Antibodies and reagents

Rabbit phosphor-specific anti-Src (pY418), recognizing both Y423 in mouse Src and Y419 in mouse Fyn, as well as anti-Src (pY529), recognizing both Y534 in mouse Src and Y530 in mouse Fyn due to the highly conserved sequence of these residues [22] were purchased from BioSource, rabbit anti-Csk (C-20) and anti-Ctk from Santa Cruz, mouse-anti-Csk (clone 52) and mouse anti-CHK from BD BioSciences, mouse anti-Src (clone GD11) from Upstate (Lake Placid, NY), rabbit anti-PSD93 from Alomone Labs Ltd., rabbit anti-c-Src (Y215) from ECM Biosciences, and mouse anti-β-actin (clone AC-15) from Sigma. Mouse-anti-phosphotyrosine (4G10) antibodies were produced in our institute from the hybridoma cells. Secondary antibodies goat-anti-mouse-HRP and goat-anti-rabbit-HRP were obtained from Dianova.

Rabbit polyclonal anti-PAG (residues 97-432) and mouse anti-Fyn (Fyn 02) were kindly provided by Vaclav Horejsi (Prague, CZ). Anti-phospho-PAG (pY317/pY314) was developed by Burkhart Schraven [23]. Rabbit polyclonal anti-PAG (Ig452) against the peptide CGDLQQGRDVTRL was developed in collaboration with ImmunoGlobe (Berlin, Germany). The antibodies against PAG, Fyn and Src used here recognize the respective proteins phospho-independently (Fig. S1). Chemicals were purchased from Sigma unless stated otherwise.

Pag1-knockout mice

Mice with a deletion in the Pag1 gene were generated using modified bacterial artificial chromosome (BAC) technology as previously described [24]. In brief, we obtained BAC clones spanning the Pag1 locus from Research Genetics (Invitrogen Life Technologies). Two short sequences flanking exons 6 were cloned into the 5′ and 3′ insertion sites of the selection cassette of the pSKY replacement vector. BAC host cells were transformed with the pBADred plasmid, which helped produce electroporation-competent cells. The linear fragment released from the pSKY backbone was then electroporated into the BAC host, and the transformants were selected for simultaneous resistance to chloramphenicol (from the BAC backbone) and zeocin (from the insert). The resulting mutant BAC is shown in Fig. S2A.

As shown in Fig. S2B, PAG1/PAG2/Pzeo primers (pag1: ttctttcagaagacagcacgctg; pag2: gcgtccaccggtcccttctgcag), identify a predicted 473-bp PCR product in the mutant BAC confirming 5′ targeting. As predicted, the Psv/PAG1/PAG2 primers identify a 745-bp PCR product in the mutant BAC and 581-bp PCR product in the wild-type BAC. Restriction digestion with BamHI and HindIII confirms the identity of WT and mutant BACs (Fig. S2C). Fluorescence in situ hybridization was performed as described previously and confirmed targeting in clones 7 and 35 (Fig. S2D). Pag1^–/– mice from clone 7 were born in the expected Mendelian frequency of 25% in Pag1 ^+/− crossings with a male/female ratio of 1∶1. In Pag1^-/- breedings the male/female ratio was 1∶0.94 (66 animals analyzed). All experiments were performed on tissue from euthanized animals in accordance with the German National Guidelines for the Use of Experimental Animals (Animal Protection Act, Tierschutzgesetz, TierSchG, in particular paragraph 7 and 8). Animals were handled in accordance with the European Communities Council Directive 86/609/EEC. All possible efforts were made to minimize animal suffering and the number of animals used.

In situ-hybridization

In situ-hybridization was carried out on 18- µm-thick cryosections of mouse brains as previously described [25], [26]. For the antisense-probe, a pBluescript II SK plasmid containing the complete mouse PAG cDNA (accession number AF250192) [14] was linearized with BamHI (internal BamHI site), in vitro transcribed with T7 RNA polymerase yielding a cRNA of ∼900 bases. To produce sense cRNA for control the plasmid was linearized with Hind III, yielding a ∼800 bases long antisense cRNA (internal HindIII site); the cRNA was in vitro transcribed with T3 RNA polymerase. The specific activity of the probes was ∼10⁸ cpm/µg. Radioactivity was adjusted to 3,3×10⁶ cpm/100 µl hybridization buffer and used immediately. The slides were dipped, developed, and counterstained Mayer's hematoxylin solution and eosin as previously described.

RNA extraction

RNA was isolated from whole brains of C57Blc6 mice at the indicated age (except E12: whole embryo head) using peqGOLD TriFast according to the manufacturer's instructions (Peqlab, Erlangen, Germany). RNA samples were dissolved in water and quantified spectrophotometrically at 260 nm. After treatment with TURBO-DNase (TURBO DNA-freeTM, Ambion Inc.) according to the manufacturer's instructions, 2 µg of total RNA were transcribed into cDNA using RevertAidTM H Minus M-MuLV Reverse Transcriptase and the RevertAidTM H Minus First Strand cDNA Synthesis Kit according to manufacturer's instructions (Fermentas).

RT-PCR

Primer sequences were designed to span intron regions to insure that no false positive PCR fragments would be generated from pseudogenes in the contaminating genomic DNA. The following primers were used:

PAG-r (AGTTCCTTGTCATACAAGTCTCG),

PAG-f (CCACTTCTGCCTTGAAGGAGCTTC),

Fyn-r (TGGCACAGGAGCAGCTATTTA C),

Fyn-f (GAGCTGGTCACCAAAGGAAGAG),

Lyn-r (TCTGACTGTGGTCCCATTGAGC),

Lyn-f (GATTGTCACCTATGGGAAGATTC),

Csk-r (ACAGGCAGGTACAGAGGCAAG),

Csk-f (CGTTCGGTGCTAGGTGGAGAC),

Ctk-r (ACTATTTTGCGGAAGGGTGGTC),

Ctk-f (CGTGCTCTTGTGAGCACCTCTC),

GAPDH-r (CTTACTCCTTGGAGGCCATG),

GAPDH-f (TTAGCACCCCTGGCCAAGG).

For each gene, the linear amplification range was optimized. Reactions were performed on a PCR cycler (GeneAmp, PCR System 9700, PE Applied Biosystems) using cDNA (1.1 ng), oligonucleotide primer (10 pmol each), of each dNTP (200 µM each), SAWADY Taq-DNA-Polymerase (2 units, PEQLAB) and 1X reaction buffer S in a 50 µl volume. Amplification started with a 95°C denaturation for 5 min, followed by the optimized number of cycles of 95°C/30 sec, 55°C/30 sec, 72°C/1 min. The PCR products were visualized by electrophoresis on 2% agarose gels in TBE buffer (89 mM Tris-base pH 7.6, 89 mM boric acid, 2 mM EDTA) with 10 µg/ml ethidium bromide and photographed using a UV light box.

GEM-Preparation

To isolate glycosphingolipid-enriched microdomains, C57Blc6 mice brains were homogenized with ULTRA-TURRAX T25 (Janke & Kunkel GmbH, IKA-Labortechnik) and lysed at a concentration of 1 g/3 ml in ice-cold Brij 58-containing lysis buffer (3% Brij 58, 50 mM Hepes pH 7.4, 100 mM NaCl, 1 mM AEBSF (AppliChem GmbH), 5 mM EDTA, 1 mM sodium orthovanadate, 50 mM sodium fluoride, 10 mM sodium pyrophosphate) for 10 min on ice. Lysates were then subjected to sucrose gradient centrifugation as previously described [14]. GEM-containing fractions were detected by dot blot probed with biotinylated cholera toxin subunit B (Sigma) and streptavidin-HRP (Dako A/S, Glostrup, Denmark).

Immunoprecipitation and Western blot analysis

Brain homogenates in GEM buffer were incubated with 1% N-dodecyl β-D-maltoside [lauryl maltoside] (Calbiochem) for 30 min on ice. After incubation, lysates were centrifuged for 15 min at 15,700xg. For direct Western blot analysis supernatants were heated in 1x reducing sample buffer for 5 min at 95°C. For immunoprecipitation, the postnuclear lysate was immunoprecipitated with the respective antibodies/-sera as previously described [14]. Gel electrophoresis of immunoprecipitates and lysates as well as ECL-Western blotting have also been described [14].

In vitro-kinase assays

Fyn and Src were immunoprecipitated from pooled GEM-containing fractions following incubation with 2% lauryl-maltoside for 30 min on ice and centrifugation for 15 min at 15,700xg at 4°C, using either 0.5 µl Fyn 02 and 30 µl protein A sepharose; or 4 µl anti-Src, 1 µl rabbit-anti-mouse (Dako) and 30 µl protein A sepharose in the presence of 1 mg/ml BSA for 18 h at 4°C with gentle rotation. Immunoprecipitates were washed and subjected to the kinase reaction as previously described [14]. Samples were separated by 10% SDS-PAGE, dried and exposed to film at –70°C with intensifying screen and on Phosphoimager plates. Quantification from films and phosphoimager plates yielded the same results.

PAG constructs

To express N-terminally Flag-tagged PAG, an oligonucleotide containing the CD8a leader sequence (aa 1–21) and FLAG tag was ligated into pGEM-5Zf vector using the Aat II-Nco I sites. The PAG sequence was then inserted at the Nco I-Not I site. The Flag-tagged PAG was excised from the pGEM vector and inserted into pEF-IRES using Sma I-Not I ligation. The Nhe I site within the CD8-Flag tag was used for screening the colonies. Sequence integrity was verified by sequencing (GATC Biotech). Stop mutants were generated using the Quick-change site directed mutagenesis kit II (Stratagene) following the manufacturers instructions. The primer sequences used were:

STOP1-f (ACAGCATAGTGGGGACCATTAGAACCTGATGAACGTGC),

STOP1-r (GCACGTTCATCAGGTTCTAATGGTCCCCACTATGCTGT),

STOP2-f (GATCTGCTGGATTCCTAGGACAGCACAGGGAAAC),

STOP2-r (GTTTCCCTGTGCTGTCCTAGGAATCCAGCAGATC),

STOP3-f (CGTCAAAGTGTTAATGTATAGAGTATCCTTGG AAATTC),

STOP3- r (GAATTTCCAAGGATACTCTATACATTAACACTTTGACG),

STOP4-f (GCTACTGTTAAAGACTTCTAAAAAACTCCAAACAGCAC),

STOP4-r (GTGCTGTTTGGAGTTTTTTAGAAGTCTTTAACAGTAGC).

Developmental expression of PAG in brain

The function of PAG was first defined as a Csk-binding protein. However, Csk expression in brain is strongly developmentally regulated and expression in adult brain was reported to be limited to the olfactory bulb [27]. Therefore, we tested the mRNA expression of PAG as well as candidate interaction partners at different stages in mouse brain development. Time points were chosen to reflect early embryonal Csk expression at a time when the embryos head can first be separately analyzed (E12), the peak of Csk expression (P1), myelinating juvenile brain (P42), and adult brain (P60). RT-PCR analysis (Fig. 1A) shows that PAG is expressed at all of these time points. We confirm that Csk expression peaks around P1, but contrary to previous reports [27] we show considerable expression in juvenile and adult brain. In agreement with previous work, we demonstrate that the expression of the Csk-homologous kinase CHK is regulated opposite to that of Csk with expression detected from P1 onwards, while Fyn is expressed throughout. We now focused our analysis on postnatal and adult brains as these time points showed the strongest differences in Csk-expression, as well as in 6 week old brains, where Fyn activity is important for proper myelination [4]. Western blot analysis (Fig. 1B) shows that PAG protein expression is strongest at P1 whereas it is decreased in 6 week and 3 month old brains. Csk protein expression is strong at P1, but hardly detectable at 6 weeks and 3 months, while CHK expression remains strong throughout. Fyn expression is well visible at P1 and decreases slightly at the later time points, while expression of Src remains fairly constant. Interestingly, phosphorylation of Y529, the negative regulatory site within SFKs phosphorylated by Csk and CHK, is very high at P1 and is much weaker at the later time points. This difference cannot simply be explained by changes in the expression levels of Fyn and Src, but fits rather well with the higher expression of Csk and CHK at P1.

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Figure 1. Expression of PAG during brain development.

A) Total RNA was isolated from whole C57Bl6 mouse brains (head or whole embryo for E12) of different ages as indicated. The expression of PAG-mRNA and functionally related genes was analyzed following an RT-reaction and PCR using gene-specific primers. CHK-RT-PCR produced a band at the expected molecular weight (460 bp) as well as a much weaker band at 560 bp. Sequencing revealed that the latter band represented an incompletely spliced product including intron 10. One representative out of three similar experiments is shown. B) Expression of PAG and functionally related proteins was analyzed by Western blot from whole brain lysate of postnatal C57Bl6 mice of different ages as indicated. PAG was detected here with the antiserum against the whole cytoplasmic domain. Detection with the anti-PAG peptide antiserum Ig452 resulted in a similar signal. As all structural proteins tested showed differential expression during development, equal loading was assured by determination of protein concentration (50 µg/lane) and controlled for by Coomassie staining of the gels (not shown). A double band for CHK at P1 was consistently shown with both a polyclonal anti-CHK-antiserum and a monoclonal antibody against this protein and may represent two different isoforms or phosphorylated forms. A similar double band has previously been shown in Western blot [55]. One representative out of four similar experiments is shown.

https://doi.org/10.1371/journal.pone.0023978.g001

Localization of PAG expression in postnatal and adult mouse brain

As postnatal and adult mouse brain showed striking differences in the levels of Csk and, to a lesser extent, PAG expression, we next studied whether the localization of PAG-mRNA expression differed at these time points. Measuring the mean density in autoradiographs we found that overall expression of PAG-mRNA in adult brains was 50% of that in P1 brains (Fig. 2), correlating well to the difference in protein expression (Fig. 1B). At both ages, a neuronal expression pattern dominated. At P1, PAG-mRNA expression was high in most areas of gray matter, namely cerebral cortex, hippocampus, septal nuclei, habenula, olfactory bulb, and striatum. In adult mouse brain PAG-mRNA expression was concentrated in the limbic system and in cerebellum. The highest expression levels were found in the hippocampus, particularly in the CA3 area and the dentate gyrus (Fig. 3), in the septal nuclei, medial habenula, and the pineal gland. Furthermore, cerebellar cortex showed a striking expression in the Purkinje cell layer. Intermediate expression levels were found in cerebral cortex, thalamus, and olfactory bulb, particularly in the mitral cell layer and inner granule cell layer. Brain stem showed a lower PAG expression and no particular nuclei could be delineated. In spinal cord, PAG-mRNA was concentrated in gray matter and expression showed a gradient towards higher expression in the dorsal horns (not shown). White matter showed a low expression of PAG-mRNA, which nevertheless exceeded background levels.

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Figure 2. In situ distribution of PAG transcripts.

Film autoradiographs of horizontal mouse brain sections showing PAG mRNA distribution in A) adult and B) postnatal (P1) mice. The respective sense controls are shown below (C, D). In the adult brain most prominent mRNA expression was detectable in septum (S), medial habenula (MHb), thalamic nuclei (Th), hippocampus (Hi), and cerebellum (Cb). One representative out of two similar experiments is shown.

https://doi.org/10.1371/journal.pone.0023978.g002

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Figure 3. Localization of PAG transcripts in specific regions of adult brain.

Representative dark-field micrographs (A, C, E, G, I, L) illustrating the hybridization and the respective bright-field (B, D, F, H, K, M) micrographs in adult mouse brain. Pictures are taken from horizontal sections, with the exception of L and M, which are photographed from frontal sections. A, B) Septal nuclei (SepN), C, D) habenula (MHb), E, F) hippocampus: CA2 and 3 and dentate gyrus (DG), G, H) cerebellum (ML: molecular layer, Pu: Purkinje cell layer, GL: granular cell layer), I, K) thalamus (Th), L, M) pineal gland (PG). Scale bar 200 µm.

https://doi.org/10.1371/journal.pone.0023978.g003

PAG binding partners

Within the immune system, the binding and recruitment of Csk into lipid rafts, thereby regulating the activity of Src family kinases, has been defined as a crucial function of PAG. We show here, that Y314 of PAG, the residue critical for Csk binding, is phosphorylated with little difference in developing and adult brain (Fig. 4A). Given the low expression of Csk and the specific localization of PAG expression in adult brain, we tested whether Csk can still be found associated at this time point. We could readily reproduce Csk-binding to PAG at P1; at 6 weeks and 3 months very little Csk can be co-precipitated. As the SH2 domain of CHK is highly homologous to Csk and CHK expression, contrary to Csk, increases during brain maturation, we tested whether CHK can also associate to PAG. Using both a polyclonal anti-CHK-serum and a monoclonal anti-CHK-antibody, we could co-precipitate CHK with PAG in developing and adult brain. As both Csk and CHK run at similar molecular weights and the overall homology between both proteins is ∼50% (this is also true of the C-terminal 100 amino acids to which the antibodies were generated) the specificity of our antibodies was tested in Csk-and CHK immunoprecipitates, where no cross-reactivity was shown (Fig. 4B). Furthermore, both the anti-CHK-antiserum and the anti-CHK–antibody did not cross-react with mouse Csk overexpressed in HEK-293 cells. Thus, we can demonstrate a specific association of CHK to PAG in mouse brain.

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Figure 4. Binding partners of PAG in postnatal and adult brain.

A) PAG immunoprecipitates from whole brain lysates of newborn, 6 month old, and adult mice were analyzed by Western blot. Each association was shown in at least three independent experiments. B) Csk and CHK were immunoprecipitated from lysates of adult mouse brain. Western blot analysis with CHK and Csk-antibodies, respectively, reveals no cross-reactivity. C) HEK-293 cells were transfected with a mouse-Csk-CFP construct versus vector containing CFP alone. Over-expression is demonstrated with the anti-Csk-antibody. There is no cross-reactivity of the anti-CHK-antibody with the over-expressed Csk. Csk-CFP is indicated with an arrow, endogenous Csk with an asterisk.

https://doi.org/10.1371/journal.pone.0023978.g004

PAG has been shown to be phosphorylated by Src kinases, particularly Fyn. In brains of postnatal Fyn-deficient mice a reduced total tyrosine phosphorylation of PAG was shown [20], however, the binding of Fyn to PAG in CNS cells or tissue has not been demonstrated to date. We show that in postnatal, 6 week, and three month old brains Fyn is associated to PAG. Moreover, we demonstrate the binding of Src in developing and mature brain (Fig. 4A).

We could not detect an association of Lyn to PAG in our whole brain extracts (data not shown), which had been demonstrated in mast cells [18]. However, this may be explained by the lower expression levels of Lyn during development and its specific concentration in the cerebellum.

PAG contributes to the recruitment of Csk to lipid rafts in postnatal brain

To analyze PAG function, we generated Pag1-knockout mice by homologous recombination as described in the Materials and Methods (Fig. S1). Pag1-knockout mice are negative for the PAG protein (Fig. 5 and Fig. S3). Note that additional bands appear in Western blots from 3 month old wild type and Pag1^-/- brains that are recognized by our antiserum (Ig452), however these bands are peptide-unspecific (Fig. 6B) and thus do not represent PAG. Using an antiserum against the N-terminal peptide (P18, 1–18) and a different antiserum against the cytoplasmic domain (Rabbit anti-PAG, 97-432) we could also not detect a truncated protein (Fig. S3). Pag1^-/- mice had no alteration in birth weight, showed no obvious neurological phenotype, and appear to live to normal age with the oldest animal in our colony now reaching 2.5 years.

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Figure 5. Reduced Csk-recruitment to lipid rafts in P1- Pag1^-/- mice.

Whole brains from A) P1 wild type C57Bl6 (WT) and Pag1^-/- mice or B) 3 month old WT/ Pag1^-/- littermate pairs were lysed in GEM-lysis buffer and subjected to sucrose-density centrifugation. Fractions were analyzed by Western blotting. PAG was detected using the Ig452 antiserum. Lipid raft fractions were identified by binding of cholera toxin subunit B (Ctx) binding to GM1-lipids in a dot blot from the fractions. * Arrowheads indicate non-specific bands in 3 months old Pag1^-/- and wild type brain extracts, see also Fig. 6A.

https://doi.org/10.1371/journal.pone.0023978.g005

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Figure 6. Quantification of kinases in GEM gradients.

The kinase bands in each fraction represented in Fig. 5 were quantified from three independent experiments for A) the P1 and B) the 3 month time point. The summative signal from GEM fractions in relation to the total signal is presented as ratio to wildtype for each kinase. GEM containing fractions were determined by choleratoxin staining. For phosphotyrosine 529 the total signal in GEMs and the total signal on the blot are given in separate graphs, as most of the signal localizes to GEM fractions and the total amount of pY529 is reduced in PAG1^-/- mice (see also Fig. 6). Given are the means +/− SEM. •p<0.05, Student's t-test, all other pairs did not show significant differences.

https://doi.org/10.1371/journal.pone.0023978.g006

PAG predominantly localizes to lipid rafts in lymphocytes and postnatal mouse brain [14], [20]. We confirm that the majority of PAG is found in the lipid raft fractions in postnatal brains (Fig. 5A). In adult brains, lipid rafts are consistently found one fraction lower than at P1, probably due to the high lipid content of myelinated brain. However, rafts can clearly be isolated, demonstrated by the binding of cholera toxin to GM1-lipids. Similar to P1, PAG strongly associates with the lipid raft fractions (Fig. 5B).

The Src family kinases Fyn and Src are found both inside and outside of lipid rafts, as previously described [20]. Interestingly, while the majority of Fyn is localized to the lipid rafts in both newborn and adult brain, only a minor proportion of Src is raft-associated in newborn murine brain. In adult brain the distribution of Fyn and Src is similar. Notably, given the association of PAG with Fyn or Src in wild type-animals (Fig. 3), neither the distribution of Fyn nor Src is altered in the brains of Pag1-deficient mice (Fig. 5A and B, 6A). We next investigated whether the localization of Csk is altered in the brains of Pag1-knockout mice. We found that the amount of Csk within GEMs is reduced to 25 % of wildtype in P1 Pag1^-/- brains. (Fig. 5A, 6A, p<0,05). In agreement with this finding, the phosphorylation of the inhibitory tyrosine Y529 in Src/Fyn within GEMs, which is dependent upon Csk or CHK, is reduced to 35% in postnatal (P1) brains of Pag1-deficient mice (Fig. 5A, 6A, p<0.05). Note that the majority of the pY529 signal is found within the lipid rafts in both postnatal and adult animals. However, the amount of Csk that can be detected in lipid rafts of adult wild type mice is minute. Interestingly, the amount of lipid raft-associated Csk does not appear to differ in adult Pag1-knockouts (Fig. 5B and 6B). Phosphorylation of Y529, which is generally much lower than in newborn mice, is also unchanged in lipid rafts of adult knockout animals (Fig. 5B and 6B). Despite its association to PAG in wild type mice, the distribution of CHK is not altered in either newborn or adult Pag1^-/- mice (Fig. 5A, B, and 6A, B).

To compare total expression levels and tyrosine phosphorylation, we investigated whole brain lysate of wild type and Pag1^-/- mice (Fig. 7). Pag1-deficiency (Fig. 7A) did not lead to a change in the expression of Csk and CHK or the Src-kinases Fyn and Src in either postnatal or adult brain (Fig. 7B). In postnatal brain however, phosphorylation of the inhibitory tyrosine in SFKs was reduced by 42% in knockout mice (analyzed over 4 independent experiments), paralleling the reduction of Csk in the lipid raft fractions (Fig. 7B and C). In brain lysate of adult mice, a trend to a reduction of around 14% in the pY529 signal is observed, which is not significant on statistical testing (p = 0.18), indicating at least a partial compensation for the lack of PAG during brain maturation (6 independent experiments; Fig. 7C).

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Figure 7. Decreased phosphorylation of Src-kinase negative-regulatory tyrosine 529 in P1- Pag1^-/- mice.

For P1-material, protein extracts were prepared from separate newborn litters of time-mated Pag1^-/- mice and wild type C57Bl6 mice. For 3 months-material, protein extracts were prepared from adult Pag1^-/- and wild type littermates of Pag1^+/- crossings. A) Incubation with anti-PAG-antiserum Ig452 detects a band at 75-80 kDa in brain extracts of 3 month old Pag1^-/- mice. Co-incubation with the antigenic peptide abolished the specific PAG-band in WT mice, but left the additional band unchanged in both WT and Pag1^-/- extracts, indicating that this band is not peptide-specific. B) Equal concentrations of protein from each sample were analyzed by immunoblotting for PAG (Ig452), Csk, CHK, pY529, Fyn, and Src. Actin staining served as loading control. C) Phosphorylation of the negative regulatory tyrosine (pY529) was quantified in different experiments and is presented as the ratio to wild type. Mean and SEM are given for n = 4 (P1) and n = 6 (3 months) independent experiments. ** p<0.01, n.s. not significant, Student's t-test.

https://doi.org/10.1371/journal.pone.0023978.g007

PAG differentially modulates Src kinase activity in postnatal and adult brain

To test whether the decreased phosphorylation of the inhibitory tyrosine is associated with increased kinase activity in postnatal Pag1^-/- mice, we next performed in vitro kinase assays for Fyn and Src from whole brain lysates. No difference was observed (data not shown). However, as PAG is predominantly found within the rafts, we hypothesized that it might exert its regulatory function only on a subset of SFKs. Thus, when the Src kinases were precipitated from the lipid rafts, Pag1^-/- mice showed an increase in both auto- and substrate phosphorylation. The basal activity of Fyn was increased by 50% (p<0,05), Src activity showed a similar trend, however the result was not significant (p = 0.31) (Fig. 8A, C). This corresponded well to a 40% decrease of Y529 phosphorylation, which was significant in both Fyn- and Src-immunoprecipitates (Fig. 8E). To our surprise, adult Pag1^-/- brains showed the reverse phenotype with a decrease in basal Fyn and Src kinase activity of −20% and −28%, respectively (p<0.05 and p<0.01, resp., Fig. 8B, D), despite normal Csk-distribution and nearly normal Y529 phosphorylation (Fig. 8F), indicating a net change of 70–80% in kinase activity within three months. The phosphorylation of other regulatory tyrosines (Y418, Fyn Y215) was not altered in adult Pag1^-/- brains (data not shown). As a possible substitute for PAG in brain we explored LIME, another lipid-raft-associated Csk-binding phosphoprotein with adaptor function [28], [29]. Although in situ-hybridisation data suggest that LIME is indeed expressed within this organ (http://www.brain-map.org), we were unable to confirm protein expression in mouse brain due to strong cross-reactivity of our antibodies/-sera. However, LIME is unlikely to function as the main compensator for the lack of PAG as Lime1^-/-/ Pag1^-/- double knockout mice are viable and fertile (J. Lindquist, unpublished observation). Another lipid-raft –bound Fyn-substrate, which phospho-dependently binds Csk, is PSD93, an important component of neuronal postsynaptic densities [30]. Belonging to the family of membrane-associated guanylate kinases, PSD93 also functions as an adaptor. We showed increasing expression in the first postnatal weeks (Fig. 9A). Furthermore, in adult brain a greater proportion of the cellular PSD93 is localized in lipid rafts of WT and Pag1^-/- mice (Fig. 9B). At 3 months a much stronger association to Csk compared to P1 could be found (Fig. 9C). After repeated immunoprecipitation of PSD93 from GEMs, Csk was also reduced (Fig. 9D), indicating that PSD93 binds Csk within the GEMs and can recruit Csk to the membrane possibly substituting for PAG in the brains of older mice. Note, PSD93 can be co-precipitated with Csk in abundance, while the Csk-PAG-association can in our hands only be shown via immunoprecipitating PAG, not vice versa. Therefore, one roles of PSD93 in adult WT mice might be the recruitment of Csk, and the amount of PSD93 that could be additionally bound to Csk to substitute for PAG in adult Pag1^-/- mice may not be detectable (Fig. 9E).

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Figure 8. Src kinase activity is altered in both postnatal and adult Pag1^-/- brain.

GEM-containing fractions (identified via cholera toxin subunit B-binding) of A) postnatal or B) adult wild type and Pag1^-/- brains were pooled, 10% was retained for a Western blot control, the rest was split into two samples, from which Fyn and Src, respectively, were precipitated. Precipitates were again split in halves and subjected to either in vitro kinase assay (upper panels) or Western blot (lower panels) which controlled for equal amounts of kinase precipitated. C) and D) Kinase activities are presented as ratio to wild type. E) and F) Phosphorylated Y529 was quantified in the Western blot controls of Fyn and Src immunoprecipitates and normalized to the amount of precipitated SFK. Given are the means +/- SEM, n =  number of independent experiments. p<0.05, ** p<0.01, n.s. not significant, Student's t-test.

https://doi.org/10.1371/journal.pone.0023978.g008

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Figure 9. Developmental expression and Csk-binding of PSD93.

A) Whole brain lysates from WT mice of the indicated ages were Western blotted and stained for PSD93. B) Brains of P1 wild type and Pag1^-/- mice and 3 month old WT/ Pag1^-/- littermate pairs were lysed at concentrations of 3 ml/g and 4.5 ml/g, respectively, in GEM-lysis buffer and subjected to sucrose-density centrifugation. Fractions were analyzed by Western blotting and staining for PSD93. Lipid raft fractions were identified by binding of cholera toxin subunit B (Ctx) binding to GM1-lipids in a dot blot from the fractions. C) Densitometric quantification of the PSD93 signal in GEM-fractions as percentage of the total PSD93-signal. For both time points, the PSD93 signal in fractions 2-5 was expressed as a ratio to control. This most likely overestimates the lipid raft localized material in P1, as only fraction 2 and 3 contain rafts (n = 3 independent experiments for each time point) D) Csk-immunoprecipitates from whole brain lysates of WT mice (ages as indicated), stained for PSD93 and Csk. Densitometric quantification of the relative amount of PSD93 bound to Csk in brains of P1 and 3 month old mice (n = 3 independent experiments) E) Csk-immunoprecipitates from whole brain lysates of 3 month old WT and Pag1^-/- mice stained for PSD93 and Csk. Two exposures are given for the PSD93-signal in the left panel. Comparison of whole brain lysates of 3 month old WT and Pag1^-/- to P1. Given are the means +/- SEM, n.s. not significant, Student's t-test.

https://doi.org/10.1371/journal.pone.0023978.g009

SH2-dependent binding of Fyn to PAG may lead to an active conformation

The surprising finding that SFK activity is decreased in the absence of PAG lead us to hypothesize that one function of PAG may be to keep Src kinases in an open conformation. Thus we investigated the Fyn binding site in PAG. We constructed several N-terminally tagged STOP-mutants of PAG (Fig. S4) and expressed them in HEK 293T cells (Fig. S3). Membrane targeting of the STOP mutants is shown in Fig. S5. In vitro kinase assays demonstrated that Fyn kinase activity was associated with WT PAG as well as with the STOP3 and STOP4 constructs. However, kinase activity was not seen with either STOP1 or STOP2, which lack the N-terminal proline rich region (Fig. S4B). Previously, the PAG-Fyn-association was proposed to be constitutive, mediated by the Fyn-SH3 domain [14], however, a contribution of the SH2-domain was suggested [14], [31]. To confirm this result, Fyn immunoprecipitates were performed from transfected cells and probed with anti-Flag (Fig. S4C). Surprisingly, Fyn binding is observed with all mutants, except STOP 1, indicating that Fyn can also bind to Y105. Together these results identify the membrane proximal proline-rich region and Y105 as potential binding sites for the SH3 and SH2 domains of Fyn, respectively. Binding of the Fyn SH2-domain to PAG may prevent the intramolecular binding of the C-terminus, when phosphorylated at the inhibitory tyrosine. By this mechanism, PAG may prevent SFKs from adapting the closed inactive conformation.