Home | Help | Feedback | Subscriptions | Archive | Search | Table of Contents

This Article Abstract Full Text (PDF, 5379K) PPT slides of all figures Alert me when this article is cited Citation Map Services Email this article Similar articles in this journal Similar articles in PubMed Alert me to new content in the JCB Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via CrossRef Citing Articles via Google Scholar Google Scholar Articles by Hortsch, M. Articles by Dubreuil, R. R. Search for Related Content PubMed PubMed Citation Articles by Hortsch, M. Articles by Dubreuil, R. R. Pubmed/NCBI databases Gene GEO Profiles HomoloGene Protein UniGene Compound via MeSH Substance via MeSH Hazardous Substances DB L-TYROSINE Social Bookmarking                            What's this?

© The Rockefeller University Press, 0021-9525/1998//251 $5.00
The Journal of Cell Biology, Volume 142, Number 1, , 1998 251-261

Structural Requirements for Outside-In and Inside-Out Signaling by Drosophila Neuroglian, a Member of the L1 Family of Cell Adhesion Molecules

Michael Hortsch^*, Diahann Homer^*, Jyoti Dhar Malhotra^*, Sherry Chang^*, Jason Frankel, Gregory Jefford, and Ronald R. Dubreuil

^* University of Michigan, Department of Anatomy and Cell Biology, Ann Arbor, Michigan 48109-0616; and University of Chicago, Department of Pharmacological and Physiological Sciences, Chicago, Illinois 60637

Expression of the Drosophila cell adhesion molecule neuroglian in S2 cells leads to cell aggregation and the intracellular recruitment of ankyrin to cell contact sites. We localized the region of neuroglian that interacts with ankyrin and investigated the mechanism that limits this interaction to cell contact sites. Yeast two-hybrid analysis and expression of neuroglian deletion constructs in S2 cells identified a conserved 36-amino acid sequence that is required for ankyrin binding. Mutation of a conserved tyrosine residue within this region reduced ankyrin binding and extracellular adhesion. However, residual recruitment of ankyrin by this mutant neuroglian molecule was still limited to cell contacts, indicating that the lack of ankyrin binding at noncontact sites is not caused by tyrosine phosphorylation. A chimeric molecule, in which the extracellular domain of neuroglian was replaced with the corresponding domain from the adhesion molecule fasciclin II, also selectively recruited ankyrin to cell contacts. Thus, outside-in signaling by neuroglian in S2 cells depends on extracellular adhesion, but does not depend on any unique property of its extracellular domain. We propose that the recruitment of ankyrin to cell contact sites depends on a physical rearrangement of neuroglian in response to cell adhesion, and that ankyrin binding plays a reciprocal role in stabilizing the adhesive interaction.

Key Words: ankyrins • cell aggregation • cells, cultured • cytoskeleton • Drosophila

Abbreviations used in this paper: CAM, cell adhesion molecule.

MEMBERS of the L1 family of cell adhesion molecules (CAMs)¹ have emerged as important molecules during embryonic nervous system development and during regeneration after nerve injury (Hortsch, 1996). They are involved in processes such as myelination, long-term potentiation, neuronal migration, axonal guidance and fasciculation, and synaptogenesis. L1 family members are also thought to transduce neurite growth-promoting signals by activation of neuronal FGF receptors (Walsh and Doherty, 1997).

There is compelling evidence linking mutations in human L1-CAM to neurodevelopmental phenotypes. These phenotypes include hydrocephalus, motor neuron defects, agenesis of the corpus callosum and the corticospinal tract, and others (Wong et al., 1995b; Dahme et al., 1997). Mutations in the Drosophila L1 homologue, neuroglian, result in embryonic lethality and defects in neuronal morphology and axonal pathfinding (Bieber et al., 1989; Hall and Bieber, 1997). Which of L1's many molecular functions are affected by these mutations and are therefore responsible for the observed phenotypes is currently unknown.

L1 family members with their conserved pattern of extracellular immunoglobulin (Ig) and fibronectin type III protein domains share a number of molecular functions, such as homo- and heterophilic adhesion (Hortsch, 1996). The cytoplasmic domain binds directly to ankyrin which, in turn, interacts with the spectrin cytoskeleton (Davis et al., 1993; Davis and Bennett, 1994; Dubreuil et al., 1996; Hortsch et al., 1998). Expression of the Drosophila L1 homologue, neuroglian, in Drosophila S2 tissue culture cells results in a selective recruitment of ankyrin and spectrin to sites of cell contacts (Dubreuil et al., 1996). Ankyrin recruitment is strictly limited to cell contacts, even though neuroglian is abundantly expressed over the entire cell surface. Thus, neuroglian can function as a signaling molecule that transmits the positional value of cell adhesion to the cytoplasmic assembly of ankyrin and spectrin. This outside-in signaling function appears to be conserved among L1 family members, since expression of human L1 in S2 cells also results in the assembly of ankyrin at cell contact sites (Hortsch et al., 1998). The adhesion-induced rearrangement of ankyrin and spectrin can be conveyed to other membrane proteins that interact with ankyrin and spectrin and might thereby provide a mechanism for the assembly of unique plasma membrane subdomains. For example, the NaK-ATPase, which is known to interact with ankyrin in vertebrates (Nelson and Veshnock, 1987), was found to accumulate along with spectrin and ankyrin at sites of neuroglian-mediated adhesion in S2 cells (Dubreuil et al., 1997). Thus, L1-mediated adhesion events result in a reorganization and compartmentalization of the plasma membrane, which may constitute an important biological function of L1 family members.

Recent studies of the L1 family member rat neurofascin have begun to elucidate the structural requirements of the L1 family–ankyrin interaction. Deletion of a five-amino acid sequence from the conserved distal region of the neurofascin cytoplasmic domain abolished ankyrin binding (Garver et al., 1997), indicating that this sequence contributes to the ankyrin-binding site. Two tyrosine residues in this distal region (corresponding to Y1217 and Y1234 in the Drosophila neuroglian protein sequence) are conserved in all but two members of the L1 family. In vitro studies of neurofascin revealed that phosphorylation of one of these tyrosines (Y1234 in neuroglian) can inhibit the binding of ankyrin to neurofascin (Garver et al., 1997). Furthermore, inhibition of the ankyrin–neurofascin interaction, either by deleting or phosphorylating the critical tyrosine residue, had an inhibitory effect on neurofascin-mediated cell adhesion (Tuvia et al., 1997). Together, these observations suggest an elegant mechanism to explain the inside-out regulation of the extracellular adhesion of an L1 family member by the intracellular phosphorylation of its cytoplasmic domain.

Here we investigate the mechanisms governing outside-in signaling by neuroglian. We take advantage of the unique features of S2 cells to study not only adhesion, but also the redistribution of the spectrin cytoskeleton in response to neuroglian expression (Dubreuil et al., 1996). We used yeast two-hybrid analysis and expression of deletion constructs in S2 cells to map the region of neuroglian that is necessary and sufficient for binding to ankyrin. Similarly, we investigated the effects of cytoplasmic domain tyrosine mutations on the ability of neuroglian to interact with ankyrin in yeast and to recruit ankyrin to cell contacts in S2 cells. Finally, we tested the possibility that neuroglian outside-in signaling depends on unique features of the neuroglian extracellular domain by expressing a fasciclin II-neuroglian chimera in S2 cells. The results of these studies expand the repertoire of molecular mechanisms that are relevant to our understanding of L1 family function and the relationship between specific L1 defects and their complex phenotypes.

	Materials and Methods

Top Abstract Materials and Methods Results Discussion References

 
Materials and Antibodies
The 1B7 and 3F4 mAbs against Drosophila neuroglian, a rat antiserum specific for the neuroglian¹⁶⁷ protein (Bieber et al., 1989; Hortsch et al., 1995) and affinity-purified rabbit anti-Drosophila ankyrin (Dubreuil and Yu, 1994) have been described earlier. The rat antiserum and the mouse 1D4 mAb against Drosophila fasciclin II, as well as the cDNA for the PEST sequence-containing, transmembrane protein form of Drosophila fasciclin II were kind gifts of C. Goodman (University of California, Berkeley, CA). Rabbit anti-phosphotyrosine antibody (She et al., 1997) was a gift of C. Palfrey (University of Chicago, Chicago, IL). Schneider's medium, penicillin/streptomycin solution, and fetal calf serum were from Life Technologies, Inc. (Gaithersburg, MD).

Construction of cDNAs for S2 Cell Transfection Experiments
Cytoplasmic domain deletions were produced by PCR with neuroglian¹⁶⁷ cDNA as template and PCR products were initially subcloned in the pAS-CYH2 vector. 5' PCR primers used in these PCRs contained a NcoI site (maintaining an open reading frame with the GAL4 DNA-binding domain), followed by a NsiI site; 3' PCR primers contained a SalI site. The numbers in the designation of individual deletion constructs refer to the 85 amino acid residues of the cytoplasmic domain of the neuroglian¹⁶⁷ protein form. Carboxy-terminal deletions were created by the introduction of in-frame stop codons along the neuroglian sequence using the 3' PCR primer; deletions in the amino-terminal region of the neuroglian cDNA by using several 5' PCR primers with homology to different regions of the neuroglian cDNA. The fidelity of the PCR amplification reactions was verified by DNA sequence analysis (Sanger et al., 1977).

Constructs incorporating the cytoplasmic deletions into the complete neuroglian open reading frame were derived from the first set of verified pAS1-CYH2 plasmids. NsiI/SalI cDNA fragments were isolated from the pAS1-CYH2 DNAs and introduced into the context of the entire neuroglian open reading frame by subcloning into pRmHa3:nrg^NsiI vector DNA. This vector was created by using PCR to introduce a silent C to A point mutation at position 3,480 of the neuroglian sequence at the end of the region encoding the transmembrane segment, thereby creating a unique NsiI site.

Neuroglian cDNAs with point mutations converting cytoplasmic tyrosine residues into phenylalanine residues were created using the following strategy. The unique BamHI site at position 3,710 of the neuroglian¹⁶⁷ cDNA sequence was used in a two-step PCR process to create initially single and subsequently double point mutations. This was accomplished by converting the flanking codons encoding tyrosine 1,217 and tyrosine 1,234 into phenylalanine-encoding codons. PCR primers including the BamHI site and one of the Y to F mutated codons (TAT/C to TTT/C) were used in separate PCR reactions and subsequently subcloned into BamHI and either NcoI- or SalI-digested pAS1-CYH2:nrg^wt (construct no. 1, wt) vector DNA. The incorporation of only the desired point mutation(s) was verified by DNA sequence analysis. As described above for the deletion mutations, all three cDNA fragments encoding Y to F mutated, neuroglian¹⁶⁷ cytoplasmic domains were subsequently subcloned into the pRmHa3:nrg^NsiI vector for transfection of S2 cells.

A chimeric cDNA was constructed by the in-frame fusion of DNA fragments encoding the extracellular domain of Drosophila fasciclin II and the transmembrane segment plus the cytoplasmic domain of Drosophila neuroglian¹⁶⁷. A 0.45-kb KpnI/SalI PCR product encoding the neuroglian transmembrane segment and the cytoplasmic domain was derived from a Drosophila neuroglian¹⁶⁷ cDNA and subcloned into pRmHa3 vector DNA. Besides the KpnI cloning site, the 5' PCR primer also introduced an AatII site which was in-frame with the AatII site at position 2,581 in the fasciclin II cDNA. This interim construct was cut with KpnI and AatII and then ligated to a 2.6-kb fasciclin II cDNA fragment, resulting in the final pRmHa3–fasII^EC–nrg^TM+CP construct. The entire open reading frame of the transmembrane, PEST sequence-containing fasciclin II cDNA, was subcloned into the pRmHa3 vector yielding the pRmHa3–fasII^PEST construct.

Generation and Maintenance of S2 Cell Lines
All Drosophila S2 cell lines were transfected using Lipofectin^® (Life Technologies, Inc.) and clonal lines were maintained as previously described (Bieber, 1994). After induction with 0.7 mM of CuSO₄, subclones were analyzed by Western blotting for high level expression of recombinant proteins and subclones expressing comparable quantities of neuroglian were selected for further experiments.

Cell Aggregation Experiments
The ability of mutated neuroglian to induce homophilic cell aggregation of transfected S2 cells was tested as described earlier (Hortsch et al., 1995). Cell lines were adjusted to a concentration of 10⁶ cells/ml and neuroglian synthesis was induced by the addition of 0.7 mM of CuSO₄. Duplicate cultures (10⁶ cells in 1 ml) were grown in six-well tissue culture plates and induced at 25°C for 15 h. Cells were transferred to sterile 50-ml centrifuge tubes and further incubated on a shaking platform (model 62; New Brunswick Sci. Co., Edison, NJ) at 200 rpm. For a quantitative analysis, the number of nonaggregated cells was counted in a hemocytometer (Bright-Line^®; Reichert, Buffalo, NY). Since cell clusters of up to five cells were occasionally observed in untransfected S2 cells, only aggregates containing more than five cells were considered to be aggregated. Eight fields, each representing 0.01 µl of cell suspension, were counted per culture. Based on the starting number of cells, the results are presented as percent aggregated cells of total cells.

SDS-PAGE and Western Blot Analysis
For Western blots, transfected S2 cells were pelleted and solubilized in SDS-containing buffer. Total cell proteins were separated by PAGE, transferred onto nitrocellulose filters, and then probed with specific antibodies as described (Hortsch et al., 1985; Dubreuil et al., 1987). Proteins were separated on either 7.5/0.2% or 8.0/0.08% acrylamide:bisacrylamide gels.

Yeast Two-Hybrid Analysis
The yeast two-hybrid system was used as described by Durfee et al. (1993). The pACTII–ankyrin construct has been characterized previously (Dubreuil et al., 1996). The pACTII-control plasmid was kindly provided by J. Clemens (University of Michigan, Ann Arbor, MI). Yeast selection plates and media were made and yeast transformations were performed using established protocols (Ausubel et al., 1988). Staining for β-galactosidase expression in yeast cell colonies was assayed using the substrate 5-bromo-4-chloro-3-indolyl-β-D-galactopyranoside as described (Bartel et al., 1993). Quantitative determinations of β-galactosidase expression were done on 4-ml liquid yeast cultures using O-nitrophenyl-β-D-galactoside as substrate (Ausubel et al., 1988).

Immunofluorescence Staining and Microscopy
Immunofluorescence analysis of Drosophila ankyrin distribution in S2 cell aggregates was performed as described previously (Dubreuil et al., 1996). Briefly, cells were attached to alcian blue–coated microscope slides, fixed in 4% paraformaldehyde, permeabilized in 0.1% Triton X-100, and then reacted with antibodies and washed in pH 7.5 Tris-buffered saline containing 5% newborn calf serum.

	Results

Top Abstract Materials and Methods Results Discussion References

 
A Conserved Distal Region of the Neuroglian Cytoplasmic Domain Binds Ankyrin
To determine the cytoplasmic neuroglian subdomains that are involved in ankyrin binding, we engineered a series of neuroglian deletion constructs to test their ability to interact with Drosophila ankyrin (Fig. 1). Deletion breakpoints were selected to isolate several protein segments that are broadly conserved among members of the L1 gene family. It has previously been shown that these conserved regions form functionally and structurally important L1 subdomains, such as the ankyrin-binding site (Davis and Bennett, 1994; Garver et al., 1997; Tuvia et al., 1997).

View larger version (18K): [in this window] [in a new window] [Download PPT slide]   Figure 1 cDNA constructs introducing various deletions and point mutations into the cytoplasmic domain of Drosophila neuroglian. Truncations at the amino- and carboxyl-terminal end of the neuroglian167 cytoplasmic domain, an internal deletion, and tyrosine to phenylalanine point mutations were generated by PCR as described in the Materials and Methods section. Lines represent the wild-type or mutated neuroglian cytoplasmic domains, starting at the first basic amino acid residue after the membrane-spanning segment and ending at the carboxy-terminus of the protein. The results of the yeast two-hybrid interaction between Drosophila ankyrin and the neuroglian cytoplasmic deletion proteins, as well as the ability of these deleted neuroglian molecules to induce S2 cell aggregation and to recruit ankyrin to S2 cell contacts are summarized on the righ.Wild-type activity levels are indicated with ++. At the bottom of the figure, cytoplasmic amino acid residues which are conserved in more than 90% of all known L1 family members are shown.

View larger version (73K): [in this window] [in a new window] [Download PPT slide]   Figure 2 A qualitative and quantitative yeast two-hybrid analysis maps the minimal ankyrin binding site to a 17-amino acid segment within the Drosophila neuroglian cytoplasmic domain with the next 19 carboxy-terminal amino acid residues being required for high efficiency binding. (A) Qualitative yeast two-hybrid analysis of the interaction between neuroglian cytoplasmic domain fragments and Drosophila ankyrin. Blue colonies result from the induction of β-galactosidase activity and indicate an interaction between the two GAL4 fusion proteins. Top row, yeast colonies containing a pACTII–Drosophila ankyrin construct (expressing a GAL4 activation domain–Drosophila ankyrin fusion protein) as well as a pAS1–CYH2 construct (expressing a fusion protein consisting of the GAL4 DNA-binding domain and a wild-type or deleted neuroglian cytoplasmic domain); bottom row, yeast colonies containing the same pAS1–CYH2 constructs and a pACTII vector control that did not result in an activation of β-galactosidase expression. (B) Quantitative analysis of the effects of neuroglian cytoplasmic deletions on the yeast two-hybrid neuroglian–ankyrin interaction. Data bars represent the mean ± SD from three different yeast colonies performed in triplicate determinations.

View larger version (45K): [in this window] [in a new window] [Download PPT slide]   Figure 3 Quantitative evaluation of S2 cell aggregation induced by the expression of mutated neuroglian. For a quantification of S2 cell aggregation, duplicate cultures were prepared, induced for 15 h at low cell density, and then processed as described in the Materials and Methods section. Cells that had not aggregated were counted (minimal aggregate size >5 cells) and the number of aggregated cells was calculated as the difference to the total number of cells. Shown is the percentage of total cells which had aggregated after 2 h of shaking. Data bars represent the mean ± SD from two independent experiments.

View larger version (83K): [in this window] [in a new window] [Download PPT slide]   Figure 4 A conserved membrane-proximal segment of the neuroglian cytoplasmic domain is dispensable for recruitment of ankyrin to cell contacts in S2 cells. S2 cells expressing wild-type or cytoplasmic deletion Drosophila neuroglian were allowed to aggregate and were double stained with a polyclonal rabbit anti- Drosophila ankyrin (left column) and a mouse anti-Drosophila neuroglian antibody (right column) followed by fluorescently- labeled secondary antibodies. Cells were permeabilized before staining by treatment with 0.1% Triton X-100. Drosophila ankyrin was recruited to cell contact sites (arrows) in cell aggregates expressing either wild-type neuroglian (A) or neuroglian in which the first 18 amino acid residues of the cytoplasmic domain had been deleted (construct no. 2 shown in row B). All other deletions in the cytoplasmic neuroglian domain abolished ankyrin recruitment (as shown for construct no. 9 in panels C). Bar, 10 µm.

18N

19C

Functional Analysis of Conserved Tyrosine Residues in the Cytoplasmic Domain of Neuroglian
A conserved cytoplasmic tyrosine residue in rat neurofascin, corresponding to Y1234 in neuroglian, was previously shown to have a possible regulatory role, since phosphorylation of this residue inhibited the binding of ankyrin to neurofascin in vitro (Garver et al., 1997). Here the effects of tyrosine to phenylalanine mutations at two positions of the Drosophila neuroglian cytoplasmic domain on ankyrin binding were evaluated using a yeast two-hybrid assay. The residues Y1217 and Y1234 in neuroglian correspond to the tyrosine residues in rat neurofascin which were mutated and analyzed by Garver et al. (1997). Replacement of Y1217 with a phenylalanine had no detectable effect on ankyrin binding (Fig. 5). However, the Y1234F mutation had a significant effect, reducing ankyrin binding by 50%. The double mutant Y1217F/Y1234F form reduced ankyrin binding to a similar extent. Thus, the conserved Y1234 contributes to the interaction between ankyrin and neuroglian. However, in contrast to rat neurofascin (Tuvia et al., 1997), substitution of the tyrosine residue with phenylalanine in neuroglian greatly reduced its ability to bind ankyrin.

View larger version (83K): [in this window] [in a new window] [Download PPT slide]   Figure 5 Qualitative and quantitative yeast two-hybrid analysis of the interaction between Drosophila ankyrin and neuroglian167 cytoplasmic domains with tyrosine to phenylalanine amino acid substitutions. (A) Qualitative yeast two-hybrid analysis of the interaction between Y to F neuroglian cytoplasmic domain mutations and Drosophila ankyrin. Blue colonies result from the induction of β-galactosidase activity and indicate an interaction between the two GAL4 fusion proteins. Top row, yeast colonies containing a pACTII–Drosophila ankyrin construct (expressing a GAL4 activation domain–Drosophila ankyrin fusion protein) as well as a pAS1-CYH2 construct (expressing a fusion protein consisting of the GAL4 DNA-binding domain and a neuroglian cytoplasmic domain, which was either wild-type or contained one or two point mutations resulting in Y to F amino acid substitutions); bottom row, yeast colonies containing the same pAS1–CYH2 constructs and a pACTII vector control. (B) Quantitative evaluation of β-galactosidase expression in the yeast cells shown in A. Data bars represent the mean ± SD from two different experiments performed in triplicate determinations.

View larger version (92K): [in this window] [in a new window] [Download PPT slide]   Figure 6 A cytoplasmic tyrosine residue is required for efficient recruitment of ankyrin to cell contacts in neuroglian-expressing S2 cells. S2 cells were induced to express wild-type neuroglian (A), nrgY1217F (B), nrgY1234F (C and D), or double mutant neuroglian (E–G) for 24 h before processing for antibody labeling of neuroglian (left panels) and ankyrin (right panels) as in Fig. 4. Arrows, abundance of neuroglian at noncontact regions of the plasma membrane; arrowheads, cell contact sites in mutant cells with little or no recruitment of ankyrin. Bar, 10 µM.

View larger version (57K): [in this window] [in a new window] [Download PPT slide]   Figure 7 Quantification of ankyrin recruitment in S2 cells expressing neuroglian proteins mutated at cytoplasmic tyrosines. Populations of transfected S2 cells expressing wild-type neuroglian (Nrg167) or the indicated tyrosine mutations of neuroglian were double labeled with mouse anti-neuroglian and rabbit anti-ankyrin antibodies as in Fig. 3. In each experiment, 100 S2 cell clusters were identified by virtue of their neuroglian expression and then scored for the presence or absence of detectable ankyrin staining at cell contacts. Data bars represent the mean ± SD from two independent experiments.

Drosophila Neuroglian Is Not Detectably Phosphorylated at Tyrosine Residues in S2 Cells
Further evidence that tyrosine phosphorylation is not responsible for neuroglian regulation in S2 cells was obtained by staining Western blots of neuroglian-expressing S2 cell lysates with a phosphotyrosine-specific antibody (Fig. 8). After induction, neuroglian was readily detected with a neuroglian-specific antibody (Fig. 8, lane 2, left column), but not with the anti-phosphotyrosine antibody (Fig. 8, lane 2, right column). Faint bands in the region of neuroglian were also detected by the anti-phosphotyrosine antibody in uninduced cells (Fig. 8, lane 1, right column) where neuroglian was undetectable (Fig. 8, lane 1, left column). PC12 cells treated with nerve growth factor were used as a positive control. Tyrosine-phosphorylated mitogen-activated protein (MAP) kinase was readily detected in growth factor-induced PC12 cells (Fig. 8, lane 4, **) but not in control untreated cells (Fig. 8, lane 3) (Boulton et al., 1991).

View larger version (77K): [in this window] [in a new window] [Download PPT slide]   Figure 8 Neuroglian is not phosphorylated on tyrosine residues in S2 cells. Western blots of total S2 cell proteins from uninduced cells (lane 1) or cells induced to express neuroglian (lane 2) were stained with mouse anti-neuroglian (lanes 1 and 2, left columns) or rabbit anti-phosphotyrosine antibodies (right columns). Antibody binding was detected with alkaline phosphatase-conjugated secondary antibodies. Total proteins from control PC12 cells (lane 3) and nerve growth factor-stimulated PC12 cells (lane 4) were also stained with anti-phosphotyrosine antibody. The positions of neuroglian (*), MAP kinase (**) and molecular weight standards (left) are indicated.

View larger version (98K): [in this window] [in a new window] [Download PPT slide]   Figure 9 S2 cells expressing neuroglian with a cytoplasmic Y1234F mutation exhibit a reduced level of cell aggregation. S2 cell lines that had been transfected with either wild-type (B) or mutated neuroglian cDNA constructs (C, NrgY1217F; D, NrgY1234F; and E, NrgnrgY1217/1234F) were induced for 15 h with Cu2+ ions and subsequently incubated at room temperature on a shaking platform at 200 rpm for 4 h. (A) Control cells not expressing neuroglian. S2 cells cultures were processed in parallel for Western blot analysis and probed with the neuroglian-specific 3F4 mAb (F). The equivalent of 5 x 105 cells was loaded in each lane. Bar, 200 µm.

View larger version (80K): [in this window] [in a new window] [Download PPT slide]   Figure 10 Western blots of fasciclin II, neuroglian, and fasciclin IIEC-neuroglianTM+CP hybrid proteins expressed in S2 cells. S2 cells, which had been transfected with a fasciclin II (PEST form) (lanes 1), a neuroglian167 (lanes 2), or a fasciclin IIEC-neuroglianTM+CP (lanes 3) cDNA construct, were induced overnight and processed for Western blot analysis. Blot A was incubated with the neuroglian-specific mAb 3F4 which recognizes an epitope on the neuroglian extracellular domain, blot B with a rat polyclonal antiserum which was raised against the entire fasciclin II protein, blot C with the mAb 1D4 which binds to a cytoplasmic epitope of the fasciclin II (PEST) protein form, and blot D with a polyclonal rat antiserum which was raised against a small peptide representing the eight carboxy-terminal amino acid residues of the neuroglian167 form.

View larger version (85K): [in this window] [in a new window] [Download PPT slide]   Figure 11 Selective recruitment of ankyrin to cell contacts in S2 cells expressing a chimeric neuroglian molecule. S2 cells were induced to express the adhesion molecule fasciclin II (A and B) or a chimeric molecule (fasciclin IIEC-neuroglianTM+CP) in which the extracellular neuroglian domain was replaced with the corresponding domain from fasciclin II (C–F). Cells were induced for 48 h and then processed for immunofluorescent staining with antibodies against ankyrin (A, C, and E) and against the extracellular domain of either fasciclin II (B and D) or neuroglian (F). Control experiments (D, inset) revealed that fasciclin II was abundantly detected at all regions of the plasma membrane when the detergent permeabilization step was omitted. Bar, 10 µM.

	Discussion

Top Abstract Materials and Methods Results Discussion References

Whereas the inside-out regulation of neuroglian's adhesive function is one finding of the present study, our approach has largely been directed toward the mechanism of outside-in signaling. Drosophila S2 cells provide a unique model system in which to study the recruitment of ankyrin to the plasma membrane, since ankyrin is not ordinarily associated with the plasma membrane of these cells. We previously demonstrated that both Drosophila neuroglian (Dubreuil et al., 1996) and human L1-CAM (Vallejo et al., 1997; Hortsch et al., 1998) induce the selective recruitment of ankyrin to sites of cell contact, even though the adhesion molecules themselves are broadly expressed over the entire cell surface. Once neuroglian has interacted with ankyrin at cell–cell contact sites, it becomes resistant to extraction by nonionic detergents (Dubreuil et al., 1996). This change in the solubility of neuroglian precludes an analysis of the neuroglian–ankryin interaction by immunoprecipitation techniques and, when using immunofluorescence microscopy, results in an underrepresentation of neuroglian staining at noncontact areas of the S2 plasma membrane.

It was previously shown that the FIGQY sequence, which is highly conserved throughout the L1 family, provides an essential part of the ankyrin-binding domain in rat neurofascin (Davis and Bennett, 1994; Garver et al., 1997). Through a combination of yeast two-hybrid analysis and expression of mutated neuroglian molecules in S2 cells, we have mapped a larger, 36-amino acid segment in the neuroglian cytoplasmic domain, which includes this conserved motif, that is both necessary and sufficient to allow the interaction between neuroglian and ankyrin.

The demonstration that ankyrin binding to rat neurofascin can be regulated by phosphorylation of the tyrosine residue in the FIGQY motif (Garver et al., 1997; Tuvia et al., 1997) suggested a possible mechanism to explain outside-in regulation of neuroglian. Phosphorylation of this conserved tyrosine in the cytoplasmic domain of neurofascin caused an 40% reduction in ankyrin binding and a comparable decrease in cell aggregation. Based on these properties of neurofascin, we hypothesized that the association of ankyrin with neuroglian in S2 cells could also be regulated by tyrosine phosphorylation, assuming that the phosphorylation of the tyrosine residue in the FIGQY motif is regulated by cell adhesion.

If neuroglian were phosphorylated on tyrosine residues in S2 cells, and phosphorylation was responsible for the lack of ankyrin binding to neuroglian at noncontact sites of aggregated S2 cells, then the mutation of tyrosine residue 1234 in Drosophila neuroglian would be expected to cause ankyrin binding indiscriminately at all regions of the plasma membrane. Although the neuroglian Y1234F mutation greatly reduced the extent of ankyrin binding to neuroglian, it did not affect the selective association of ankyrin at sites of cell–cell contact or the lack of ankyrin at noncontact regions of the plasma membrane. Thus, another mechanism must be responsible for the outside-in regulation of ankyrin recruitment in S2 cells. We therefore suggest that the previously observed effects of tyrosine phosphorylation on rat neurofascin constitutes a mechanism of regulation that might be specific for the neurofascin subfamily. Alternatively, tyrosine phosphorylation may operate in regulating ankyrin binding to L1 molecules in some cell types, such as the B104 neuroblastoma cell line, but not in other cells. S2 cells may simply lack a tyrosine kinase of the appropriate specificity for the FIGOY motif to produce an effect on ankyrin binding. It is important to note that these two mechanisms for regulating the interaction between ankyrin and L1 molecules are not mutually exclusive, and the phosphorylation of the conserved tyrosine residue in the FIGQY motif might provide an additional way to inhibit L1-mediated cell adhesion and L1 binding to the membrane skeleton.

Other types of protein phosphorylation might also be involved in regulating the association of ankyrin with neuroglian in vivo or in S2 cells. Several cytoplasmic serine residues are also highly conserved throughout the L1 family and some have been shown to be the target of protein kinases (Wong et al., 1996a,b). The phosphorylation of these residues might have an effect on ankyrin binding to L1 family members and play an important role in the regulation of this interaction in S2 cells.

The regulation of ankyrin binding to L1-type molecules might also involve the adhesion-induced clustering of several L1 molecules within the plane of the plasma membrane, similar to the mechanism of growth factor receptor activation (Schlessinger and Ullrich, 1992). Alternatively, the homophilic adhesion process could induce an allosteric change in the neuroglian molecule. However, the finding that a chimeric molecule, composed of the extracellular domain of a distantly related adhesion molecule coupled to the cytoplasmic and transmembrane domains of neuroglian, exhibits the same regulated association with ankyrin as wild-type neuroglian argues against the allosteric model.

Our results indicate that the tyrosine residue in the conserved FIGQY motif plays an important role in L1's interaction with the membrane skeleton and its adhesive function. One of the identified L1-CAM mutations, which causes a range of neurological phenotypes in humans, results in the exchange of tyrosine 1229 in the human L1 protein for a histidine residue (Van Camp et al., 1996). Residue Y1229 in human L1-CAM is homologous to Y1234 in the Drosophila neuroglian sequence. Considering that the cytoplasmic domain of human L1 CAM is dispensable for its adhesive function (Wong et al., 1995a), it has been an enigma why mutations in the cytoplasmic domain of human L1-CAM can cause the same range of phenotypes as mutations in the extracellular domain. It now appears that extracellular adhesive and intracellular cytoskeletal interactions of L1 molecules are functionally connected and therefore influence each other. Members of the L1 family are expressed on advancing growth cones during development and during regeneration after nerve injury and by other motile neuronal cells, such as migrating granule cells (Lindner et al., 1983; Kamiguchi and Lemmon, 1997). A precise regulation of neuronal adhesiveness must be very important in these cells to allow dynamic interactions with their cellular environment. Any mutation interrupting this delicate adhesive balance might therefore cause the observed wide range of L1 mutant phenotypes (Wong et al., 1995b; Dahme et al., 1997; Hall and Bieber, 1997).

	Acknowledgments

 
We would like to thank C. Goodman (University of California, Berkeley, CA) for making the fasciclin II cDNA and the anti-fasciclin II antibodies available to us, C. Palfrey for providing the anti-phosphotyrosine antibody, and M. Wert (both from University of Chicago, Chicago, IL) for PC12 cell samples. We would also like to thank M. Wyche (Alabama A & M University, Normal, AL) and M. Hadeed for help with several of the described experiments and S. Brown and S. Ernst (all three from University of Michigan, Ann Arbor, MI) for a critical reading of the manuscript.

Submitted: 17 February 1998

Revised: 2 June 1998

The work described in this publication has been supported by grants from the National Institutes of Health to R.R. Dubreuil (GM 49301 and DK 42086) and to M. Hortsch (HD 29388).

Address all correspondence to Michael Hortsch, Department of Anatomy and Cell Biology, University of Michigan, Ann Arbor, MI 48109-0616. Tel.: (734) 647-2720. Fax: (734) 763-1166. E-mail: hortsch{at}umich.edu

	References

Top Abstract Materials and Methods Results Discussion References

 

Ausubel, F.M., R. Brent, R.E. Kingston, D.D. Moore, J.G. Seidman, J.A. Smith, and K. Struhl. 1988. Current Protocols in Molecular Biology. J. Wiley & Sons, Inc., New York.

Bartel, P.L., C.-t. Chien, R. Sternglanz, and S. Fields. 1993. Using the two- hybrid system to detect protein-protein interactions. In Cellular Interactions in Development: A Practical Approach. D.A. Hartley, editor. IRL Press, Oxford, UK. 153–179.

Bieber, A.J. 1994. Analysis of cellular adhesion in cultured cells. In Drosophila melanogaster: Practical Uses in Cell Biology. L. Goldstein and E. Fyrberg, editors. 44:683–696. Academic Press, San Diego, CA.

Bieber AJ, Snow PM, Hortsch M, Patel NH, Jacobs JR, Traquina ZR, Schilling J & Goodman CS. Drosophilaneuroglian: a member of the immunoglobulin superfamily with extensive homology to the vertebrate neural adhesion molecule L1, Cell, 1989, 59, 447–460.[Medline]

Boulton TG, Nye SH, Robbins DJ, Ip NY, Radziejewska E, Morgenbesser SD, DePinho RA, Panayotatos N, Cobb MH & Yancopoulos GD. ERKs: a family of protein-serine/threonine kinases that are activated and tyrosine phosphorylated in response to insulin and NGF, Cell, 1991, 65, 663–675.[Medline]

Clark EA & Brugge JS. Integrins and signal transduction pathways: the road taken, Science, 1995, 268, 233–239.[Abstract/Free Full Text]

Dahme M, Bartsch U, Martini R, Anliker B, Schachner M & Mantei N. Disruption of the mouse L1 gene leads to malformations of the nervous system, Nat Genet, 1997, 17, 346–349.[Medline]

Davis JQ & Bennett V. Ankyrin binding activity shared by the neurofascin/L1/NrCAM family of nervous system cell adhesion molecules, J Biol Chem, 1994, 269, 27163–27166.[Abstract/Free Full Text]

Davis JQ, McLaughlin T & Bennett V. Ankyrin-binding proteins related to nervous system cell adhesion molecules: candidates to provide transmembrane and intercellular connections in adult brain, J Cell Biol, 1993, 121, 121–133.[Abstract/Free Full Text]

Dubreuil RR & Yu J-Q. Ankyrin and beta-spectrin accumulate independently of alpha-spectrin in Drosophila. , Proc Natl Acad Sci USA, 1994, 91, 10285–10289.[Abstract/Free Full Text]

Dubreuil RR, Byers TJ, Branton D, Goldstein LSB & Kiehart DP. Drosophiliaspectrin. I. Characterization of the purified protein, J Cell Biol, 1987, 105, 2095–2102.[Abstract/Free Full Text]

Dubreuil RR, MacVicar G, Dissanayake S, Liu C, Homer D & Hortsch M. Neuroglian-mediated cell adhesion induces assembly of the membrane skeleton at cell contact sites, J Cell Biol, 1996, 133, 647–655.[Abstract/Free Full Text]

Dubreuil RR, Maddux PB, Grushko TA & MacVicar GR. Segregation of two spectrin isoforms: polarized membrane-binding sites direct polarized membrane skeleton assembly, Mol Biol Cell, 1997, 8, 1933–1942.[Abstract/Free Full Text]

Durfee T, Becherer K, Chen PL, Yeh SH, Yang Y, Kilburn AE, Lee WH & Elledge SJ. The retinoblastoma protein associates with the protein phosphatase type 1 catalytic subunit, Genes Dev, 1993, 7, 555–569.[Abstract/Free Full Text]

Garver TD, Ren Q, Tuvia S & Bennett V. 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, 1997, 137, 703–714.[Abstract/Free Full Text]

Grenningloh G, Rehm EJ & Goodman CS. Genetic analysis of growth cone guidance in Drosophila: fasciclin II functions as a neuronal recognition molecule, Cell, 1991, 67, 45–57.[Medline]

Gumbiner BM. Signal transduction of beta-catenin, Curr Opin Cell Biol, 1995, 7, 634–640.[Medline]

Hall SG & Bieber AJ. Mutations in the Drosophilaneuroglian cell adhesion molecule affect motor neuron pathfinding and peripheral nervous system patterning, J Neurobiol, 1997, 32, 325–340.[Medline]

Hortsch M. The L1 family of neural cell adhesion molecules: old proteins performing new tricks, Neuron, 1996, 17, 587–593.[Medline]

Hortsch M, Avossa D & Meyer DI. A structural and functional analysis of the docking protein. Characterization of active domains by proteolysis and specific antibodies, J Biol Chem, 1985, 260, 9137–9145.[Abstract/Free Full Text]

Hortsch M, O'Shea KS, Zhao G, Kim F, Vallejo Y & Dubreuil RR. A conserved role for L1 as a transmembrane link between neuronal adhesion and membrane cytoskeleton assembly, Cell Adh Comm, 1998, 5, 61–73.[Medline]

Hortsch M, Wang YM, Marikar Y & Bieber AJ. The cytoplasmic domain of the Drosophilacell adhesion molecule neuroglian is not essential for its homophilic adhesive properties in S2 cells, J Biol Chem, 1995, 270, 18809–18817.[Abstract/Free Full Text]

Kamiguchi H & Lemmon V. Neural cell adhesion molecule L1: signaling pathways and growth cone motility, J Neurosci Res, 1997, 49, 1–8.[Medline]

Lindner J, Rathjen FG & Schachner M. L1 mono- and polyclonal antibodies modify cell migration in early postnatal mouse cerebellum, Nature, 1983, 305, 427–430.[Medline]

Nelson WJ & Veshnock PJ. Ankyrin binding to (Na⁺, K⁺)ATPase and implications for the organization of membrane domains in polarized cells, Nature, 1987, 328, 533–536.[Medline]

Sanger F, Nicklen S & Coulson AR. DNA sequencing with chain-terminating inhibitors, Proc Natl Acad Sci USA, 1977, 74, 5463–5467.[Abstract/Free Full Text]

Schlessinger J & Ullrich A. Growth factor signaling by receptor tyrosine kinases, Neuron, 1992, 9, 383–391.[Medline]

She H-y, Rockow S, Tang J, Nishimura R, Skolnik EY, Chen M, Margolis B & Li W. Wiskott-Aldrich Syndrome protein is associated with the adapter protein Grb2 and the epidermal growth factor receptor in living cells, Mol Biol Cell, 1997, 8, 1709–1721.[Abstract]

Tuvia S, Garver TD & Bennett V. The phosphorylation state of the FIGQY tyrosine of neurofascin determines ankyrin-binding activity and patterns of cell segregation, Proc Natl Acad Sci USA, 1997, 94, 12957–12962.[Abstract/Free Full Text]

Vallejo Y, Hortsch M & Dubreuil RR. Ethanol does not inhibit the adhesive activity of Drosophila neuroglian or human L1 in DrosophilaS2 tissue culture cells, J Biol Chem, 1997, 272, 12244–12247.[Abstract/Free Full Text]

Van Camp G, Fransen E, Vits L, Raes G & Willems PJ. A locus-specific mutation database for the neural cell adhesion molecule L1CAM (Xq28), Hum Mutat, 1996, 8, 391, .[Medline]

Walsh FS & Doherty P. Neural cell adhesion molecules of the immunoglobulin superfamily: Role in axon growth and guidance, Annu Rev Cell Dev Biol, 1997, 13, 425–456.[Medline]

Wong EV, Cheng GH, Payne HR & Lemmon V. The cytoplasmic domain of the cell-adhesion molecule L1 is not required for homophilic adhesion, Neurosci Lett, 1995a, 200, 155–158.[Medline]

Wong EV, Kenwrick S, Willems P & Lemmon V. Mutations in the cell adhesion molecule L1 cause mental retardation, Trends Neurosci, 1995b, 18, 168–172.[Medline]

Wong EV, Schaefer AW, Landreth G & Lemmon V. Casein kinase-II phosphorylates the neural cell-adhesion molecule L1, J Neurochem, 1996a, 66, 779–786.[Medline]

Wong EV, Schaefer AW, Landreth G & Lemmon V. Involvement of p90rsk in neurite outgrowth mediated by the cell adhesion molecule L1, J Biol Chem, 1996b, 271, 18217–18223.[Abstract/Free Full Text]

CiteULike

Complore

Connotea

Del.icio.us

Digg

Facebook

Reddit

Technorati

Twitter

This article has been cited by other articles:

• Buhusi, M., Schlatter, M. C., Demyanenko, G. P., Thresher, R., Maness, P. F. (2008). L1 Interaction with Ankyrin Regulates Mediolateral Topography in the Retinocollicular Projection. J. Neurosci. 28: 177-188 [Abstract] [Full Text]  
• Boiko, T., Vakulenko, M., Ewers, H., Yap, C. C., Norden, C., Winckler, B. (2007). Ankyrin-Dependent and -Independent Mechanisms Orchestrate Axonal Compartmentalization of L1 Family Members Neurofascin and L1/Neuron-Glia Cell Adhesion Molecule. J. Neurosci. 27: 590-603 [Abstract] [Full Text]  
• Parks, A. L., Stout, J. R., Shepard, S. B., Klueg, K. M., Dos Santos, A. A., Parody, T. R., Vaskova, M., Muskavitch, M. A. T. (2006). Structure-Function Analysis of Delta Trafficking, Receptor Binding and Signaling in Drosophila. Genetics 174: 1947-1961 [Abstract] [Full Text]  
• Whittard, J. D., Sakurai, T., Cassella, M. R., Gazdoiu, M., Felsenfeld, D. P. (2006). MAP Kinase Pathway-dependent Phosphorylation of the L1-CAM Ankyrin Binding Site Regulates Neuronal Growth. Mol. Biol. Cell 17: 2696-2706 [Abstract] [Full Text]  
• Banerjee, S., Pillai, A. M., Paik, R., Li, J., Bhat, M. A. (2006). Axonal ensheathment and septate junction formation in the peripheral nervous system of Drosophila.. J. Neurosci. 26: 3319-3329 [Abstract] [Full Text]  
• Cheng, L., Itoh, K., Lemmon, V. (2005). L1-Mediated Branching Is Regulated by Two Ezrin-Radixin-Moesin (ERM)-Binding Sites, the RSLE Region and a Novel Juxtamembrane ERM-Binding Region. J. Neurosci. 25: 395-403 [Abstract] [Full Text]  
• Szafranski, P., Goode, S. (2004). A Fasciclin 2 morphogenetic switch organizes epithelial cell cluster polarity and motility. Development 131: 2023-2036 [Abstract] [Full Text]  
• Nishimura, K., Yoshihara, F., Tojima, T., Ooashi, N., Yoon, W., Mikoshiba, K., Bennett, V., Kamiguchi, H. (2003). L1-dependent neuritogenesis involves ankyrinB that mediates L1-CAM coupling with retrograde actin flow. JCB 163: 1077-1088 [Abstract] [Full Text]  
• Buhusi, M., Midkiff, B. R., Gates, A. M., Richter, M., Schachner, M., Maness, P. F. (2003). Close Homolog of L1 Is an Enhancer of Integrin-mediated Cell Migration. J. Biol. Chem. 278: 25024-25031 [Abstract] [Full Text]  
• Malhotra, J. D., Koopmann, M. C., Kazen-Gillespie, K. A., Fettman, N., Hortsch, M., Isom, L. L. (2002). Structural Requirements for Interaction of Sodium Channel beta 1 Subunits with Ankyrin. J. Biol. Chem. 277: 26681-26688 [Abstract] [Full Text]  
• Dickson, T. C., Mintz, C. D., Benson, D. L., Salton, S. R.J. (2002). Functional binding interaction identified between the axonal CAM L1 and members of the ERM family. JCB 157: 1105-1112 [Abstract] [Full Text]  
• Kamiguchi, H., Yoshihara, F. (2001). The Role of Endocytic L1 Trafficking in Polarized Adhesion and Migration of Nerve Growth Cones. J. Neurosci. 21: 9194-9203 [Abstract] [Full Text]  
• Bennett, V., Baines, A. J. (2001). Spectrin and Ankyrin-Based Pathways: Metazoan Inventions for Integrating Cells Into Tissues. Physiol. Rev. 81: 1353-1392 [Abstract] [Full Text]  
• Bai, J, Chiu, W, Wang, J, Tzeng, T, Perrimon, N, Hsu, J (2001). The cell adhesion molecule Echinoid defines a new pathway that antagonizes the Drosophila EGF receptor signaling pathway. Development 128: 591-601 [Abstract]  
• Moulding, H. D., Martuza, R. L., Rabkin, S. D. (2000). Clinical Mutations in the L1 Neural Cell Adhesion Molecule Affect Cell-Surface Expression. J. Neurosci. 20: 5696-5702 [Abstract] [Full Text]  
• Bouley, M., Tian, M.-Z., Paisley, K., Shen, Y.-C., Malhotra, J. D., Hortsch, M. (2000). The L1-Type Cell Adhesion Molecule Neuroglian Influences the Stability of Neural Ankyrin in the Drosophila Embryo But Not Its Axonal Localization. J. Neurosci. 20: 4515-4523 [Abstract] [Full Text]  
• Malhotra, J. D., Kazen-Gillespie, K., Hortsch, M., Isom, L. L. (2000). Sodium Channel beta Subunits Mediate Homophilic Cell Adhesion and Recruit Ankyrin to Points of Cell-Cell Contact. J. Biol. Chem. 275: 11383-11388 [Abstract] [Full Text]  
• Malhotra, J. D., Tsiotra, P., Karagogeos, D., Hortsch, M. (1998). Cis-activation of L1-mediated Ankyrin Recruitment by TAG-1 Homophilic Cell Adhesion. J. Biol. Chem. 273: 33354-33359 [Abstract] [Full Text]  
• Scotland, P., Zhou, D., Benveniste, H., Bennett, V. (1998). Nervous System Defects of AnkyrinB (-/-) Mice Suggest Functional Overlap between the Cell Adhesion Molecule L1 and 440-kD AnkyrinB in Premyelinated Axons. JCB 143: 1305-1315 [Abstract] [Full Text]  
• Zhang, X., Davis, J. Q., Carpenter, S., Bennett, V. (1998). Structural Requirements for Association of Neurofascin with Ankyrin. J. Biol. Chem. 273: 30785-30794 [Abstract] [Full Text]  
• Jefford, G., Dubreuil, R. R. (2000). Receptor Clustering Drives Polarized Assembly of Ankyrin. J. Biol. Chem. 275: 27726-27732 [Abstract] [Full Text]  

This Article Abstract Full Text (PDF, 5379K) PPT slides of all figures Alert me when this article is cited Citation Map Services Email this article Similar articles in this journal Similar articles in PubMed Alert me to new content in the JCB Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via CrossRef Citing Articles via Google Scholar Google Scholar Articles by Hortsch, M. Articles by Dubreuil, R. R. Search for Related Content PubMed PubMed Citation Articles by Hortsch, M. Articles by Dubreuil, R. R. Pubmed/NCBI databases Gene GEO Profiles HomoloGene Protein UniGene Compound via MeSH Substance via MeSH Hazardous Substances DB L-TYROSINE Social Bookmarking                            What's this?