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Previous Article | Next Article
The Journal of Neuroscience, October 15, 2002, 22(20):8827-8837
A Receptor for Activated C Kinase Is Part of Messenger Ribonucleoprotein Complexes Associated with PolyA-mRNAs in Neurons
Frank Angenstein1, Anne M. Evans2, Robert E. Settlage2, 4, Stewart T. Moran1, Shuo-Chien Ling1, Anna Y. Klintsova1, Jeffrey Shabanowitz2, Donald F. Hunt2, 3, and William T. Greenough1 1 Beckman Institute/Neuronal Pattern Analysis, University of Illinois, Urbana, Illinois 61801, Departments of 2 Chemistry and 3 Pathology, University of Virginia, Charlottesville, Virginia 22904, and 4 ProteoMS, LLC, Charlottesville, Virginia 22903
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Long-lasting changes in synaptic functions after an appropriate stimulus require altered protein expression at the synapse. To restrict changes in protein composition to activated synapses, proteins may be synthesized locally as a result of transmitter receptor-triggered signaling pathways. Second messenger-controlled mechanisms that affect mRNA translation are essentially unknown. Here we report that a receptor for activated C kinase, RACK1, is a component of messenger ribonucleoprotein (mRNP) complexes. RACK1 is predominantly associated with polysome-bound, polyA-mRNAs that are being actively translated. We find it to be present in a complex with
-tubulin and at least two mRNA-binding proteins, polyA-binding protein 1 and a 130 kDa polyA-mRNA binding protein (KIAA0217). Activation of PKC
Key words: translational control; messenger ribonucleoproteins; metabotropic glutamate receptor; protein kinase C; protein phosphorylation; polyA-mRNA; mass spectrometry
INTRODUCTION
Rapid receptor-mediated control of local, postsynaptic protein synthesis is an intriguing mechanism for producing long-lasting changes in the efficiency of synaptic transmission. Moreover, there is now increasing evidence that activity-dependent control of protein synthesis, at the level of translation, is mediated at least partly by metabotropic glutamate receptor-triggered signaling pathways (Huber et al., 2000
; Raymond et al., 2000
Localized changes in mRNA translation near activated synapses could be achieved by at least three different mechanisms: (1) receptor-mediated control of mRNA transport to dendrites, as has been described recently for Arc (Roberts et al., 1998
On the basis of the possibility that translational control at synapses leads to a selective rather than a general change in protein synthesis, we focused in this study on mRNPs that could serve as a detector for synapse activity and in response could locally affect the translation of particular mRNAs. Here, we demonstrate that a receptor for activated C kinase, RACK1, is associated with polyA-mRNAs and, furthermore, that in rat hippocampal slices mGluR stimulation controls the movement and binding of RACK1 together with activated protein kinase C
MATERIALS AND METHODS
Preparation of mRNPs. Cortex or hippocampal slices of 15- to 19-d-old Long-Evans rats were homogenized in buffer A containing 125 mM NaCl, 100 mM sucrose, 50 mM HEPES, 2 mM potassium acetate, and 40 U/ml of an RNase-inhibitor, RNasin (Promega), and centrifuged for 2 min at 4000 × g (postnuclear supernatant) followed by 10 min at 14,000 × g (postmitochondrial supernatant). The supernatant was lysed (final concentration: 50 mM Tris/HCl, pH 7.5, 1% NP40, 50 mM NaCl, 4 mM MgCl2, 45 µg/ml cycloheximide) and layered on a discontinuous sucrose gradient (4.5 ml of 12% sucrose and 4.5 ml of 33.5% sucrose). The tubes were centrifuged for 90 min at 41,000 rpm in a SW41 rotor (Beckman L8-70M centrifuge). To dissociate ribosomes/polysomes and release polyA-mRNA/mRNP complexes, the resulting pellet (monosomes and polysomes; see Fig. 1A) was resuspended in a solution (pellet buffer) containing 30 mM EDTA, 0.5% NP40, 20 mM Tris/HCl, pH 7.5, and kept on ice for 10 min. The interfaces were recovered and centrifuged again for 20 min at 400,000 ×g in a Beckman TL-100 ultracentrifuge. The resulting pellets, which contained mRNPs, free 40S, and 60S ribosomal subunits, and a small subfraction of monosomes (see Fig. 1A) were resuspended in the pellet buffer and kept for 10 min at 4°C. The suspension was centrifuged for 2 min at 14,000 × g, and the supernatant was used for both the oligo(dT)-cellulose binding assay and for RACK1 immunoprecipitation (see below). The KCl concentration was adjusted to 200 mM and then 40 µl of prewashed oligo(dT)-cellulose (100 µg/ml; Sigma, St. Louis, MO) was added. After 90 min of constant rotation at 4°C, the cellulose was washed three times with 1 ml wash buffer (20 mM Tris/HCl, pH 7.5, 100 mM KCl, 5 mM MgCl2). PolyA-mRNAs and attached mRNPs were eluted with 200 µl of 10 mM Tris/HCl, pH 7.5, and proteins were then precipitated with 1 ml of 10% trichloroacetic acid in acetone. Precipitated proteins were washed with acetone and finally solubilized in 70 µl of SDS sample buffer (4% SDS, 250 mM Tris, 50 mM DTT, 3 mM EDTA, 20% glycerol, pH 8.0). The sample was boiled, and 25 µl of aliquot was loaded on a 5-20% polyacrylamide gel.
Polysome profile. For each profile, one cortex of a 15- to 19-d-old rat was homogenized in 2 ml of buffer A. The homogenate was first centrifuged for 5 min at 4000 × g, and the supernatant was centrifuged again for 10 min at 14,000 × g. The resulting postmitochondrial supernatant was then lysed as described above. The lysate was layered on 1.5 ml of 15% sucrose and centrifuged for 11 min at 400,000 × g. The resulting pellet was resuspended in 500 µl of a buffer containing 20 mM Tris/HCl, pH 7.5, 10 mM MgCl2, 100 mM NH4Cl, 2 mM KAc, 225 µg/ml cycloheximide. The suspension was then layered on 10.4 ml of a 15-45% continuous sucrose gradient in 20 mM Tris/HCl, pH 9.0, 80 mM NaCl, 3 mM MgCl2, and 0.02%
RACK1 immunoprecipitation. mRNA/mRNP complexes were released from polysomes on treatment with 30 mM EDTA as described above. After centrifugation the supernatant was adjusted to 20 mM TBS, pH 8.0, 0.5% NP40, and precleared by incubation with 50 µl of anti-IgM agarose (Sigma) or 40 µl of protein A agarose (Santa Cruz Biotechnology, Santa Cruz, CA). For immunoprecipitation, RACK1 monoclonal antibody (mAb) [3 µl, IgM (Transduction Laboratories, Lexington, KY) or IgG (Santa Cruz Biotechnology, Inc., Santa Cruz, CA)] bound either to 30 µl of anti-IgM-agarose or to 30 µl of protein A-agarose was then added to the precleared supernatant and incubated, with constant agitation, for 2 hr at 4°C.
Samples were washed two times with 1 ml TBS/0.5% NP40 and two times with TBS, and the resulting pellet was boiled for 4 min with 70 µl of solubilizer. Anti-IgM-agarose or protein A-agarose was removed by centrifugation, and the resulting supernatant was used for Western blot analysis. For detection of RACK1-interacting proteins, RACK1-containing protein complexes were released from the anti-IgM-agarose beads after incubation with 60 µl of 0.1 M glycine, pH 3.0. Released proteins were either analyzed directly by mass spectrometry or solubilized and separated by SDS-PAGE and then analyzed by mass spectrometry. Coimmunoprecipitated proteins were cut out and identified by mass spectrometry.
Northwestern blot assay. RACK1 and coimmunoprecipitated proteins were separated by SDS-PAGE and blotted onto nitrocellulose. Detection of putative mRNA-binding proteins was performed as described by Holcik and Liebhaber (1997)
-32P ATP and poly(A) polymerase (USB Corp., Cleveland OH), precipitated with ammonium acetate/ethanol, washed, and finally resuspended in 10 mM Tris/HCl, pH 8.0. Labeled polyA-mRNA was added to the hybridization solution (final concentration ~200,000 cpm/ml), and the nitrocellulose membrane was incubated in this solution for 120 min at room temperature. After a series of washes, the blot was dried, and bound radioactivity was detected by phosphoimaging (Fujix-Bas1000).
Yeast two-hybrid assay. A full-length ORF of RACK1 was amplified from cerebellar cDNA by the PCR, with EcoRI and BamHIII sites added at the end of the 3' end primer and 5' end primer, respectively. The construct was inserted into a TOPO-TA vector (Invitrogen) and subsequently subcloned into the pGBKT7 (bait) vector (Clonetech). To get the full-length ORF of PABP1, we amplified the 3' end (1-707, an internal HindIII sequence) by PCR using a PABP1-pBSK+ vector (a generous gift from Dr. E. Mohr, University of Hamburg, Hamburg, Germany), with EcoRI and HindIII added to the primer. The PABP1-pBSK+ vector was digested with EcoRI and HindIII, and the resulting fragment PABP1-708-1911 was ligated with the PCR product (PABP1-1-707) and inserted into a pGAD424 (prey) vector (Clonetech). Proper orientation of the insert was tested by control digestion with HindIII-BamHI or KpnI-DraIII. Both vectors were transformed into yeast, and a possible direct protein interaction between RACK1 and PABP1 was measured using a
In vitro phosphorylation assay. mRNPs were prepared from the 33.5% sucrose pellet as described above. Washed oligo(dT)-cellulose containing bound proteins was resuspended in kinase buffer (20 mM Tris/HCl, pH 7.5, 10 mM MgCl2, 8% glycerol, 100 mM KCl). For detection of endogenous kinase activity, one aliquot of this sample was treated with 1 µCi 33P-
ATP (final ATP concentration 50 µM). For PKC
In situ phosphorylation of mRNP. Approximately 40 transverse 400-µM-thick hippocampal slices from 17-d-old rats were prepared and incubated in interface chambers in a medium containing (in mM): NaCl 134.0, KCl 6.24, MgSO4 1.3, CaCl2 2.0, NaHCO3 16, and glucose 10 (pH 7.4, 32°C). The medium was aerated with carbogen (95% O2, 5% CO2) throughout the experiment. After 60 min of preincubation, 200 µCi 33Pi (final concentration in the medium 100 µCi/ml; Amersham) was added, and the slices were labeled for 90 min. During the last 30 min of slice incubation, 1 µM okadaic acid was present to inhibit phosphatase activities. Then slices were homogenized in 1.5 ml buffer A, and mRNP was prepared as described above except that 1 µM okadaic acid was added to all buffers.
Identification of mRNPs by mass spectrometry. In-gel digestion and extraction of the proteins was accomplished using a modification of the method of Wilm et al. (1996)
Extraction was accomplished by alternating dehydration-hydration steps, collecting, and pooling the solutions resulting from each step as follows. First the gel pieces were dehydrated (50% ACN, 5% formic acid) and dried in the vacuum centrifuge. The gel pieces were then rehydrated (AMBIC) and dehydrated (50% ACN, 5% formic acid) again. This was followed by two more steps of dehydration (100% ACN) and rehydration (AMBIC). The pooled supernatants were reduced to near dryness, reconstituted to 50 µl (1% acetic acid), reduced to near dryness again, and finally reconstituted to 40 µl with 1% acetic acid to give the final solution.
Aliquots (5 µl) of the gel digests were analyzed by nano-reverse phase HPLC-micro-electrospray ionization-mass spectrometry on an LCQ mass spectrometer (MS) (Finnigan, San Jose, CA). Data from ~1 hr of run time (~1000 MS/MS spectra per hour) were acquired on each sample. The data were acquired using data-dependent analysis in which one MS scan was followed by collisionally activated dissociation (CAD) of the top five most abundant ions present in the MS scan. Isotope exclusion was used to exclude analysis of isotope ions. Dynamic exclusion was used to reduce the redundancy of the data. Dynamic exclusion settings were repeat count 1, pre-exclude time 30 sec, exclude time 1 min. Filtering software was used to (1) reduce the number of low quality CADs, (2) determine the charge state of the peptides analyzed, and (3) recalibrate the parent mass. Data passing through the above filters were searched against the all nonredundant GenBank [National Center for Biotechnology Information (NCBI)] database using Sequest (Finnigan, San Jose, CA). All reported hits were verified manually.
Immunocytochemistry. Two female and two male 15-d-old Long-Evans rats were anesthetized deeply and perfused transcardially with 10 ml of heparin saline (1000 U/ml), followed first by 50 ml of fixative containing 3.75% acrolein and 2% paraformaldehyde in 0.1 M phosphate buffer (PB), pH 7.4, and then with 200 ml of 2% paraformaldehyde in PB. The brains were removed, postfixed in the final fixative for 1 hr, and sectioned at 40 µm on a vibratome. The sections were collected in PB and then treated with 1% sodium borohydride for 30 min to improve antigenicity and reduce nonspecific immunolabeling. To further reduce the nonspecific labeling before incubation in primary antibody, the sections were treated for 30 min in a washing solution consisting of 0.8% BSA and 0.1% fish gelatin in 0.01 M PBS. Sections were incubated in primary anti-RACK1 antibody (1:2000) in washing solution for 24 hr at 4°C. Sections were rinsed in washing buffer and transferred for 30 min to a 1:50 dilution of goat anti-mouse gold-conjugated IgM (Amersham). The gold particles were enlarged by reaction with silver solution from an IntenS-EM kit (Amersham). For electron microscopy the sections were postfixed in 2% osmium tetroxide in 0.1 M phosphate buffer, dehydrated, and flat-embedded between a slide and a coverslip that had been treated with liquid release agent (Electron Microscopy Sciences). Ultrathin sections from the CA1 subfield of the hippocampus, somatosensory cortex, and cerebellar cortex were collected on Formvar-coated slot grids, stained with uranyl acetate and lead citrate, and examined with a Philips CM-200 electron microscope.
RESULTS
RACK1 is a component of mRNP complexes associated with translated mRNAs
To characterize proteins that were part of the mRNP complex associated with translated (polysome-bound) or nontranslated (not ribosome-bound) mRNAs, we first separated polysomes from free ribosomal subunits/monosomes by discontinuous sucrose gradient centrifugation (Fig. 1A). The polyA-mRNAs/mRNP complexes were purified using oligo(dT)-cellulose and released by 10 mM Tris, pH 7.5, either for direct mass spectrometry analysis or for SDS-PAGE separation. Proteins, which were first separated by SDS-PAGE, were excised, eluted, and then identified by mass spectrometry or, alternatively, transferred onto nitrocellulose and detected by Western blot assay. With this approach we found, in addition to a number of known mRNA-binding proteins, such as heterogeneous nuclear (hn) RNP-A/B/C/D/E/G/H/K/l/Q3/R/U, HuA/B/C/D/R/, pRENT1, nucleolin, FMRP, staufen, and polyA binding protein 1 (unpublished observations), the RACK1 protein in fractions corresponding to translated mRNAs. The identity of RACK1 was determined from the detection of 13 different peptide sequences (Table 1), all of which were specific for RACK1 protein as determined with BLAST2.0 using all nonredundant GenBank databases provided by NCBI. Furthermore, the presence of RACK1 in this fraction was confirmed by Western blot assay and is comparable to the localization of FMRP, which is already known to be associated with polyA-mRNAs in actively translating polysomes (Corbin et al., 1997
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Figure 1. Preparation of mRNPs and detection of RACK1. A, Nontranslated mRNAs were separated from translated mRNAs by discontinuous sucrose density gradient centrifugation. Separation of the resulting interfaces and pellet by a 15-45% continuous sucrose gradient revealed that free mRNA/mRNP complexes and particles smaller than 40S were enriched in the first interface and free ribosomal subunits and monosomes were enriched in the second (12%-33% sucrose density) interface, whereas polysomes were found in the 33% sucrose pellet (right side). B, PolyA-mRNAs were purified from each fraction by binding to oligo(dT)-cellulose and, together with copurified proteins, eluted with 10 mM Tris/HCl, separated by SDS-PAGE, and silver-stained. C, Western blot analysis of the same samples using monoclonal antibodies recognizing RACK1, FMRP, PABP1 (location indicated by an arrow), and G3BP-2a. 1, Fraction 1; 2, fraction 2; 3, fraction 3.
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Table 1. Detected amino acid sequences specific for RACK1 within the protein fraction associated with translated mRNAs Although the detection of PABP1 and other well known mRNPs in this fraction confirms the validity of the method used to enrich mRNPs, the simultaneous identification of RACK1 in this fraction was surprising, because RACK1 does not contain any known mRNA binding domains. However, by releasing the entire mRNP complex from polyA-mRNAs, we also might have obtained proteins that were linked to mRNAs via other proteins. One problem of using oligo(dT)-cellulose to purify proteins assumed to be bound to polyA-mRNAs is that a number of proteins bind in a polyA-mRNA-independent manner to oligo(dT)-cellulose, especially in fraction one (Fig. 2). Thus, treatment of the sample before oligo(dT)-cellulose binding with RNase A (10 µg/ml) did not prevent the binding of a number of proteins to the beads (data not shown). To reduce the presence of unspecific bound proteins, we focused therefore only on proteins that can be released from oligo(dT)-cellulose by 10 mM Tris/HCl, pH 7.5. Because the interaction between polyA-mRNA and oligo(dT)-cellulose is impaired in a salt-free buffer, mainly polyA-mRNAs together with associated proteins should be released under this condition. This procedure clearly reduced the presence of proteins that are not part of mRNP complexes, because after treatment with RNase-A, no proteins were present in the released fraction. However, it should be noted that there is not a complete release of polyA-mRNAs under this condition. Thus, mRNA-binding proteins such as PABP1 are still detectable among oligo(dT)-cellulose bound proteins after elution with 10 mM Tris/HCl (data not shown). To further determine whether RACK1 is in fact part of the mRNP complex and was not nonspecifically captured by the tracer cellulose, we added polyA and polyU oligonucleotides to compete with the binding of polyA-mRNAs to oligo(dT)-cellulose (Fig. 3A). Furthermore, elution of polyA-mRNAs by 10 mM Tris/HCl from both oligo(dT)-cellulose and polyU-agarose coreleased the RACK1 protein, indicating that RACK1 does not simply bind nonspecifically to cellulose (Fig. 3B). That RACK1 binds in fact via polyA-mRNAs to oligo(dT)-cellulose is supported by the finding that RNase A (10 µg/ml) in the binding buffer completely abolished the binding of RACK1 to oligo(dT)-cellulose (Fig. 3B).
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Figure 2. Comparison of oligo(dT)-cellulose bound proteins with proteins that can be eluted with polyA-mRNAs by 10 mM Tris/HCl. A postmitochondrial supernatant was stimulated with PS/DAG, and oligo(dT)-cellulose bound proteins were prepared from both interfaces and the 33% sucrose pellet and released either by SDS-sample buffer (4% SDS, 250 mM Tris, 50 mM DTT, 3 mM EDTA, 20% glycerol, pH 8.0) or by 10 mM Tris/HCl, pH 7.5. Although a number of proteins bind to oligo(dT)-cellulose, only a fraction of them can be eluted together with polyA-mRNAs by 10 mM Tris/HCl (silver stain). Thus, PKC
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Figure 3. Binding of RACK1 to oligo(dT)-cellulose is mediated by polyA-mRNAs. A, PolyA and polyU oligonucleotides compete with the binding of RACK1 to oligo(dT)-cellulose. The locations of PABP1 and RACK1 in a silver-stained gel, as identified by mass spectrometry, are indicated by an arrow. Preincubation of oligo(dT)-cellulose with polyA (A) or incubation of the sample with polyU (U) during the binding resulted in decreased binding of a number of proteins, including PABP1 and RACK1, relative to control preparations (C). In contrast, the presence of polyG (G) did not affect the binding of PABP1 and RACK1 to oligo(dT)-cellulose. B, RNase A (10 µg/ml) treatment abolished the binding of RACK1 to oligo(dT)-cellulose. Under control conditions (top, first 3 lanes), RACK1 can be captured with oligo(dT)-cellulose from fraction 3 (Figs. 1, 2), which includes translated mRNAs. Treatment of these fractions with RNase A resulted in a complete absence of RACK1 among the proteins that are bound to oligo(dT)-cellulose (top, last 3 lanes). C, RACK1 can be released with polyA-mRNAs from both oligo(dT)-cellulose (first 3 lanes) and polyU-agarose (last 3 lanes). PolyA-mRNA/mRNP complexes were prepared from each fraction and incubated with oligo(dT)-cellulose or polyU-agarose and released with 10 mM Tris/HCl, pH 7.5, further indicating that RACK1 binds via polyA-mRNA and not nonspecifically to cellulose.
In an additional set of experiments we determined the localization of RACK1 within a 15-45% continuous sucrose gradient. From each fraction the polyA-mRNA/mRNP complexes were again purified using oligo(dT)-cellulose, and the presence of RACK1 and the polyA-binding protein 1 (PABP1) were detected by Western blot assay (Fig. 4). In the presence of 3 mM MgCl2 within the sucrose gradient, which is crucial for the ribosome association, RACK1 is present in fractions containing 40S ribosomal subunits and larger components (Fig. 4A). Omitting MgCl2 in the sucrose gradient led to a dissociation of ribosomes/polysomes, and therefore no polysomes were detectable. Under this condition, RACK1, comparable to PABP1, could be captured only in the first fraction containing the released polyA-mRNA/mRNP complexes as well as free mRNA/mRNP complexes (Fig. 4B). Therefore, we conclude that RACK1 is part of a protein complex that is associated with polyA-mRNAs.
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Figure 4. RACK1 is preferentially associated with translated mRNAs. Seventeen fractions of a continuous sucrose gradient (15-45%) were collected, and those containing polyA-mRNAs/mRNP complexes were purified using oligo(dT)-cellulose. The presence of RACK1 and PABP1 (indicated by arrows) was determined by Western blot assay. For that the blot was cut (at ~55 kDa); the top part was stained for PABP1 and the lower part for RACK1. A, Under the control condition, PABP1 was detectable in all fractions, whereas RACK1 appeared in the fraction that contained 40S and heavier particles (fractions 4-17). B, Absence of Mg2+ within the sucrose gradient caused a complete dissociation of polysomes, and therefore only one peak containing free ribosomal subunits was detectable. Under this condition RACK1 was not detectable in fractions higher than 11. The distribution of PABP1 changed in a similar way, except that we could detect PABP1 in fraction 17, which might correspond to translationally arrested RNA granules (Krichevsky and Kosik, 2001
RACK1 is in a complex with at least two mRNA-binding proteins
Although RACK1 does not contain any known mRNA binding domains, the protein binds to polyA-mRNAs as well as to RNA homopolymers (data not shown). However, this does not prove a direct interaction of RACK1 with mRNAs. It is also possible that RACK1 is linked by another protein to mRNAs. To search for possible candidates, we prepared the fraction used for the oligo(dT)-cellulose binding assay and performed an immunoprecipitation using a RACK1-specific antibody (clone 20, an IgM; Transduction Laboratories). To identify a possible polyA-mRNA binding protein within the RACK1-containing mRNP complex, we performed a Northwestern blot assay using 32P-labeled total polyA-mRNAs prepared from rat cortex. On the basis of this assay, RACK1 does not bind directly to polyA-mRNAs but is in a complex with at least two mRNA-binding proteins [RACK1-interacting mRNA-binding protein (Rimb)] with apparent molecular weights of 75 kDa (Rimb1) and 130 kDa (Rimb2), respectively (Fig. 5). Rimb1 and Rimb2, which coimmunoprecipitated with two different RACK1-specific monoclonal antibodies [clone 20 (Transduction Laboratories) and clone B-3, an IgG (Santa Cruz Biotechnology)] (Figs. 5, 6), were excised from the gel, and the composition was analyzed by mass spectrometry. The Rimb1 band was identified as polyA-binding protein 1 (PABP1), HSP70, and the Ras-GTPase-activating-(GAP-120)-SH3-domain-binding protein 2a (G3BP-2a) (Table 2); the presence of the PABP1 and G3BP-2a within this 75 kDa band was confirmed by Western blot assay (Fig. 6). It remains unclear why G3BP-2a appears in our preparation at 75 kDa given the fact that the calculated molecular weight of G3BP-2a is 54 kDa (Kennedy et al., 1996
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Figure 5. RACK1 is in a complex with at least two polyA-mRNA binding proteins. A, To determine whether RACK1 binds directly or via another protein to polyA-mRNAs, a Northwestern blot analysis was performed. RACK1 and coimmunoprecipitated proteins were blotted on nitrocellulose, renatured, and incubated with 32P-labeled polyA-mRNAs [ , immunoprecipitation was performed without the RACK1 IgM-mAb (negative control); +, immunoprecipitation with RACK1 IgM-mAb]. Two proteins, with an apparent molecular weight of 75 kDa (Rimb1) and 130 kDa (Rimb2), were found to bind polyA-mRNAs. RACK1, at ~32 kDa, did not bind polyA-mRNAs in this assay. The presence of RNase A (last lane) did not prevent the interaction of these proteins with RACK1. B, To identify the mRNA-binding proteins, RACK1-IgM coimmunoprecipitated proteins were released from the agarose beads by 0.1 M glycine, pH 3.0, and silver-stained. The 75 kDa (Rimb1) and 130 kDa (Rimb2) bands were cut out and analyzed by mass spectrometry. The Rimb1 protein band contained (1) the polyA-binding protein (PABP1), (2) HSP70, and (3) the Ras-GTPase-activating protein (GAP120) SH3-domain-binding protein 2a (G3BP-2a) (Table 2). The Rimb2 protein band was found to contain the protein KIAA0217, a protein with an RNA-binding domain (Nagase et al., 1996
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Figure 6. RACK1 coimmunoprecipitates with PABP1. A, RACK1 was immunoprecipitated from the protein fraction that was released from a polysomal pellet by 30 mM EDTA with two different monoclonal antibodies [left side, clone B-3, an IgG2a (Santa Cruz Biotechnology); right side, clone 20, an IgM (Transduction Laboratories)]. The immunoprecipitate was separated using SDS-PAGE and silver-stained. In confirmation of a previous experiment (Fig. 5), the additional protein at 75 kDa (left side, arrow) that was not detectable in the negative control (
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Table 2. Identification of Rimb1 (75 kDa) (Fig. 5) that coimmunoprecipitates with RACK1 (clone B-3) Rimb2 contains a number of protein sequences that correspond to a protein, KIAA0217, predicted from a partial cDNA D86971 (Nagase et al., 1996
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Table 3. Identification of Rimb2 (130 kDa) (Fig. 5) that coimmunoprecipitates with RACK1 (clone B-3) To discern whether RACK1 is in the same protein complex as PABP1, G3BP-2a, and Rimb2 (KIAA0217), a parallel immunoprecipitation was performed in the absence or presence of RNase A (final concentration 10 µg/ml) using the same starting material. To avoid protein precipitation by RNase A treatment, we first performed the immunoprecipitation, washed the beads, and then added RNase A (10 µg/ml) for 20 min at room temperature. After this treatment, we were still able to coimmunoprecipitate Rimb1 and Rimb2 with RACK1, pointing to an mRNA-independent association of RACK1 to these proteins (Fig. 5). Western blot analysis using a specific monoclonal antibody for PABP1 (clone 10E10) or a polyclonal antiserum for G3BP-2a (rabbit poly-576) revealed that only PABP1 is associated with RACK1 in an mRNA-independent manner, whereas G3BP-2a is linked to RACK1 via mRNA (Fig. 6). However, it is not clear whether RACK1 and PABP1 interact physically with each other. Using a direct yeast two-hybrid screen with RACK1 fused to the DNA-binding domain (bait) and PABP1 fused to the activation domain (prey), we could not detect a direct interaction. Therefore, we conclude that RACK1 and PABP1 are together in one protein complex. In summary, we found that RACK1 is in a complex with two mRNA-binding proteins, PABP1 and Rimb2, and in addition is linked to another mRNA-binding protein, G3BP-2a, via mRNA, which further supports the conclusion that RACK1 is a component of mRNP particles associated with poly-mRNAs.
Activation of PKC
On the basis of these findings, we concluded that RACK1 binds to mRNAs in a complex that contains PABP1 and Rimb2 and might therefore be involved in targeting of two kinases, activated PKC
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Figure 7. Stimulation of PKC
PKC
To search for putative substrates for PKC
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Figure 8. PKC
RACK1 is localized in dendrites and within dendritic spines
To further assess whether RACK1-dependent mechanisms might be involved in dendritic protein translation, we examined the cellular distribution of RACK1.
Light microscopic distribution of RACK1
In sections from the rat brain, RACK1 immunolabeling was found by light microscopy to be selectively associated with neuronal perikarya and dendrites in hippocampal CA1 (in both pyramidal neurons and interneurons in stratum radiatum). In somatosensory cortex, neurons in all layers had RACK1-immunopositive somata and prominent staining of apical dendrites (Fig. 9A), and the staining became more sparse and punctate farther away from the neuronal cell body. In cerebellar cortex, the Purkinje cell layer was especially densely labeled by RACK1 antibodies, although Golgi neurons, basket cells, and some granule cells were also positively stained for RACK1. Primary dendrites of Purkinje cells were immunopositive for RACK1, and staining became punctate higher in the molecular layer.
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Figure 9. Subcellular localization of RACK1. A, Light micrograph illustrating immunogold-silver staining for RACK1 in a pyramidal neuron in somatosensory cortex. Strong immunolabeling is seen in the neuronal soma and the apical dendrite, and punctate staining in the neuropil suggests synaptic localization of RACK1. Scale bar, 50 µm. B, C, Immunogold-silver labeling for RACK1 (black arrows) in the neuronal cytoplasm (B) and the neuronal nucleus (C). In the cytoplasm the gold-silver particles are localized over ribosomal aggregates (B, white arrows). Scale bars: B, 0.5 µm; C, 1 µm. D, RACK1 immunolabeling in a postsynaptic spine (arrow) close to the postsynaptic density in the spine head. The labeled synapse is surrounded by nonlabeled ones (asterisks) in the neuropil of the somatosensory cortex. Scale bar, 0.5 µm. E, Localization of RACK1 in the cytoplasm of a dendrite. Labeling is associated with cisternae in dendritic cytoplasm. Scale bar, 0.5 µm.
Electron microscopic distribution of RACK1
RACK1 localization was studied in somatosensory cortex, in the CA1 subfield of the hippocampus, and in the molecular layer of the cerebellar cortex. In all areas, RACK1 immunolabeling was observed most often in dendrites and in somata, although occasional staining in neuronal nuclei was detected as well (Fig. 9B,C). No staining was detected when the RACK1 antibody was omitted. RACK1 immunoreactivity was rarely observed in glial cells. In the soma, RACK1 was frequently colocalized with rough endoplasmic reticulum or polyribosomal clusters in Nissl bodies (Fig. 9B). In large and mid-size dendrites, RACK1 immunolabeling was scattered through the cytoplasm (Fig. 9E) and occasionally associated with cisterns of rough endoplasmic reticulum. Interestingly, dendritic spines were frequently labeled for RACK1, containing one or two immunogold-silver particles per spine (Fig. 9D). These particles were most often localized in the spine head. There was no distinct presynaptic or axonal RACK1 labeling.
DISCUSSION
Receptor-mediated activation of PKC
Local changes in protein synthesis can be controlled by phosphorylation and subsequent activation/inhibition of (1) translation initiation factors (Clemens, 1996
The entire functional mRNP complex consists of primary mRNA-binding proteins and secondary proteins, which are bound to it. If we assume that different proteins can bind, possibly in a competitive way, to a trans-acting factor, this could allow changes in mRNP complex composition, corresponding to the relative concentration or the activation state of these proteins in different compartments within the cell. One of these proteins that could control the composition of the mRNP complex, and subsequently its function, is the RACK1 protein. RACK1, originally described as a receptor for activated C kinase (Ron et al., 1994
Our results imply that RACK1, like FMRP, is primarily associated with mRNAs engaged in translation. This could indicate that (1) RACK1 is also associated with ribosomes, (2) RACK1 binds to specific mRNA sequences that become accessible only during or after translation initiation, or (3) immediately after binding of RACK1 to the appropriate mRNAs, translation initiation is promoted.
Recently, mGluR-triggered mechanisms have been implicated in the control of protein synthesis (Weiler and Greenough, 1993
One interesting property of RACK1 is the ability to bind PKC
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Figure 10. Proposed model for an mGluR-mediated control of postsynaptic protein synthesis. 1, A polyA-mRNA/mRNP complex is transported along microtubules through the dendrite in both anterograde and retrograde directions. The mRNA might be masked by specific mRNPs to prevent premature translation. 2, Synaptic stimulation activates protein kinase C
The extent to which RACK1 might also be involved in sequestering of mRNAs to specific subcellular domains remains to be determined; an indication of such participation comes from the detection of
FOOTNOTES Received May 14, 2002; revised July 23, 2003; accepted July 26, 2002.
This work was supported by the FRAXA-Research Foundation, Grants HD 37175 (W.T.G.), MH 35321 (W.T.G.), and GM 37537 (D.F.H.). We thank Dr. Susan Sesack (University of Pittsburgh, Pittsburgh, PA) for generous advice on immuno-EM methods, Dr. G. Dreyfuss (Howard Hughes Medical Institute and Department of Biochemistry and Biophysics, University of Pennsylvania School of Medicine, Philadelphia, PA) for the PABP1 (clone 10E10) antibody, Dr. D. Kennedy (Griffith University, Brisbane, Australia) for the G3BP-2a staining, Dr. E. Mohr (University of Hamburg, Hamburg, Germany) for the PABP1-pBSK+ vector, and Dr. J. Chen (Cell and Structural Biology, University of Illinois at Urbana/Champaign, Urbana, IL), Dr. C. Seidenbecher, and Dr. U. Thomas (Institute for Neurobiology, Magdeburg, Germany) for their generous help.
Correspondence should be addressed to Dr. Frank Angenstein, Institute for Neurobiology, Brenneckestrasse 6, 39120 Magdeburg, Germany. E-mail: angenstein{at}ifn-magdeburg.de.
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