final concentration of 10 µg/ml. Stock solutions of 13 mM 4-amino-5-(4-chlorophenyl)-7-(t-butyl)pyrazolo[3,4-d]pyrimidine (PP2), PP3 and of 10 mM SU6656 (Calbiochem-Novabiochem, CA, USA) were prepared in DMSO and diluted before use in TH medium to final concentrations of either 10–100 µM (PP2, PP3) or 1–5 µM (SU6656).
Immunoprecipitation and immunoblotting
Batches of 400 eggs were lysed in 100 µl NP-40 lysis buffer and immunoprecipitated with anti-Fyn-3 peptide pAb, as described previously (Talmor et al. 1998). Western blot analysis was performed with an anti-ß tubulin mAb (1:200). Bound antibody was recognized by horseradish peroxidase conjugated to anti-mouse antibody (1:5000; Sigma). Detection was performed by ECL (Pierce, Rockford, IL, USA). Approximate molecular masses were determined by comparison with the migration of prestained protein standards (Amersham).
CAF construction
In order to create a form of Fyn kinase that would be constitutively active (CAF), we modified it’s C-terminal phosphorylation site to a non-phosphorylatable residue. A mutation was induced in the Fyn sequence of Xenopus that substituted Tyr 532 by Phe. This was done by PCR, using a sense primer 5' TAG AAT TCG ATA ATG GGC TGT GTG CAA T3' and an antisense primer 5' TAG CTC GAG GTT GTC TCC AGG CTG AAA TT 3'. The PCR product was cloned into pGEX4T3 and the sequence GST-Fyny532f was confirmed. The fusion protein was expressed in Escherichia coli and purified by affinity chromatography (GST Technical Manual; Pharmacia Biotech, Piscataway, NJ, USA). Further purification was accomplished by chromatography on a diethylaminoethyl (DEAE) column followed by elution by a 50–500 mM KCl gradient. Fractions containing protein tyrosine kinase (PTK) activity were pooled, concentrated and dialyzed to KPS buffer (150 mM KCl, 3 mM NaCl, 10 mM KH2PO4, pH 7.2). Catalytic activity was confirmed by a kinase assay using a synthetic peptide substrate.
Microinjection
CAF was microinjected into unfertilized eggs (~10 pl per oocyte). Control eggs were microinjected with KPS buffer alone or with a boiled CAF protein. The estimated concentration of CAF that would be within the egg cytoplasm is indicated in the Results section. Microinjections (Narishige Micromanipulators, Japan) were performed under differential interference contrast (DIC; inverted microscope TE-200, Nikon, Japan), at x 20 (objective) magnification, by intracytoplasmic injection micropipettes (Perry, Medical Instrumental Development Ltd, Ra’anana, Israel). All microinjection experiments were performed on a warm stage (30 ± 0.5°C) in TH medium supplemented with 10% fetal calf serum (FCS; Biological Industries, Beit-Haemek, Israel). The microinjected eggs were allowed 1 h of recovery in TH medium at 37 ° C, 5% CO2 in air, prior to fixation (3% paraformaldehyde and 0.01% glutaraldehyde in Dulbecco’s phosphate-buffered saline (DPBS)) and to zona pellucida (ZP) removal. Eggs were monitored for morphological criteria that indicate progression through the activation process (the chromosomal stage was detected by a DNA-specific fluorochrome (Hoechst 33342, Sigma); cortical granules exocytosis (CGE) was detected by lens culinaris aectin (LCA) and Texas-red streptavidin (Vector; Eliyahu & Shalgi 2002). Data are expressed as a percentage: the number of treated eggs that resumed meiosis successfully, or demonstrated CGE, per total number of injected eggs.
Immunofluorescent staining and laser-scanning confocal microscopy
Oocytes/eggs at various stages of meiosis were fixed and permeabilized (Talmor et al. 1998), then incubated in the presence of two primary antibodies: either anti-Fyn-3 peptide pAb (1:10) or anti-ß tubulin mAb (1:5000), followed by an incubation with Cy-conjugated secondary antibodies (Jackson Immunoresearch Laboratories, West Grove, PA, USA): donkey anti-rabbit IgG-Cy2 (1:500) or donkey anti-mouse IgG-Cy3 (1:500) respectively. Data collected from three experiments were pooled. Groups of three to four oocytes from each experiment were recorded.
DNA was detected by Hoechst 33342. Stained oocytes/ eggs were visualized and photographed using a Zeiss confocal laser scanning microscope (CLSM; Rufas et al. 2000). The dye intensity was measured using the corrected mean density values obtained by the LSM software.
In vitro phosphorylation of tubulin
Samples of purified bovine brain tubulin (1 µg) were incubated with 10 ng GST-Fyny532f bound to glutathione-sepharose (Pharmacia Biotech) in kinase buffer (15 mM HEPES, 10 mM MgCl2, 1 mM 2-mercaptoethanol, 1 mM[32P]ATP (3 mCi/µmol); pH 7.2) for 10 min at 25 °C. The reaction was stopped by an addition of 2 x Laemmli sample buffer and the products were resolved by SDS-PAGE. The gel was treated with 1 M KOH for 1 h at 50 °C to hydrolyze any P-Ser and P-Thr, then dried and analyzed by autoradiography.
Statistical analysis
The significance of differences between experimental groups was determined by Fisher’s exact probability test or by one-way ANOVA test, combined with Tukey’s method for multiple comparisons; P < 0.05 was considered significant.
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Results |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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). Exposure of MII eggs to 5 µM SU6656 caused a disintegration of the barrel-shaped spindle and appearance of dispersed tubulin fibers throughout the cytoplasm. Moreover, the chromosomes were no longer aligned on a metaphase plate (Fig. 1B'). PP2 did not have such a dramatic effect on the metaphase plate but caused a minor disorganization of the spindle (Fig. 1C'). SFK inhibitors did not cause depolymerization of the MTs in MII eggs, as was the case for nocodazole (Fig. 1D'), which suggests a different mechanism of action.
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, demonstrating short MTs surrounding the chromosomes of an oocyte undergoing GVBD (Fig. 2A'). A bipolar spindle was observed 6 h post hCG injection, and the chromosomes gathered at the equatorial plane (Fig. 2B'), as in the MII stage (Fig. 2C'). As a specificity control for each experiment, a synthetic peptide antigen was coincubated with the primary antibody to act as a competitive inhibitor. The antibody staining was completely blocked by the synthetic peptide (data not shown). Our findings indicate that localization of Fyn kinase at the spindle MT is a general phenomenon, observed, in the present study, during oocyte maturation (Fig. 2A, B and C), and as shown in a previous work, during fertilization in both the meiotic and the mitotic spindles (Talmor et al. 1998).
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). Nocodazole treatment caused dispersal of Fyn staining from the spindle, and was observed throughout the cytoplasm of all eggs tested (Fig. 3B); it also caused abolishment of tubulin staining (Fig. 3B'). After washing off the drug most of the eggs (69/75) re-exhibited a fully recovered spindle (Fig. 3C') accompanied by Fyn staining (Fig. 3C). These results suggest that the association of Fyn with the spindle MTs is dynamic and can be disrupted and re-established when MTs are allowed to depolymerize and repolymerize respectively.
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). We were able to detect a weak tubulin band when Fyn was immunoprecipitated from lysates of non-activated MII eggs (Fig. 4, lane a). The tubulin band became more prominent after activation by ionomycin (Fig. 4, lane b). Control samples containing only culture media were devoid of any band (Fig. 4, lane c) as were samples immunoprecipitated by a non-related control antibody (data not shown). The detected ß-tubulin band served as an indicator for the presence of the tubulin heterodimer in the precipitate.
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, the kinase reaction containing GST- Fyny532f resulted in a single 85 kDa band representing the autophosphorylated kinase, although some lower molecular weight contaminants or proteolytic fragments are also phosphorylated. Tubulin alone had no kinase activity (Fig. 5, lane B). Addition of tubulin to the kinase reaction resulted in phosphorylation of a doublet (approx 45 kDa) representing 
- and ß-tubulin (Fig. 5, lane C). While tubulin is similar in Mr to some of the faint bands in lane A, the 45 kDa doublet is phosphorylated at a higher level relative to other contaminants and is therefore unlikely to represent a phosphorylated contaminant.
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), whereas most of the eggs injected with boiled CAF remained at the MII stage (Fig. 6Ab and B (gray bars)). Completion of meiosis in response to injection of CAF occurred in a dose-dependent fashion (Fig. 6B, black bars). Some 77% of eggs injected with CAF at a concentration of 555 µg/ml (calculated as final concentration within the egg of 6.4 µM), resumed meiosis, whereas only 28% resumed meiosis at concentration of 37 µg/ml (within the egg 0.4 µM). Only 21% of MII eggs injected with boiled CAF, at any injected dose, resumed meiosis (Fig. 6B, gray bars), compared with 11% of MII eggs that resumed meiosis after being injected with KPS buffer alone (data not shown).
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Discussion |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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In a previous study we were able to show that completion of meiosis is an SFK-dependent process (Talmor-Cohen et al. 2004). In the present study we demonstrated that inhibition of SFKs caused the disintegration of the spindle and dispersion of tubulin fibers in the cytoplasm. Moreover, as a result of this treatment the chromosomes were not aligned on the metaphase plate. For a successful fertilization, the spindle of vertebrate eggs must remain stable and correctly organized during the second meiotic metaphase arrest (Terret et al. 2003, Wassmann et al. 2003). Thus, we have suggested that SFKs mediate some functions during the organization of a proper MII spindle. However, we have not yet determined whether the SFK function during fertilization controls meiotic arrest either by maintaining MPF stability or by ensuring that the spindle is properly organized during the arrest.
Potential function of Fyn in microtubule signaling
Fyn kinase is the only one of the three SFKs studied that is localized to meiotic and mitotic spindles (Talmor et al. 1998, Talmor-Cohen et al. 2004). Our findings that the proper organization of the MII spindle is an SFK-dependent process, and that Fyn kinase is localized to the MTs, lead us to investigate the involvement of Fyn in microtubule function.
Fyn kinase was found to be associated with (Katagiri et al. 1993, Marie-Cardine et al. 1995) or localized to (Ley et al. 1994, Yasunaga et al. 1996) the spindle MTs during the M-phase of various cells. In the present study, localization of Fyn to the egg’s spindle MTs was observed during various stages of oocyte maturation, and during the M-phase of the meiotic division.
Our results demonstrate an association of Fyn with tubulin. The band of tubulin which has been coimmunoprecipitated by Fyn kinase appears more intense in activated eggs than in MII-arrested eggs. We would like to suggest that during the M-phase, Fyn kinase interacts, directly or indirectly, with only a small number of tubulin units, while after egg activation, either the number of interacting units increases or the affinity between tubulin and Fyn increases, hence allowing a more efficient coimmunoprecipitation. Studies involving other cell systems have shown that mito-genic stimuli induce phosphorylation of the tyrosine residues of -tubulin and that the phosphorylated -tubulin is capable of binding the Fyn SH2 domain (Katagiri et al. 1993, Ley et al. 1994, Marie-Cardine et al. 1995). The spindle is a complex structure that is known to associate with a variety of proteins, including motor proteins such as kine-sin (Neighbors et al. 1988) and dynein (Pfarr et al. 1990), MT-associated proteins (MAPs; Sherline & Mascaro 1982) and Ca2+ calmodulin kinase II (Ohta et al. 1990). It has also been shown that Fyn binds MAP-2c (Zamora-Leon et al. 2001) and dynein complex (Campbel et al. 1998). The present study allows us to conclude that Fyn kinase is not merely colocalized to, but is also associated with tubulin, before and during egg activation induced by ionomycin, as demonstrated by the use of nocodazole and by coimmunoprecipitation. Fyn can phosphorylate tubulin in vitro, as implied by our in vitro phosphorylation experiment. The question whether Fyn interacts with tubulin directly or indirectly remains open. Fyn, like other SFKs, is commonly involved in multi-protein complexes involving interaction with the SH2 and SH3 domains. It is therefore possible that the localization of Fyn to the microtubules involves other MT-associated proteins.
Our findings demonstrated that CAF stimulates the completion of meiosis in rat eggs. This result should be taken with reservation because the constructed CAF is cytosolic, and as such it is incapable of bonding with a myristic acid chain. This diminished its efficiency in finding its suitable substrate, although it did not hinder its kinase activity. As a result, we were forced to employ a relatively high concentration of the activated kinase.
The CAF injection result is supported by another study concerning SFK inhibitors (Talmor-Cohen et al. 2004) and is in accordance with yet another study, performed with mouse eggs (Sette et al. 2002). In view of the CAF injection experiment and of the pronounced concentration of Fyn kinase at the spindle, we suggest that Fyn may play an important role in some aspects of spindle functions, possibly those involving the MTs themselves.
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Acknowledgements |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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Footnotes |
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References |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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