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Previous Article | Next Article
The Journal of Neuroscience, September 15, 2002, 22(18):7948-7958
A New Activity of Doublecortin in Recognition of the Phospho-FIGQY Tyrosine in the Cytoplasmic Domain of Neurofascin
Krishnakumar Kizhatil, Yi-Xin Wu, Anindita Sen, and Vann Bennett Howard Hughes Medical Institute and Departments of Cell Biology, Biochemistry, and Neuroscience, Duke University Medical Center, Durham, North Carolina 27710
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Doublecortin is a cytoplasmic protein mutated in the neuronal migration disorder X-linked lissencephaly. This study describes a novel activity of doublecortin in recognition of the FIGQY-phosphotyrosine motif present in the cytoplasmic domain of the L1 cell adhesion molecule neurofascin. Phospho-FIGQY-neurofascin (186 kDa) coimmunoprecipitated with doublecortin from detergent extracts of embryonic brain membranes, and this doublecortin-phospho-FIGQY neurofascin complex was disassociated by a synthetic phospho-FIGQY neurofascin peptide but not by a dephospho-FIGQY peptide. Doublecortin specifically recognized the phospho-FIGQY tyrosine in the context of a synthetic phospho-FIGQY neurofascin peptide and in phospho-FIGQY neurofascin isolated from cells treated with pervanadate. Mutations of doublecortin causing lissencephaly (R59H, D62N, and G253D) abolished binding to the phospho-FIGQY peptide and to phospho-FIGQY neurofascin. Finally, phospho-FIGQY neurofascin and doublecortin colocalize in developing axon tracts and in zones enriched in migrating neurons in the embryonic cerebral cortex. In the adult rostral migratory stream, doublecortin colocalizes in migrating neurons with a phospho-FIGQY bearing L1 CAM different from neurofascin. The finding that doublecortin associates with FIGQY-phosphorylated neurofascin provides the first connection of doublecortin with the plasma membrane and could be important for a function of doublecortin in directing neuronal migration.
Key words: doublecortin; phospho-FIGQY; neurofascin; L1 CAM; neuronal migration; axons
INTRODUCTION
L1 cell adhesion molecules (CAMs) are transmembrane proteins in the Ig superfamily that engage in stable protein interactions as well as signaling pathways (Brummendorf et al., 1998
; Hortsch, 2000
L1 CAM cytoplasmic domains contain a highly conserved binding site for ankyrin, a protein that provides a linkage to the spectrin-actin network (Davis and Bennett, 1993
FIGQY-phosphorylated L1 CAMs have been detected in multiple tissues of vertebrates, D. melanogaster, and C. elegans using antibodies that recognize the phospho-FIGQY tyrosine epitope (Chen et al., 2001
This paper presents evidence that doublecortin, a cytoplasmic protein mutated in a neuronal migration disorder [X-linked lissencephaly (XLIS)] (des Portes et al., 1998a,b; Gleeson et al., 1998
MATERIALS AND METHODS
cDNAs and antibodies. Plasmids encoding hemagglutinin (HA)-neurofascin and HA-FIGQY/F-neurofascin have been described (Zhang et al., 1998
III tubulin (Covance), phosphotyrosine (clone 4G10; Upstate Biotechnologies), neurofascin (Davis et al., 1996
Cell culture. B104 rat neuroblastoma cells were cultured as described (Garver et al., 1997
Fractionation of embryonic brain and immunoprecipitation. Approximately 3 gm of embryonic rat brain was harvested in cold Leibovitz L-15 (Invitrogen) containing 0.32 M sucrose, 2 mM sodium fluoride, 1 mM phenylarsine oxide, 1 mM Na3VO4, 1 mM PMSF, 1 mM 4-(2-aminomethyl)benzenesulfonylfluoride hydrochloride (AEBSF), and 10 µg/ml leupeptin. Brains were homogenized in 4 vol of buffer containing 100 mM PIPES, 50 mM HEPES, 100 mM NaCl, 1 mM NaEDTA, 1 mM magnesium sulfate, 1 mM ATP, 0.32 M sucrose, 1 mM NaF, 1 mM AEBSF, 10 µg/ml leupeptin, 10 µg/ml pepstatin, and 1 mM Na3VO4, pH 6.9. The homogenate was centrifuged at 100 × g to remove the nuclei. The postnuclear supernatant was centrifuged at 20,000 × g, and the pellet was extracted with homogenization buffer containing 1% Triton X-100 (extraction buffer) for 30 min on ice to solubilize membrane proteins. The supernatant from the 20,000 × g spin was subjected to a 100,000 × g spin for 1 hr. The supernatant from this step was designated the cytosolic fraction. Immunoprecipitation was performed by incubating 10 µg of rabbit anti-doublecortin with 2 ml of Triton X-100 extract of membranes followed by addition of Protein A Sepharose beads. The Sepharose was then washed five times with extraction buffer and extracted with SDS for electrophoresis.
Isolation of recombinant doublecortin. Glutathione S-transferase (GST)-doublecortin fusion proteins were affinity purified using glutathione Sepharose beads and released from the beads using Precision protease (80 U), which cleaves the polypeptide chain between the GST moiety and doublecortin. Proteins were further purified by gel filtration chromatography on a Superose 12 column to obtain monodisperse preparations with full-length doublecortin eluting at a Ve/Vo of 1.5, DCN at a Ve/Vo of 1.74, and DCC at a Ve/Vo of 1.84. Concentrations of purified doublecortin, DCN, and DCC were estimated on the basis of the extinction coefficients of 0.5, 0.6, and 0.15, respectively, which were derived from the amino acid sequence. Wild-type doublecortin protein and mutated doublecortin protein preparations were affinity purified using glutathione Sepharose beads and centrifuged at 100,000 × g for 45 min after enzymatic removal of the GST tag to remove aggregated protein.
In vitro doublecortin-phospho-FIGQY peptide binding assay. Synthetic peptides (18-mer) KQFNEDGSFIGQpYTVRKD, KQFNEDGSFIGQYTVRKD, and KQFNEDGSFIGQFTVRKD bearing biotin conjugated to the NH2-terminal lysine were immobilized on streptavidin-coated wells (Pierce). The wells were blocked with 3% w/v BSA in PBS. Purified doublecortin (400 nM) was added to the wells after removal of the blocking solution and incubated overnight at 4°C. Wells were washed with PBS with 0.1% Tween 20. Binding was detected using doublecortin antibodies and secondary antibodies conjugated to alkaline phosphatase (AP). AP activity was detected using the colorimetric substrate p-nitrophenol (absorbance at 405 nm).
In vitro doublecortin-native phospho-FIGQY neurofascin binding assay. B104 cells, enriched for the expression of exogenous HA-neurofascin or FIGQY/F HA-neurofascin by a 2 week selection in geneticin (750 µg/ml), were incubated in the presence and absence of 100 µM sodium pervanadate for 45 min (Garver et al., 1997
Immunocytochemistry. Immunocytochemistry was performed on 10-µm-thick frozen sections of adult rat brain from animals perfused with 2% paraformaldehyde and from whole embyros (Davis et al., 1996
RESULTS
Doublecortin binds directly to a phospho-FIGQY synthetic peptide derived from the cytoplasmic domain of neurofascin
Doublecortin was identified as a candidate phospho-FIGQY binding protein by screening a rat fetal brain phage expression library with a biotinylated 30-mer synthetic peptide containing the phospho-FIGQY motif (KDSLVDpYGEGGEGQFNEDGSFIGQpYTVRKD) derived from the cytoplasmic domain of neurofascin (data not shown). Doublecortin has a closely related homolog on chromosome 13 (DC13) that encodes for alternatively spliced forms that include a doublecortin-like protein, and a doublecortin domain fused to a protein kinase domain (Burgess et al., 1999
A doublecortin-phospho-FIGQY motif interaction was evaluated by ELISA using NH2-terminally biotinylated peptides immobilized on streptavidin-coated wells of a 96-well plastic plate (see Materials and Methods). Purified recombinant doublecortin (see Materials and Methods) was incubated with a biotinylated phospho-FIGQY peptide (QFNEDGSFIGQpYTVRKD) derived from the cytoplasmic domain of neurofascin as well as equivalent peptides that either were not phosphorylated on the FIGQY tyrosine or had phenylalanine substituted for tyrosine (FIGQY/F). A Coomassie blue-stained SDS-PAGE gel of the purified monodisperse recombinant doublecortin revealed a single polypeptide band of ~40 kDa (Fig. 1A). The phospho-FIGQY-bearing peptide elicited a doublecortin-binding signal that was 12-fold over nonspecific binding (Fig. 1B). A similar increase in signal was observed in two other experiments. Doublecortin did not show significant binding to either the nonphosphorylated FIGQY peptide or the FIGQF peptide, as indicated by lack of increase in signal over nonspecific binding of doublecortin to the wells.
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Figure 1. Doublecortin binds directly to a synthetic peptide bearing the phospho-FIGQY motif, and mutations in doublecortin that cause X-linked lissencephaly abolish the doublecortin-phospho-FIGQY motif interaction. A, Coomassie blue-stained gel of purified monodisperse recombinant doublecortin (2 µg). B, Results of a representative peptide-binding assay. The y-axis of the graph represents the doublecortin binding to the synthetic peptides in arbitrary units (A.U.) and was obtained as described in Materials and Methods. C, Coomassie blue-stained gel of partially purified recombinant doublecortin and doublecortin mutants: R59H, D62N, and G253D. D, Results of a representative peptide-binding assay. The y-axis of the graph represents in arbitrary units the doublecortin binding to the synthetic peptides. Black bars represent binding for wild-type doublecortin, white bars represent binding for R59H doublecortin, diagonally striped bars represent binding for D62N doublecortin, and horizontally striped bars represent binding for G253D doublecortin. In B and D, the peptides used are listed below each bar representing doublecortin binding, phospho-FIGQY, FIGQY, FIGQF, or no peptide.
Doublecortin mutations that cause lissencephaly abolish binding to the phospho-FIGQY neurofascin peptide
We next determined the effect of mutations of doublecortin that cause lissencephaly on the ability of doublecortin to bind to the phospho-FIGQY neurofascin peptide. Doublecortin mutations cluster within two repeated domains in the NH2-terminal domain (Sapir et al., 2000
Phospho-FIGQY neurofascin coimmunoprecipitates with doublecortin from embryonic brain extracts
An in vivo interaction between doublecortin and phospho-FIGQY L1 CAMs was evaluated by immunoprecipitating doublecortin from Triton X-100 extracts of embryonic day (E) 18 rat brain membranes under nondenaturing conditions and then immunoblotting immunoprecipitated proteins with an affinity-purified anti-phospho-FIGQY antibody (Jenkins et al., 2001
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Figure 2. Doublecortin and phospho-FIGQY L1 CAMs form a complex in embryonic rat brain. A, Left panel, Immunoblot of equivalent volumes (10 µl) of total embryonic brain homogenate (T), cytosolic fraction (C), and Triton X-100 extract of membrane fraction (M) with a rabbit polyclonal doublecortin antibody. Right panel, Doublecortin in the different fractions (see Materials and Methods) is represented as a percentage of the amount in the starting homogenate (T). B, Immunoblot analysis of immunoprecipitates obtained using doublecortin antibodies from Triton X-100 membrane lysates (Materials and Methods). Antibodies used in immunoprecipitation are shown at the top of the blots. Antibodies used for immunobloting are shown on the right-hand side of the blots. DCX, Doublecortin; IP, immunoprecipitation. C, Immunoblot analysis of immunoprecipitates obtained using doublecortin antibody as well as total Triton X-100 membrane lysate with anti-NCAM antibody. D, Immunoblot analysis of immunoprecipitates obtained using doublecortin antibody as well as total Triton X-100 membrane lysate with antibodies against neurofascin, L1, and NrCAM. The antibody used for immunoblot is shown on the top of the blots. Tot, Triton X-100 membrane lysate; DCX IP, doublecortin immunoprecipitate.
A 186 kDa phospho-FIGQY L1 CAM coimmunoprecipitated with antibody against doublecortin, whereas neither doublecortin (Fig. 2B, bottom panel) nor phospho-FIGQY L1 CAM was immunoprecipitated with nonspecific rabbit IgG. Heat treatment of the Triton X-100 brain membrane extracts to 55°C abolished the phospho-FIGQY L1 CAM-doublecortin interaction (Fig. 2B, right panel). These results indicate that a doublecortin 186 kDa phospho-FIGQY L1 CAM complex exists in vivo and requires native folding for one or both of these proteins. In contrast, NCAM, a cell adhesion molecule prominently expressed in embryonic brain (Fig. 2C, Tot) that does not belong to the L1 family and lacks the FIGQY motif in its cytoplasmic domain, does not coimmunoprecipitate with doublecortin (Fig. 2C).
The identity of the phospho-FIGQY L1 CAM that coimmunoprecipitated with doublecortin was evaluated using antibodies against neurofascin, L1, and NrCAM (Fig. 2D). The extent of enrichment of each of these proteins in the immunoprecipitated fraction was determined by measuring blot intensity of polypeptides in the immunoprecipitate and an equivalent volume of the total membrane extract. Neurofascin is enriched sevenfold in the doublecortin immunoprecipitate (Fig. 2D, compare neurofascin Tot, DCX IP). L1, although detectable in immunoprecipitates (Fig. 2D, L1 DCX IP), is not enriched relative to the starting extract. NrCAM, although evident in the total extract (Fig. 2D, NrCAM Tot) is not coimmunoprecipitated (Fig. 2D, NrCAM DCX IP). Similar results were obtained in two other experiments. These data indicate that neurofascin is a major L1 CAM coimmunoprecipitating with doublecortin from E18 brain extracts. CHL1 was not evaluated and could also be present.
We next showed that the in vivo association of neurofascin with doublecortin is mediated through the phospho-FIGQY motif. The addition of increasing concentrations of the phospho-FIGQY neurofascin peptide (NEDGSFIGQpYTVRKD) to the Triton X-100 brain membrane lysate before immunoprecipitation of doublecortin resulted in reduction (0.25 mM peptide) and >90% elimination (0.5 mM peptide) of the 186 kDa phospho-FIGQY neurofascin that coimmunoprecipitated with doublecortin (Fig. 3). In contrast, the unphosphorylated FIGQY peptide at 0.5 mM had no effect on coimmunoprecipitation of phospho-FIGQY L1 CAM with doublecortin. Comparable levels of doublecortin were immunoprecipitated in the presence and absence of the peptides.
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Figure 3. Doublecortin-phospho-FIGQY L1 CAM complex in embryonic brain membranes is disrupted by a phospho-FIGQY synthetic peptide but not a dephospho-FIGQY peptide. Shown is immunoblot analysis of immunoprecipitated polypeptides obtained using antibody against doublecortin (Fig. 2) after preincubation of Triton X-100 lysate with synthetic peptides containing either the phospho-FIGQY or the FIGQY motif. The amount and nature of the synthetic peptide used are indicated above the blot. Antibodies used for the immunoblot are shown to the right of the blot.
Doublecortin binds to phospho-FIGQY neurofascin in vitro
We next studied the doublecortin interaction with the phospho-FIGQY motif in the context of full-length neurofascin. Purified recombinant doublecortin (Fig. 1A) was tested for the ability to bind neurofascin bearing an NH2-terminal HA-peptide (HA-neurofascin) that was FIGQY tyrosine phosphorylated, unphosphorylated, or with phenylalanine substituted for tyrosine (FIGQY/F). HA-neurofascin polypeptides were isolated from cell extracts and immobilized on Protein G Sepharose using an anti-HA antibody (see Materials and Methods). FIGQY tyrosine phosphorylation was achieved by treating the cells with the tyrosine phosphatase inhibitor, sodium pervanadate, before immunoisolation of neurofascin (Garver et al., 1997
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Figure 4. Doublecortin binds directly to FIGQY tyrosine-phoshorylated full-length neurofascin. A, Phospho-FIGQY native neurofascin binds doublecortin in the in vitro binding assay (Materials and Methods). B, Mutants of doublecortin that cause neuronal migration defects do not bind to full-length neurofascin. In A and B, the antibodies used for immunoblotting are shown to the right of the blots. The doublecortin proteins used are shown above each of the four columns of blots. In A and B, pervanadate treatment of the B104 cells transfected with HA-tagged neurofascin before immunoprecipitation is indicated by +, and the lack of treatment is indicated by above the blots. The type of neurofascin is indicated above the blots in A and B: wt, wild type; Y/F, FIGQY/F neurofascin. In A, none indicates nonspecific mouse IgG used instead of anti-HA antibody. In A, wild-type purified doublecortin was used in all binding sets as indicated above the blots; wt denat refers to heat-denatured wild-type doublecortin. In B the identities of doublecortin proteins used are shown above each of the four columns of blots. C, Graphical representation of the results of the binding assay shown in B. The y-axis represents in arbitrary units the ratio of doublecortin signal to the neurofascin signal after background correction. The neurofascin used in the binding is shown below the x-axis. wt, Wild type; Y/F, FIGQY/F neurofascin. Pervanadate treatment or lack of it is indicated by + or
Doublecortin mutations that result in neuronal migration defects and block recognition of phospho-FIGQY peptides (Fig. 2) also disrupt binding to phospho-FIGQY neurofascin. The blots in Figure 4B are arranged as in Figure 4A. The first set of blots confirms that wild-type doublecortin prepared without gel filtration binds (Fig. 1C) phospho-FIGQY neurofascin but not dephospho-FIGQY neurofascin or FIGQY/F neurofascin. The next three sets of blots show that mutated doublecortin polypeptides (Fig. 1C) fail to specifically bind phospho-FIGQY neurofascin. 125I-signals representing immunoreactive doublecortin were normalized with respect to the amount of neurofascin signal and are presented in bar graphs (Fig. 4C). Wild-type doublecortin binds phospho-FIGQY neurofascin with an ~10-fold higher efficiency than unphosphorylated or FIGQY/F neurofascin (Fig. 4C, black bars). In marked contrast, R59H and D62N mutated doublecortin polypeptides fail to bind phospho-FIGQY neurofascin (Fig. 4C, white and diagonally striped bars). The G253D mutant binds fivefold less efficiently than wild-type doublecortin to phospho-FIGQY neurofascin in this experiment (Fig. 4C, horizontally striped bars). The binding of mutant doublecortin to unphosphorylated neurofascin is nonspecific, because this binding is observed when the mutant proteins are heat denatured. These results demonstrate that clinically relevant doublecortin mutations abolish or reduce binding of doublecortin to phospho-FIGQY neurofascin.
Interaction with the phospho-FIGQY motif requires the full-length doublecortin protein
NH2-terminal sequencing of polypeptides produced by limited proteolysis of purified doublecortin with trypsin, chymotrypsin, and V8 protease revealed two independently folded protease-resistant domains composed of amino acids 45-270 and amino acids 271-360 (our unpublished data). These experimentally determined domain boundaries are in agreement with boundaries predicted from sequence analysis by other groups by the analysis of the doublecortin amino acid sequence (Sapir et al., 1997
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Figure 5. Individual domains of doublecortin fail to bind the phospho-FIGQY motif. A, Coomassie blue-stained gel of purified monodisperse recombinant doublecortin, DCN domain, and DCC domains. B, Peptide binding assay. The graph on the left shows the result of assay testing the ability of the DCN domain to bind peptides bearing the phospho-FIGQY motif. Black bars, Doublecortin; gray bars, DCN domain. The graph on the right shows the result of assay testing the ability of the DCC domain to bind peptides bearing the phospho-FIGQY motif. Black bars, Doublecortin; gray bars, DCC domain. Binding is represented as arbitrary units. The peptides used are listed below each bar representing doublecortin binding. C, Binding of native doublecortin and DCN domain to immunoisolated native neurofascin was performed as described (Materials and Methods). The antibodies used for immunoblotting are shown to the right of the blots. The graphical representation of the binding is shown to the right of the blots also. D, Binding of native doublecortin and DCC domain to immunoisolated native neurofascin was performed as described in Materials and Methods. The antibodies used for immunoblotting are shown to the right of the blots. In C and D, the neurofascin used in the binding is also indicated above the blot. wt, Wild type; Y/F, FIGQY/F neurofascin. Pervanadate treatment or lack of it is indicated by + or
Doublecortin and phospho-FIGQY L1 CAMs colocalize in migrating neurons and in tracts of developing axons
The sites of coexpression of doublecortin and phospho-FIGQY neurofascin were determined by immunofluorescence of sections of embryonic rat brain. In the E15 rat cerebral cortex, the first wave of postmitotic neurons have migrated from the neuroepithelial germinal zone lining the ventricles of the brain and have settled in a region called the preplate below the pial surface. Continued neuronal migration eventually splits the preplate to form the six-layered cortical plate. The anti-phospho-FIGQY antibody shows a preference for phospho-FIGQY neurofascin but also recognizes other FIGQY tyrosine-phosphorylated L1 CAMs (Jenkins et al., 2001
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Figure 6. Migrating neurons coexpress phospho-FIGQY L1 CAMs and doublecortin in embryonic brain. A, Double immunofluorescence staining of a parasagittal section of E15 rat brain with anti-phospho-FIGQY antibody and goat anti-doublecortin (Materials and Methods): phospho-FIGQY L1 CAMs (red, left), doublecortin (green, middle), and overlay (right). Scale bar, 10 µm. B, Double immunofluorescence labeling of a parasagittal section of E15 rat brain with rabbit anti-neurofascin antibody and goat anti-doublecortin: neurofascin (red, left), doublecortin (green, middle), and overlay (right). Scale bar, 25 µm. C, Double immunofluorescence labeling of a parasagittal section of E15 rat brain with rabbit anti-doublecortin-13 antibody and goat anti-doublecortin: doublecortin-13 (red, left), doublecortin (green, middle), and overlay (right). Scale bar, 25 µm.
Double labeling for doublecortin and DC13, the autosomal doublecortin homolog, is shown in Figure 6C. The pattern of labeling of phospho-FIGQY L1 CAMs (Fig. 6A) is similar to localization of DC13 (Fig. 6C, red, left panel) (Lin et al., 2000
In adult rats, neuroblasts from the SVZ migrate along the rostral migratory stream to renew the neuronal population within the olfactory bulb (Lois and Alvarez-Buylla, 1994
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Figure 7. Migrating neurons in the rostral migratory stream coexpress phospho-FIGQY L1 CAMs and doublecortin in the adult brain. A, Doublecortin and phospho-FIGQY L1 CAMs are coexpressed in migrating neurons of the rostral migratory stream in adult brain. Shown is double immunofluorescence labeling of a parasagittal section of the rostral cortex of adult rat brain using rabbit anti-phospho-FIGQY antibody and goat anti-doublecortin: phospho-FIGQY L1 CAM (red, left), doublecortin (green, middle), and overlay (right). Arrows indicate the chain-like structures formed by the migrating neurons. Scale bar, 50 µm. B, Doublecortin and phospho-FIGQY L1 CAMs are coexpressed in primary cultures of SVZ neurons. Cultures (Materials and Methods) were subjected to immunofluorescence with anti-phospho-FIGQY L1 CAM antibody, goat anti-doublecortin, and monoclonal anti-
SVZ explants were cultured in a three-dimensional extracellular matrix (Matrigel) (Wichterle et al., 1997
Doublecortin and phospho-FIGQY-L1 CAMs also are coexpressed in developing axon tracts (Fig. 8). Double immunofluorescence demonstrates that phospho-FIGQY L1 CAMs (red, left panels) and doublecortin (green, middle panels) colocalize (yellow, right panels) in the axon fascicles in the dorsal root ganglion (a-c), the axon tracts that extend into the developing olfactory bulb from the olfactory placode as well as the developing vomeronasal organ (d-f), and the axon fascicles belonging to the intraalary group of sensory nerves in the lower mandible (g-i). These results suggest that a complex between doublecortin and phospho-FIGQY L1 CAMs could exist in developing axons in addition to migrating neurons.
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Figure 8. Doublecortin and phospho-FIGQY L1 CAMs colocalize in axon fascicles during development. Double immunofluorescence of sections of rat tissue was performed with anti-phospho-FIGQY antibody and goat anti-doublecortin antibody. Phospho-FIGQY L1 CAM (a, d, g, red), doublecortin (b, e, h, green), and overlap (c, f, i). a-c, Axon tracts in the dorsal root ganglion; overlap (c). DCX, Doublecortin; DRG, dorsal root ganglion; phospho-FIGQY, phospho-FIGQY L1 CAM. Scale bar, 100 µm. d-f, Axon fascicle (arrows) in olfactory placode. axf, Axon fascicle; nb, neuroblastoma; ob, developing olfactory bulb; op, olfactory placode; vno, vomeronasal organ. Scale bar, 100 µm. g-i, Axon fascicle (arrow) in the developing mandible. Scale bar, 50 µm.
DISCUSSION
This study describes a new activity of doublecortin in recognition of the phospho-FIGQY tyrosine present in the cytoplasmic domain of neurofascin, a member of the L1 family of cell adhesion molecules. Phospho-FIGQY-neurofascin (186 kDa) coimmunoprecipitated with doublecortin from detergent extracts of embryonic brain membranes, and this doublecortin-phospho-FIGQY-neurofascin complex was disassociated by a synthetic phospho-FIGQY neurofascin peptide but not by a dephospho-FIGQY peptide. Doublecortin specifically recognized the phospho-FIGQY tyrosine in the context of a synthetic phospho-FIGQY neurofascin peptide and in phospho-FIGQY neurofascin isolated from cells treated with pervanadate. Mutations of doublecortin causing XLIS (R59H, D62N, and G253D) abolished binding to the phospho-FIGQY peptide and to phospho-FIGQY neurofascin. Finally, phospho-FIGQY neurofascin and doublecortin colocalize in developing axon tracts and in zones enriched in migrating neurons in the embryonic cerebral cortex. In the adult rostral migratory stream, doublecortin colocalizes in migrating neurons with a phospho-FIGQY bearing L1 CAM different from neurofascin.
These findings suggest the possibility that doublecortin functions as a phosphotyrosine adapter that serves as a link between neurofascin and other proteins that are capable of interacting with doublecortin. Candidate proteins to be coupled by doublecortin to phospho-FIGQY neurofascin include microtubules (Francis et al., 1999
The phospho-FIGQY motif-binding activity of doublecortin requires the contribution of the two domains in doublecortin. This is in contrast to SH2 and PTB domains, which are capable of independently binding phosphotyrosine motifs in various proteins. The doublecortin amino acid sequence does not show similarity to the amino acid sequence of SH2 domain or PTB domains that are found in the currently identified phosphotyrosine adapter proteins. Moreover, the stretch of amino acid residues encompassing the FIGQY motif shows little homology to peptides that bind to known SH2 or protein tyrosine binding domains, or to conventional substrates for protein tyrosine kinases (Scansite, http://scansite.mit.edu). Doublecortin could thus represent a new class of phosphotyrosine adapters with a novel sequence preference. Alternatively, the doublecortin-phospho-FIGQY interaction may be restricted to phospho-FIGQY-tyrosine of neurofascin and possibly the other L1 CAMs.
L1 and NrCAM share an identical sequence with neurofascin up to the FIGQY tyrosine and have similar COOH-terminal residues (SGKKE) that differ from the neurofascin sequence (TVRKD). The presence of the FIGQY motif in L1 and NrCAM raises the possibility that these L1 CAMs also can bind doublecortin when the FIGQY tyrosine is phosphorylated. However, neurofascin was the only L1 CAM that was enriched in immunoprecipitates of doublecortin from embryonic brain, although small amounts of L1 were also present. One possible explanation is that neurofascin is the major L1 CAM coexpressed with doublecortin during this developmental period, whereas at later times doublecortin is associated with other L1 CAMs. Further structural analysis of the sequence required for doublecortin binding should resolve this issue.
FIGQY phosphorylation of L1 CAMs has been demonstrated in the developing epithelium of the lung and midgut and neuromuscular junction in rat (Jenkins et al., 2001
This study is the first report of the expression of doublecortin in developing axon tracts outside the brain. Francis et al. (1999)
Doublecortin binds to LIS1, another protein involved in neuronal migration disorders (Caspi et al., 2000
FOOTNOTES Received April 16, 2002; revised May 30, 2002; accepted June 17, 2002.
We thank Dr. J. Gleeson for his generous gift of the cDNA encoding human doublecortin, Dr. L. Cantley for permission to use the Scansite software program, Dr. O. Reiner for her generous gift of the antibody against DCLK, and Dr. S. M. Jenkins for providing the phospho-FIGQY antibody.
Correspondence should be addressed to Krishnakumar Kizhatil, Box 3892, Duke University Medical Center, Durham, NC 27710. E-mail: k.kizhatil{at}cellbio.duke.edu.
REFERENCES
- Bieber AJ, Snow PM, Hortsch M, Patel NH, Jacobs JR, Traquina ZR, Schilling J, Goodman CS (1989) Drosophila neuroglian: a member of the immunoglobulin superfamily with extensive homology to the vertebrate neural adhesion molecule L1. Cell 59:447-460[Web of Science][Medline].
- Brummendorf T, Kenwrick S, Rathjen FG (1998) Neural cell recognition molecule L1: from cell biology to human hereditary brain malformations. Curr Opin Neurobiol 8:87-97[Web of Science][Medline].
- Burgess HA, Martinez S, Reiner O (1999) KIAA0369, doublecortin-like kinase, is expressed during brain development. J Neurosci Res 58:567-575[Web of Science][Medline].
- Caspi M, Atlas R, Kantor A, Sapir T, Reiner O (2000) Interaction between LIS1 and doublecortin, two lissencephaly gene products. Hum Mol Genet 9:2205-2213
[Abstract/Free Full Text] .- Chen L, Ong B, Bennett V (2001) LAD-1, the Caenorhabditis elegans L1 CAM homologue, participates in embryonic and gonadal morphogenesis and is a substrate for fibroblast growth factor receptor pathway-dependent phosphotyrosine-based signaling. J Cell Biol 154:841-856
[Abstract/Free Full Text] .- Cohen NR, Taylor JS, Scott LB, Guillery RW, Soriano P, Furley AJ (1998) Errors in corticospinal axon guidance in mice lacking the neural cell adhesion molecule L1. Curr Biol 8:26-33[Web of Science][Medline].
- Dahme M, Bartsch U, Martini R, Anliker B, Schachner M, Mantei N (1997) Disruption of the mouse L1 gene leads to malformations of the nervous system. Nat Genet 17:346-349[Web of Science][Medline].
- Davis JQ, Bennett V (1993) Ankyrin-binding activity of nervous system cell adhesion molecules expressed in adult brain. J Cell Sci [Suppl] 17:109-117[Medline].
- Davis JQ, Bennett V (1994) Ankyrin binding activity shared by the neurofascin/L1/NrCAM family of nervous system cell adhesion molecules. J Biol Chem 269:27163-27166
[Abstract/Free Full Text] .- Davis JQ, Lambert S, Bennett V (1996) Molecular composition of the node of Ranvier: identification of ankyrin-binding cell adhesion molecule neurofascin (mucin +/third FN111 domain) and NrCam at nodal axon segments. J Cell Biol 135:1355-1367
[Abstract/Free Full Text] .- Demyanenko GP, Tsai AY, Maness PF (1999) Abnormalities in neuronal process extension, hippocampal development, and the ventricular system of L1 knock-out mice. J Neurosci 19:4907-4920
[Abstract/Free Full Text] .- Demyanenko GP, Shibata Y, Maness PF (2001) Altered distribution of dopaminergic neurons in the brain of L1 null mice. Brain Res Dev Brain Res 126:21-30[Medline].
- des Portes V, Francis F, Pinard JM, Desguerre I, Moutard ML, Snoeck I, Meiners LC, Capron F, Cusmai R, Ricci S, Motte J, Echenne B, Ponsot G, Dulac O, Chelly J, Beldjord C (1998a) Doublecortin is the major gene causing X-linked subcortical laminar heterotopia (SCLH). Hum Mol Genet 7:1063-1070
[Abstract/Free Full Text] .- des Portes V, Pinard JM, Billuart P, Vinet MC, Koulakoff A, Carrie A, Gelot A, Dupuis E, Motte J, Berwald-Netter Y, Catala M, Kahn A, Beldjord C, Chelly J (1998b) A novel CNS gene required for neuronal migration and involved in X-linked subcortical laminar heterotopia and lissencephaly syndrome. Cell 92:51-61[Web of Science][Medline].
- Dubreuil RR, MacVicar G, Dissanayake S, Liu C, Homer D, Hortsch M (1996) Neuroglian-mediated cell adhesion induces assembly of the membrane skeleton at cell contact sites. J Cell Biol 133:647-655
[Abstract/Free Full Text] .- Francis F, Koulakoff A, Boucher D, Chafey P, Schaar B, Vinet MC, Friocourt G, McDonnell N, Reiner O, Kahn A, McConnell SK, Berwald-Netter Y, Denoulet P, Chelly J (1999) Doublecortin is a developmentally regulated, microtubule-associated protein expressed in migrating and differentiating neurons. Neuron 23:247-256[Web of Science][Medline].
- Fransen E, Lemmon V, Van Camp G, Vits L, Coucke P, Willems PJ (1995) CRASH syndrome: clinical spectrum of corpus callosum hypoplasia, retardation, adducted thumbs, spastic paraparesis and hydrocephalus due to mutations in one single gene, L1. Eur J Hum Genet 3:273-284[Web of Science][Medline].
- Fransen E, Van Camp G, D'Hooge R, Vits L, Willems PJ (1998) Genotype-phenotype correlation in L1 associated diseases. J Med Genet 35:399-404
[Abstract/Free Full Text] .- Friocourt G, Chafey P, Billuart P, Koulakoff A, Vinet MC, Schaar BT, McConnell SK, Francis F, Chelly J (2001) Doublecortin interacts with mu subunits of clathrin adaptor complexes in the developing nervous system. Mol Cell Neurosci 18:307-319[Web of Science][Medline].
- Fukuda T, Kawano H, Ohyama K, Li HP, Takeda Y, Oohira A, Kawamura K (1997) Immunohistochemical localization of neurocan and L1 in the formation of thalamocortical pathway of developing rats. J Comp Neurol 382:141-152[Web of Science][Medline].
- Garver TD, Ren Q, Tuvia S, Bennett V (1997) Tyrosine phosphorylation at a site highly conserved in the L1 family of cell adhesion molecules abolishes ankyrin binding and increases lateral mobility of neurofascin. J Cell Biol 137:703-714
[Abstract/Free Full Text] .- Gleeson JG, Allen KM, Fox JW, Lamperti ED, Berkovic S, Scheffer I, Cooper EC, Dobyns WB, Minnerath SR, Ross ME, Walsh CA (1998) Doublecortin, a brain-specific gene mutated in human X-linked lissencephaly and double cortex syndrome, encodes a putative signaling protein. Cell 92:63-72[Web of Science][Medline].
- Gleeson JG, Lin PT, Flanagan LA, Walsh CA (1999) Doublecortin is a microtubule-associated protein and is expressed widely by migrating neurons. Neuron 23:257-271[Web of Science][Medline].
- Gonczy P, Grill S, Stelzer EH, Kirkham M, Hyman AA (2001) Spindle positioning during the asymmetric first cell division of Caenorhabditis elegans embryos. Novartis Found Symp 237:164-175[Medline].
- Horesh D, Sapir T, Francis F, Wolf SG, Caspi M, Elbaum M, Chelly J, Reiner O (1999) Doublecortin, a stabilizer of microtubules. Hum Mol Genet 8:1599-1610
[Abstract/Free Full Text] .- Hortsch M (1996) The L1 family of neural cell adhesion molecules: old proteins performing new tricks. Neuron 17:587-593[Web of Science][Medline].
- Hortsch M (2000) Structural and functional evolution of the L1 family: are four adhesion molecules better than one? Mol Cell Neurosci 15:1-10[Web of Science][Medline].
- Jenkins SM, Kizhatil K, Kramarcy NR, Sen A, Sealock R, Bennett V (2001) FIGQY phosphorylation defines discrete populations of L1 cell adhesion molecules at sites of cell-cell contact and in migrating neurons. J Cell Sci 114:3823-3835
[Abstract/Free Full Text] .- Lee MK, Tuttle JB, Rebhun LI, Cleveland DW, Frankfurter A (1990) The expression and posttranslational modification of a neuron-specific beta-tubulin isotype during chick embryogenesis. Cell Motil Cytoskeleton 17:118-132[Web of Science][Medline].
- Lin PT, Gleeson JG, Corbo JC, Flanagan L, Walsh CA (2000) DCAMKL1 encodes a protein kinase with homology to doublecortin that regulates microtubule polymerization. J Neurosci 20:9152-9161
[Abstract/Free Full Text] .- Lois C, Alvarez-Buylla A (1994) Long-distance neuronal migration in the adult mammalian brain. Science 264:1145-1148
[Abstract/Free Full Text] .- Lois C, Garcia-Verdugo JM, Alvarez-Buylla A (1996) Chain migration of neuronal precursors. Science 271:978-981[Abstract].
- Morris NR, Efimov VP, Xiang X (1998) Nuclear migration, nucleokinesis and lissencephaly. Trends Cell Biol 8:467-470[Web of Science][Medline].
- Nacher J, Crespo C, McEwen BS (2001) Doublecortin expression in the adult rat telencephalon. Eur J Neurosci 14:629-644[Web of Science][Medline].
- Needham LK, Thelen K, Maness PF (2001) Cytoplasmic domain mutations of the L1 cell adhesion molecule reduce L1-ankyrin interactions. J Neurosci 21:1490-1500
[Abstract/Free Full Text] .- Sapir T, Elbaum M, Reiner O (1997) Reduction of microtubule catastrophe events by LIS1, platelet-activating factor acetylhydrolase subunit. EMBO J 16:6977-6984[Web of Science][Medline].
- Sapir T, Horesh D, Caspi M, Atlas R, Burgess HA, Wolf SG, Francis F, Chelly J, Elbaum M, Pietrokovski S, Reiner O (2000) Doublecortin mutations cluster in evolutionarily conserved functional domains. Hum Mol Genet 9:703-712
[Abstract/Free Full Text] .- Taylor KR, Holzer AK, Bazan JF, Walsh CA, Gleeson JG (2000) Patient mutations in doublecortin define a repeated tubulin-binding domain. J Biol Chem 275:34442-34450
[Abstract/Free Full Text] .- Tuvia S, Garver TD, Bennett V (1997) The phosphorylation state of the FIGQY tyrosine of neurofascin determines ankyrin-binding activity and patterns of cell segregation. Proc Natl Acad Sci USA 94:12957-12962
[Abstract/Free Full Text] .- Vallee RB, Tai C, Faulkner NE (2001) LIS1: cellular function of a disease-causing gene. Trends Cell Biol 11:155-160[Web of Science][Medline].
- Wichterle H, Garcia-Verdugo JM, Alvarez-Buylla A (1997) Direct evidence for homotypic, glia-independent neuronal migration. Neuron 18:779-791[Web of Science][Medline].
- Wynshaw-Boris A, Gambello MJ (2001) LIS1 and dynein motor function in neuronal migration and development. Genes Dev 15:639-651
[Free Full Text] .- Xiang X, Osmani AH, Osmani SA, Xin M, Morris NR (1995) NudF, a nuclear migration gene in Aspergillus nidulans, is similar to the human LIS-1 gene required for neuronal migration. Mol Biol Cell 6:297-310[Abstract].
- Zhang X, Davis JQ, Carpenter S, Bennett V (1998) Structural requirements for association of neurofascin with ankyrin. J Biol Chem 273:30785-30794
[Abstract/Free Full Text] .
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