The Role of Endocytic L1 Trafficking in Polarized Adhesion and Migration of Nerve Growth Cones

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The Journal of Neuroscience, December 1, 2001, 21(23):9194-9203

The Role of Endocytic L1 Trafficking in Polarized Adhesion and Migration of Nerve Growth Cones
Hiroyuki Kamiguchi and Fumie Yoshihara
Developmental Brain Science Group, RIKEN Brain Science Institute, Wako, Saitama 351-0198, Japan

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Motility of the nerve growth cone is highly dependent on its dynamic interactions with the microenvironment mediated by celladhesion molecules (CAMs). These adhesive interactions can bespatially regulated by changing the density and avidity of CAMson the growth cone. Previous studies have shown that L1, a memberof the immunoglobulin superfamily of CAMs, is endocytosed at thecentral domain of the growth cone followed by centrifugal vesiculartransport and reinsertion into the plasma membrane of the leadingedge. The present paper focuses on the functional significanceof endocytic L1 trafficking in dorsal root ganglia neurons invitro. We demonstrate that the rate of L1-based neurite growthhas a positive correlation with the amount of endocytosed L1 inthe growth cone, whereas stimulation of neurite growth via anN-cadherin-dependent mechanism does not increase L1 endocytosis.A growth cone that migrates on an L1 substrate exhibits a steepgradient of L1-mediated adhesion (strong adhesion at the growthcone's leading edge and weak adhesion at the central domain).This gradient of L1 adhesion is attenuated after inhibition ofL1 endocytosis in the growth cone by intracellular loading ofa function-blocking antibody against $alpha$ -adaptin, a subunit of theclathrin-associated AP-2 adaptor. Inhibition of L1 endocytosisby this antibody also decreased the rate of L1-dependent growthcone migration. These results indicate that the growth cone activelytranslocates CAMs to create spatial asymmetry in adhesive interactionswith its environment and that this spatial asymmetry is importantfor growth conemigration.

Key words: cell adhesion molecule; L1; N-cadherin; nerve growth cone; endocytosis; neurite growth

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Axonal elongation during neural development is highly dependent on the regulated motility of nerve growth cones (Mueller,1999). Adhesive interactions of the growth cone with its microenvironmentplay an integral role in determining the motile behavior of growthcones (Isbister and O'Connor, 2000). Such interactions are mediatedby cell adhesion molecules (CAMs) on the growth cone that recognizelocalized guidance cues present on neighboring cells and in theextracellular matrix (ECM). The in vivo importance of CAMs inaxon tract development has been confirmed, for example, by thefact that mutations of L1, a member of the Ig superfamily of CAMs(IgCAMs), cause defects in the corticospinal tract and the corpuscallosum in humans and mice (Dahme et al., 1997; Cohen et al.,1998; Fransen et al., 1998; Kamiguchi et al., 1998a; Demyanenkoet al., 1999; Kenwrick et al., 2000).

Although CAMs mediate cell-cell and cell-ECM adhesion, a cytoplasmic tail of many CAMs binds the cytoskeleton, which alsoplays a critical role in growth cone motility (Tanaka and Sabry,1995; Letourneau, 1996). Spatially localized actin polymerization/depolymerizationand actin-myosin interactions generate retrograde flow of actinfilaments (Mitchison and Cramer, 1996), which then produces atraction force to pull the growth cone forward when coupled mechanicallyto CAMs (Suter et al., 1998). Forward translocation of the growthcone requires not only the CAM-cytoskeletal linkage but also agradient of adhesive interactions with its environment (strongadhesion at the leading edge of the growth cone and weak adhesionat the rear) (Lauffenburger and Horwitz, 1996). In this way, thecytoskeletal machinery is able to move the growth cone forwardas attachments at its rear are released. To create such polarizedadhesion by spatial regulation of CAM density, CAMs that havebeen translocated into the central (C) domain of growth conesby coupling to the retrograde actin flow should be recycled tothe leading edge. Indeed, it has been shown that CAMs, such asneural CAM (NCAM) and $beta$ 1 integrin, undergo bidirectional movementon the growth cone surface, suggesting the centrifugal transportfor CAM recycling (Sheetz et al., 1990; Schmidt et al., 1995;Grabham et al., 2000). In addition to this cell surface pathway,an intracellular pathway for CAM recycling has been demonstratedpreviously (Kamiguchi et al., 1998b; Kamiguchi and Lemmon, 2000b):L1 is endocytosed preferentially at the C-domain followed by centrifugaltransport into the peripheral (P) domain and reinsertion intothe plasma membrane of the leading edge. So there seem to be atleast two distinct traffic pathways for CAM recycling. However,the involvement of CAM recycling in producing polarized adhesionand directed migration of the growth cone has not been testedexperimentally.

In the present paper, we demonstrate that L1-based neurite growth is associated with increased endocytic trafficking of L1in the growth cone and that the L1 trafficking is required forpolarized adhesion and migration of the growth cone mediated byL1. These revelations will help elucidate the biophysical mechanismsby which CAMs regulate growth conemotility.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antibodies. Ng-CAM, a chick homolog of L1 (Buchstaller et al., 1996), will be termed chick L1 in this paper. Rabbit polyclonalantibodies against human L1, rat L1, chick L1, and chick NCAM,and mouse monoclonal antibody against chick L1 (8D9) were kindlyprovided by Dr. Vance Lemmon (Case Western Reserve University,Cleveland OH). These antibodies have been described previously(Lemmon and McLoon, 1986; Hlavin and Lemmon, 1991; Long et al.,2001). All the antibodies against CAMs used in the present studyrecognize their extracellular domain. Polyclonal goat antibodyagainst the Fc region of human IgG was obtained from Sigma (St.Louis, MO). Alexa-conjugated and unconjugated secondary antibodiesraised in goats were purchased from Molecular Probes (Eugene,OR) and Jackson ImmunoResearch Laboratories (West Grove, PA),respectively.

To produce a highly concentrated solution of the mouse monoclonal antibody against $alpha$ -adaptin (AP.6), mouse ascites obtainedby intraperitoneal injection of the AP.6 hybridoma cells (AmericanType Culture Collection, Rockville, MD) were processed by ammoniumsulfate precipitation and protein A column chromatography. Nonspecificmouse IgG used in control experiments was purchased from JacksonImmunoResearch Laboratories. These IgG solutions were dialyzedagainst Leibovitz's L-15 medium (Life Technologies, Gaithersburg,MD) and then loaded into neurons byelectroporation.

Production of CAM-Fc chimeric proteins. Three chimeric proteins (human L1-Fc, chick L1-Fc, and N-cadherin-Fc), which consistof the whole extracellular domain of CAMs (human L1, chick L1,and chick N-cadherin, respectively) and the Fc region of humanIgG, were used in the present study. The pIg vector containingan insert of human L1-Fc was reported previously (Fransen et al.,1998). The pIg vector with an insert of N-cadherin-Fc was providedby Dr. Patrick Doherty (Guy's Hospital, London, UK) (Schnadelbachet al., 2000). Chick L1-Fc was constructed using chick L1 cDNA(a kind gift of Dr. Peter Sonderegger, University of Zurich, Zurich,Switzerland) (Buchstaller et al., 1996) and the pIg-tail expressionsystem (Novagen, Madison, WI). First, a cDNA encoding the extracellulardomain of chick L1 was obtained by PCR from the pUC19 that containsa cDNA encoding the full-length chick L1 in its HindIII site.Primers used for the PCR amplification were as follows: a senseprimer corresponding to nucleotides 2779-2796 of the chick L1cDNA, and an antisense primer 5'-GATGAAGAATTCACTTACCTGTCTTGGTGGCAAACCCCC-3'.The latter primer contains a cDNA fragment (nucleotides 3413-3429)encoding for the C-terminal end of the L1 extracellular domain,which is immediately followed by a splice donor sequence and anEcoRI restriction site. The PCR product was digested with SacI(located at nucleotide 2827) and EcoRI and ligated into a SacI-EcoRI-digestedpUC19 containing the full-length chick L1 cDNA. A HindIII-EcoRIfragment of the resulting plasmid, which contains a cDNA encodingthe L1 extracellular domain followed by a splice donor sequence,was then ligated into a HindIII-EcoRI-digested pIg vector. ThePCR-amplified region and the insert-vector junctions were confirmedbysequencing.

COS-7 cells were transfected with the pIg vectors using FuGENE6 transfection reagent according to the manufacturer's protocol(Roche, Indianapolis, IN). The culture media were conditionedfor 72 hr, and the CAM-Fc chimeras were purified from the culturesupernatant by a recombinant protein A-Sepharose column (AmershamPharmacia, Uppsala, Sweden). Integrity of the chimeric proteinswas ascertained by Western blotting using polyclonal antibodiesthat recognize the extracellular domain of human L1, chick L1,and chick N-cadherin. Purity of the preparation was checked bysilver staining. The preparations of human and chick L1-Fc yieldeda single band at ~200 kDa, and the preparation of N-cadherin-Fchad a major band at ~135 kDa and a minor degradation band at ~55kDa, as reported previously (Schnadelbach et al., 2000). Unlessnoted otherwise, a culture supernatant of the transfected COS-7cells was used as a neuronal culture substrate instead of affinity-purifiedCAM-Fc chimeras, because the supernatant contained 1-2 µg/ml ofCAM-Fc, a saturating concentration for neurite growth (see Fig.1).

For control experiments, the Fc fragment that is not fused to any CAM extracellular domain was also generated. COS-7 cellswere transfected with the pIg vector (R & D Systems, Minneapolis,MN) that contains cDNAs coding for the CD33 signal peptide followedby a factor Xa cleavage site and the Fc region of human IgG. Theconditioned medium was applied to a recombinant protein A-Sepharosecolumn followed by treatment with 2 U of factor Xa (Roche) for6 hr at room temperature. After washing out the cleaved fragmentthat contained the CD33 signal peptide, the Fc fragment remainingbound to the column waseluted.

Neuronal culture and electroporatic loading of IgG. Dorsal root ganglia (DRGs) were dissected from embryonic day 10 chicksor embryonic day 18 rats, and dissociated sequentially with 2.4U/ml dispase II (Roche) and 0.1 mg/ml DNase (Roche) in Ca²⁺/Mg²⁺-free PBS. The dissociated cells were resuspended in RPMI Medium1640 (Life Technologies) supplemented with 10% fetal bovine serum(FBS) and 20 ng/ml nerve growth factor (NGF), and then platedon a two-chamber glass slide (Lab-Tek, Naperville, IL) that hadbeen coated sequentially with poly-D-lysine (70-150 kDa; 0.1 mg/ml;Sigma), anti-Fc antibody (40 µg/ml), and CAM-Fc chimeras. To detectaxonal L1 by immunocytochemistry using species-specific anti-L1antibodies without cross-labeling L1 presented as a substrate,chick neurons were cultured on human L1-Fc, and rat neurons onchick L1-Fc. The cultures were maintained in a humid atmosphereof 95% air, 5% CO₂ at 37°C.

In the experiment designed to load IgG into neurons, the dissociated cells were resuspended in Leibovitz's L-15 medium andmixed with the IgG solution (either AP.6 or nonspecific mouseIgG). In some experiments, fluorescein isothiocyanate (FITC)-conjugateddextran (150 kDa; Sigma) was also added to the mixture to identifypositively loaded neurons during live cell imaging. One hundredand fifty microliters of the mixed solution, which contained 5× 10⁵ cells, 5 mg/ml IgG, and 1 mg/ml FITC-dextran were transferredto a cuvette (0.4 cm gap; Bio-Rad, Hercules, CA), incubated onice for 10 min, and then electroporated at 450 V/cm and 950 µF(Gene Pulser II and Capacitance Extender Plus; Bio-Rad). After10 min incubation on ice, the cells were washed three times withLeibovitz's L-15 medium. The cells were resuspended in RPMI Medium1640 supplemented with 10% FBS and 20 ng/ml NGF, and then platedon a two-chamber glassslide.

For live cell imaging, the dissociated neurons were resuspended in Leibovitz's L-15 medium containing N2 supplements (LifeTechnologies), 20 ng/ml NGF, and 750 µg/ml bovine serum albumin(BSA). The cells were then plated on a glass-based 35 mm dish(Iwaki, Chiba, Japan) that had been coated sequentially with poly-D-lysine,anti-Fc antibody, and CAM-Fc. The cultures were maintained ina humid atmosphere of 100% air at 37°C on a microscopestage.

Immunocytochemistry. In the experiment designed to double-label cell surface NCAM and internalized L1 (see Fig. 2), chickDRG neurons were incubated with the mouse anti-chick L1 antibody(8D9 hybridoma supernatant) at 37°C for 15 min to allow for endocytosisof the antibody bound to L1. After being rinsed three times withPBS at 4°C, the cells were fixed with 4% formaldehyde for 30 min,washed, and incubated with unconjugated anti-mouse IgG (100 µg/ml)to block the primary antibody remaining on the cell surface. Thecells were fixed again with 4% formaldehyde for 10 min to immobilizethe unconjugated secondary antibody. After being blocked with10% horse serum (HS) in PBS for 1 hr, cell surface NCAM was labeledwith the rabbit anti-chick NCAM antisera (1:500). The cells werepermeabilized and blocked with 0.1% Triton X-100 and 10% HS inPBS for 1 hr. Internalized L1 was visualized with Alexa 594-conjugatedanti-mouse IgG (10 µg/ml), and cell surface NCAM was visualizedwith Alexa 488-conjugated anti-rabbit IgG (10 µg/ml).

In the experiment designed to double label internalized L1 and electroporatically loaded IgG (see Fig. 5), rat DRG neuronswere incubated with the rabbit anti-rat L1 antisera (1:2000) at37°C for 15 min to allow for endocytosis of the antibody boundto L1. After being rinsed at 4°C, the cells were fixed with 4%formaldehyde for 30 min followed by incubation with unconjugatedanti-rabbit IgG (100 µg/ml). After 10 min refixation, the cellswere permeabilized and blocked with 0.1% Triton X-100 and 10%HS in PBS for 1 hr. Then, internalized L1 was visualized withAlexa 594-conjugated anti-rabbit IgG and electroporatically loadedIgG with Alexa 488-conjugated anti-mouseIgG.

In the experiments designed to double label cell surface L1 and electroporatically loaded IgG (see Fig. 7), rat DRG neuronswere fixed with 4% formaldehyde, washed, blocked, and incubatedwith the rabbit anti-rat L1 antisera (1:2000). After permeabilizationand blocking, L1 was visualized with Alexa 594-conjugated anti-rabbitIgG and electroporatically loaded IgG with Alexa 488-conjugatedanti-mouse IgG. The labeled cells were mounted with ProLong (MolecularProbes).

Confocal microscopy and image analyses. Images of nerve growth cones were taken with a Bio-Rad confocal imaging system (Radiance2000;Hempstead, UK) attached to a Nikon inverted microscope (TE300;Tokyo, Japan), using an argon/krypton laser (excitation lines,488 and 568 nm) and a 100× Plan Apochromat, numerical aperture1.4, oil objective. Pinhole settings were chosen to give singleoptical sections of 0.6 µm inthickness.

Growth cones were randomly selected on the basis of NCAM staining or electroporatically loaded IgG visualized by Alexa 488-conjugatedanti-mouse IgG. Then, a single-section confocal slice of the growthcone was obtained such that the section contained the maximalnumber of L1-positive endocytic compartments in that growth cone.The number of L1-positive compartments was counted by an observerwho was unaware of the treatment conditions (blind). The sizeof a growth cone was also measured by a blind observer, usingLaser Pix version 4.0 (Bio-Rad).

Neurite growth assay. Images of DRG neurons taken with a cooled digital CCD camera (ORCA; Hamamatsu Photonics, Hamamatsu,Japan) were analyzed using Aquacosmos version 1.3 (Hamamatsu Photonics).Neurite length was measured as the distance between the tip ofthe longest neurite and the periphery of the cell soma where theneurite emerges. Only the neurites that met the requirements describedpreviously (Lemmon et al., 1989) were included in this study.Neurite growth rates (micrometers per hour) were assayed withtime-lapse imaging of living growth cones. Growth cones includedin this analysis were limited to single growth cones that grewunobstructed and without retraction during the time-lapseimaging.

Bead preparation. Protein A-conjugated beads were prepared as described by Thompson et al. (1996). A 1% (w/v) aqueous suspensionof silica beads (800 nm in diameter) with aminopropyl functionalgroups (Micromod, Rostock, Germany) was mixed with an equal volumeof 8% glutaraldehyde (Grade I; Sigma) and incubated for 6 hr atroom temperature. The beads were pelleted (500 × g, 10 min) andresuspended three times at 1% (w/v) in 25 mM Na-phosphate buffer,pH 7.0. Recombinant protein A (Calbiochem, La Jolla, CA) was addedto the glutaraldehyde-activated bead suspension at 400 µg/ml proteinin 25 mM Na-phosphate buffer, pH 7.0, and mixed gently for 4 hrat room temperature. The protein A-conjugated beads were washedthree times in 50 mM Tris buffer, pH 8.0, and 7.5 mg/ml BSA wasadded to block any residual cross-linking sites. The beads werethen incubated with either 10 µg/ml of CAM-Fc chimeras or 1 mg/mlof rabbit antibodies for at least 30 min at 4°C. The beads incubatedwith either Fc fragments or nonspecific rabbit IgG were used incontrol experiments. After being washed, a 1% (w/v) suspensionof the coated beads was diluted 2000-fold when added to neuronalcultures for laser trappingstudies.

Laser tweezers. The optical trap system consisted of the Laser Tweezers 980/1000 module (1 W diode laser at 985 ± 10 nm; CellRobotics, Albuquerque, NM) and a CCD camera (C5985; HamamatsuPhotonics) attached to a Nikon inverted microscope (TE300), usinga 100× Plan Fluor, numerical aperture 1.3, oil objective. Movementof the microscope stage and focus drive was controlled by MicroscopeWorkstation System version 4.0 (Cell Robotics). Under video-enhancedcontrast/differential interference contrast (VEC-DIC) image observation,a silica bead was trapped with the laser in the culture medium,manipulated to the growth cone surface, held there for 3-4 sec,and then released. The bead behavior after release from the tweezerswas analyzed as described in Results. The laser power used inthis study exerted a maximal force of ~2.5 pN on the bead fordisplacements in the xy-direction, as calculated from Stokes'Law.

Statistics. Data were expressed as the mean ± SEM. Statistical analyses were performed using GraphPad Prism version 3.0a (GraphPadSoftware, San Diego, CA). Unless noted otherwise, a comparisonbetween two groups was performed by an unpaired t test, and acomparison among three or more groups by one-way ANOVA followedby Tukey's post-test. p values <0.05 were judged significantlydifferent.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

L1-based neurite growth is accompanied by increased L1 endocytosis in the growth cone

L1 presented as a substrate promotes neurite growth by binding homophilically to L1 expressed on the growth cone (Grumet andEdelman, 1988; Lemmon et al., 1989). If the growth cone activelyrecycles axonal L1 to migrate on an L1 substrate, the activityof L1 recycling should have a positive correlation with the rateof L1-dependent neurite growth. This possibility can be testedby quantifying L1 endocytosis in growth cones that migrate atdifferent rates either dependently or independently of L1. Wedecided to use N-cadherin as a control substrate for the followingreasons. (1) N-cadherin stimulates neurite growth via a homophilicbinding mechanism that is independent of L1 (Matsunaga et al.,1988; Bixby and Zhang, 1990). (2) Neurites grow at comparablerates on N-cadherin and L1 substrates (Lemmon et al., 1992). (3)Growth cone morphology (shape and cytoskeletal organization) onan N-cadherin substrate resembles that on an L1 substrate (Payneet al., 1992; Burden-Gulley and Lemmon, 1996). Therefore, usingvarious concentrations of the CAM-Fc chimeric proteins (eitherL1-Fc or N-cadherin-Fc) as substrates, the dose-response relationshipwas obtained between the CAM-Fc density and neurite length (Fig.1). For both L1 and N-cadherin substrates, neurite growth fromchick DRG neurons was promoted significantly when culture slideswere coated with CAM-Fc at a concentration as low as 150 ng/ml.This neurite-growth-promoting activity was saturated at ~600 ng/mlof L1-Fc or N-cadherin Fc. On the basis of this result, we decidedto quantify the amount of endocytosed L1 in growth cones thatmigrate on culture substrates prepared with either 150 or 600ng/ml of CAM-Fc.

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Figure 1. The dose-response relationship between the substrate density and neurite growth from chick DRG neurons. The neurons were plated on culture slides that had been coated sequentially with poly-D-lysine, anti-Fc antibody, and increasing concentrations of either L1-Fc (A) or N-cadherin-Fc (B). Fourteen hours after plating, the length of neurites was measured (n = 50-54 for each data set). ***p < 0.001; compared with 0 ng/ml of the Fc chimeras.

A traditional method for studying the endocytic movement of membrane proteins is to label them with specific antibodies atthe cell surface (Teter et al., 1998; Cao et al., 1999). Thisexperimental paradigm has also been shown to specifically visualizeL1 in endocytic compartments (Kamiguchi et al., 1998b; Kamiguchiand Lemmon, 2000b). Living chick DRG neurons were incubated withmonoclonal anti-L1 antibody at 37°C for 15 min to allow for endocytosisof the antibody bound to L1. After blocking the primary antibodyremaining on the cell surface with an unconjugated secondary antibody,internalized L1 was visualized by incubating the permeabilizedcells with Alexa 598-conjugated secondary antibody. Representativeimages of growth cones migrating on an L1 substrate (150 or 600ng/ml of L1-Fc) are shown (Fig. 2A-D). As demonstrated previously(Kamiguchi and Lemmon, 2000b), endocytosed L1 at this time point(15 min incubation with anti-L1 antibody) was confined to theC-domain in the majority of growth cones examined. A similar distributionpattern of endocytosed L1 was observed in growth cones migratingon an N-cadherin substrate (150 or 600 ng/ml of N-cadherin-Fc;data not shown). To quantify the amount of endocytosed L1, thenumber of endocytic compartments (most likely endosomes) labeledby the anti-L1 antibody was counted by a blind observer. As shownin Figure 2E, the growth cone migrating on a high-density substrateof L1-Fc contained a greater number of L1-positive endocytic compartmentsthan the growth cone on a low-density substrate of L1-Fc. Thesize of a growth cone was 461.6 ± 29.6 µm² (n = 139) or 462.7 ± 23.5 µm² (n = 121) on substrates prepared with 150 or 600 ng/ml of L1-Fc,respectively, indicating that the observed difference in L1 endocytosisis not attributable to a change in the growth cone size. In contrastto L1 substrates, the number of L1-positive endocytic compartmentswas not affected by a density of N-cadherin-Fc substrates on whichthe growth cone migrates. The size of a growth cone was 281.8± 20.3 µm² (n = 121) or 271.7 ± 18.5 µm² (n = 124) on substrates prepared with 150 or 600 ng/ml of N-cadherin-Fc,respectively. Although 600 ng/ml of L1-Fc or N-cadherin-Fc stimulatedneurite growth to a similar extent (Fig. 1), the number of L1-positiveendocytic compartments in growth cones migrating on L1-Fc wassignificantly greater than that on N-cadherin-Fc (Fig. 2E). Thiswas also true if the number of L1-positive endocytic compartmentswas normalized by the mean size of a growth cone: 9.8 ± 0.9/100µm² (n = 121; 600 ng/ml of L1-Fc) versus 3.7 ± 1.0/100 µm² (n = 124; 600 ng/ml of N-cadherin-Fc), which showed a statisticaldifference at the p < 0.001 level. These results indicate thatL1-dependent neurite growth is accompanied by increased L1 endocytosisin the growth cone.

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Figure 2. A-D, L1 endocytosis in the growth cone migrating on different densities of L1-Fc. Chick DRG neurons were plated on culture slides that had been coated with either 150 ng/ml (A, B) or 600 ng/ml (C, D) of L1-Fc. The cells were then incubated with monoclonal anti-L1 antibody for 15 min to allow for internalization of the antibody bound to L1. The cells were double labeled for NCAM to outline the growth cone structure. In superimposed images (A, C), endocytosed L1 is colored red, and NCAM is colored green. To facilitate visualization of endocytosed L1, only the red channel is shown in black and white (B, D). Scale bars: A, B, 10 µm; C, D, 10 µm. E, The number of L1-positive endocytic vesicles in the growth cone on different substrates. Intracellular vesicles containing endocytosed L1 were visualized as described above, and the number of vesicles per growth cone was counted. Distribution was plotted as percentage of the growth cones that contained a greater number of the vesicles than a given value on the x-axis. In the growth cones that were not labeled for endocytosed L1, the number of the vesicles was regarded as zero. The number of growth cones included in this study was 139 (150 ng/ml L1-Fc), 121 (600 ng/ml L1-Fc), 121 (150 ng/ml N-cadherin-Fc), and 124 (600 ng/ml N-cadherin-Fc). The difference between 150 and 600 ng/ml of L1-Fc was statistically significant (p < 0.001).

L1-based neurite growth is accompanied by increased polarity of L1 adhesion on the growth cone

As demonstrated previously, L1 is endocytosed preferentially at the C-domain followed by centrifugal transport into the P-domainand reinsertion into the plasma membrane of the leading edge.Therefore, the endocytic L1 trafficking is expected to createpolarized L1 density and adhesion on the growth cone (strong adhesionat the leading edge and weak adhesion at the C-domain). Theoretically,such polarized adhesion on the substrate-facing plasma membranebut not on the apical membrane should be required for growth conemigration. However, it is very difficult to assess CAM densityor adhesiveness on the substrate-facing surface for technicalreasons. Therefore, many investigators analyze CAM behavior byligating CAMs on the apical surface (Suter et al., 1998; Nishizakaet al., 2000), which is believed to mimic CAM ligation by culturesubstrates (Galbraith and Sheetz, 1999). As described previously(Kamiguchi and Lemmon, 2000b), immunocytochemistry of traffickingL1 used in the present study preferentially labels L1 that isbeing recycled to and from the apical plasma membrane but notthe substrate-facing membrane of growth cones. This is most likelycaused by the limited accessibility of antibodies to the substrate-facingsurface. This observation, taken together with the result shownin Figure 2, suggests that L1 presented as a substrate is ableto upregulate L1 endocytosis from the apical plasma membrane leadingto an increased polarity of L1 density and adhesion on the apicalsurface. Results consistent with this hypothesis have been publishedby Stoeckli et al. (1996), who studied the distribution patternof chick L1 (Ng-CAM) on the apical growth cone surface by conventional,confocal, and electron microscopy. In their report, homogeneousL1 distribution was observed on a laminin substrate, whereas L1distribution was highly polarized on an L1 substrate (L1 was concentratedon the filopodia and the lamellipodial leading edge but was removedfrom the C-domain). Therefore, we decided to test whether an L1substrate is able to influence L1 density and adhesion on theapical plasma membrane via the regulation of endocytic L1trafficking.

First, L1 distribution on chick DRG growth cones migrating on either L1 or N-cadherin substrate was examined immunocytochemically,using a mixture of formaldehyde and glutaraldehyde for fixation.On both substrates, the P-domain expressed higher density of L1than the C-domain in the majority of growth cones examined. However,the growth cone on an L1 substrate tended to show more polarizedL1 distribution than that on an N-cadherin substrate (data notshown). Although this observation was consistent with the findingthat L1 endocytosis increases when the growth cone migrates onan L1 substrate, there were several problems in quantifying L1distribution by this approach. (1) The L1 distribution patternwas highly sensitive to immunocytochemical protocols. Live celllabeling with the primary antibody or formaldehyde fixation followedby incubation with the primary antibody yielded a more punctatepattern of L1 distribution with much less polarity than fixationwith a mixture of formaldehyde and glutaraldehyde (data not shown).(2) A variation in the thickness of growth cones (especially inthe C-domain) might have caused some areas of the apical plasmamembrane to be situated out of the focal plane of a microscope,thereby affecting the spatial distribution of fluorescent signalintensities. (3) The L1 staining pattern might have been affectedby different antibody accessibility to the substrate-facing plasmamembrane depending on the culture substrate used. Therefore, wedecided to use another experimental approach to assess the distributionof L1 and L1-mediated adhesion on the growthcone.

CAM-mediated adhesion has been studied by manipulating ligand-coated beads on the cell surface using laser optical tweezers(Thompson et al., 1996; Nishizaka et al., 2000). To analyze L1adhesion on the leading edge versus the C-domain of growth cones,an L1-Fc-coated bead was held in position against the apical plasmamembrane with the laser trap for 3-4 sec and then released. Accordingto previous reports (Thompson et al., 1996; Nishizaka et al.,2000), the bead behavior after release was categorized as eitheradherent or nonadherent. The nonadherent beads were defined asthose that either diffused away from the growth cone or couldbe pulled off the plasma membrane with the laser trap. The adherentbeads were further categorized as (1) those that showed retrogradedirectional movement and/or little visible diffusion and couldnot be dragged after being retrapped with the tweezers (Fig. 3A-C)(designated as cytoskeletal association) or (2) those that showedtwo-dimensional Brownian motion and could be dragged within theplane of the plasma membrane (Fig. 3D-G;) (designated as Brownianmotion). The velocity of the retrograde movement of an L1-Fc-coatedbead was 4.1 ± 0.4 µm/min (n = 8; on the growth cone on an L1substrate) and 4.0 ± 0.3 µm/min (n = 7; on an N-cadherin substrate),which corresponds to the velocity of the retrograde flow of actinfilaments (Forscher and Smith, 1988). A similar result was obtainedwith a bead coated with anti-L1 antibody: 3.8 ± 0.3 µm/min (n= 9; on an L1-substrate) and 4.0 ± 0.3 µm/min (n = 8; on an N-cadherinsubstrate). We did not observe L1-coupled beads being internalizedat the C-domain of growth cones; perhaps an 800 nm bead is toobig to be internalized via clathrin-coated pits.

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Figure 3. A-C, VEC-DIC micrographs showing retrograde directional movement of an L1-Fc-coated bead on a chick DRG growth cone. A, A bead was placed on the leading edge with laser tweezers (0 sec). B, Time sequence of the bead movement in the area of interest indicated in A (0-90 sec). C, The bead had moved into the C-domain at 90 sec after placement on the leading edge. D-G, Brownian motion of an L1-Fc-coated bead on a chick DRG growth cone. D, A bead was placed on the leading edge with laser tweezers (0 sec). E, A magnified view of the area of interest indicated in D. The line sketch indicates the path of the bead tracked for a total of 27 sec at 3 sec intervals. F, The bead was still beside the leading edge at 3 min after placement. G, The bead could be dragged within the plane of the plasma membrane after being retrapped with the tweezers but could not be pulled off the membrane. Scale bars: A, C, 10 µm; D, F, G, 10 µm.

On growth cones migrating on an L1-substrate, the majority of L1-Fc-coated beads adhered to the leading edge showing eithercytoskeletal association or Brownian motion, whereas <50% of thebeads attached to the plasma membrane of the C-domain (Fig. 4A).As a control, the majority of beads coated with the Fc fragmentalone did not attach to either the leading edge or the C-domain.On growth cones migrating on an N-cadherin substrate, the differencein the behavior of L1-Fc-coated beads between the leading edgeand the C-domain is not as significant as that on an L1 substrate.Furthermore, the bead binding behavior at the leading edge ofgrowth cones on an L1-substrate is statistically different fromthat on an N-cadherin substrate (p < 0.05). Because the growthcone also expresses heterophilic binding partners for L1, suchas integrins (Ruppert et al., 1995; Felding-Habermann et al.,1997), the observed attachment of L1-Fc-coated beads in theseexperiments is not attributable exclusively to L1-L1 homophilicadhesion. L1 on the cell surface can be assessed more specificallywith antibody-coated beads than with L1-Fc-coated beads (Winckleret al., 1999). Therefore, we have repeated the laser tweezersexperiments using beads coated with anti-chick L1 antibody andhave obtained similar results (Fig. 4B). On the basis of theseobservations, we concluded that the growth cone migrating viaan L1-dependent mechanism has the increased polarity of L1 densityand adhesion compared with the growth cone on an N-cadherin substrate.

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Figure 4. Histograms of the bead-binding behavior at different regions of chick DRG growth cones migrating on either L1-Fc or N-cadherin-Fc substrate. A, An L1-Fc-coated bead was held in position against the plasma membrane of either the leading edge (defined as the region within 0.5 µm of the lamellipodial edge) or the C-domain for 3-4 sec and then released. The bead behavior was categorized as cytoskeletal association, Brownian motion, or no membrane attachment. Data from three independent experiments were pooled, and probability of the binding behavior of a total of 100 beads is shown. As a control, a bead coated with the Fc fragment alone was tested for its binding to the growth cone. B, Shown is probability of the binding behavior of a total of 100 beads coated with anti-L1 antibody (pooled from three independent experiments). As a control, a bead coated with nonspecific rabbit IgG was tested for its binding to the growth cone. The p values between two groups were calculated from a Mann-Whitney U test, with a Kruskal-Wallis test (nonparametric ANOVA) confirming that there was a significant difference at the p = 0.0001 level.

Endocytic L1 trafficking is required for polarized L1 adhesion on the growth cone

To test whether the polarity of L1 adhesion on the growth cone migrating on an L1-substrate is created and maintained by endocyticL1 trafficking, we have developed a neuronal culture in whichthe L1 trafficking in the growth cone is disrupted. It has beendemonstrated previously that L1 internalization occurs via itsinteraction with AP-2 (Kamiguchi et al., 1998b), a clathrin adaptorthat captures plasma membrane proteins for endocytosis by coatedpits (Kirchhausen et al., 1997). The AP-2 adaptor consists offour subunits ( $alpha$ -adaptin, $beta$ 1/ $beta$ 2-adaptin, µ2 chain, and $sigma$ 2 chain).The mouse monoclonal antibody AP.6 that recognizes $alpha$ -adaptin hasbeen shown to block AP-2 function and inhibit endocytic traffickingat least at two steps: receptor-mediated endocytosis from theplasma membrane (Chin et al., 1989) and AP-2-dependent vesicleaggregation in vitro, which is thought to represent an initialstep in the formation of endosomes in vivo (Beck et al., 1992).The purified AP.6 antibody recognized a single band at ~110 kDa(corresponding to $alpha$ -adaptin) by Western blotting of rat brainmembrane extracts but not chick extracts (data not shown). Byimmunocytochemistry, the AP.6 antibody labeled vesicular structuresin rat DRG growth cones but not in chick cells (data not shown).The labeled structures were situated throughout the growth coneexcluding the filopodia. On the basis of these results, we decidedto apply this antibody to rat DRG neurons to inhibit endocyticL1trafficking.

Either the AP.6 antibody or nonspecific mouse IgG was loaded into rat DRG neurons by electroporation, with a loading efficiencyof ~50%. Shown in Figure 5A-D are representative images of thegrowth cones on an L1-substrate that were double labeled for theloaded IgG and endocytosed L1. The distribution of AP.6 in thegrowth cone appeared punctate, whereas control IgG distributedrelatively homogeneously, consistent with the AP.6 antibody associatingwith AP-2-positive vesicular structures. To quantify L1 endocytosis,the number of endocytic compartments labeled by anti-L1 antibodywas counted. As shown in Figure 5E, the growth cones loaded withAP.6 contained a smaller number of L1-positive endocytic compartmentsthan the control growth cones. The size of a growth cone was 237.5± 20.0 µm² (n = 95; control IgG loaded) or 232.0 ± 21.4 µm² (n = 85; AP.6 loaded), indicating that the observed differencein L1 endocytosis is not attributable to a change in the growthcone size. These results indicate that AP.6 inhibits endocyticL1 trafficking in the growth cone. To examine a possible effectof AP.6 on N-cadherin trafficking, we tested whether N-cadherinis endocytosed in rat DRG growth cones by immunocytochemistryusing a rabbit polyclonal antibody against the ectodomain of N-cadherin(Santa Cruz Biotechnology, Santa Cruz, CA). However, we couldnot detect the antibody internalized in the growth cone aftereither 15 or 30 min of incubation, whereas the antibody did labelcell-surface N-cadherin (data not shown). In contrast, internalizedL1 was visualized in parallel experiments. This suggests thatno or only a small amount of N-cadherin is endocytosed in thegrowth cone.

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Figure 5. The effect of the anti- $alpha$ -adaptin antibody (AP.6) on L1 endocytosis in the growth cone. A-D, Rat DRG neurons that had been loaded with either control mouse IgG (A, B) or AP.6 (C, D) by electroporation were plated on an L1-Fc substrate. Endocytosed L1 was visualized by incubating the cells with rabbit anti-L1 antibody for 15 min to allow for internalization of the antibody bound to L1. The cells were double labeled for electroporatically loaded IgG with Alexa 488-conjugated anti-mouse IgG. In superimposed images (A, C), endocytosed L1 is colored red, and loaded IgG is colored green. To facilitate visualization of endocytosed L1, only the red channel is shown in black and white (B, D). Scale bars: A, B, 10 µm; C, D, 10 µm. E, Intracellular vesicles containing endocytosed L1 were visualized as described above, and the number of vesicles per growth cone was counted. Distribution was plotted as percentage of the growth cones that contained a greater number of the vesicles than a given value on the x-axis. The number of growth cones included in this study was 95 (control IgG loaded) and 85 (anti- $alpha$ -adaptin loaded). The difference between the two groups was statistically significant (p < 0.001).

We next tested whether polarized L1 adhesion on the growth cone is altered after inhibiting L1 endocytosis. Rat DRG neuronswere loaded with either control mouse IgG or AP.6 together withFITC-conjugated dextran (150 kDa) and then plated on an L1-Fcsubstrate. Positively loaded neurons were identified by FITC fluorescence.Using laser tweezers, the binding probability of an L1-Fc-coatedbead on the growth cone (leading edge vs C-domain) was examined(Fig. 6). On the control growth cone, the majority of L1-Fc-coatedbeads adhered to the leading edge showing either cytoskeletalassociation or Brownian motion, whereas 60% of the beads did notattach to the plasma membrane of the C-domain. This polarity ofthe bead binding probability between the leading edge and theC-domain was significantly attenuated by AP.6 loading, indicatingthat endocytic L1 trafficking is required for polarized L1 adhesionon the growth cone.

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Figure 6. Histograms of the bead-binding behavior on rat DRG growth cones loaded with either control mouse IgG or the anti- $alpha$ -adaptin antibody (AP.6). An L1-Fc-coated bead was held in position against the plasma membrane of either the leading edge (defined as the region within 0.5 µm of the lamellipodial edge) or the C-domain for 3-4 sec and then released. The bead behavior was categorized as cytoskeletal association, Brownian motion, or no membrane attachment. Data from three independent experiments were pooled, and probability of the binding behavior of a total of 50-54 beads is shown. The p values between two groups were calculated from a Mann-Whitney U test, with a Kruskal-Wallis test (nonparametric ANOVA) confirming that there was a significant difference at the p = 0.0001 level.

Endocytic L1 trafficking is required for L1-based neurite growth

Given that the polarized adhesion between the growth cone and its substrate is required for migration of the growth cone,endocytic L1 trafficking should play an important role in neuritegrowth on an L1 substrate. To test this possibility, rat DRG neuronsthat had been loaded with either AP.6 or nonspecific mouse IgGwere plated on several substrates, including L1-Fc. As shown inFigure 7A-D, positively loaded neurons were identified by immunocytochemistrywith anti-mouse IgG, and the length of their neurites was measured.On an L1-Fc substrate, neurons loaded with AP.6 had significantlyshorter neurites than neurons loaded with control IgG (Fig. 7E).Considering that the control substrate (no Fc chimera) stimulatedneurite growth to some extent, AP.6 loading caused a ~50% reductionin L1-dependent neurite growth. In contrast, AP.6 loading hadno effect on N-cadherin-dependent neurite growth, which is consistentwith the result that the growth cone does not actively internalizeN-cadherin. We also measured the percentage of rat DRG neuronsbearing neurites on an L1-Fc substrate: 76.0 ± 1.8% of controlIgG-loaded neurons and 75.0 ± 3.5% of AP.6-loaded neurons boreneurites at 6 hr after plating (four independent determinations).Therefore, AP.6 loading should have decreased the length of neuriteson an L1-Fc substrate by inhibiting growth cone migration butnot by delaying neurite initiation. This possibility was furtherconfirmed by measuring the rate of growth cone migration. To identifyliving neurons loaded with mouse IgG, FITC-conjugated dextran(150 kDa) was loaded concomitantly. The AP.6-loaded growth conesmigrated at a rate of 9.7 ± 1.6 µm/hr (n = 16) on an L1-Fc substrate,whereas the growth cones loaded with control mouse IgG migratedat 20.1 ± 2.4 µm/hr (n = 13) on an L1-Fc substrate. There wasa statistical difference at the p < 0.001 level. On the basisof these results, we concluded that endocytic L1 trafficking isrequired for L1-dependent migration of the growth cone.

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Figure 7. The effect of the anti- $alpha$ -adaptin antibody (AP.6) on L1-based neurite growth. A-D, Rat DRG neurons that had been loaded with either control mouse IgG (A, B) or AP.6 (C, D) by electroporation were plated on an L1-Fc substrate. Loaded IgG was labeled by immunocytochemistry with anti-mouse IgG (B, D). To visualize the whole population of neurons in culture, the cells were double labeled for a neuronal marker, L1, with rabbit anti-rat L1 antibody (A, C). Scale bars: A, B, 50 µm; C, D, 50 µm. E, Rat DRG neurons that had been loaded with either control mouse IgG or AP.6 were cultured on the following substrates: L1-Fc, N-cadherin-Fc, and the control substrate (poly-D-lysine and anti-Fc antibody but no Fc chimera). Shown is the length of neurites measured at 12 hr after plating (n = 97-112 for each bar). ***p < 0.001; compared with control IgG-loaded neurons on L1-Fc.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

CAMs mediate not only static cell-cell adhesion but also dynamic biological processes, such as cell migration and synapticremodeling, that require temporally and spatially regulated celladhesion. Therefore, a cell must be able to modulate CAM-mediatedadhesion in response to external stimuli or in a cell-autonomousmanner. Such regulation of IgCAM adhesion can be achieved viafour distinct mechanisms: lateral oligomerization of CAMs, CAMtrafficking, proteolytic cleavage of the CAM ectodomain, and transcriptionalregulation of CAM expression (Kamiguchi and Lemmon, 2000a). Althoughthe three post-translational regulatory mechanisms should be ableto modulate IgCAM adhesion rapidly in the growth cone, there hasbeen no experimental evidence that these mechanisms are involvedin the spatial regulation of growth cone adhesion or the promotionof neurite growth. The present study demonstrates that the growthcone migrating via an L1-dependent mechanism actively internalizesL1 at the C-domain and potentiates a gradient of L1 adhesion,and that endocytic L1 trafficking is required for the polarizedadhesion and migration of the growth cone mediated by L1. Theseresults establish a mechanism by which growth cone adhesion isspatially regulated in a manner important for growth conemigration.

How does CAM trafficking control its adhesiveness? One obvious explanation is that CAM density is spatially regulated by preferentialinternalization at some region of a cell followed by recyclinginto a different region. This should be the case with L1 traffickingbecause beads coated with anti-L1 antibody preferentially boundto the leading edge rather than the C-domain, whereas the assaywith L1-Fc-coated beads could be detecting changes in the adhesivestate of L1 itself. Another possibility is that rapid endocytosisof CAMs decreases cell adhesion by shortening the dwell time ofthe CAMs on the cell surface. Early modeling studies suggestedthat, after homophilic trans-binding of CAMs, individual pairsof bound CAMs rapidly cycle between the bound and unbound states(Bell, 1978). Rapid internalization would cause CAMs to be quicklyremoved from the cell surface after trans-binding of the CAMs.Slow internalization would cause CAMs to remain on the cell surfacefor a long period so that they could be engaged in trans-bindingmultiple times before being removed from the cell surface. Thispossibility has been supported by recent observation that homophilicL1 adhesion is regulated by L1 endocytosis rates without affectingthe amount of L1 expression on the cell surface (Long et al.,2001). They were able to double L1-mediated cell aggregation ratesafter inhibiting L1 endocytosis, either by altering the L1 cytoplasmicdomain (L1CD) or by blocking the clathrin endocytic pathway. Therefore,it is likely that endocytic L1 trafficking creates a gradientof growth cone adhesion by regulating both L1 density and thedwell time of L1 on the cellsurface.

So far, three major classes of CAMs have been identified in the nervous system: integrins, cadherins, and IgCAMs. Althoughmany CAMs in the three classes mediate cell migration, integrinsare the best-studied family using several non-neuronal cells.These studies have introduced a model of cell migration (Sheetzet al., 1998; Palecek et al., 1999) that can be applied to migrationof the nerve growth cone (Suter and Forscher, 2000): (1) assemblyof actin filaments at the cell front generates protrusion of theleading edge; (2) the newly formed leading edge adheres to thesubstrate via CAMs; (3) linkage of CAMs to the retrograde actinflow generates a traction force that pulls the cell body or thegrowth cone forward; (4) the cell rear detaches from the substratefollowed by tail retraction, although this tail retraction stepis modified in the growth cone by the presence of the neuriteshaft; and (5) CAMs are recycled to the cell front. In this model,CAMs can be viewed as the "feet" needed to crawl on a relevantsubstrate, using the underlying actin cytoskeleton as a force-generatingsystem. CAMs bind the cytoskeleton preferentially at the leadingfront, move rearward as the cell migrates forward, and are releasedfrom the cytoskeleton at the ectoplasm-endoplasm boundary in fibroblasts(Nishizaka et al., 2000), which corresponds to the boundary betweenthe P- and C-domains in growth cones. As reported previously (Faivre-Sarrailhet al., 1999), Ng-CAM-related cell adhesion molecule, anothermember of the L1 family, displays actin-dependent retrograde movementon the growth cone. Our study also demonstrated that L1 movesbackward on the growth cone at ~4 µm/min, corresponding to thevelocity of the retrograde actin flow. These results stronglysuggest that the L1 family CAMs associate with retrogradely movingactin filaments in the P-domain, thereby transmitting a tractionforce that pulls the growth cone forward on an L1 substrate. Becauseit is not economical for the growth cone to use the feet (CAMs)for only a single forward step, a mechanism would be requiredto bring them up to the leading front for reuse. Such CAM recyclingcan occur either by cell surface transport or by intracellularvesicular transport, as has been demonstrated in non-neuronalcells (Bretscher, 1992; Schmidt et al., 1993; Lawson and Maxfield,1995). The present paper, together with our previous results (Kamiguchiand Lemmon, 2000b), clearly demonstrate that L1 recycling viaintracellular vesicular transport plays a significant role ingrowth cone migration, although involvement of cell surface transportis also possible. The fact that we failed to detect N-cadherinendocytosis in the growth cone suggests that N-cadherin recyclingoccurs predominantly via a cell surface pathway. This is in strongcontrast to the observation that adherens junctions are dynamicallyregulated by endocytosis and recycling of E-cadherin in epithelialcells (Le et al., 1999; Akhtar and Hotchin, 2001). Perhaps eachCAM has a different preference for its trafficking pathway, whichalso depends on the celltype.

Although we observed the behavior of L1 present on the apical surface of growth cones in this paper, it is widely acceptedthat the CAM behavior triggered by ligand binding on the apicalsurface reflects the CAM behavior on the substrate-facing surfacethat actually participates in cell migration (Galbraith and Sheetz,1999; Suter and Forscher, 2000). Zheng et al. (1994) have measuredgrowth cone adhesion to culture substrates by dislodging the growthcone with calibrated glass needles. They revealed that the distalends of filopodia and lamellipodia adhered most firmly to thesubstrates including L1, which is consistent with our result onL1 adhesion assessed on the apical surface. Another techniquesuited for examining growth cone-substrate interactions is interferencereflection microscopy (IRM). IRM reveals the spatial separationbetween the growth cone and its substrate, although it may notprovide a reliable estimation of adhesive strength between thegrowth cone and its substrate (Zheng et al., 1994). It was foundthat, in growth cones migrating on an L1 substrate, dark grayspots indicative of close apposition appeared near the leadingedge and moved toward the C-domain at a mean rate of 5.8 µm/min(Drazba et al., 1997). This suggests that these small areas ofclose apposition of the growth cone membrane to the L1 substratemove in association with the retrograde actin flow. An intriguingspeculation is that this type of membrane flow on the substrate-facingsurface observed by IRM is functionally related to retrogradeL1 movement on the apical surface observed in the presentstudy.

In addition to the initial idea that CAMs regulate neurite growth on the basis of their ability to mediate adhesive interactions,it has become evident that CAM-associated intracellular signalsare also critical. For example, cross-linking of L1 on the cellsurface activates the mitogen-activated protein kinase pathway(Schaefer et al., 1999), which is required for neurite growthon an L1 substrate (Wong et al., 1996; Schmid et al., 2000). Othersignals implicated in L1-based neurite growth include calciumsignaling (Williams et al., 1992), the fibroblast growth factorreceptor (Saffell et al., 1997), and the non-receptor tyrosinekinase pp60^c-src (Ignelzi et al., 1994). These signaling events are likely toregulate neurite growth by modulating the pathway and the rateof L1 trafficking in the growth cone. For example, the kinaseactivity of pp60^c-src is required for L1 endocytosis (Schmid et al., 2000). It hasalso been found that L1 endocytosis may be triggered by tyrosinedephosphorylation in the L1CD (A. W. Schaefer, S. Storms, H. Kamiguchi,M. Pendergast, I. Rapoport, G. Landreth, T. Kirchhausen, and V.Lemmon, unpublished observations). Furthermore, interactions ofthe L1 family CAMs with the actin cytoskeleton via ankyrin isdependent on the phosphorylation state of another tyrosine inthe L1CD (Garver et al., 1997; Hortsch et al., 1998). These resultssuggest that the pathway of L1 trafficking is controlled by L1-associatedkinases and phosphatases. Furthermore, L1-induced localized calciuminflux in the growth cone (Archer et al., 1999) may acceleratevesicle endocytosis/exocytosis (Geppert and Südhof, 1998; Sankaranarayananand Ryan, 2001) and influence actin dynamics (Welnhofer et al.,1999), thereby regulating the rate of L1 trafficking. Future studiesshould be directed to elucidate how dynamic interactions betweenCAMs and the trafficking machinery are spatially regulated byCAM-associated signals in a way important for growth conemigration.

  FOOTNOTES

Received June 26, 2001; revised Aug. 21, 2001; accepted Sept. 5, 2001.

This study was partially supported by a grant-in-aid for Scientific Research of the Japan Society for the Promotion of Science(13680857) and grants from the Japan Intractable Diseases ResearchFoundation and the School of Medicine of Keio University (MedicalSchool Faculty and Alumni Grants) to H.K. We are grateful to Drs.Patrick Doherty, Vance Lemmon, and Peter Sonderegger who providedantibodies and DNA constructs. We also thank Dr. Vance Lemmonfor helpful comments on thismanuscript.
Correspondence should be addressed to Hiroyuki Kamiguchi, Developmental Brain Science Group, RIKEN Brain Science Institute,2-1 Hirosawa, Wako, Saitama 351-0198, Japan. E-mail: kamiguchi{at}brain.riken.go.jp.

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ABSTRACT
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MATERIALS AND METHODS
RESULTS
DISCUSSION
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