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Address correspondence to Ronald D.G. McKay, 36 Convent Drive, MSC 4092, Bethesda, MD 20892. Tel.: (301) 496-6574. Fax: (301) 402-1340. E-mail: mckay{at}codon.nih.gov
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Abstract |
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Key Words: bone morphogenetic protein; stem cell; SMAD; STAT; mammalian FRAP
P. Rajan's present address is Psychiatric Genomics, Inc., 19 Firstfield Road, Gaithersburg, MD 20878.
* Abbreviations used in this paper: bFGF, basic FGF; BMP, bone morphogenetic protein; BMPR-IA, BMP receptor type one A; CNS, central nervous system; CNTF, ciliary neurotrophic factor; EMSA, electrophoretic mobility shift assay; FRAP, FKBP12/rapamycin-associated protein; FRB, FKBP12-rapamycin binding; GFAP, glial fibrillary acidic protein; SMA, smooth muscle
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Introduction |
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Cultured stem cells are increasingly used to analyze mechanisms of cellular differentiation because of the easy access to large numbers of self-renewing cells that exhibit rapid, controlled and reproducible differentiation. We have previously shown that CNS stem cells isolated from the embryonic rodent brain can be expanded in large numbers using the mitogen basic FGF (bFGF) to maintain self-renewal (Vicario-Abejon et al., 1995; Johe et al., 1996). Upon bFGF withdrawal, these cells will differentiate into the three characteristic CNS lineages: neurons, astrocytes, and oligodendrocytes (Johe et al., 1996). Furthermore, they can be efficiently redirected to specific CNS fates by the addition of single extracellular factors such as platelet-derived growth factor, triiodothyronine, and ciliary neurotrophic factor (CNTF) (Johe et al., 1996). CNTF rapidly and robustly instructs CNS stem cells to a glial fate and requires the actions of Stat3 (Bonni et al., 1997; Rajan and McKay, 1998).
Bone morphogenetic proteins (BMPs) have diverse actions on the fate choice and differentiation of CNS stem cells during development. BMPs induce dorsal precursor fates, including roof plate, choroid plexus epithelium, and neural crest (Shah et al., 1996; Liem et al., 1997; Sela-Donenfeld and Kalcheim, 1999; Panchision et al., 2001), and induce apoptosis or terminal differentiation in the developing neural tube (Graham et al., 1996; Furuta et al., 1997; Li et al., 1998; Panchision et al., 2001). BMP stimulation of CNS precursors in vitro leads to differentiation into CNS neurons (Mabie et al., 1999) and glia (Gross et al., 1996) and neural crest derivatives such smooth muscle, peripheral neurons, and Schwann cells (Mujtaba et al., 1998; Molne et al., 2000; Panchision et al., 2001). These diverse responses to BMPs may be due to (a) other signals that modulate the response to BMPs (Sun et al., 2001; White et al., 2001) and/or (b) the activation of different BMP signal transduction pathways. Here we show that the differentiation of two distinct cell fates, smooth muscle and glia, is modulated by density and is controlled by alternative use of two distinct cytoplasmic BMP pathways.
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Results |
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Neurons were also generated in both low- and high-density cultures, but in the absence of additional survival factors, the BMP-generated neurons usually died during differentiation. Thus, all clones in these BMP-treated cultures consisted predominantly of smooth muscle and glia. In contrast, stem cell clones grown to either low or high local density in the absence of BMP treatment generated only CNS neurons, astrocytes, and oligodendrocytes, as reported in previous studies (Johe et al., 1996). This indicates that the BMP-induced generation of neural crest derivatives, such as smooth muscle (Table I), is an efficient response of cortical stem cells and not of any contaminating cell type. On the basis of these observations, we sought to determine how this difference in cell density affects the fate choice of stem cells in response to BMPs.
BMP regulates smooth muscle and glial fates by signaling through the SMAD and STAT pathways, respectively
BMPs generate many responses by activating the SMAD family of DNA binding proteins (Miyazono, 1999). Transient transfection assays were used to determine if SMAD activation was necessary for generation of either or both of the fates. Cells were transfected with a construct that constitutively expresses high levels of HA-tagged Smad7, an endogenous inhibitory SMAD that functions as a dominant negative (Souchelnytskyi et al., 1998; Ishisaki et al., 1999). The transfected protein was allowed to express for 3 d, after which BMP treatment was initiated. Of all HASmad7-transfected cells, 77% differentiated into glia whereas <16% differentiated into smooth muscle (Table II).
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These data suggest that smooth muscle and glial fates are independently controlled by SMAD and STAT activation, respectively. We verified the biochemical activation of SMAD proteins by performing immunoblotting assays with an antibody recognizing the phosphorylated forms of Smad1, 5, and 8 (Faure et al., 2000) on whole cell extracts prepared after a 1-h factor treatment. Although bFGF and CNTF each have strong proliferative and differentiative effects on stem cells (Johe et al., 1996; Rajan and McKay, 1998), they had no effect on the activation of Smad1/5/8 (Fig. 2 A). In contrast, BMP4 robustly activated Smad1/5/8 in both low- and high-density cultures (Fig. 2 A, lanes 3 and 6). This activation occurred within 30 min and continued beyond 4 h of BMP4 treatment (Fig. 2 B).
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Maximal activation of STAT proteins by BMP was seen at 8 h. This treatment is prolonged when compared with CNTF, which causes maximal STAT activation at 15 min to 1 h. The long time required for BMP4 to activate STAT proteins suggests that some intermediary signal, perhaps a CNTF-like activity, becomes transcriptionally activated and that this is responsible for the activation of Stat3. We tested this possibility by treating the stem cells with the transcriptional inhibitor -amanitin, which acts as a competitive inhibitor of RNA polymerase II (Wieland and Faulstich, 1978). Cotreatment of stem cells with
-amanitin did not block BMP4-mediated Stat3 binding (Fig. 4, compare lanes 4 and 5 with 9 and 10). These results make it unlikely that Stat3 activation requires a transcriptionally induced intermediate and instead suggests that BMP4 activates Stat3 directly through cytoplasmic signaling.
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The observations that BMP-mediated activation is blocked by rapamycin and the correlated release of FKBP12 from the BMP receptor implicate FRAP as the mediator of STAT activation. A previous study has shown that FRAP can phosphorylate STAT proteins in response to CNTF (Yokogami et al., 2000). As this would involve direct interaction between FRAP and Stat3, we determined if BMP signaling increases complex formation between the two proteins. FRAP was immunoprecipitated from nondenaturing cell extracts, and the immunoprecipitated proteins were subsequently immunoblotted with an anti-Stat3 antibody. BMP treatment of CNS stem cells led to increased interaction of FRAP and Stat3 proteins by coimmunoprecipitation, greater than that seen with CNTF (Fig. 5 C). The binding of FRAP to Stat3 in response to BMP stimulation (Fig. 5 C) and the inhibition of Stat3 activation by rapamycin (Fig. 5 B) suggest that BMP4 activates Stat3 via a FRAP-mediated pathway.
As more direct evidence that FRAP is instrumental in mediating STAT activation, and hence glial differentiation, downstream of BMP, we determined the effect of two dominant-negative forms of FRAP on BMP-mediated astrocytic differentiation. The Trp2027Phe point mutation renders FRAP defective in the FKBP12-rapamycin binding (FRB) domain, whereas Asp2357Glu point mutation deletes the kinase function of FRAP (Vilella-Bach et al., 1999). Both the constructs we have used are NH2-terminal FLAG tagged. About 25% of stem cells transfected with the dominant-negative forms of FRAP differentiate into glia upon BMP treatment (Fig. 5, D and E), whereas in a control transfection with a GFP construct under identical experimental conditions, 80% of the culture differentiated into glia. These data indicate that FRAP activation is required for BMP-mediated glial differentiation.
BMP4-induced glial differentiation is rapamycin sensitive, whereas smooth muscle differentiation is rapamycin insensitive
We additionally looked at rapamycin inhibition of FRAP on fate choice. Stem cells that received no treatment before mitogen withdrawal generated glia with weak to moderate GFAP staining and an immature morphology (Fig. 6 A). Stem cells that received CNTF before mitogen withdrawal generated intensely stained GFAP+ cells with a mature, stellate astrocytic morphology (Fig. 6 B), as described previously (Johe et al., 1996; Rajan and McKay, 1998). Treatment with BMP4 before mitogen withdrawal generated glia with strong GFAP staining and distinctly flattened morphology (Fig. 6 C). Stem cells that received BMP4 and rapamycin showed a dramatically reduced number of GFAP+ cells, even in areas with high local density (Fig. 6 D). Additionally, we treated stem cells with FK506, another drug that complexes with FKBP12 but inhibits the phosphatase calcineurin (Abraham and Wiederrecht, 1996). We found that FK506 had no effect on the generation of glia by BMP4 (Fig. 6 E).
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We then looked at the effect of rapamycin in adult stem cells. These cells are multipotent based on clonal assays (Johe et al., 1996), but BMP treatment promotes efficient glial differentiation even at lower densities that would promote smooth muscle differentiation in fetal stem cells. In these cells, rapamycin treatment caused a twofold reduction in the generation of glia and caused a twofold increase in the number of smooth muscle cells (Fig. 6 H). Thus, inhibition of FRAP specifically blocks the glial fate in both fetal and adult stem cells and redirects adult stem cells to a smooth muscle fate. These results are all consistent with the conclusion that BMP4 causes glial differentiation by FRAP-mediated Stat3 activation and smooth muscle differentiation by a FRAP-independent, SMAD-mediated mechanism.
BMP4 and CNTF have additive effects on glial differentiation
CNTF and BMPs both cause STAT activation and glial differentiation but do so by using different kinases. CNTF predominantly activates the janus kinases (Kisseleva et al., 2002), whereas we show that BMPs require a density-dependent signal in addition to FRAP (Fig. 5). Because distinct pathways are used to activate STAT proteins and cause glial differentiation, the simultaneous treatment of stem cells with both ligands might accelerate glial differentiation. Stem cells were plated at a medium density and treated with either ligand alone or together. As measured by GFAP expression, 25% of stem cells were differentiated by 24 h after CNTF treatment, whereas 50% of stem cells differentiated after 48 h. Cotreatment with BMP4 and CNTF increased glia number from 25 to 60% at 24 h and from 50 to 85% at 48 h (Fig. 7 A).
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Discussion |
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Our results show that fate choice decisions leading to glial or nonglial fates downstream of BMPs can be made in the cytoplasm. This provides a novel complement to previous studies showing that glial differentiation in response to BMPs is regulated in the nucleus. In these studies, glial differentiation requires the coactivators cyclic AMP response elementbinding protein (CBP)/p300 in a complex with STAT and SMAD proteins (Nakashima et al., 1999). The differentiation of glia by either BMPs or CNTF is inhibited by the basic helix-loop-helix protein neurogenin1, which acts in part by sequestering the CBPSmad1 complex from association with STAT proteins. In CNS stem cells expressing high levels of neurogenin1, BMPs induce neuronal, rather than glial, differentiation (Sun et al., 2001). Our results show that glial versus nonglial fates can also be regulated by alternative cytoplasmic signals. These alternative pathways are subject to control by density-dependent signals, consistent with our previous findings (Tsai and McKay, 2000). Whereas BMP4 activates SMADs at both low and high densities, its activation of Stat3 at high density results in glial differentiation regardless of SMAD activation (Table II; Figs. 2 and 3). Furthermore, glial differentiation can occur even when SMAD signaling is inhibited (Table II). One interpretation of this result is that sufficiently high levels of STAT activation promote glial differentiation without the requirement for SMADs. Alternatively, SMAD activation may modify the type of glia that is generated, as evidenced by the morphological difference in glia generated from CNTF- versus BMP-treated stem cells (Figs. 6 and 7).
In addition to density-dependent biases, stem cells also exhibit age-dependent biases in fate choice that mirror the in vivo developmental progression of cell type differentiation. Activating BMP signals in vivo results in apoptosis in early gestation precursors and neurogenesis in midgestation precursors (Panchision et al., 2001). Similarly, neural stem cells isolated from progressively older embryos respond to BMPs first with apoptosis, and then with neuronal and finally glial differentiation (Gross et al., 1996; Mabie et al., 1999). Our FRAP inhibition experiments suggest that the same mechanisms for glial differentiation are accessible in both fetal and adult stem cells and that age-intrinsic differences between stem cells can be reversible (Fig. 6).
Previous studies have shown that the same signaling molecules can promote either stem cell self-renewal or gliogenesis. Notch activation is required for the maintenance of early gestation neural stem cells (Hitoshi et al., 2002a) but also promotes gliogenesis in stem cells from older embryos (Tanigaki et al., 2001; White et al., 2001). Stat3, which we show to be activated by BMPs through FRAP, has been shown to promote both glial differentiation in neural stem cells (Bonni et al., 1997; Rajan and McKay, 1998) and self-renewal of embryonic stem cells (Niwa et al., 1998; Nishinakamura et al., 1999; Boeuf et al., 2001) in response to CNTF or Leukemia inhibitory factor. FRAP signaling is required for proliferation in mouse embryos and the loss-of-function phenotype is mimicked by the treatment of embryos with rapamycin (Hentges et al., 2001). Our results show a novel pathway in which FRAP is recruited to promote gliogenesis by activating Stat3. Presumably this is due to other signals that provide a different context to FRAP and STAT signaling, but the mechanisms that mediate this changing context remain to be identified. In our in vitro stem cell system, this potentially translates into a density-mediated signal. Our results add FRAP to a growing list of signaling molecules whose actions are redirected from self-renewal/proliferation to gliogenesis during development.
A novel mechanism for signal integration
Our results suggest that the immunophilin FKBP12 is involved in glial differentiation, but its exact role is unclear. FKBP12 binds TGFß receptors (Wang et al., 1996) and inhibits the basal activity of the receptor in the absence of ligand (Chen et al., 1997). We show that FKBP12 complexes with BMPR-IA in stem cells and is released upon binding of BMP4 to its receptor (Fig. 5). The timing of the release of FKBP12 from the BMP receptor correlates with activation of Stat3 (6 h), suggesting that FKBP12 is also involved in the kinetics of FRAP activation. FKBP12 can complex with the antibiotic drugs FK506 and rapamycin to inhibit distinct signaling pathways. FK506 binding to FKBP12 inhibits the activity of calcineurin in T cells, causing immunosuppression (Clipstone et al., 1994), whereas rapamycin binding to FKBP12 inhibits the activation of FRAP (Hamilton and Steiner, 1998). We show that rapamycin, but not FK506, specifically inhibits the BMP-mediated augmentation of Stat3 activation and glial differentiation (Fig. 6). It is important to note that all our studies are performed with endogenous cellular proteins, with the exception of dominant-negative inhibitory proteins that we have overexpressed. This, and the fact that our cultures are dynamically undergoing differentiation, may allow us to speculate on novel functions for FKBP12. We could not isolate a complex of FKBP12 and FRAP in BMP-treated cells (unpublished data), in agreement with a previous crystallographic analysis showing that FKBP12 does not bind directly to FRAP (Choi et al., 1996). FKBP12 may complex with other proteins, or be modified, as it is released from the receptor. The intrinsic peptidyl-prolyl isomerase activity (Siekierka et al., 1990) may be significant in these signaling interactions. The region of FRAP required for binding to FKBP12rapamycin complex is also required for the activation of its serine-threonine kinase activity (Vilella-Bach et al., 1999). This may suggest an endogenous cellular analogue of rapamycin that functions in FKBP12-mediated activation of FRAP. However, we cannot discount the likelihood that FKBP12 is acting strictly as an inhibitor of both BMP receptor and FRAP activity, so the signaling molecules linking BMP receptor activation with FRAP activation remain undetermined.
The serine-threonine kinase FRAP is an important regulator of cell growth and proliferation (Hentges et al., 2001; Fingar et al., 2002). FRAP acts by promoting the synthesis of proteins crucial to increasing cell size and to cell cycle progression (Gingras et al., 2001; Fingar et al., 2002). FRAP activity is nutrient dependent and increases with rising amino acid levels and insulin signaling (Gingras et al., 2001). One possibility is that rapamycin may mimic an endogenous inhibitor of otherwise constitutively active FRAP (Gingras et al., 2001). Overexpressed FRAP causes Stat3 phosphorylation at serine residue 727 (Yokogami et al., 2000). This suggests a model where BMPs, by causing serine phosphorylation of STAT proteins, can integrate with other signals that tyrosine phosphorylate STAT proteins; this concerted action would raise STAT activation above a threshold required for differentiation to the glial fate and would override a SMAD proteinmediated smooth muscle fate (Fig. 8).
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Materials and methods |
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Antibodies.
The following antibodies were used: monoclonal anti-GFAP from ICN Biomedicals; polyclonal anti-GFAP from DakoCytomation; monoclonal anti-SMA and anti-FLAG from Sigma-Aldrich; polyclonal anti-HA from BABCO; monoclonal anti-FKBP12, anti-FRAP, and anti-Stat3 from Transduction Laboratories; polyclonal anti-phosphoStat3 (Tyr705 and Ser727) from Santa Cruz Biotechnology, Inc.; monoclonal antiBMPR-IA from R&D Systems; polyclonal anti-phosphoSmad1/5/8 (a gift of P. ten Dijke, Netherlands Cancer Institute, Amsterdam, Netherlands; or purchased from Cell Signaling); fluorescent-labeled secondary antibodies from Jackson ImmunoResearch Laboratories; and peroxidase-conjugated secondaries for ECL from Boehringer.
Other reagents.
Other reagents included ECL reagents from Pierce Chemical Co., polyacrylamide gradient gels from Novex, protein ASepharose from Amersham Biosciences, Ponceau S from Sigma-Aldrich, Lipofectamine Plus from Invitrogen, rapamycin and -amanitin from Calbiochem, FK506 from American Qualex, and BMP2 and BMP4 from Genetics Institute.
Plasmids.
The Stat3 mutant (a gift from J.E. Darnell, The Rockefeller University, New York, NY) has a three amino acid substitution in the DNA binding domain as previously described (Horvath et al., 1995) and was tagged with a synthetic FLAG epitope. The Smad7 construct (a gift from P. ten Dijke, Netherlands Cancer Institute, Amsterdam, Netherlands) (Ishisaki et al., 1999) was modified such that it expressed the protein with an NH2-terminal HA epitope under the control of the ß-actin promoter (a gift from J. Rossant, Children's Hospital, Toronto, Canada). The kinase-dead FRAP construct has a Trp2027 to Phe inactivating mutation in the kinase domain (Vilella-Bach et al., 1999). The FRB-defective FRAP construct has an Asp2357 to Glu mutation that prevents protein interactions via the FRB domain (Vilella-Bach et al., 1999). Both FLAG constructs (gifts from J. Chen, University of Illinois, Urbana-Champaign, IL) were tagged with an NH2-terminal synthetic FLAG epitope.
Cell culture and treatments
Embryonic and adult rat stem cells were grown as previously described (Johe et al., 1996; Rajan and McKay, 1998). To grow adult stem cells, ventricular and subventricular tissue was dissected from the brains of young adult female rats (200250 g weight), enzymatically dissociated, and plated in serum-free DME/F12 medium with N2 supplement. bFGF was included at 10 ng/ml to promote rat stem cell proliferation. Stem cells from E13 mouse cortex were required for one experiment using a mouse-specific Stat3 (pSer727) antibody and were grown as described for rat, except mouse cells were incubated in 5% oxygen and 20 ng/ml bFGF. Cells were fed with bFGF daily, and medium was replaced on alternate days during stem cell expansion. Passaging was performed nonenzymatically using Ca2+/Mg2+-free HBSS. All experiments were performed on first- or second-passage cells.
For mass culture experiments, cells were plated at 7,000 cells/cm2 and BMP treatment was initiated after 1 d (low density) or 4 d (high density). Alternatively, cells were plated at 350 cells/cm2 and BMP treatment was initiated immediately (low density) or after 4 d (high density). For clonal analysis, cells were plated at 35 cells/cm2 and BMP treatment was initiated immediately (low density) or after 6 d (high density). BMP4 was added daily, usually for 2 d in the presence of bFGF and for another 4 d after bFGF withdrawal to promote efficient terminal differentiation of stem cells.
Drug inhibition experiments were performed using the 350 cells/cm2 plating paradigm described above. When needed, CNTF (10 ng/ml), rapamycin (1 µM), or FK506 (1 µg/ml) were used in the same manner as BMP4. Separate experiments involving BMP/CNTF cotreatment were performed using the 7,000 cells/cm2 plating paradigm; cells were treated with BMP4 for 3 d in the presence of bFGF and for another 3 d in the absence of bFGF.
For the biochemical assays, cells were treated with factors and harvested at the time points mentioned in the figure legends. For transcriptional inhibition experiments, cells were preincubated with -amanitin (5 µg/ml) for 20 min before and along with BMP treatment before harvesting of cells. Transfections were performed with Lipofectamine Plus reagent according to the manufacturer's instructions (Invitrogen). For Stat3 and Smad7 manipulations, cells were plated at 3,500 cells/cm2 and cultured with 10 ng/ml bFGF for 1 d before transfection and for 3 d after transfection to allow the dominant-negative Stat3FLAG or Smad7HA plasmid to express before BMP4 treatment. Cells were then treated with 10 ng/ml BMP4 for 3 d with bFGF mitogen and for 3 d after mitogen withdrawal. For FRAP manipulations, cells were plated at 350 cells/cm2 and cultured with 10 ng/ml bFGF for 4 d before transfection and for 1 d after transfection to allow the kinase-dead or FRB-defective FRAP plasmid to express before BMP4 treatment. The transfection efficiency was
10%, as measured by epitope tag staining.
Immunofluorescent staining of cells
Cells were fixed with 4% paraformaldehyde for 1015 min at room temperature, blocked for 30 min in PBS with 0.1% triton and 5% normal goat serum, and incubated with the primary antibody for 24 h at room temperature. Cells were stained as directed with anti-SMA to detect smooth muscle cells and anti-GFAP to detect glia. After two washes in PBS, the secondary antibody was applied at a 100-fold dilution for 1 h at room temperature. Cultures were then washed with PBS and mounted in Vectashield containing DAPI (Vector Laboratories). Images were photographed under fluorescent filters using a Carl Zeiss MicroImaging, Inc. Axioplan microscope and Spot digital camera (Diagnostic Instruments, Inc.). Statistical analysis and histogram illustration of cell numbers were performed using SigmaPlot 5.0 (SPSS, Inc.). Other graphic illustrations were generated using Powerpoint for Windows (Microsoft). All images were combined for figures using Adobe Photoshop 5.0® for Windows.
EMSA
Nuclear extract preparation and EMSA were performed as described previously (Rajan and McKay, 1998). Autoradiography was performed using Biomax Mr film (Eastman Kodak Co.), and images were digitally imported using a Duoscan T2500 flatbed scanner (AGFA) and processed for figures using Adobe Photoshop 5.0® for Windows.
Immunoprecipitation and immunoblotting
Total cell lysates were prepared in nondenaturing lysis buffer (1% Triton X-100, 10% glycerol, 50 mM Tris, pH 7.4, 150 mM NaCl, 2 mM EGTA, 2 mM MgCl2, 1 mM DTT, 1 mM PMSF, and phosphatase inhibitors) and were normalized for protein concentration. For immunoprecipitation, normalized lysates were incubated with primary antibody overnight at 4°C. After incubation with protein ASepharose (1:1 vol/vol), the immune complexes were washed twice with PBS and heated to 70°C in SDS-PAGE loading buffer. Samples were resolved in denaturing gels and transferred onto nitrocellulose. Filters were blocked overnight in Tris-buffered saline (20 mM Tris, pH 7.6, 137 mM NaCl) with 0.1% Tween 20 (TBST) containing 3% bovine serum albumin. Filters were incubated with primary antibody (1:1,000 dilution in blocking buffer) for 4 h at room temperature and then washed three times in TBST for 1 h. Filters were then incubated with the appropriate secondary antibody (1:20,000 dilution in blocking buffer) for 1 h and then washed for 1 h. Relevant bands were detected with ECL according to the manufacturer's instructions. Ponceau S staining (0.1% in 5% acetic acid) was performed for 30 s, followed by destaining in several changes of purified water. Banding patterns were digitally scanned as described above.
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Acknowledgments |
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L. Newell is funded by the Howard Hughes Medical Institute National Institutes of Health Research Scholar's Program.
Submitted: 5 November 2002
Revised: 23 April 2003
Accepted: 23 April 2003
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References |
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