Dual Regulation of Actin Rearrangement through Lysophosphatidic Acid Receptor in Neuroblast Cell Lines: Actin Depolymerization by Ca2+-alpha -Actinin and Polymerization by Rho

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Originally published as MBC in Press, 10.1091/mbc.01-09-0465 on June 6, 2002

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Vol. 13, Issue 8, 2692-2705, August 2002

Dual Regulation of Actin Rearrangement through Lysophosphatidic Acid Receptor in Neuroblast Cell Lines: Actin Depolymerization by Ca²⁺- $alpha$ -Actinin and Polymerization by Rho

Nobuyuki Fukushima,^* Isao Ishii,^§ Yoshiaki Habara, Cara B. Allen,^¶ and Jerold Chun^¶^#^@

^*Department of Molecular Biochemistry, Hokkaido University Graduate School of Medicine, Sapporo 060-8638, Japan; Department of Pharmacology, ^¶Neurosciences Program, ^#Biomedical Sciences Program, School of Medicine, University of California, San Diego, La Jolla, California 92093-0636; ^@Molecular Neuroscience, Merck Research Laboratories, San Diego, California 91212; and Department of Biomedical Sciences, Hokkaido University Graduate School of Veterinary Medicine, Sapporo 060-0818, Japan

Submitted September 24, 2001; Revised April 11, 2002; Accepted April 22, 2002
Monitoring Editor: Howard Riezman

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Lysophosphatidic acid (LPA) is a potent lipid mediator with actions on many cell types. Morphological changes involving actinpolymerization are mediated by at least two cognate G protein-coupledreceptors, LPA₁/EDG-2 or LPA₂/EDG-4. Herein, we show that LPAcan also induce actin depolymerization preceding actin polymerizationwithin single TR mouse immortalized neuroblasts. Actin depolymerizationresulted in immediate loss of membrane ruffling, whereas actinpolymerization resulted in process retraction. Each pathway wasfound to be independent: depolymerization mediated by intracellularcalcium mobilization, and $alpha$ -actinin activity and polymerizationmediated by the activation of the small Rho GTPase. $alpha$ -Actinin-mediateddepolymerization seems to be involved in growth cone collapseof primary neurons, indicating a physiological significance ofLPA-induced actin depolymerization. Further evidence for dualregulation of actin rearrangement was found by heterologous retroviraltransduction of either lpa₁ or lpa₂ in B103 cells that neitherexpress LPA receptors nor respond to LPA, to confer both formsof LPA-induced actin rearrangements. These results suggest thatdiverging intracellular signals from a single type of LPA receptorcould regulate actin depolymerization, as well as polymerization,within a single cell. This dual actin rearrangement may play anovel, important role in regulation of the neuronal morphologyand motility during braindevelopment.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Lysophosphatidic acid (LPA), a simple yet potent bioactive phospholipid, has been shown to elicit diverse cellular responsesin many types of cells (Moolenaar, 1995; Moolenaar et al., 1997;Contos and Chun, 1998; Moolenaar, 1999). These responses are mediatedby specific cell-surface G protein-coupled receptors, which areencoded by three cognate genes: lpa₁/edg-2, lpa₂/edg-4, and lpa₃/edg-7(Hecht et al., 1996; An et al., 1998; Contos and Chun, 1998; Bandohet al., 1999; Chun, 1999; Chun et al., 1999; Fukushima et al.,2001). LPA₁ shares many downstream intracellular signaling pathwayswith LPA₂, including inhibition of adenylyl cyclase (AC) and activationof phospholipase C (PLC) and the small GTPase Rho (Fukushima etal., 1998, 2001; Ishii et al., 2000). In contrast, LPA₃ linksto the former two pathways: AC inhibition and PLC activation,but not Rho stimulation (Ishii et al., 2000).

One prominent cellular response evoked by LPA is rearrangement of the actin cytoskeleton. In fibroblasts, LPA induces actinpolymerization, resulting in the formation of cytoplasmic stressfibers that consist of filamentous actin (f-actin) and are associatedwith cell contraction (Ridley and Hall, 1992). In neuroblastomacells or primary neuroblasts, LPA induces actin polymerizationthat produces neurite retraction/cell rounding (Jalink et al.,1993; Fukushima et al., 1998, 2000). In both cell types, LPA inducesactin polymerization through the activation of Rho and its downstreamRho-associated kinase (Amano et al., 1997; Hirose et al., 1998).One difference between these cell types is the amount of f-actinthat is present under resting conditions. Unlike resting fibroblaststhat have little f-actin, resting neuronal cells have abundantf-actin throughout their cell bodies, in both cytoplasm and processes(Jalink et al., 1993; Fukushima et al., 1998, 2000). This raisesthe question of how LPA affects preexisting abundant f-actin duringthe remodeling of neuronal cell morphology. In addition, the intracellularactions of LPA through direct interactions with actin-bindingproteins have been demonstrated (Meerschaert et al., 1998). Herein,we provide the first evidence that LPA induces both actin depolymerizationand polymerization within a single neuronal cell through distinct,receptor-mediated signaling pathways. Actin depolymerization furtherseems to be involved in regulation of neuronal growth conemorphology.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell Cultures

TR mouse cerebral cortical immortalized neuroblast cells and B103 rat neuroblastoma cells were grown as described previously(Chun and Jaenisch, 1996; Hecht et al., 1996; Fukushima et al.,1998; Ishii et al., 2000). Cells were maintained in DMEM (Invitrogen,Carlsbad, CA) containing 10% fetal calf serum and penicillin/streptomycin.For experiments, cells were grown on (poly)lysine-coated glasscoverslips (12 or 40 mm in diameter, 500 cells/coverslip, unlessstated otherwise; Fisher Scientific, Tustin, CA). The next day,cells were washed with serum-free Opti-MEM I (Invitrogen) supplementedwith 55 µM $beta$ -mercaptoethanol, 20 mM glucose, and penicillin/streptomycin,and were further incubated in the serum-free medium for 1 d beforeanalyses. Primary cortical neurons were prepared using embryonicday 12 mice as described previously (Fukushima et al., 2000),seeded on Cell-TaK (BD Biosciences, Franklin Lakes, NJ)-coatedglass coverslips (12 mm in diameter, 500-2000 cells/coverslip),and cultured in Opti-MEM containing 5% fetal calfserum.

Time-Lapse Video Microscopy

Time-lapse, video-enhanced differential interference contrast (DIC) microscopy was carried out as described previously (Fukushimaet al., 2000). The 40-mm coverslips were mounted onto a heat-controlledperfusion apparatus (FCS-2; Bioptechs, Butler, PA) set at 37°C,and cells were observed with an inverted microscope (Axiovert135; Carl Zeiss, Thornwood, NY) by using a 63× oil immersion objective(Plan-Apochromat; Carl Zeiss). Replacement of culture medium witha buffer containing 0.1% fatty acid-free bovine serum albumin(Sigma-Aldrich, St. Louis, MO) was manually performed with a syringe(~2 ml/min). DIC images were collected every 15 s with a cooledcharge-coupled device camera (DEI-47; Carl Zeiss) by using theScion Image software (Scion, Frederick,MA).

Immunocytochemistry

Cells were fixed for 15 min with 3.7% formaldehyde in the presence of 0.5% Triton X-100 and were then washed with phosphate-bufferedsaline. To visualize f-actin, cells were incubated with AlexaFluor 546-labeled phalloidin (1 U/ml; Molecular Probes, Eugene,OR). For double-labeling studies, cells were blocked with 10%normal goat serum and 0.5% bovine serum albumin and incubatedfor 2 h with a primary antibody. The antibody used was an anti- $alpha$ -actininmonoclonal antibody (mAb) (1:300; Sigma-Aldrich), anti-gelsolinmAb (2 µg/ml; BD Biosciences), anti-GFP polyclonal antibody forlabeling enhanced green fluorescent protein (EGFP) (1:1000; CLONTECH,Palo Alto, CA), or anti-FLAG M2 mAb (1 µg/ml; Sigma-Aldrich).Cells were further incubated with biotinylated anti-mouse IgM,anti-rabbit IgG, or anti-mouse IgG antibodies (5 µg/ml; all fromVector Laboratories, Burlingame, CA), followed by incubation withAlexa 488 streptavidin (1 µg/ml; Molecular Probes) and Alexa 546phalloidin. For double labeling of transfected TR cells for FLAGand $alpha$ -actinin, cells were first labeled for FLAG. Cells were thenincubated with anti- $alpha$ -actinin antibody, followed by incubationwith Cy3-labeled anti-mouse IgM antibody (1.5 µg/ml; Jackson ImmunoresearchLaboratories, West Grove, PA). For double labeling of B103 cellsfor EGFP and $alpha$ -actinin, cells were first labeled for EGFP andthen stained for $alpha$ -actinin. Approximately 200 cells/coverslipwere observed with an inverted microscope (Axiovert 135) and a40× objective (Plan NEOFLUAR; Carl Zeiss), and counted in at leastfive fields, which were selected randomly, but substantially inthe middle, top, and bottom of the middle and right and left ofthe middle of coverslips. Cells were also photographed using a40× (Plan NEOFLUAR) or 63× oil immersion objective (Plan-Apochromat)and Cy3 or fluorescein filters, and jpg format images created.In some cases, fluorescent images were captured using a charge-coupleddevice camera (DXM1200; Nikon, Tokyo, Japan) and software ACT-1(version 2.0; Nikon), and converted to jpg files. All figuresof stained cells were generated by using Adobe Photoshop 6.0 (AdobeSystems, Mountain View,CA).

Ca²⁺ Imaging

Cells were cultured on 40-mm coverslips, loaded with 10-20 µM fura 2-acetoxymethyl ester, and subjected to Ca²⁺ image analysis (Habara and Kanno, 1991). Briefly, the coverslipwas mounted onto a heat-controlled perfusion apparatus (FCS-2;35°C), and fluorescence images were analyzed by the digital imageprocessor (Argus-100/Ca; Hamamatsu Photonics, Hamamatsu, Japan).The buffer was Opti-MEM I (without phenol red) containing 0.1%fatty acid-free bovine serum albumin. LPA stimulation was performedby the replacement with LPA (1 µM)-containing buffer at 2 ml/min.The images were collected at a 30-s interval before (2 images)and after LPA exposure (12 images) and displayed usingpseudocolor.

PLC Assay

TR cells on 12-well plates were prelabeled with [³H]inositol (2 µCi/well), stimulated with LPA for 20 min, and radioactivityin the inositol phosphate fractions measured, as described previously(Ishii et al., 2000).

Rho Assay

Cells on 40-mm (poly)lysine-coated coverslips (20,000 cells seeded/coverslip) were stimulated with LPA and lysed in 500 µlof Rho-binding buffer (50 mM Tris-HCl, 500 mM NaCl, 10 mM MgCl₂,1% Triton X-100, 0.5% sodium deoxycholate, 0.1% SDS, and 1× proteaseinhibitor cocktail, pH 7.2). Cell lysates were centrifuged andthe resultant supernatants (450 µl) incubated with agarose beads-conjugatedrhotekin Rho binding domain (Upstate Biotechnology, Lake Placid,NY) for 45 min on ice. The beads were washed four times and bead-bound,GTP-bound active forms of Rho specifically detected by Westernblot analysis by using anti-RhoA mAb (50 ng/ml; Santa Cruz Biotechnology,Santa Cruz, CA), peroxidase-labeled anti-mouse IgG antibody (100ng/ml; Vector Laboratories), and ECL Plus (Amersham Biosciences,Piscataway, NJ), according the manufacturers' protocols. An aliquot(15 µl) of the cell lysates was used for detection of total amountsofRho.

Construction of FLAG-tagged $alpha$ -Actinin Expression Plasmids

Chick nonmuscle $alpha$ -actinin cDNA (Waites et al., 1992) was a kind gift from Dr. David R. Critchley (University of Leicester,Leicester, United Kingdom). A full-length $alpha$ -actinin DNA that encodes893 amino acids and an $alpha$ -actinin mutant DNA that lacks Ca²⁺-binding domain sequences and encodes 711 amino acids [designatedherein as $alpha$ -actinin^(-EF)] were amplified with polymerase chain reaction by using PlatinumTaq DNA polymerase high-fidelity (Invitrogen). They were subclonedin frame into the NotI/XbaI and NotI/ClaI sites of a pFLAG-CMV-2mammalian expression vector (Sigma-Aldrich), respectively. Thenucleotide sequences were confirmed by BigDye terminator cyclesequencing (Applied Biosystems, Foster City,CA).

Transfection of TR Cells or Primary Cortical Neurons

TR cells were transfected with expression plasmids by using LipofectAMINE PLUS (Invitrogen). Cells were seeded on (poly)lysine-coatedglass coverslips (500 cells/12 mm in diameter for immunostainingor 20,000 cells/40 mm in diameter for Western blotting) and incubatedfor 15 h with DNA-lipid complex (0.1 µg of DNA-1 µl of PLUS reagent-0.5µl of LipofectAMINE/cm²). Cells were washed and further cultured in serum-free mediumfor 1 d before use. Transfection of cortical neurons was performed3 d after seeding using LipofectAMINE2000 (0.15 µg of DNA-0.4µl of lipid/cm²; Invitrogen). Cells were washed after 24 h and further culturedin serum-free Opti-MEM for 1 d beforeuse.

f-Actin Binding Assay

TR cells on a 9-cm dish were transfected with expression plasmids by using LipofectAMINE2000. Cells were sonicated in 100µl of lysis buffer (50 mM Tris-Cl, 0.6 M KCl, 1 mM EDTA, 1% TritonX-100, 0.5% deoxycholate-Na, and 1× protease inhibitor cocktail,pH 7.4), and cell lysates diluted with 500 µl of lysis bufferwithout KCl and deoxycholate-Na. FLAG-tagged proteins were immunoprecipitatedusing anti-FLAG M2 antibody (3 µg) and protein G-agarose (SantaCruz Biotechnology) and eluted in 0.1 M glycine-HCl containing0.1% Triton X-100, pH 3.5. The elutes (100 µl) were neutralizedwith 10 µl of 0.6 M Tris-Cl, pH 8.2, and subjected to f-actinbinding assay. Eluted proteins (40 µl) were incubated with f-actin(10 µg) in 200 µl of binding buffer (20 mM Tris-Cl, 2 mM MgCl₂,1 mM EDTA, and 0.5 mM dithiothreitol, pH 7.4) with or without1.1 mM CaCl₂ for 1 h on ice. f-Actin was prepared by incubatingrabbit muscle actin (Sigma-Aldrich) in polymerization buffer (5mM Tris-Cl, 1 mM MgCl₂, 50 mM KCl, and 1 mM ATP, pH 8) at 4°Cfor 4 h. Reaction mixtures were centrifuged at 65,000 rpm (TLA100,3; Beckman Coulter, Fullerton, CA) for 1 h and the supernatants(unbound proteins) precipitated by adding trichloroacetic acid.The trichloroacetic acid precipitates and ultracentrifuge precipitates(f-actin-bound proteins) were analyzed by Western blot analysisby using anti-FLAG M2 antibody (50 ng/ml). Bound antibodies werevisualized by subsequent incubation with peroxidase-labeled anti-mouseIgG antibody and ECL plus. Images were captured by using ATTOLight Capture (AE-6960; ATTO, Tokyo,Japan).

Western Blotting

Cells were harvested in phosphate-buffered saline and mixed with 2× SDS-sample buffer (Laemmli, 1970). Cell extracts (50 µgof protein) were separated on 10% polyacrylamide gels, and proteinswere transferred to polyvinylidene difluoride membranes (Millipore,San Jose, CA), which was followed by probing with anti-FLAG M2antibody. Membranes were further incubated with peroxidase-labeledanti-mouse IgG antibody and ECL plus and exposed to x-rayfilms.

Infection of B103 Cells with Retroviruses Expressing LPA Receptors

Production of retroviruses expressing LPA₁ or LPA₂ and infection of B103 cells with these viruses were performed as describedpreviously (Ishii et al., 2000).

Reagents

LPA was purchased from Avanti Polar Lipids (Alabaster, AL). Cytochalasin D, pertussis toxin, bisindolylmaleimide I (Go6850),1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraacetic acid-acetoxymethylester (BAPTA-AM), R-(+)-trans-N-(4-pyridyl)-4-(l-aminoethyl)-cyclohexanecarboxamide (Y27632), and genistein were purchased from Calbiochem(La Jolla,CA).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Effects of LPA on Cell Shape and Actin Cytoskeleton

To examine the effects of LPA on neuronal cell morphology, we used TR cells, which are immortalized neuroblasts derived fromembryonic mouse cerebral cortex (Chun and Jaenisch, 1996; Hechtet al., 1996; Ishii et al., 2000). TR cells extend their bipolaror multipolar processes on (poly)lysine-coated glass coverslipsunder serum-free culture condition (Chun and Jaenisch, 1996; Ishiiet al., 2000). These cells express lpa₁ and lpa₂ but not lpa₃,and respond to LPA with rapid retraction of their processes, resultingin cell rounding (Hecht et al., 1996; Ishii et al., 2000). Closerobservation of TR cells revealed that most cells possess membraneruffling at the tips of processes (Figure 1). After LPA exposure,these structures began to disappear within 1 min and completelydisappeared by 4 min (Figure 1). In contrast, the well-documentedphenomenon of process retraction (Hecht et al., 1996; Ishii etal., 2000) was also detectable at 1 min after LPA stimulationand was completed by 10-15 min, resulting in cell rounding (seebelow). LPA-induced loss of membrane ruffling was also observedin TSM cells (Chun and Jaenisch, 1996), another immortalized neuroblastcell type derived from cerebral cortex (our unpublished data).Because membrane ruffling has been shown to contain enriched actinmicrofilaments (Bray, 1992; Matsudaira, 1994), we examined actinrearrangement during the loss of membrane ruffling.

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Figure 1. LPA induces a rapid loss of membrane ruffling in TR cells. Cells were treated with 0.5 µM LPA and cell morphology monitored by DIC microscopy. Arrows indicate membrane ruffling. Arrowheads indicate retracted processes that have lost membrane ruffling. Bar, 10 µm.

TR cells were labeled with Alexa Fluor 546 phalloidin, allowing the visualization of f-actin (Figure 2). In most of the resting(control) cells, f-actin was distributed throughout cell bodiesand was particularly enriched within membrane ruffling (Figure2, a and b). This type of labeling was observed in ~75% of totalcells, with the remaining cells showing no prominent stainingat the tips (~15%) or rounded morphologies without processes (~10%).In this study, cells with these three typical morphologies arereferred to as E(+) (extended process with f-actin-enriched membraneruffling), E( $-$ ) (extended processes without f-actin-enriched membraneruffling), and R (rounded cell body) (Figure 2e).

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Figure 2. LPA induces actin rearrangement in TR cells. (a-d) f-Actin labeling of cells treated without (a and b) or with 0.5 µM LPA for 2 min (c) or 15 min (d). Arrows (b) indicate f-actin-enriched membrane ruffling. Arrowheads (c) indicate processes without enriched f-actin. (e) Classification of three typical cell shapes: E(+) cells, cells with extended processes with f-actin-enriched membrane ruffling; E( $-$ ) cells, cells with extended processes without f-actin-enriched membrane; and R cells, cells with rounded cell bodies without processes. Graded shading shows accumulation of f-actin. (f) Time course of LPA-induced changes in populations of E(+), E( $-$ ), and R cells. Data are the means ± SEM (n = 8). Bar, 50 µm (a) and 20 µm (b-d).

One to four minutes after 0.5 µM LPA exposure, E(+) cell population decreased, whereas E( $-$ ) cell population increased (Figure2, c and f). The f-actin staining observed in E( $-$ ) cells was indistinguishablefrom that observed in cells treated with 200 nM cytochalasin D(CD) (our unpublished data), a drug that promotes actin depolymerizationand also inhibits actin polymerization. This suggested that LPArapidly induced actin depolymerization within ruffling membranes,as CD did (Figure 3a). The E(+) cell population decreased between4 and 15 min and then increased, whereas the E( $-$ ) cell populationdecreased to a basal level between 4 and 60 min (Figure 2f). Incontrast, the R cell population reached a peak at 15-30 min andthen gradually decreased (Figure 2, d and f). The increase inthe R cell population at 15 min was significantly inhibited bypretreatment with CD (Figure 3c), consistent with previous resultsshowing that process retraction and cell rounding require actinpolymerization (Jalink et al., 1994). These results indicatedthat LPA induced rapid actin depolymerization that was associatedwith loss of membrane ruffling, which was followed by actin polymerizationthat induced process retraction and cell rounding.

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Figure 3. BAPTA-AM inhibits a loss of membrane ruffling, whereas Y27632 inhibits process retraction in LPA-stimulated TR cells. (a) Effects of various specific inhibitors on E( $-$ ) population. To examine effects of CD alone, cells were treated with 200 nM CD for 4 min. After pretreatment with inhibitors (100 ng/ml PTX for 18 h, 100 nM Go6850 for 5 min, 10 µM BAPTA-AM for 15 min, 5 µM Y27632 for 5 min, and 100 µM genistein for 5 min), cells were stimulated with 0.5 µM LPA for 4 min. Fixed cells were labeled for f-actin, and E( $-$ ) cells were counted at 4 min. Data are the means ± SEM (n = 3-6). #p < 0.05 vs. control (no treatment) and *p < 0.05 vs. none (LPA alone). (b) f-Actin labeling of Y27632-pretreated cells exposed to LPA for 4 min. (c) Effects of various specific inhibitors on R population. Cells were pretreated with inhibitors, as described in the legend of a. CD was pretreated for 5 min. Cells were stimulated with 0.5 µM LPA for 15 min and R cells counted. Data are the means ± SEM (n = 3-6). #p < 0.05 vs. control (no treatment) and *p < 0.05 vs. none (LPA alone). (d-f) Time course of LPA-induced changes in populations of E(+), E( $-$ ), and R cells when pretreated with BAPTA-AM or Y27632. Fixed cells were labeled for f-actin, and E(+), E( $-$ ), and R cells were counted (d, e, and f, respectively). Data are the means ± SEM (n = 4-8). (f, inset) Typical cell type that has a retracted process but still retains a small portion of f-actin-enriched membranes indicated by an arrow. This population likely resulted from retraction of processes with f-actin-enriched structures and was categorized as R cells. Bar, 25 µm.

Effects of BAPTA-AM and Y27632 on LPA-induced Actin Cytoskeletal Changes

LPA receptors drive multiple signaling pathways through several types of G proteins, including G_i/o, G_q, and G_12/13 (Contoset al., 2000; Ishii et al., 2000; Fukushima et al., 2001). TheG_i/o pathway is predominantly linked to mitogen-activated proteinkinase activation and AC inhibition, but not to actin rearrangement(Weiner and Chun, 1999; Ishii et al., 2000). The G_q pathway islinked to PLC activation (Ishii et al., 2000; Kimura et al., 2001),which leads to intracellular Ca²⁺ mobilization and protein kinase C (PKC) activation. These moleculescan modulate actin rearrangement by means of Ca²⁺-sensitive, actin-associated proteins such as $alpha$ -actinin or gelsolin,and by phosphorylation of these proteins (Janmey, 1994; Keenanand Kelleher, 1998). The G_12/13 pathway activates Rho and Rho-associatedkinases (ROCKs), resulting in actin polymerization (Gohla et al.,1998; Kranenburg et al., 1999). Specific pharmacological inhibitors,which are well established and widely used, were used to determinewhich pathways were involved in LPA-induced actindepolymerization.

Pretreatment of cells with pertussis toxin (PTX), which inhibits G_i/o activation (Katada et al., 1986), did not alter LPA-inducedchanges in the E( $-$ ) or R cell populations (Figure 3, a and c).Pretreatment of cells with a PKC inhibitor Go6850 (Toullec etal., 1991) also failed to alter the changes in those populations(Figure 3, a and c). At the used concentration (100 nM), thiscompound shows high selectivity for PKC but does not affect otherkinases (Toullec et al., 1991). These results indicated that bothG_i/o and PKC pathways were not involved in LPA-induced actin rearrangement.In contrast, when cells were pretreated with BAPTA-AM, which isknown to prevent LPA-induced increase in intracellular Ca²⁺ concentrations in many types of cells (Manning and Sontheimer,1997; Shahrestanifar et al., 1999), LPA-induced transient increasesin the numbers of E( $-$ ) cells were completely blocked (Figure 3,a and e). The E(+) cell population remained at relatively higherpercentages in BAPTA-AM-treated cells compared with the percentagesfound in control cells (Figure 3d). The R cell population increasedwith time in BAPTA-AM-treated cells, similar to that in controlcells (Figure 3f). Treatment with BAPTA-AM alone did not significantlyaffect the populations of E(+), E( $-$ ), and R, suggesting that thiscompound showed no effect on actin rearrangement under the restingconditions. These results indicated that Ca²⁺ signaling was involved in LPA-induced actin depolymerizationbut not actin polymerization. Consistent with this, thapsigargin,a reagent that depletes Ca²⁺ stores and increases intracellular Ca²⁺ concentrations (Thastrup et al., 1990), induced the loss of membraneruffling in TR cells, accompanied by actin depolymerization [E( $-$ )population; 78% at 15 min after thapsigargin alone treatment].

A highly specific and well-characterized ROCK inhibitor, Y27632 (Uehata et al., 1997; Hirose et al., 1998), was used to examinethe involvement of the Rho pathway. Pretreatment of cells withY27632 did not affect LPA-induced decreases in the E(+) cell populationpercentages during the first several minutes after LPA exposure(Figure 3d). However, in Y27632-treated cell populations, therewas no increase in the R cell population (Figure 3, c and f).Instead, a greater increase in the E( $-$ ) cell percentages was observedin Y27632-treated cells than observed in nontreated cells (Figure3, a, b, and e). These results suggested that cells remained inthe E( $-$ ) cell stage without progressing to the R cell stage. Similarresults were obtained in cells pretreated with genistein, a generaltyrosine kinase inhibitor (Akiyama et al., 1987) (Figure 3, aand c), consistent with the previous report (Kranenburg et al.,1999). Because genistein has little effect on PKC and other proteinkinases at the concentration used (100 nM), our results indicatedthe involvement of tyrosine kinase in LPA-induced actin polymerization.However, how genistein-sensitive tyrosine kinase(s) interactswith the Rho pathway remains to bedetermined.

LPA-induced Ca²⁺ Mobilization and Rho Activation

Our pharmacological experiments have suggested two intracellular signals involved in actin rearrangement in TR cells: Ca²⁺ mobilization and Rho activation. To further confirm the datafrom these experiments, we directly measured both signals andPLC activity. Ca²⁺ mobilization was monitored using fura 2, a fluorescent Ca²⁺ indicator. No Ca²⁺ mobilization was observed before LPA exposure (Figure 4, a andb). However, a transient increase in Ca²⁺ concentration was detected throughout a cell body, includingmembrane ruffling, process shaft, and the soma after LPA exposure(Figure 4, a and b). Maximal increase was observed at 2 min afterLPA stimulation, consistent with an increase of E( $-$ ) cells (Figure2f). Such Ca²⁺ mobilization was likely to be induced by inositol trisphosphate,because LPA stimulated PLC activity in TR cells (Figure 4c). LPA-inducedRho activation was tested in pull down assay by using agarosebeads-conjugated rhotekin Rho binding domain, which specificallybinds active GTP-bound forms of Rho (Ren and Schwartz, 2000).Within 4 min after LPA exposure, Rho was activated, and this activationsustained for at least 1 h (Figure 4d). Together with the resultsusing Y27632 (Figure 3), these data indicated that the Rho pathwaywas involved in LPA-induced process retraction by actin polymerization,as reported previously (Jalink et al., 1993; Hirose et al., 1998;Kranenburg et al., 1999), but not in actin depolymerization.

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Figure 4. Increase in Ca²⁺ mobilization and Rho activity by LPA in TR cells. (a) Effects of LPA on Ca²⁺ mobilization. Cells were loaded with fura 2-acetoxymethyl ester and subjected to Ca²⁺ image analyses. DIC and Ca²⁺ images before LPA (1 µM) exposure and Ca²⁺ image 110 s after LPA exposure are shown. Note an increase in Ca²⁺ concentration within membrane ruffling after LPA exposure. An arrow indicates membrane ruffling. (b) Time course of fluorescence ratio. Fluorescence ratios (340 nm/380 nm) were determined within small portions in membrane ruffling and cytosol squared in a. The drop of ratio in the ruffling after 5 min is due to the disappearance of cell structures by process retraction. (c) Effects of LPA on PLC activity. Cells were labeled with [³H]inositol and stimulated with LPA, and PLC activity was measured as accumulation of radiolabeled total inositol phosphates (IPs). (d) Effects of LPA on Rho activity. Cells were stimulated with LPA for the indicated time and extracted for the detection of active and total Rho. Bar, 20 µm.

Subcellular Localization of $alpha$ -Actinin and f-Actin

The state of actin polymerization is controlled with actin-binding proteins, such as actin-capping or actin cross-linkingproteins. These proteins regulate polymerization of globular actin,depolymerization of f-actin, and cross-linking of f-actin in responseto intracellular signaling molecules (e.g., Ca²⁺) (Bamburg and Bernstein, 1991; Bray, 1992; Janmey, 1994; Matsudaira,1994). In view of our data suggesting the role of Ca²⁺ in LPA-induced actin depolymerization (Figures 3 and 4), theinvolvement of $alpha$ -actinin or gelsolin, both of which are Ca²⁺-regulated actin-binding proteins, was examined. $alpha$ -Actinin isan actin cross-linking protein, which has been shown to play arole in neurite outgrowth in neuronal cells and to exist withinmembranes ruffling of motile cells (Jockusch et al., 1983; Bamburgand Bernstein, 1991; Sobue, 1993). Binding of Ca²⁺ to a nonmuscle type of $alpha$ -actinin stimulates its dissociationfrom f-actin, resulting in the accumulation of free f-actin (Condeelisand Vahey, 1982). On the other hand, gelsolin is a Ca²⁺-regulated actin-severing protein, and binding of Ca²⁺ to gelsolin leads to actin depolymerization (Bamburg and Bernstein,1991; Janmey, 1994).

When TR cells were double labeled for $alpha$ -actinin and f-actin, expression of $alpha$ -actinin was observed throughout the soma, particularlywithin membrane ruffling where prominent f-actin labeling wasobserved (Figure 5, a and b). We also treated TR cells with LPA,followed by labeling for $alpha$ -actinin. Within 2 min after LPA exposure, $alpha$ -actinin labeling either weakened or vanished at the tips ofprocesses with a concomitant reduction in f-actin labeling (Figure5, c and d). Cell populations with prominent $alpha$ -actinin labelingat the tips of processes decreased between 2 and 8 min, and thengradually recovered with time (Figure 5e). This temporal profilewas consistent with that of E(+) cells (Figure 5e). In contrast,gelsolin distribution showed no obvious overlap with that of f-actinboth in control and LPA-treated cells (Figure 5, f and g). Theseresults indicated that LPA-induced actin depolymerization/polymerizationwithin ruffling membranes was correlated with $alpha$ -actinin accumulation,but not gelsolin, and allowed us to focus on a role of $alpha$ -actinin.

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Figure 5. Colocalization of f-actin and $alpha$ -actinin within membrane ruffling in TR cells. (a-d) Cells treated without (a and b) or with 0.5 µM LPA for 2 min (c and d) were labeled for f-actin (a and c) or $alpha$ -actinin (b and d). Arrows indicate colocalization of f-actin and $alpha$ -actinin within membrane ruffling, and arrowheads indicate LPA-induced concomitant reduction in f-actin and $alpha$ -actinin labeling within membrane ruffling. (e) Time course of LPA-induced changes in E(+) cell population and those cells with prominent $alpha$ -actinin labeling within membrane ruffling. Cells were treated with 0.5 µM LPA for the indicated time, fixed, and double labeled for f-actin and $alpha$ -actinin. Data are the means ± SEM (n = 6). (f and g) Gelsolin staining of cells treated without (f) or with 0.5 µM LPA for 2 min (g). Bar, 20 µm.

The signaling pathways regulating $alpha$ -actinin distribution were explored using BAPTA-AM or Y27632. Cells were pretreated withBAPTA-AM or Y27632, exposed to LPA, and then double labeled for $alpha$ -actinin and f-actin. In BAPTA-AM-treated cells, $alpha$ -actinin labelingwas prominent and correlated with an accumulation of f-actin withinmembrane ruffling (Figure 6, a and b). In contrast, cells treatedwith Y27632 showed loss of both f-actin and $alpha$ -actinin labelingat the tips of processes after LPA exposure (Figure 6, c and d),as was found in control cells (Figure 5, c and d). These dataindicated that Ca²⁺ signaling, but not Rho pathways, was involved in LPA-inducedloss of $alpha$ -actinin and f-actin labeling within membranes ruffling.

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Figure 6. BAPTA-AM, but not Y27632, inhibits LPA-induced concomitant reduction in f-actin and $alpha$ -actinin labeling. (a and b) f-Actin (a) and $alpha$ -actinin (b) labeling of TR cells treated with 0.5 µM LPA for 2 min in the presence of 10 µM BAPTA-AM. Arrows indicate colocalization of f-actin and $alpha$ -actinin within membrane ruffling. (c and d) f-Actin (c) and $alpha$ -actinin (d) labeling of TR cells treated with 0.5 µM LPA for 2 min in the presence of 5 µM Y27632. Arrowheads indicate concomitant reduction in f-actin and $alpha$ -actinin labeling within membrane ruffling. Bar, 20 µm.

Effects of an $alpha$ -Actinin Mutant on LPA-induced Cytoskeletal Changes

$alpha$ -Actinin consists of an actin-binding domain, a domain containing spectrin-like repeats, and two EF hand Ca²⁺-binding motifs (Baron et al., 1987a,b; Arimura et al., 1988;Youssoufian et al., 1990; Waites et al., 1992) (Figure 7a). Toexamine the requirement of $alpha$ -actinin for f-actin depolymerization,a mutant form of $alpha$ -actinin that lacks two EF hand motifs [designatedherein as $alpha$ -actinin^(EF)] and thereby could act as Ca²⁺-inseisitive $alpha$ -actinin was constructed (Figure 7a). The expressionof FLAG-tagged proteins in TR cells was confirmed by Western blotanalysis by using anti-FLAG antibody (Figure 7b). Both FLAG-tagged $alpha$ -actinin and $alpha$ -actinin^(EF) showed f-actin-binding activities in the absence of Ca²⁺ (Figure 7c), as expected from the reports that truncated $alpha$ -actinin(without spectrin-like domains and EF motifs, or without onlyEF motifs) can bind f-actin (Tokuue et al., 1991; Hemmings etal., 1992). In addition, f-actin-binding activity of $alpha$ -actinin^(EF) was expectedly Ca²⁺ insensitive under conditions where FLAG-tagged full-length $alpha$ -actininlost the binding activity (Figure 7c). In TR cells transfectedwith FLAG-tagged $alpha$ -actinin or $alpha$ -actinin^(EF) plasmid, FLAG immunolabeling always colocalized with f-actin,particularly within membrane ruffling (Figure 7d). However, whenthese cells were double labeled for FLAG and $alpha$ -actinin, no orweak labeling of $alpha$ -actinin was observed within membrane rufflingof FLAG-tagged $alpha$ -actinin^(EF)-expressing cells, whereas clear labeling in FLAG-tagged $alpha$ -actinin-expressingcells. Because anti- $alpha$ -actinin antibody recognized $alpha$ -actinin butnot $alpha$ -actinin^(EF) (our unpublished data), these results indicated that the levelof endogenous $alpha$ -actinin decreased within membrane ruffling of $alpha$ -actinin^(EF)-expressing cells. Therefore, exogenously expressed $alpha$ -actinin^(EF) could replace endogenous $alpha$ -actinin to cross-link f-actin withinmembrane ruffling, and perhaps fail to respond to intracellularCa²⁺ mobilization by dissociating f-actin and thereby acts as a dominant-negativeform.

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Figure 7. Overexpression of Ca²⁺-insensitive mutant $alpha$ -actinin inhibits LPA-induced actin depolymerization in membrane ruffling. (a) Schematic illustration of protein structures of $alpha$ -actinin and $alpha$ -actinin^(EF), a mutant form lacking two EF hands. (b) Western blot analyses of transfected TR cells to detect overexpressed FLAG-tagged proteins. Nontransfected or transfected cells with a control vector (FLAG-BAP), $alpha$ -actinin^(EF), or $alpha$ -actinin expression vector were analyzed using anti-FLAG antibody. Arrowheads indicate overexpressed FLAG-tagged proteins. (c) f-Actin binding of FLAG-tagged $alpha$ -actinin and $alpha$ -actinin^(EF). Tagged proteins were immunoprecipitated from TR cell extracts and used for f-actin-binding assay in the absence or presence of Ca²⁺. Unbound (s) and bound (p) fractions were subjected to Western blot analysis to detect FLAG. (d) FLAG, f-actin, and $alpha$ -actinin labeling of transfected TR cells. Transfected cells were double labeled for FLAG and f-actin, or FLAG and $alpha$ -actinin. Arrows indicate typical membrane ruffling that contains $alpha$ -actinin^(EF) and f-actin. Arrowheads indicate typical membrane ruffling that contains $alpha$ -actinin^(EF) and low levels of endogenous $alpha$ -actinin. (e) Effects of $alpha$ -actinin^(EF) overexpression on LPA-induced increase in E( $-$ ) cell population. TR cells were transfected and treated without or with 0.5 µM LPA. Cells were fixed at 4 min and double labeled for f-actin and FLAG, and E( $-$ ) cells were counted. Data are the means ± SEM (n = 4). *p < 0.05 $alpha$ -actinin^(EF) vs. BAP.

TR cells were transfected with a control vector (FLAG-bacterial alkaline phosphatase; BAP), or experimental vectors [FLAG- $alpha$ -actininand FLAG- $alpha$ -actinin^(EF)], exposed to LPA for 4 min and then double labeled for f-actinand FLAG. The E( $-$ ) and E(+) cells were counted in the FLAG-positivepopulation. In cells transfected with a control vector, LPA increasedthe E( $-$ ) cell population (28% increase in Figure 7e) with a concomitantdecrease in the E(+) cell population (46% decrease), indicatingthat actin depolymerization occurred as in nontransfected cells(Figure 2f). Similar results were obtained in cells overexpressingthe wild-type $alpha$ -actinin (Figure 7e). In contrast, even althoughthe expression of FLAG-tagged $alpha$ -actinin^(EF) was much lower than that of FLAG-tagged wild-type $alpha$ -actinin intransfected TR cells (Figure 7b), the LPA-induced increase inthe E( $-$ ) cell population was significantly attenuated by $alpha$ -actinin^(EF) overexpression (16% increase in Figure 7e). There was also asignificant inhibition of the LPA-induced decrease in the E(+)cell population (29% decrease). These results indicated that overexpressionof a mutant $alpha$ -actinin^(EF) inhibited LPA-induced actin depolymerization, suggesting thatCa²⁺-regulation through EF hands in $alpha$ -actinin was, at least in part,responsible for LPA-induced actin depolymerization within membraneruffling.

Effects of $alpha$ -Actinin^(EF) on LPA-induced Morphological Changes in Growth Cone of Primary Neurons

$alpha$ -Actinin is known to be enriched in neuronal growth cone and suggested to be involved in its morphology (Sobue, 1993). Ourfinding that $alpha$ -actinin also accumulated in membrane ruffling atthe tips of growing processes of TR cells led us to examine arole of LPA-induced actin depolymerization in growth cone morphologyof primary neurons. We used primary cultures consisting of youngcortical neurons in which neurite outgrowth was underway and lpa₂was expressed (Fukushima et al., 2002). These neurons expressedendogenous $alpha$ -actinin at their growth cone and cell body, colocalizedwith f-actin (Figure 8, a and b). This overlap was similar tothat observed in TR cells, although the fluorescence intensitiesof these components were not as high as those in TR cells. Incontrol, 38.9% of total neurons possessed intact growth cones,defined as f-actin-enriched, flat and wider structures than neurites.When LPA was exposed to these neurons for 4 min, the populationwith growth cones was decreased to 16.7%, indicating that LPAinduced growth cone collapse. However, no marked process retractionand cell rounding were not observed, probably because these cellularresponses were reduced with the progress of morphological maturationof neurons (Fukushima et al., 2002). Similar growth cone collapsewas observed in neurons transfected with a control FLAG-BAP vector(Figure 8, c-f, the population with growth cone in transfectedneurons; 46.2% in control vs. 23.8% in LPA treatment). In contrast,LPA treatment failed to induce marked changes in growth cone morphologyof $alpha$ -actinin^(EF)-expressing neurons (Figure 8, g-j, the population with growthcone in transfected neurons; 46.5% in control vs. 43.8% in LPAtreatment). These results indicated that LPA-induced actin depolymerizationthrough $alpha$ -actinin was involved in regulation of growth cone morphologyof primary neurons.

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Figure 8. Overexpression of $alpha$ -actinin^(EF) inhibits LPA-induced growth cone collapse. (a and b) $alpha$ -Actinin (a) and f-actin (b) labeling of primary cortical neurons cultured for 5 d. (c-f) Typical FLAG (c and e) and f-actin (d and f) labeling of cortical neurons transfected with a FLAG-BAP plasmid. Neurons were treated without (c and d) or with 0.5 µM LPA for 4 min (e and f), and double labeled for FLAG and f-actin. (g-j) Typical FLAG (g and i) and f-actin (h and j) labeling of cortical neurons transfected with a FLAG- $alpha$ -actinin^(EF) plasmid. Neurons were treated without (g and h) or with 0.5 µM LPA for 4 min (i and j), and double labeled for FLAG and f-actin. Insets are 3× magnifications of growth cones. Growth cones in b, d, h, and j are defined to be intact by f-actin-enriched, flat, and wider structures than neurites, whereas growth cone in f is collapsed. Bar, 20 µm.

Heterologous Expression of LPA Receptors lpa₁ or lpa₂

Two LPA receptors expressed in TR cells, LPA₁ and LPA₂, have similar signaling properties, including PLC activation and Rhostimulation (Fukushima et al., 1998, 2001; Ishii et al., 2000;Kimura et al., 2001). On the other hand, the LPA molecule itselfcan directly interact with actin-binding proteins (Meerschaertet al., 1998), and these interactions might be involved in theLPA-induced actin depolymerization. To determine whether LPA receptorsor nonreceptor mechanisms are involved in actin depolymerization,either lpa₁ or lpa₂ was heterologously expressed using retrovirusexpression systems in a B103 rat neuroblastoma cell line. Thiscell line expresses none of the three known LPA receptors andshows no cytoskeletal responses to LPA, but responds to LPA withprocess retraction when either lpa₁ or lpa₂ is introduced (Fukushimaet al., 1998; Ishii et al., 2000; Kimura et al., 2001).

Cells were infected with lpa₁-expressing retroviruses that coexpress EGFP, and then double labeled for EGFP and either f-actinor $alpha$ -actinin. Infected (EGFP-positive) cells showed marked f-actinlabeling as well as $alpha$ -actinin labeling within membrane rufflingas was observed in TR cells (Figure 9, a, b, e, and f). LPA treatmentfor 2 min resulted in reduced labeling within the tips of processes(Figure 9, c, d, g, h, and i). Such changes in f-actin and $alpha$ -actininlabeling were also observed in lpa₂-expressing cells (Figure 9i).In the absence of exogenous lpa₁ or lpa₂ expression, actin depolymerizationwas not observed (Figure 9i). Combined with our previous data(Fukushima et al., 1998; Ishii et al., 2000), both LPA₁ and LPA₂appeared capable of explaining LPA-induced actin depolymerizationassociated with membrane ruffling as well as actin polymerizationin neurite shafts.

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Figure 9. Heterologous expression of LPA₁ or LPA₂ is sufficient for LPA-induced actin depolymerization in B103 cells. (a-d) f-Actin (a and c) and EGFP (b and d) labeling of B103 cells infected with retroviruses expressing lpa₁. Cells were treated without (a and b) or with 0.5 µM LPA for 2 min (c and d), and double labeled for f-actin and EGFP. An arrow (a) indicates a process with f-actin-enriched membrane ruffling. An arrowhead (c) indicates a process without f-actin-enriched structures. (e-h) $alpha$ -Actinin (e and g) and EGFP (f and h) labeling of B103 cells infected with retroviruses expressing lpa₁. Cells were treated without (e and f) or with 0.5 µM LPA for 2 min (g and h) and double labeled for $alpha$ -actinin and EGFP. An arrow (e) indicates a process with $alpha$ -actinin-enriched membrane ruffling. An arrowhead (g) indicates a process without $alpha$ -actinin-enriched structures. (i) Time course of LPA-induced reduction in B103 cell populations with enriched f-actin or $alpha$ -actinin. B103 cells infected with retroviruses expressing lpa₁ or lpa₂ were treated with 0.5 µM LPA. Cells were fixed at the indicated time and double labeled for f-actin and EGFP or $alpha$ -actinin and EGFP. E(+) cells and cells with prominent $alpha$ -actinin labeling within membrane ruffling were counted in naive cells (left) or cells infected to express lpa₁ (middle) or lpa₂ (right). Data are the means ± SEM (n = 4-6). Bar, 20 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We have shown herein that LPA induces two distinct forms of actin rearrangement within single neuroblasts: depolymerizationassociated with loss of membrane ruffling, and polymerizationassociated with process retraction. A single type of LPA receptorregulates each actin rearrangement by activating distinct cellularsignaling pathways: depolymerization via Ca²⁺- $alpha$ -actinin and actin polymerization via Rho. These results suggesta novel role for receptor-mediated LPA signaling in regulationof the actin cytoskeleton in neuronalcells.

LPA Induces Both Actin Depolymerization and Polymerization within a Single Cell

Actin microfilaments are primarily regulated through their interactions with actin-binding proteins and/or intracellular signalingmessengers produced by extracellular stimuli such as growth factorsand extracellular matrix (ECM) (Bamburg and Bernstein, 1991; Bray,1992; Janmey, 1994; Matsudaira, 1994). Depending on the typesof interactions, cells can undergo either polymerization or depolymerizationto change their morphologies (e.g., leading edge of migratingcells).

LPA has been shown to be a potent inducer of actin polymerization (Moolenaar, 1995, 1997). LPA-induced actin polymerizationresults in process retraction and cell rounding in neuronal cellssuch as N1E-115, or stress fiber formation in fibroblast cells(Ridley and Hall, 1992; Jalink et al., 1993). These cellular responsesare mediated by actomyosin interactions through activation ofthe Rho pathway, producing contractile forces that induce cellshape changes (Jalink et al., 1994; Tigyi et al., 1996; Kozmaet al., 1997; Hirose et al., 1998; Kranenburg et al., 1999; Fukushimaet al., 2000; Weiner et al., 2001). Herein, we have also shownthat Rho is activated by LPA in TR cells and LPA-induced processretraction is blocked by a ROCK inhibitor or CD, which indicatesthe possible involvement of Rho and actomyosin for process retractionin TR cells (Figure 10).

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Figure 10. Proposed model for dual regulation of actin rearrangement by diverging intracellular signals from a single LPA receptor. Either LPA₁ or LPA₂ receptors can mediate two distinct types of actin rearrangement in TR cells: actin depolymerization and polymerization. In membrane ruffling, actin is depolymerized through Ca²⁺- $alpha$ -actinin interactions, whereas in neurite shafts, actin is polymerized via the Rho pathway. These distinct pathways may coordinate to regulate morphology of neuronal cells.

In addition to actin-polymerizing effects, LPA induced more rapid, transient actin depolymerization within the same cell.It is possible that depolymerized actin could be the source forsubsequent actin polymerization during process retraction. However,this is unlikely because BAPTA-AM did not block LPA-induced processretraction, whereas Y27632 failed to inhibit LPA-induced lossof f-actin within membrane ruffling. Therefore, LPA appears toactivate two independent signaling pathways, with opposing effectson the actin rearrangement, and apparently using distinct poolsof actin. Our results also suggest that actin rearrangement inducedby LPA may be compartmentalized; actin depolymerization associatedwith membrane ruffling occurs at the tips of processes, whereasactin polymerization occurs in the shaft of processes (Figure10).

LPA-induced actin depolymerization has not been documented previously, perhaps because of the use of different cell typesor different techniques that focused on longer time periods afterLPA exposure. For example, fibroblasts have little cytoplasmicf-actin in resting conditions (i.e., G₀ phase of cell cycle) (Ridleyand Hall, 1992), and actin depolymerization might not be detectableafter stimulation of the cells. In neuronal cells, actin rearrangementhas been examined by fluorometric methods that monitor changesin f-actin in the entire cell body (Jalink et al., 1993), andthese methods might not detect local fine changes in f-actinlevels.

LPA-induced Actin Depolymerization Involves Ca²⁺- $alpha$ -Actinin but Not Rho

Several lines of evidence in the present study support an idea that LPA-induced actin depolymerization is mediated by Ca²⁺- $alpha$ -actinin interactions: 1) $alpha$ -actinin was colocalized with enrichedf-actin within membrane ruffling, and both dissipated after LPAexposure; 2) pretreatment with a Ca²⁺ chelator, BAPTA-AM, inhibited LPA-induced loss of membrane ruffling;3) intracellular Ca²⁺ mobilization was induced in membrane ruffling after LPA stimulation;and 4) overexpression of Ca²⁺-insensitive $alpha$ -actinin^(EF), which binds f-actin and replaces endogenous $alpha$ -actinin, attenuatedLPA-induced actin depolymerization. LPA-induced increases in Ca²⁺ concentration within membrane ruffling perhaps inhibit the actincross-linking activity of $alpha$ -actinin through its EF hands, whichin turn leads to the dissociation of $alpha$ -actinin from f-actin (Bamburgand Bernstein, 1991; Janmey, 1994) (Figure 10). However, actindepolymerization observed as the disappearance of f-actin labelingshould normally require actin-depolymerizing or actin-severingactivity, which has not been documented for $alpha$ -actinin. This suggestsinvolvement of another mechanism for actin depolymerization afterdissociation of actin filaments resulting from the inhibitionof $alpha$ -actininactivity.

$alpha$ -Actinin is also known to link actin filaments to receptors for ECM molecules (Pavalko et al., 1991). It has been shown thatcomplexes containing $alpha$ -actinin, ECM, and ECM receptors are involvedin the formation of membrane ruffling (Jockusch et al., 1983;O'Connor et al., 2000). We detected the distribution of $beta$ 1-integrin,one of the ECM receptors, in membrane ruffling of TR cells byimmunocytochemical labeling (our unpublished data). LPA-inducedloss of membrane ruffling may involve dissociation of actin filamentsfrom those complexes as well as betweenfilaments.

Our data show a role for $alpha$ -actinin in actin rearrangement that is different from previous results observed in several celltypes. In fibroblasts, $alpha$ -actinin is recruited along f-actin stressfibers and focal adhesions in response to serum or LPA stimulation(Barry and Critchley, 1994). These cells are likely to use $alpha$ -actininin actin rearrangement primarily directed toward polymerizationin a Rho-dependent manner, which is different from our data onneuronal cells presented herein. Whether $alpha$ -actinin is also involvedin actin polymerization in TR cells remains to be determined.However, this seems unlikely because overexpression of $alpha$ -actininor $alpha$ -actinin^(EF) did not alter LPA-induced process retraction (our unpublisheddata). Thus, in LPA-stimulated TR cells, $alpha$ -actinin appears toplay a role in actin depolymerization but not in actinpolymerization.

Both LPA₁ and LPA₂ Could Mediate LPA-induced Actin Depolymerization and Polymerization

Both LPA₁ and LPA₂ can stimulate PLC through PTX-insensitive G proteins (e.g., G_q) in neuronal cells (Ishii et al., 2000;Kimura et al., 2001), producing inositol trisphosphate that inducesCa²⁺ release from intracellular Ca²⁺ stores (Berridge, 1993). This Ca²⁺ mobilization by activation of the G_q-PLC pathway has been alsoconfirmed in the present study (Figure 4) and is probably involvedin the inhibition of $alpha$ -actinin activity (Bamburg and Bernstein,1991; Janmey, 1994). Both LPA receptors can also activate theRho pathway that is linked to myosin stimulation, which leadsto actin polymerization (Amano et al., 1998; Fukushima et al.,1998; Ishii et al., 2000). Thus, a single LPA receptor is likelyto use two independent signaling pathways for actin regulation.This idea is supported by the data from our heterologous experimentsusing B103 cells, which demonstrated that expression of eitherLPA receptor was enough for dual regulation of actinrearrangement.

Possible Roles for LPA-induced Actin Rearrangements in Neuronal Cell Morphology

TR cells show many features of cortical neuroblasts (e.g., expression of neuroblast markers, such as brain factor-1, lpa₁,and nestin [an intermediate filament protein]), but also expressearly neuronal markers, such as neurofilament proteins (Chun andJaenisch, 1996). Therefore, these cells provide a good, homogenousmodel system to study intracellular events that occur in primaryneuroblasts or migrating or differentiating neurons. Corticalneuroblasts express lpa₁ (Hecht et al., 1996) and extend radiallyoriented processes and undergo a "to-and-fro movement," calledinterkinetic nuclear migration, in which process retraction andextension are repeated with a radial nuclear movement (Seymourand Berry, 1975). Our previous study has shown that LPA signalingaffects cortical neuroblast morphology through actin polymerization(Fukushima et al., 2000). However, how actin depolymerizationis involved in the neuroblast morphology remains uncertain. $alpha$ -Actininmay form a complex with actin filaments and focal adhesion proteins,which functions as scaffolds for signal transduction and/or theattachment of processes (Barry and Critchley, 1994), althoughits precise localization in neuroblasts remains to be determined.Actin depolymerization through Ca²⁺- $alpha$ -actinin interactions may produce loss of these scaffolds and/orthe detachment of processes, an essential step of interkineticnuclear migration (Fukushima et al., 2000).

Migrating or differentiating neurons express lpa₂ (Fukushima et al., 2002) and extend leading processes during migration oraxons and dendrites at their final destination, respectively.Ca²⁺ is an important factor for the regulation of growth cone morphologyin these processes (Letourneau, 1996), and both $alpha$ -actinin andf-actin are concentrated in the filopodia of growth cone (Sobueand Kanda, 1989). Our data from the experiments using primaryneurons suggest the involvement of Ca²⁺- $alpha$ -actinin interactions in LPA-induced changes in growth conemorphology, which would implicate LPA as a guidance molecule formigrating or differentiating neurons. Clearly, further investigationshould be necessary for clarifying the biologically relevant rolesfor LPA-induced dual actin rearrangement in the nervoussystem.

	ACKNOWLEDGMENTS

We thank Carol Akita and Marisa Fontanoz for technical assistance, Drs. Joshua A. Weiner and Dhruv Kaushal for reading themanuscript, Dr. Takaharu Yamamoto for f-actin binding assay, andCasey Cox for copyediting the manuscript. This work was supportedby the National Institute of Mental Health and an unrestrictedgift from Merck Research Laboratories (to J.C.) and by the Ministryof Education, Science, Sports and Culture of Japan (to N.F. andY.H.).

	FOOTNOTES

^§ Present address: Department of Molecular Genetics, National Institute of Neuroscience, 4-1-1 Ogawahigashi, Kodaira, Tokyo187-8502, Japan

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.01-09-0465. Article and publication date are at www.molbiolcell.org/cgi/doi/10.1091/mbc.01-09-0465.

Corresponding author. E-mail address: nfuku{at}med.hokudai.ac.jp.

ABBREVIATIONS

Abbreviations used: BAP, bacterial alkaline phosphatase; CD, cytochalasin D; DIC, differential interference contrast; ECM, extracellular matrix; EGFP, enhanced green fluorescent protein; f-actin, filamentous actin; LPA, lysophosphatidic acid; PKC, protein kinase C; PLC, phospholipase C; PTX, pertussis toxin.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Akiyama, T., Ishida, J., Nakagawa, S., Ogawara, H., Watanabe, S., Itoh, N., Shibuya, M., and Fukami, Y. (1987). Genistein, a specific inhibitor of tyrosine-specific protein kinases. J. Biol. Chem. 262, 5592-5595[Abstract/Free Full Text].
Amano, M., Chihara, K., Kimura, K., Fukata, Y., Nakamura, N., Matsuura, Y., and Kaibuchi, K. (1997). Formation of actin stress fibers and focal adhesions enhanced by Rho-kinase. Science 275, 1308-1311[Abstract/Free Full Text].
Amano, M., Chihara, K., Nakamura, N., Fukata, Y., Yano, T., Shibata, M., Ikebe, M., and Kaibuchi, K. (1998). Myosin II activation promotes neurite retraction during the action of Rho and Rho-kinase. Genes Cells 3, 177-188[Abstract].
An, S., Bleu, T., Hallmark, O.G., and Goetzl, E.J. (1998). Characterization of a novel subtype of human G protein-coupled receptor for lysophosphatidic acid. J. Biol. Chem. 273, 7906-7910[Abstract/Free Full Text].
Arimura, C., Suzuki, T., Yanagisawa, M., Imamura, M., Hamada, Y., and Masaki, T. (1988). Primary structure of chicken skeletal muscle and fibroblast $alpha$ -actinins deduced from cDNA sequences. Eur. J. Biochem. 177, 649-655[Medline].
Bamburg, J.R., and Bernstein, B.W. (1991). Actin and actin-binding proteins in neurons. In: The Neuronal Cytoskeleton, ed. R.D. Burgoyne, New York: Wiley-Liss, 121-160.
Bandoh, K., Aoki, J., Hosono, H., Kobayashi, S., Kobayashi, T., Murakami-Murofushi, K., Tsujimoto, M., Arai, H., and Inoue, K. (1999). Molecular cloning and characterization of a novel human G-protein-coupled receptor, EDG7, for lysophosphatidic acid. J. Biol. Chem. 274, 27776-27785[Abstract/Free Full Text].
Baron, M.D., Davison, M.D., Jones, P., and Critchley, D.R. (1987a). The sequence of chick $alpha$ -actinin reveals homologies to spectrin and calmodulin. J. Biol. Chem. 262, 17623-17629[Abstract/Free Full Text].
Baron, M.D., Davison, M.D., Jones, P., Patel, B., and Critchley, D.R. (1987b). Isolation and characterization of a cDNA encoding a chick $alpha$ -actinin. J. Biol. Chem. 262, 2558-2561[Abstract/Free Full Text].
Barry, S.T., and Critchley, D.R. (1994). The RhoA-dependent assembly of focal adhesions in Swiss 3T3 cells is associated with increased tyrosine phosphorylation and the recruitment of both pp125FAK and protein kinase C- $delta$ to focal adhesions. J. Cell Sci. 107, 2033-2045[Abstract].
Berridge, M.J. (1993). Inositol trisphosphate and calcium signaling. Nature 361, 315-325[CrossRef][Medline].
Bray, D. (1992). Cell Movements, New York: Garland Pub.
Chun, J. (1999). Lysophospholipid receptors: implications for neural signaling. Crit. Rev. Neurobiol. 13, 151-168[Medline].
Chun, J., Contos, J.J.A., and Munroe, D. (1999). A growing family of receptor genes for lysophosphatidic acid (LPA) and other lyso-phospholipids (LPs). Cell Biochem. Biophys. 30, 213-242[Medline].
Chun, J., and Jaenisch, R. (1996). Clonal cell lines produced by infection of neocortical neuroblasts using multiple oncogenes transduced by retroviruses. Mol. Cell. Neurosci. 7, 304-321[CrossRef][Medline].
Condeelis, J., and Vahey, M. (1982). A calcium- and pH-regulated protein from Dictyostelium discoideum that cross-links actin filaments. J. Cell Biol. 94, 466-471[Abstract/Free Full Text].
Contos, J.J.A., and Chun, J. (1998). Complete cDNA sequence, genomic structure, and chromosomal localization of the LPA receptor gene, lp_A1/vzg-1/Gpcr26. Genomics 51, 364-378[CrossRef][Medline].
Contos, J.J.A., Ishii, I., and Chun, J. (2000). Lysophosphatidic acid receptors. Mol. Pharmacol. 58, 1188-1196[Abstract/Free Full Text].
Fukushima, N., Ishii, I., Contos, J.A., Weiner, J.A., and Chun, J. (2001). Lysophospholipid receptors. Annu. Rev. Pharmacol. Toxicol. 41, 507-534[CrossRef][Medline].
Fukushima, N., Kimura, Y., and Chun, J. (1998). A single receptor encoded by vzg-1/lp_A1/edg-2 couples to G proteins and mediates multiple cellular responses to lysophosphatidic acid. Proc. Natl. Acad. Sci. USA 95, 6151-6156[Abstract/Free Full Text].
Fukushima, N., Weiner, J.A., and Chun, J. (2000). Lysophosphatidic acid (LPA) is a novel extracellular regulator of cortical neuroblast morphology. Dev. Biol. 228, 6-18[CrossRef][Medline].
Fukushima, N., Weiner, J.A., Kaushal, D., Contos, J.J.A., Rehen, S.K., Kingsbury, M.A., Kim, K.-Y., and Chun, J. (2002). Lysophosphatidic acid influences the morphology, and motility of young, postmitotic cortical neurons. Mol. Cell. Neurosci. 20, 271-282[CrossRef][Medline].
Gohla, A., Harhammer, R., and Schultz, G. (1998). The G-protein G₁₃ but not G₁₂ mediates signaling from lysophosphatidic acid receptor via epidermal growth factor receptor to Rho. J. Biol. Chem. 273, 4653-4659[Abstract/Free Full Text].
Habara, Y., and Kanno, T. (1991). Dose-dependency in spatial dynamics of [Ca²⁺]c in pancreatic acinar cells. Cell Calcium 12, 533-542[CrossRef][Medline].
Hecht, J.H., Weiner, J.A., Post, S.R., and Chun, J. (1996). Ventricular zone gene-1 (vzg-1) encodes a lysophosphatidic acid receptor expressed in neurogenic regions of the developing cerebral cortex. J. Cell Biol. 135, 1071-1083[Abstract/Free Full Text].
Hemmings, L., Kuhlman, P.A., and Critchley, D.R. (1992). Analysis of the actin-binding domain of $alpha$ -actinin by mutagenesis and demonstration that dystrophin contains a functionally homologous domain. J. Cell Biol. 116, 1369-1380[Abstract/Free Full Text].
Hirose, M., Ishizaki, T., Watanabe, N., Uehata, M., Kranenburg, O., Moolenaar, W.H., Matsumura, F., Maekawa, M., Bito, H., and Narumiya, S. (1998). Molecular dissection of the Rho-associated protein kinase p160ROCK-regulated neurite remodeling in neuroblastoma N1E-115 cells. J. Cell Biol. 141, 1625-1636[Abstract/Free Full Text].
Ishii, I., Contos, J.J., Fukushima, N., and Chun, J. (2000). Functional comparisons of the lysophosphatidic acid receptors, LP_A1/VZG-1/EDG-2, LP_A2/EDG-4, and LP_A3/EDG-7 in neuronal cell lines using a retrovirus expression system. Mol. Pharmacol. 58, 895-902[Abstract/Free Full Text].
Jalink, K., Eichholtz, T., Postma, F.R., van Corven, E.J., and Moolenaar, W.H. (1993). Lysophosphatidic acid induces neuronal shape changes via a novel, receptor-mediated signaling pathway: similarity to thrombin action. Cell Growth Differ. 4, 247-255[Abstract].
Jalink, K., van Corven, E.J., Hengeveld, T., Morii, N., Narumiya, S., and Moolenaar, W.H. (1994). Inhibition of lysophosphatidate- and thrombin-induced neurite retraction and neuronal cell rounding by ADP ribosylation of the small GTP-binding protein Rho. J. Cell Biol. 126, 801-810[Abstract/Free Full Text].
Janmey, P.A. (1994). Phosphoinositides and calcium as regulators of cellular actin assembly and disassembly. Annu. Rev. Physiol. 56, 169-191[Medline].
Jockusch, B.M., Haemmerli, G., and In Albon, A. (1983). Cytoskeletal organization in locomoting cells of the V2 rabbit carcinoma. Exp. Cell Res. 144, 251-263[CrossRef][Medline].
Katada, T., Oinuma, M., and Ui, M. (1986). Two guanine nucleotide-binding proteins in rat brain serving as the specific substrate of islet-activating protein, pertussis toxin. Interaction of the $alpha$ -subunits with $beta$ $gamma$ subunits in development of their biological activities. J. Biol. Chem. 261, 8182-8191[Abstract/Free Full Text].
Keenan, C., and Kelleher, D. (1998). Protein kinase C and the cytoskeleton. Cell. Signal. 10, 225-232[CrossRef][Medline].
Kimura, Y., Schmitt, A., Fukushima, N., Ishii, I., Kimura, H., Nebreda, A.R., and Chun, J. (2001). Two novel Xenopus homologs of mammalian LP_A1/EDG-2 function as lysophosphatidic acid receptors in Xenopus oocytes and mammalian cells. J. Biol. Chem. 276, 15208-15215[Abstract/Free Full Text].
Kozma, R., Sarner, S., Ahmed, S., and Lim, L. (1997). Rho family GTPases and neuronal growth cone remodelling: relationship between increased complexity induced by Cdc42Hs, Rac1, and acetylcholine and collapse induced by RhoA and lysophosphatidic acid. Mol. Cell. Biol. 17, 1201-1211[Abstract].
Kranenburg, O., Poland, M., van Horck, F.P., Drechsel, D., Hall, A., and Moolenaar, W.H. (1999). Activation of RhoA by lysophosphatidic acid and G $alpha$ 12/13 subunits in neuronal cells: induction of neurite retraction. Mol. Biol. Cell 10, 1851-1857[Abstract/Free Full Text].
Laemmli, U.K. (1970). Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227, 680-685[CrossRef][Medline].
Letourneau, P.C. (1996). The cytoskeleton in nerve growth cone motility and axonal pathfinding. Perspect. Dev. Neurobiol. 4, 111-123[Medline].
Manning, T.J.J., and Sontheimer, H. (1997). Bovine serum albumin and lysophosphatidic acid stimulate calcium mobilization and reversal of cAMP-induced stellation in rat spinal cord astrocytes. Glia 20, 163-172[CrossRef][Medline].
Matsudaira, P. (1994). Actin crosslinking proteins at the leading edge. Semin. Cell Biol. 5, 165-174[Medline].
Meerschaert, K., De Corte, V., De Ville, Y., Vandekerckhove, J., and Gettemans, J. (1998). Gelsolin and functionally similar actin-binding proteins are regulated by lysophosphatidic acid. EMBO J. 17, 5923-5932[CrossRef][Medline].
Moolenaar, W.H. (1995). Lysophosphatidic acid signaling. Curr. Opin. Cell Biol. 7, 203-210[CrossRef][Medline].
Moolenaar, W.H. (1999). Bioactive lysophospholipids and their G protein-coupled receptors. Exp. Cell Res. 253, 230-238[CrossRef][Medline].
Moolenaar, W.H., Kranenburg, O., Postma, F.R., and Zondag, G.C. (1997). Lysophosphatidic acid: G-protein signaling and cellular responses. Curr. Opin. Cell Biol. 9, 168-173[CrossRef][Medline].
O'Connor, K.L., Nguyen, B.-K., and Mercurio, A.M. (2000). RhoA function in lamellae formation, and migration is regulated by the $alpha$ 6 $beta$ 4 integrin, and cAMP metabolism. J. Cell Biol. 148, 253-258[Abstract/Free Full Text].
Pavalko, F.M., Otey, C.A., Simon, K.O., and Burridge, K. (1991). $alpha$ -Actinin: a direct link between actin and integrins. Biochem. Soc. Trans. 19, 1065-1069[Medline].
Ren, X., and Schwartz, M. (2000). Determination of GTP loading on Rho. Methods Enzymol. 325, 264-272[Medline].
Ridley, A.J., and Hall, A. (1992). The small GTP-binding protein rho regulates the assembly of focal adhesions and actin stress fibers in response to growth factors. Cell 70, 389-399[CrossRef][Medline].
Seymour, R.M., and Berry, M. (1975). Scanning and transmission electron microscope studies of interkinetic nuclear migration in the cerebral vesicles of the rat. J. Comp. Neurol. 160, 105-125[CrossRef][Medline].
Shahrestanifar, M., Fan, X., and Manning, D.R. (1999). Lysophosphatidic acid activates NF- $kappa$ B in fibroblasts. A requirement for multiple inputs. J. Biol. Chem. 274, 3828-3833[Abstract/Free Full Text].
Sobue, K. (1993). Actin-based cytoskeleton in growth cone activity. Neurosci. Res. 18, 91-102[CrossRef][Medline].
Sobue, K., and Kanda, K. (1989). $alpha$ -Actinins, calspectin (brain spectrin or fodrin), and actin participate in adhesion and movement of growth cones. Neuron 3, 311-319[CrossRef][Medline].
Thastrup, O., Cullen, P., Drobak, B., Hanley, M., and Dawson, A. (1990). Thapsigargin, a tumor promoter, discharges intracellular Ca²⁺ stores by specific inhibition of the endoplasmic reticulum Ca²⁺-ATPase. Proc. Natl. Acad. Sci. USA 87, 2466-2470[Abstract/Free Full Text].
Tigyi, G., Fischer, D.J., Sebok, A., Marshall, F., Dyer, D.L., and Miledi, R. (1996). Lysophosphatidic acid-induced neurite retraction in PC12 cells: neurite-protective effects of cyclic AMP signaling. J. Neurochem. 66, 549-558[Medline].
Tokuue, Y., Goto, S., Imamura, M., Obinata, T., Masaki, T., and Endo, T. (1991). Transfection of chicken skeletal muscle $alpha$ -actinin cDNA into nonmuscle and myogenic cells: dimerization is not essential for $alpha$ -actinin to bind to microfilaments. Exp. Cell Res. 197, 158-167[CrossRef][Medline].
Toullec, D., et al. (1991). The bisindolylmaleimide GF 109203X is a potent and selective inhibitor of protein kinase C. J. Biol. Chem. 266, 15771-15781[Abstract/Free Full Text].
Uehata, M., et al. (1997). Calcium sensitization of smooth muscle mediated by a Rho-associated protein kinase in hypertension. Nature 389, 990-994[CrossRef][Medline].
Waites, G., Graham, I., Jackson, P., Millake, D., Patel, B., Blanchard, A., Weller, P., Eperon, I., and Critchley, D. (1992). Mutually exclusive splicing of calcium-binding domain exons in chick $alpha$ -actinin. J. Biol. Chem. 267, 6263-6271[Abstract/Free Full Text].
Weiner, J.A., and Chun, J. (1999). Schwann cell survival mediated by the signaling phospholipid lysophosphatidic acid. Proc. Natl. Acad. Sci. USA 96, 5233-5238[Abstract/Free Full Text].
Weiner, J.A., Fukushima, N., Contos, J.J.A., Scherer, S.S., and Chun, J. (2001). Regulation of Schwann cell morphology and adhesion by receptor-mediated lysophosphatidic acid signaling. J. Neurosci. 21, 7069-7078[Abstract/Free Full Text].
Youssoufian, H., McAfee, M., and Kwiatkowski, D.J. (1990). Cloning and chromosomal localization of the human cytoskeletal $alpha$ -actinin gene reveals linkage to the beta-spectrin gene. Am. J. Hum. Genet. 47, 62-71[Medline].

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