The Internal Phosphodiesterase RegA Is Essential for the Suppression of Lateral Pseudopods during Dictyostelium Chemotaxis

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Vol. 11, Issue 8, 2803-2820, August 2000

The Internal Phosphodiesterase RegA Is Essential for the Suppression of Lateral Pseudopods during Dictyostelium Chemotaxis

Deborah J. Wessels,^* Hui Zhang,^* Joshua Reynolds,^* Karla Daniels,^* Paul Heid,^* Sijie Lu, Adam Kuspa, Gad Shaulsky, William F. Loomis,^§ and David R. Soll^*

^*Department of Biological Sciences, University of Iowa, Iowa City, Iowa 52242 Department of Biochemistry and Molecular Biology, Baylor College of Medicine, Houston, TX 77030 Department of Molecular and Human Genetics, Baylor College of Medicine, Houston, TX 77030 ^§Department of Biology, University of California, San Diego, La Jolla, CA 92037

Submitted March 9, 2000; Revised May 23, 2000, and June 9, 2000; Accepted June 12, 2000
Monitoring Editor: Henry R. Bourne

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Dictyostelium strains in which the gene encoding the cytoplasmic cAMP phosphodiesterase RegA is inactivated form small aggregates.This defect was corrected by introducing copies of the wild-typeregA gene, indicating that the defect was solely the consequenceof the loss of the phosphodiesterase. Using a computer-assistedmotion analysis system, regA mutant cells were found to show little sense of direction duringaggregation. When labeled wild-type cells were followed in a fieldof aggregating regA cells, they also failed to move in an orderly direction, indicatingthat signaling was impaired in mutant cell cultures. However,when labeled regA cells were followed in a field of aggregating wild-type cells,they again failed to move in an orderly manner, primarily in thededuced fronts of waves, indicating that the chemotactic responsewas also impaired. Since wild-type cells must assess both theincreasing spatial gradient and the increasing temporal gradientof cAMP in the front of a natural wave, the behavior of regA cells was motion analyzed first in simulated temporal waves inthe absence of spatial gradients and then was analyzed in spatialgradients in the absence of temporal waves. Our results demonstratethat RegA is involved neither in assessing the direction of aspatial gradient of cAMP nor in distinguishing between increasingand decreasing temporal gradients of cAMP. However, RegA is essentialfor specifically suppressing lateral pseudopod formation duringthe response to an increasing temporal gradient of cAMP, a necessarycomponent of natural chemotaxis. We discuss the possibility thatRegA functions in a network that regulates myosin phosphorylationby controlling internal cAMP levels, and, in support of that hypothesis,we demonstrate that myosin II does not localize in a normal mannerto the cortex of regA cells in an increasing temporal gradient ofcAMP.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Chemotactically directed motility is a characteristic of many cell types including phagocytic neutrophils and nerve growthcones (Tamagnone et al., 1999; Hong et al., 2000; Servant et al.,2000). It also plays an essential role in the development of Dictyosteliumwhere it can be analyzed genetically (Parent and Devreotes, 1996;Jin et al., 2000). When Dictyostelium amoebae are washed freeof nutrients and are dispersed on a substratum saturated withbuffered salts solution, they undergo a complex and carefullyorchestrated process of aggregation driven by chemotaxis to cAMP(Konijn et al., 1967; Tomchik and Devreotes, 1981). Within a fewhours after the initiation of development, a few cells begin tospontaneously emit pulses of cAMP. Cells in the immediate environmentrespond to each pulse of cAMP in two ways. First, they surge towardthe source of the primary signal, and, second, they relay thesignal by releasing more cAMP (Shaffer, 1962; Alcantara and Monk,1974; Tomchik and Devreotes, 1981; Devreotes et al., 1983). Withina few minutes extracellular phosphodiesterase activity removesthe signal by extracellular hydrolysis of the cAMP (Franke andKessin, 1992). These characteristics result in spreading, nondissipatingwaves of cAMP that direct cells over large distances into aggregationcenters.

The shape of each outwardly radiating cAMP wave is roughly symmetric (Tomchik and Devreotes, 1981; Devreotes et al., 1983),and the average period between waves during the natural aggregationprocess is approximately 7 min (Alcantara and Monk, 1974; Devreotes,1982). As a cell encounters the front of a wave, it experiencesan increasing spatial gradient of cAMP and an increasing temporalgradient of cAMP, while in the back of each wave a cell experiencesa decreasing spatial gradient of cAMP and a decreasing temporalgradient of cAMP (Figure 1A) (Soll, 1989; Soll et al., 1993).If cells simply use the spatial information of a wave in chemotaxis,we are faced with a paradox (Soll, 1989; Soll et al., 1993). SinceDictyostelium amoebae are capable of changing direction withina few seconds in response to cAMP released from a micropipette(Gerisch et al., 1975), and since both the front and the backof each wave takes > 60 s to cross them, why do they not movetoward the aggregation center as they encounter the front of eachwave and then move away from the aggregation center as they encounterthe back of the wave? This would lead to no net movement towardthe aggregation center over time. The answer lies in the mannerin which the temporal dynamics of each wave regulate cell behaviorand has been revealed by analyzing cell behavior in temporal gradientsof cAMP (Van Haastert, 1983; Fisher et al., 1989) and by simulatingthe temporal dynamics of a natural wave in the absence of a spatialgradient (Varnum et al., 1985; Varnum-Finney et al., 1987a; Wesselset al., 1992; Wessels and Soll, unpublished observations).

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Figure 1. The behavior of a cell in the different portions of a natural cAMP wave propagated in a population of developing Dictyostelium discoideum amoebae (A) and in a temporal wave of cAMP generated in a perfusion chamber in the absence of a spatial gradient of cAMP (B). The cyclic behavior of cells responding to natural waves of cAMP is similar to that of cells responding to the different portions of a simulated wave (a, b, c, and d) in all aspects but one. While cells in the front of a natural wave all move in a persistent manner in the same direction (i.e., toward the aggregation center, the source of the wave), cells in the front of a simulated temporal wave move in a persistent manner in all directions. From the similar cyclic pattern of behaviors, the portions of the natural wave were deduced from the known portions of the in vitro generated temporal wave (Wessels et al., 1992

). The heavy arrow in (A) indicates the direction of spreading of the nondissipating, relayed natural wave. The bold print in point b refers to the one difference between the behavior in a natural wave and the behavior in a simulated temporal.

After the first in a series of simulated temporal waves, Dictyostelium amoebae exhibit the following behavior in each successivewave (Figure 1B). When cAMP first starts to rise in the increasingphase of a wave, cells extend numerous pseudopods for a shortperiod of time, then one pseudopod assumes anterior dominance(i.e., assumes the role of leading edge). Then, as the concentrationcontinues to rise, cells become highly polar and crawl in a persistentmanner because of the suppression of lateral pseudopod formation(Figure 1). At the peak of a simulated temporal wave, cells stopdirectional locomotion, and, in the back of the wave when theconcentration of cAMP decreases with time, the cells extend lateralpseudopods in random directions, become relatively unpolarized,and move in a nonpersistent, nondirectional manner, making littlenet progress in any direction (Figure 1B). This complex behaviorcycle is repeated in each successive simulated temporal wave.The behavior of cells in natural waves appears to be similar inmost respects to that in simulated temporal waves (Figure 1) (Wesselset al., 1992). As the deduced front of a natural wave crossesthem and the concentration of cAMP rises, cells move in a persistentmanner as they do in the front of a simulated temporal wave. Again,persistent translocation is facilitated by the suppression oflateral pseudopod formation. At the deduced peak of a naturalwave, cells stop directional locomotion, and, in the deduced backof a natural wave, cells make little net progress in any direction.The only difference in behavior is directionality. In the frontof a natural wave, all cells move toward the aggregation center,the source of cAMP waves (Figure 1A), while in a simulated temporalwave, cells move in all directions since they do not receive spatialcues (Figure 1B).

The gene regA encodes a cytoplasmic phosphodiesterase that is activated by phosphorelay from a histidine on RdeA to an aspartatein the N-terminal portion of RegA (Shaulsky et al., 1996; Changet al., 1998; Shaulsky et al., 1998; Thomason et al., 1998). TheregA gene is expressed shortly after the initiation of development,and its product regulates the internal concentration of cAMP throughoutdevelopment (Shaulsky et al., 1998). There is evidence that theMAP kinase ERK2 also controls the activity of RegA by threoninephosphorylation in the C-terminal portion of RegA (S. Lu, C. Su,B. Wang, A. Shaulsky, E. Snaar-Jagalska, and A. Kuspa; submitted).ERK2 is activated when extracellular cAMP binds to the surfacereceptor CAR1 (Maeda et al., 1996). ERK2 appears to inhibit RegAactivity leading to accumulation of internal cAMP (S. Lu et al.,submitted). The cAMP protein kinase PKA then would be expectedto be activated. It has been proposed that PKA activity leadsindirectly to the inhibition of both CAR1 and ERK2 activity, suchthat RegA can be reactivated and reduce the internal concentrationof cAMP (Laub and Loomis, 1998). This network would lead to periodicoscillations in PKA activity as external cAMP waves transientlystimulate CAR1. The model predicts that RegA plays an essentialrole in generating regular periodic cAMP pulses and the entrainmentof cells such that they signal in unison. Previous studies haveindicated that ERK2 also is involved in both signaling and responsesto cAMP (Segall et al., 1995; Wang et al., 1998). We have nowfound that RegA plays a role in the motile response of cells tonatural waves ofcAMP.

Using computer-assisted motion analysis systems (Soll, 1995; Soll and Voss, 1998; Wessels, 1998; Soll, 1999), the behaviorof regA cells has been quantitatively analyzed when cells are perfusedwith buffer in a chamber that excludes chemotactic signaling (Wesselset al., 1989), in natural waves of cAMP (Wessels et al., 1992),in a gradient chamber in which spatial gradients of cAMP are generatedin the absence of the temporal dynamics of waves (Zigmond, 1977;Varnum and Soll, 1984; Varnum-Finney et al., 1987b), and in temporalgradients of cAMP generated in a perfusion chamber in which spatialgradients of cAMP are not established (Varnum et al., 1985; Varnum-Finneyet al., 1987b; Wessels et al., 1992). Our results demonstratethat RegA is not involved in reading the direction of a spatialgradient or in assessing the direction (increasing versus decreasing)of a temporal wave, and responding with chemokinetic stimulationin the increasing phase. However, RegA is necessary for the suppressionof lateral pseudopod formation in response to an increasing temporalgradient of cAMP, and its role appears to be in the regulationof myosin II localization in the cortex. In the absence of pseudopodsuppression in the front of a wave, chemotaxis in an aggregationterritory isdisrupted.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Origin of Control, regA, and regA-Rescued Strains

The isolation and original characterization of the regA strain from the parent strain AX4 by saturation restriction enzyme-mediatedintegration (REMI) were described in a previous report (Shaulskyet al., 1996). The regA-rescued strain was isolated by the following procedure. GenomicDNA from the 5'-end of regA was prepared as a 1094-bp HindIII-SalIfragment, and genomic DNA from the 3' end was prepared as a 1014-bpHindIII-NcoI fragment, both from the original REMI clone-out vectorpSTB6-Hind (Shaulsky et al., 1996). An SalI-NcoI cDNA fragmentwas prepared from a full-length REGA cDNA clone (Shaulsky et al.,1998). A plasmid backbone containing the neoresistance cassettewas prepared as a 4730-bp HindIII fragment from pDdGa115(H⁺) (Harwood and Drury, 1990). The fragments were cloned sequentiallyinto the backbone vector using standard recombinant DNA techniques.All of the fragment junctions were verified by sequencing andby Southern analysis. The complete sequence of regA has been depositedin GenBank (U60170). The resulting plasmid pregAxNeo was transformedinto regA cells by CaPO₄ precipitation and glycerol shock (Nellen and Firtel,1985), and transformants were selected using 10 µg/ml G418 inHL5 medium (Cocucci and Sussman, 1970). BlasticidinS (4 µg/ml)also was added in the medium to maintain the insertion mutationin the native regA locus. G418 and blasticidin-resistant transformantswere cloned on SM agar in association with Klebsiella aerogenes.Individual colonies were randomly selected and regrown in HL5medium plus G418 and blasticidin. Total cellular protein fromeach strain was prepared, and Western blot analysis was performedwith polyclonal anti-RegA antibodies (Thomason et al., 1998) totest for the presence of the RegA protein. One such strain, pregAxNeo/regA,was chosen and used for the studies reported here. Estimates fromsemiquantitative Western analyses indicated that this strain produced1.5-fold wild-type levels of RegA (our unpublished results). Inaddition, the regA-rescued strain was tested for the restoration of large aggregatesize (aggregates of regA are abnormally small), streaming (regA cells do not stream), and normal levels of cAMP after cAMP stimulation(regA cells have threefold to fourfold more cAMP than Ax4 cells) (Luet al.,2000).

Maintenance and Development of Control, regA, and Rescued Strains

Spores of the parental Ax4 strain, the regA strain, and the rescued regA strain were frozen in 10% glycerol at $-$ 80°C and were reconstitutedevery 3 wk for experimental purposes (Sussman, 1987). Cells weregrown in suspension in HL-5 medium to a density of 2 × 10⁶ cells/ml. To initiate development, cells were washed free ofnutrients in basic salts solution (BSS; 20 mM KCl, 2.5 mM MgCl₂,and 20 mM KH₂PO₄ [pH 6.4]) and then were dispersed onto filterpads as a smooth carpet at a density of 5 × 10⁶ cells/cm² (Soll, 1987). For motility experiments in buffer, and in spatialand temporal gradients of cAMP (see below), cells were harvestedat the ripple stage, which represents the onset of aggregation(Soll, 1979).

Analysis of Cell Motility in a Spatial Gradient of cAMP

Cells were washed from filters at the ripple stage of development and were deposited on the bridge of a Plexiglas gradientchamber as a dilute suspension in BSS according to methods previoiuslydescribed (Varnum and Soll, 1984; Varnum-Finney et al., 1987b).One trough of the chamber was immediately filled with BSS aloneand the other with BSS containing 10⁶ M cAMP, and the chamber was covered with a coverslip. The chamberwas incubated undisturbed on the stage of a Leitz (Leica Microsystems,Deerfield, IL) microscope equipped with brightfield optics anda 25× objective for 5-7 min to allow the gradient to become establishedand for cells to reestablish adherence and motile behavior. Fieldsof cells were videorecorded through a DAGE camera (DAGE-MTI, MichiganCity, IN) onto half-inch videotape for 10 min. The images wereprocessed using the camera control panel so that the cells appeareddark against a lighter background, thus allowing automatic edgedetection by the threshold method in 2D DIAS (Soll, 1995; Solland Voss, 1998). Video images were digitized at a rate of 15 frames/minonto the hard disk of a PowerComputing PowerTower Pro 225 computer(Apple Computer, Cupertino, CA) equipped with a Data Translationframegrabber board (Data Translation Inc., Marlboro, MA) and 2D-DIASsoftware (Soll, 1995; Soll and Voss, 1998). Only those cells crawlingat average velocities >3 µm/min for the 10-min period of analysiswere used to compute motility parameters. This represented >80%of cells on the chamber bridge for all three celltypes.

Analysis of Cell Motility in Buffer or in Simulated Temporal Waves of cAMP

To monitor the behavior of individual amoebae in buffer, 1 ml of a dilute suspension of cells at the ripple stage of developmentwas inoculated into a Sykes-Moore chamber (Bellco Glass, Vineland,NJ) as previously described (Varnum et al., 1985; Varnum-Finneyet al., 1987a). This perfusion chamber consisted of a rubber o-ringsandwiched between two glass coverslips within a stainless steelholder. Immediately after inoculation, the chamber was closed.Cells were allowed to settle and to adhere to the coverslip, aprocess that took ~5 min. The chamber then was inverted and placedon the stage of a Leitz upright microscope fitted with a long-rangecondenser. The chamber had one inlet and one outlet port at oppositesides of the metal ring wall. The tube to the inlet port was connectedto a reservoir containing the proper perfusion solution, and thetube to the outlet port was connected to a peristaltic pump setto a flow rate of 4 ml/min, so that chamber volume was replacedevery 15 s. For behavior in the absence of cAMP, cells were continuouslyperfused with BSS. To simulate temporal waves of cAMP, amoebaewere perfused with increasing, then decreasing, temporal step-gradientsof cAMP. In each experiment, amoebae first were perfused with5 ml of BSS solution lacking cAMP and then with 2 ml of freshBSS solution containing 7.8 × 10⁹ M cAMP. Then at 30-s intervals, 2 ml of a new solution was perfusedthat contained twice the cAMP concentration of the preceding solution.After perfusion with 2 ml of the buffer solution containing 10⁶ M cAMP (the peak concentration), the last step in the increasinggradient, the decreasing temporal gradient was simulated by introducing2-ml increments of BSS into the reservoir, each containing one-halfthe previous concentration of cAMP. The second, third, and fourthwaves were created using this same technique. The rapid flow rateand round shape of the chamber prevented the establishment ofspatial gradients of cAMP, and this was verified using fluorescentdyes. Fields of cells were videorecorded, and the cell imageswere processed and digitized as describedabove.

Analysis of Cell Motility in Natural Waves of cAMP

For analyzing behavior in natural aggregation territories, exponentially growing cells were washed free of nutrients and weresuspended in BSS at 2.4 × 10⁶ cells/ml according to methods previously described (Escalanteet al., 1997) with one exception. Two milliliters of the cellsuspension were added to the uncoated surface of a 35-mm tissueculture dish. Dishes were used without an agar coating becausethe particular strain employed (Ax4) adhered more securely tothe plastic surface than previous strains used for similar studies(Wessels et al., 1992; Escalante et al., 1997). After a 30-minincubation period, the cells had settled and had attached to thesurface. One milliliter of fluid was carefully withdrawn, andthe dish was placed on the stage of a Zeiss ICM 405 inverted microscope(Carl Zeiss, Thornwood, NY). Images were recorded through a HamamatsuC-2400 Newvicon camera (Hamamatsu Photonics, Hamamatsu City, Japan)using a 10 X objective and brightfield optics. Video images weredigitized at a rate of 6 frames/min as describedabove.

Labeling Cells with DiI and Mixing with Unlabeled Cells

To test the behavior of mutant cells in wild-type aggregation territories, regA cells were stained with the vital dye DiI (Molecular Probes,Eugene OR), mixed with a majority of unlabeled Ax4 cells, andmotion analyzed during aggregation. To label regA amoebae, 8 × 10⁶ cells in the log-phase of growth were pelleted, washed threetimes in BSS, and then resuspended in 2 ml of labeling solution(3% dextrose in BSS). A 4 mM stock solution of DiI in ethanolwas stored at $-$ 20°C. Before use, the stock solution of DiI waspassed through a 5-µm filter, and then 25 µl of the filtrate wasadded to the cell suspension to give a final concentration of0.05 mM DiI. regA cells were incubated in the DiI solution for 30 min, washed threetimes in BSS, and then mixed with unlabeled Ax4 cells at a ratioof 1:4. Ax4 cells were prestarved for 2 h before mixing so thatthe developmental timing of the two strains would be comparable(see Results section). Labeled and unlabeled cells were mixed,and 5 × 10⁶ cells were dispersed evenly on the surface of a 35-mm Petri dish.The Petri dish was placed on the stage of an Axiovert 100STV Zeissmicroscope (Carl Zeiss) and examined with a NORAN laser scanningconfocal microscope (NORAN, Middleton, WI). The same procedurewas used to test the behavior of wild-type cells in mutant aggregationterritories. Transmitted light images were continuously collectedthrough a transmitted light detector. Settings in Oz IntervisionSoftware (NORAN) were selected so that cells were exposed to laserlight for 0.5 s every 20 s with a laser intensity of 20%, at anexcitation of 568 nm and an emission $>=$ 590 nm. Transmitted andfluorescent images were collected through the photomultipliertube, were mixed and averaged using the Intervision Software,and then were saved on the hard drive in Silicon Graphics (SGI,Inc., Mountain View, CA) movie format. The transmitted and fluorescentimaging format functioned automatically throughout aggregation.SGI movies acquired with the NORAN system were converted to QuickTime format, and labeled cells were outlined using 2D-DIAS (seebelow).

Two Dimensional Computer-Assisted Analysis of Cell Motility

Digitized images of cells in buffer, in spatial gradients of cAMP, in simulated temporal waves of cAMP, or in natural wavesof cAMP were image processed, and the perimeters of cells wereautomatically outlined using the grayscale threshold option ofDIAS (Soll, 1995; Soll and Voss, 1998). Perimeters were convertedto beta-spline replacement images, which were used to computethe position of the centroid (Soll, 1995; Soll and Voss, 1998).Motility parameters were computed from centroid positions, anddynamic morphology parameters were computed from the perimetercontours of the replacement images according to formulas derivedand discussed in a previous report (Soll, 1995). In brief, "instantaneousvelocity" of a cell in frame n was computed by drawing a linefrom the centroid in frame n $-$ 1 to the centroid in frame n +1 and then dividing the length of the line by twice the time intervalbetween analyzed frames. "Directional change" was computed asthe direction in the interval (n $-$ 1, n) minus the direction inthe interval (n, n + 1). If directional change was >180°, it wassubtracted from 360°, resulting in a positive value between 0°and 180°. "Positive flow" was computed from difference pictures(Soll, 1995; Soll and Voss, 1998). To generate a difference picture,the cell perimeter in frame n was superimposed on the perimeterin frame n $-$ 1. The regions in the image in frame n not overlappingthe image in frame n $-$ 1 were considered "expansion zones" andwere color-coded green. The regions in the image in frame n $-$ 1 not overlapping the image in n were considered "contractionzones" and were color-coded red. The summed area of expansionzones divided by the total cell area in frame n times 100 representspositive flow in microns squared per interval time. "Maximum length"was computed as the longest chord between any two points alongthe perimeter, and "maximum width" as the longest chord perpendicularto maximum length. "Roundness" was computed by the formula 100× 4 $pi$ (area/perimeter squared). "Convexity" and "concavity" werecomputed by first drawing line segments connecting the verticesof the final cell shape. The angles of turning from one segmentto the next were measured. Counterclockwise turns were positive,and clockwise turns were negative. Convexity was computed as theabsolute value of the sum of positive turn angles, in degrees,and concavity was computed as the absolute value of the sum ofnegative turn angles. The "chemotactic index" was computed asthe net distance moved to the source of chemoattractant dividedby the total distance moved in the time period. "Percent positivechemotaxis" was computed as the proportion of the cell populationexhibiting a positive chemotacticindex.

Quantitative Immunolocalization of Myosin II in the Front of a Temporal Wave

To quantitate the distribution of myosin II in cells responding to the front of a simulated temporal wave of cAMP, Ax4 orregA cells were washed from filters at the ripple stage of development,were inoculated into a Sykes-Moore chamber, and were treated withsuccessive simulated temporal waves of cAMP, as detailed above.Midway through the third wave, the chamber was perfused with freshlyprepared 4% paraformaldehyde in PBS supplemented with 0.01% saponin.The cells were fixed for 10 min at room temperature. The chamberwas disassembled, and the coverslip was gently washed with TBS.Before immunostaining, antigen retrieval was performed using TargetRetrieval Solution (DAKO Corp., Carpinteria, CA) in a steamerand processed for 20 min in retrieval solution heated to 90°C.The solution and coverslips were removed from heat and were allowedto cool to room temperature before TBS rinsing. Nonspecific bindingwas blocked with 10% normal donkey serum in PBS. To localize myosinII, cells were incubated with rabbit antimyosin II antibody (1/1000),a generous gift from Dr. Arturo De Lozanne (University of Texasat Austin, Austin, TX) in PBS containing 10% donkey serum for45 min at 37°C. After extensive PBS rinsing, cells were stainedwith FITC-labeled donkey anti-rabbit antibody (1/200) (JacksonImmunoResearch, West Grove, PA) for 30 min at room temperature.Coverslips were rinsed and mounted using Gelvatol (Monsanto Corp.,St Louis, MO) with azide. Images were captured with a Zeiss 510laser-scanning confocal microscope (LSM 510; Central MicroscopyFacility, University of Iowa). For quantitative analysis, an initialimage was scanned using an Ax4 cell, and the parameters were optimized.These same parameters then were used for each subsequent scan.The same scanning parameters were used for regA cells. LSM 510 software was used to convert 2D optical slicesinto filled "Pseudo 3D" projections in which the z-axis representsthe grayscale intensity distribution over the scannedarea.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Rescue of regA Phenotypes by the Wild-Type Gene

Strains in which regA is disrupted form only small aggregates and develop into misshapen fruiting bodies (Shaulsky et al.,1996, 1998). To be sure that this aberrant behavior was directlyrelated to the loss of RegA, we transformed mutant cells witha vector carrying the regA coding region and its upstream regulatorysequence (see MATERIALS AND METHODS). Stable transformants formedlarge aggregation streams and developed into normal fruiting bodies,while the parent regA strain failed to stream and formed small aberrant fruiting bodiesin the midst of aggregates that did not complete morphogenesis(Figure 2). These results demonstrate that the aberrant behavioralphenotype of regA cells can be attributed to the specific loss of regA. The defectin aggregation could result from reduced motility, defective chemotacticsignaling, or a defective behavioral response to cAMP waves.

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Figure 2. The late aggregation territories (A-C) and fruiting bodies (D-F) of Ax4, regA, and regA-rescued cell cultures, respectively. Note the abnormally small size (B) as well as the absence of streams (B) and the incomplete or small fruiting bodies (E) in regA cultures. Note the reexpression of normal traits, including large aggregates and streaming (C) and large fruiting bodies (F) in regA-rescued cultures.

Basic Motility of regA Cells

The velocity of individual cells changes during the early developmental stages of Dictyostelium (Varnum et al., 1985; Shuttet al., 1995). The instantaneous velocity of cells is low at thebeginning of the developmental program, increases to a peak valueat the onset of aggregation, and then decreases through the laterstages of development. During the preaggregative period, the instantaneousvelocity of individual Ax4 cells continually increased from 2to 10 µm/min at the onset of aggregation, then decreased duringthe later stages of aggregation (Figure 3A). Motility was developmentallyregulated in a similar manner in regA cells (Figure 3B). Aggregation began 2 h earlier in regA cultures than in Ax4 cultures, and peak instantaneous velocityalso was achieved 2 h earlier (compare Figure 3, A and B). Therefore,in the comparative studies that follow, cells of the three teststrains (Ax4, regA, and regA-rescued) were obtained from developing cultures at the observedonset of aggregation (i.e., the ripple stage; Soll, 1979).

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Figure 3. Motility is developmentally regulated in regA cells (B) as it is in parental Ax4 cells (A). Cells were removed from the respective developing cultures at the noted intervals, were dispersed on the wall of a perfusion chamber, and average instantaneous velocity were measured over a 10-min period. The mean instantaneous velocity at each time point was computed from the average instantaneous velocities of 20 amoebae at each time point.

The quantitative parameters of motility of individual Ax4 and regA cells translocating in buffer without added cAMP were similar.Ax4 and regA cells translocated with mean instantaneous velocities (±SD) of10.8 ± 3.9 and 11.1 ± 4.2 µm/min, respectively, and with meandirectional change parameters (±SD) of 44.3° ± 7.9° and 51.0°± 6.3° per minute, respectively (Table 1). Mean cell shape parameters,including mean maximum length and mean roundness, were also similar(Table 1). These results indicate that RegA plays no role inthe basic motile behavior of Dictyostelium amoebae translocatingin the absence of a chemoattractant.

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Table 1. A computer-assisted comparison of the motile behavior of regA and Ax4 cells perfused with buffer in the absence of chemoattractant

Both the Generation and Response to Natural Waves of cAMP Are Impaired in regA Cells

To assess the behavior of cells in natural aggregation territories, Ax4 or regA cells were dispersed on the surface of tissue culture dishes,and the behavior of neighboring cells was continually videorecordedthrough the aggregation process in submerged cultures (Wesselset al., 1992; Escalante et al., 1997). In Figure 4,A-C, the timeplots of instantaneous velocity and corresponding centroid tracksare presented for three representative Ax4 amoebae that were neareach other in the same localized area of an aggregation territory.For these three independent, neighboring cells, the instantaneousvelocity plots contained sharp peaks with average periods (±SD)between peaks of 5.8 ± 1.3, 5.9 ± 1.5, and 5.9 ± 1.9 min, respectively.The velocity peaks have been interpreted to represent periodsof rapid, persistent movement in the front of consecutive naturalwaves, while velocity troughs have been interpreted to representthe behavior at the peak and in the back of the consecutive waves(Figure 1A) (Wessels et al., 1992). Average peak instantaneousvelocities (±SD) for the three representative cells were 5.3 ±0.9, 5.7 ± 1.0, and 5.5 ± 1.1 µm/min, respectively, and the ratiosof average peak to trough velocity values were 2.4, 2.3, and 2.2,respectively (Figure 4, A-C). Portions of the centroid track ofeach cell representing peak and trough velocities were easilydistinguished by the expanded and contracted distances, respectively,between centroids (Figure 4, A-C). More importantly, through sequentialwaves each Ax4 cell moved in a directed manner toward the sameaggregation center. Similar behavior was observed for nine additionalsets of spatially associated Ax4 amoebae in the process of aggregation.

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Figure 4. Time plots of instantaneous velocity and corresponding centroid tracks of three representative Ax4 cells (A-C) and three representative regA cells (D-F) responding to natural waves generated in their own homogeneous aggregation territories. Arrows along Ax4 centroid tracks represent the direction toward the common aggregation center (source of waves), and "t" represents the trough regions in the respective velocity plots. In regA territories, there was no single direction reflecting the source of the wave, hence no arrows have been included in panels D-F. Pd, average period between velocity peaks; pk, average peak velocity; trh, average trough velocity; p/t, ratio of average peak to average trough velocities. Values are presented as average ± SD. Velocity plots were smoothed 10 times with Tukey windows of 10, 20, 40, 20, and 10.

In Figure 4, D-F, time plots of instantaneous velocity and corresponding centroid tracks are presented for three aggregatingregA amoebae that were near each other in the same localized areaof a culture dish. As in the case of Ax4 cells, the time plotsof instantaneous velocity were cyclic, but the period and peakvelocities were less regular. For these three regA cells, the average periods (±SD) were 3.9 ± 0.8, 5.2 ± 1.9, and3.9 ± 0.2 min, respectively. In repeat experiments, more variabilitywas evident in the average period between velocity peaks of regA cells than in those of wild-type Ax4 cells. In fact, within eachof the 10 sets of spatially localized Ax4 amoebae undergoing aggregationthat were motion analyzed, there was no significant differencein periodicity. This result suggests that regA cells may not be responding to the same source of chemotacticsignals even when they are in close spatialproximity.

The average trough values of instantaneous velocity for the three regA cells (Figure 4, D-F) were similar to those for the three Ax4cells (Figure 4, A-C). However, the average peak values were consistentlylower for the three regA cells than those for the three Ax4 cells. While the peak to troughratio of the three representative regA cells was 1.4 in each case, the ratios of the three Ax4 cellswere 2.4, 2.3, and 2.2, respectively. These results suggest thatin a developing culture, regA cells appear to release cAMP and respond to it, but they failto achieve the high peak velocities of Ax4cells.

In contrast to the relatively straight paths taken by Ax4 cells (Figure 4, A-C), regA cells zig-zagged and back-tracked (Figure 4, D-F). For the threespatially localized regA cells that were motion analyzed, no single direction reflectingthe position of an aggregation center could be discerned. Thisaberrant behavior no doubt accounts for the very small aggregatesformed by regA cells (Shaulsky et al., 1998). In addition, while the periodsof translocation representing peak and trough velocities wereeasily distinguished¹ in centroid tracks of Ax4 cells (Figure 4, A-C), they were notas easily distinguished in centroid tracks of regA cells (Figure 4, D-F), primarily because the peak velocitiesof regA cells were in many cases depressed and the tracks were not aspersistent and directional during periods of increasedvelocity.

The aberrant behavior of regA cells could be the result of an abnormality in the genesis of waves, an abnormality in the responseto waves, or both. To distinguish between these three possibilities,experiments were performed in which DiI-labeled cells of one celltype were mixed with a majority of unlabeled cells of the othertype. The fluorescent dye DiI did not affect motility, since centroidtracks and velocity plots of labeled and unlabeled AX4 cells mixedat a ratio of 1 to 4 were not significantly different (our unpublishedresults).

In Figure 5A, the time plot of instantaneous velocity and the centroid track are presented for a representative unlabeledregA cell in an aggregation territory that contained 20% DiI-labeledAx4 cells and 80% unlabeled regA cells. The velocity plot of the regA cell was generally depressed, and the centroid track was compressedand directionless (Figure 5A) in a manner that was similar tothat of regA cells in homogeneous regA territories (Figure 4, D-F). The peak velocities in the timeplots of labeled Ax4 cells in the same regA territory (Figure 5, B and C) were higher than those of regA cells, more similar in fact to those of Ax4 cells in Ax4 territories(Figure 4, A-C). However, the centroid tracks of these Ax4 cells,although expanded, exhibited no discernable directionality (Figure5, B and C). These results, obtained in several repeat experiments,suggest that although cAMP appears to be released in a pulsatilemanner in territories containing 80% regA cells and 20% Ax4 cells, the signals are not propagated froma single aggregation center even in a restricted part of the territory.Since regA cells make up the majority of cells in these territories, itappears they may not be entrained to relay the signal coordinately.In addition, the suppressed velocity peaks in instantaneous velocityplots of regA cells (Figure 5A), when compared with those of Ax4 cells (Figure5, B and C) in regA territories, suggest an aberrant behavioral response by regA cells to cAMP signals.

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Figure 5. The behavior of a representative unlabeled regA cell (A) and two DiI-labeled Ax4 cells (B and C) in the same area of a developing regA culture, and the behavior of a representative unlabeled Ax4 cell (D) and two DiI-labeled regA cells (E and F) in the same Ax4 aggregation territory. Arrows in (D-F) indicate the direction toward the aggregation center (the source of waves) of the territory in which the three representative cells are located. pd, pk, trh, and p/t and the smoothing regime are described in the legend to Figure 3.

To test whether the response of regA cells to a natural cAMP wave was defective, the behavior of DiI-labeled regA cells was analyzed in territories of unlabeled Ax4 cells in whichthe two cell types were mixed at a ratio of 1:4, respectively.In Figure 5D, the time plot of instantaneous velocity and thecentroid track are presented for an unlabeled Ax4 cell in themixed aggregation territory. The time plot was similar to thatof unlabeled Ax4 cells in homogeneous Ax4 territories (Figure4, A-C) and included high average peak velocity values at regularintervals and a high peak-to-trough velocity ratio. In addition,the centroid track included discernable peak and trough velocityperiods and a high degree of net directionality toward the aggregationcenter (Figure 5D). In contrast, the velocity plots of two labeledregA cells (Figure 5, E and F) in close spatial association with theAx4 cell followed in Figure 5D were depressed. Peak velocitiesand the ratios of average peak-to-trough velocities were similarto those of regA cells in homogeneous regA territories (Figure 4, D-F). In addition, the centroid trackswere compressed and lacked direction. Zig-zagging was rampant(Figure 5, E and F), demonstrating that the regA cells did not respond with persistent translocation to the frontof natural waves of cAMP. These results, obtained in several repeatexperiments, demonstrate that regA cells are defective not only in generating coordinated cAMP waves,but also in responding to natural cAMPwaves.

Chemotaxis in Spatial Gradients of cAMP

The aberrant behavior of regA cells in natural cAMP waves propagated by Ax4 cells could be because of their inability to reada spatial gradient and/or their inability to respond to the temporaldynamics of the wave (Wessels et al., 1992). To distinguish betweenthese possibilities, we first tested whether regA cells could assess the direction of a spatial gradient of cAMPin the absence of the temporal dynamics of the wave and whetherthey could crawl in a directed manner up the gradient. Ax4 orregA cells were dispersed on the Plexiglas bridge of a gradient chamber(Zigmond, 1977; Varnum and Soll, 1984; Varnum-Finney et al., 1987b).To one trough, BSS solution alone was added (the "sink"), andto the other trough, BSS containing 10⁶ M cAMP was added (the "source") (Varnum and Soll, 1984; Varnum-Finneyet al., 1987b). Cells were incubated for 5 min to allow the gradientto develop (Shutt et al., 1998; Shutt and Soll, 1999) and to allowthe cells to reestablish polarity and motility. Their behaviorthen was recorded and motion analyzed. There were no significantdifferences among Ax4, regA, and regA-rescued cells in instantaneous velocity and positive flow ina spatial gradient of cAMP, and although the directional changeparameter was slightly higher in regA cells, it was not significantly different (Table 2). There wasalso no significant difference in mean morphology parameters ina spatial gradient, including maximum length, maximum width, area,roundness, convexity, and concavity (Table 2). More importantly,the majority of regA cells (93%) exhibited a positive chemotactic index, as did Ax4(90%) and regA-rescued (85%) cells (Table 2). The mean chemotactic index (CI)(±SD) of regA cells was +0.48 ± 0.28, which represents a relatively strongresponse. However, this value was lower than the mean CI (±SD)of either Ax4 cells (+0.61 ± 0.34) or regA-rescued cells (+0.67 ± 0.34). This difference was statisticallysignificant (Table 2). A histogram of CIs for the three cellsrevealed that fewer regA cells achieved top-end chemotactic indices (i.e., $>=$ 0.80) thaneither Ax4 or regA-rescued cells (Figure 6). While 36 and 40% of Ax4 and regA-rescued cells exhibited CIs of $>=$ 0.80, only 14% of regA cells exhibited CIs in this high-end category.

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Table 2. 2D motility and dynamic morphology parameters of wild-type (Ax4), regA, and regA-rescued cells in a spatial gradient of cAMP

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Figure 6. Histogram of CIs indicates that regA cells are less efficient at attaining high-end CIs (i.e., >0.80-1.00) than either Ax4 or regA-rescued cells.

To investigate further the behavioral basis of this difference, the perimeter tracks of chemotaxing Ax4 and regA cells with the highest CIs were compared. The perimeter tracksof the highest end Ax4 cells were highly persistent in the directionof the gradient, with few lateral pseudopod projections and virtuallyno significant turns (Figure 7A). The perimeter tracks of thehighest end regA cells were also persistent in the direction of the gradient butexhibited more frequent lateral pseudopod activity and more frequentchanges in direction (see arrows, Figure 7B). Together, theseresults demonstrate that regA cells are capable of assessing the direction of a spatial gradientof cAMP and moving in a directed manner, but they are not as efficientas Ax4 cells in suppressing lateral pseudopod formation and turns,a behavioral characteristic that increases proportionately withincreasing CI (Varnum-Finney et al., 1987b).

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Figure 7. Computer-generated tracks of the three analyzed Ax4 cells and the three analyzed regA cells in a spatial gradient of cAMP exhibiting the highest chemotactic indices. Small arrows in (B) point to turns initiated by lateral pseudopods.

Responses to Temporal Gradients of cAMP

Since the abnormal behavior exhibited by regA cells in a natural wave does not appear to result from a defect in their abilityto read the spatial gradient, it may instead be because of anincapacity to respond to the temporal dynamics of a natural wave,in particular the increasing phase in the front of the wave. Totest this possibility, cells were subjected to sequential temporalwaves of cAMP that approximated the temporal dynamics of naturalwaves in the absence of established spatial gradients (Varnumet al., 1985; Varnum-Finney et al., 1987a). In Figure 8A, theaverage instantaneous velocities of 10 representative Ax4 cellsand 10 representative regA cells are plotted while they were subjected to four temporalwaves of cAMP generated in sequence. As previously reported forwild-type cells (Varnum et al., 1985), the instantaneous velocityof parental Ax4 and regA cells remained low throughout the first wave. In subsequent waves,instantaneous velocity increased through the first half of eachincreasing phase, reflecting positive chemokinesis, and then decreasedto a depressed level through the peak and the decreasing phase(Figure 8A). The chemokinetic responses shown by regA cells were not significantly different from those of Ax4 cells,indicating that regA cells recognize temporal changes in cAMP (increasing versus decreasingconcentration with time) and respond by altering their instantaneousvelocity accordingly, in particular by positive chemokinesis inthe front of each of a series of simulated waves, beginning withthe second wave. However, the centroid tracks of regA cells in simulated waves were abnormal. The centroid tracks ofAx4 cells contained expanded stretches representing rapid, persistent,and directional translocation in the first two-thirds of the increasingphase of waves 2, 3, and 4, and intervening compacted stretchesrepresenting depressed rates of translocation at the peak andin the decreasing phase of each wave (Figure 8, B and C). In contrast,the centroid tracks of regA cells were far more compressed, with less persistent stretches,and included constant backtracking, which indicated a higher frequencyof sharp turns (Figure 8, D and E). The persistent and directionalphases of translocation exhibited by Ax4 cells in the first halfto two-thirds of the increasing phase of simulated waves 2, 3,and 4 were, therefore, absent in the regA tracks.

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Figure 8. The behavior of Ax4 and regA cells in temporal gradients of cAMP generated in the absence of spatial gradients that mimic the temporal dynamics of natural waves of cAMP. (A) The average instantaneous velocity and estimated cAMP concentration are shown during simulated waves. Note that neither Ax4 nor regA cells increase instantaneous velocity in the front of the first simulated wave (Varnum et al., 1985

). Instantaneous velocity, measured at 1-min intervals, represents the average of 10 Ax4 cells and 10 regA cells, respectively. (B and C) The centroid tracks of Ax4 cells responding to sequential simulated temporal waves of cAMP. (D and E) The centroid tracks of regA cells responding to sequential simulated temporal waves of cAMP. 1, 2, 3, and 4 (in B and C), sequential wave number; i, increasing gradient; d, decreasing gradient. Velocity plots in (A) were smoothed 10 times with Tukey windows of 10, 20, 40, 20, and 10.

Suppression of Lateral Pseudopod Formation as cAMP Increases with Time

Wild-type cells suppress lateral pseudopod formation during rapid translocation in the increasing phase of each simulatedtemporal wave to achieve a high degree of persistent and directionaltranslocation (Varnum-Finney et al., 1987a). Since regA cells turned frequently during this phase of a temporal wave,it seemed reasonable to hypothesize that they might be impairedin this response. To test this possibility, we recorded cellsresponding to the increasing phases of consecutive temporal waves2, 3, and 4 at high magnification to directly measure the frequencyof lateral pseudopod formation. Lateral pseudopods were definedas protrusions representing $>=$ 5% of the total area of the cell,which extended at an angle of $>=$ 45° from the translocation axisof the cell (Wessels et al., 1996). The translocation axis wasdetermined by a line drawn between the centroids of the cell inthe present frame and the frame 16 s earlier. While Ax4 cellsrarely formed lateral pseudopods in the increasing phases of temporalcAMP waves (0.7 ± 0.7 per front of wave), regA cells formed lateral pseudopods at a frequency five times higher(3.6 ± 1.2 per front of wave) (Table 3). The difference in thefrequency of lateral pseudopod formation is evident in perimeterplots and difference pictures of representative Ax4 and regA cells responding to the first two-thirds of a simulated temporalwave of cAMP (Figure 9). While Ax4 cells maintained a highly polarmorphology with rare lateral extensions (Figure 9, A and C), regA cells continually extended lateral pseudopods at high frequency(Figure 9, B and D). These results demonstrate that although regA cells recognize temporal changes in cAMP (increasing versus decreasingconcentration with time) and respond by altering their instantaneousvelocity, they do not suppress lateral pseudopod formation duringthe increasing phases of simulated temporal waves, resulting ina loss of persistent, directional translocation.

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Table 3. Number of lateral pseudopods formed by Ax4 and regA cells in the increasing phases of simulated temporal waves of cAMP

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Figure 9. Behavior of Ax4 and regA cells in the first 3 min of the increasing phase of a temporal wave of cAMP that mimics the temporal dynamics of a natural wave of cAMP. (A and B) Perimeter tracks of Ax4 and regA cells, respectively. (C and D) Difference pictures of a representative Ax4 and regA cell, respectively. Black filled areas represent expansion zones, and hatched areas represent contraction zones of difference pictures. Arrows in difference pictures represent direction vectors drawn through the centroids of the earlier and later perimeter image in each difference picture.

regA Cells Are Defective in Myosin II Localization in the Front of the Wave

The cortical localization of myosin II has been implicated in the suppression of lateral pseudopods (Wessels et al., 1988;Spudich, 1989; Wessels and Soll, 1990; Stites et al., 1998; Chungand Firtel, 1999). We, therefore, tested whether myosin II localizationto the cell cortex was defective in regA cells responding to the front of a simulated temporal wave. Ax4or regA cells were fixed on the glass wall of a perfusion chamber midwaythrough the third in a series of simulated temporal waves andwere stained for myosin II. In Figure 10, confocal images are presentedof four representative Ax4 cells (Figure 10, A-D) and four representativeregA cells (Figure 10, E-H). Each image represents an optical section0.4 µm above the substratum. The great majority of Ax4 cells wereelongate, while all of the regA cells exhibited a flatter, more complex contour, reflecting continuedlateral pseudopod formation. In every Ax4 cell (20 were analyzed),myosin was highly localized to the cortex of the posterior three-fourthsof the elongate cell body. Localization was extremely weak inthe cortex of anterior pseudopods and was weak throughout theinterior cytoplasm. regA cells were analyzed at the same scanning parameters as Ax4 cells.In every regA cell (20 were analyzed), myosin II was distributed throughoutthe cytoplasm, rather than localized specifically to the cortex.In a minority of regA cells, some cortical localization was evident (e.g., Figure 10H),but in all of these cases, staining was still distributed throughoutthe interior of the cell, except for the nucleus. In Figure 11,the differences in the distribution of myosin II in the frontof a simulated temporal cAMP wave are demonstrated by mappingthe grayscale intensity distributions over the scanned areas ofa representative Ax4 cell (Figure 11A) and a representative regA cell (Figure 11B).

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Figure 10. Mysoin II distribution in representative Ax4 cells (A-D) and regA cells (E-H) midway in the front of a simulated temporal wave of cAMP (the third in a series). Images were taken 0.4 µm off the substratum, using identical confocal scanning parameters for comparison. Small arrows indicate the polarity of the cell interpreted from the parallel DIC image of each cell. The scale bar represents 10 µm.

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Figure 11. A "pseudo-3D" projection in which the z-axis represents the intensity distribution of stained myosin II over the scanned area of a representative Ax4 (Figure 10C) and a representative regA cell (Figure 10G) midway in the front of a simulated temporal wave of cAMP. Scale bar represents 10 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In the original characterization, it was demonstrated that regA cultures formed small aggregates and did not form streams, suggestingthat cell motility or some other aspect of the aggregation processwas defective (Shaulsky et al., 1996, 1998). We found that mutantcells showed the same developmentally regulated increase in cellmotility at the time of aggregation as wild-type cells, and theylocomoted in buffer in the absence of a chemotactic signal withmotility parameters similar to those of Ax4 cells. These resultsindicated, therefore, that RegA played no role in the basic motilebehavior of cells in the absence of a chemotacticsignal.

RegA Is Necessary for Normal Wave Propagation

To identify the defect in regA aggregation, we first considered whether the production and propagation of chemotactic wavesof cAMP might be impaired. RegA is the cAMP phosphodiesterasethat reduces the internal concentration of cAMP after the activationof adenylyl cyclase by the G protein-coupled receptor CAR1 (Shaulskyet al., 1996, 1998; Thomason et al., 1998). As such, the lossof RegA might be expected to result in higher intracellular cAMPlevels and in persistently high PKA activity. Analysis of thenetwork controlling adenylyl cyclase activity predicts that theloss of RegA would preclude the entrainment of cells such thatthey would no longer propagate cAMP signals coordinately (Lauband Loomis, 1998). The behavior of Ax4 cells in a predominantlyregA aggregation territory clearly showed that signaling was aberrant.Although regA cells appeared to release cAMP signals, they were not propagatedfrom a single source even within a small, restrictedterritory.

RegA Is Not Necessary for Assessing the Direction of a Spatial Gradient of cAMP

We next tested whether regA cells were capable of chemotaxing in a spatial gradient of cAMP. Mutant and wild-type cells weremotion analyzed in a gradient chamber where a steep cAMP gradientis generated by 8 min and then flattens due to diffusion (Shuttet al., 1998; Shutt and Soll, 1999). Peak chemotactic stimulationoccurs between ~4 and 14 min (D.S. Shutt and D.R. Soll, unpublishedobservations). regA cells exhibited a relatively strong chemotactic response in thesespatial gradients of cAMP. Over 90% of regA cells chemotaxed up the spatial gradient, roughly the same proportionas Ax4 cells. The chemotactic index (±SD) of regA cells was +0.48 ± 0.28, which is comparable to the chemotacticindices of several other normal strains of Dictyostelium (Shuttet al., 1995; Cox et al., 1996) but is lower than that of theparent Ax4 strain. The difference between the chemotactic indexof Ax4 and regA cells was because of a depression in high-end chemotactic indices(i.e., those $>=$ +0.80). A comparison of the perimeter tracks ofAx4 and regA cells with the highest chemotactic indices revealed that chemotaxingregA cells were not as efficient as Ax4 cells in suppressing lateralpseudopod formation (Varnum-Finney et al., 1987b). However, theresults clearly demonstrated that RegA is not essential for readingthe direction of a spatial gradient and for responding with directed,persistent movement up thegradient.

RegA Is Not Necessary for Recognizing Temporal Changes in cAMP Concentration and Adjusting Instantaneous Velocity Accordingly

Except for the initial decision on direction at the onset of the front of a natural wave, which must be extracted from thespatial dynamics of the wave, all subsequent behavior appearsto be dictated by the temporal dynamics of the wave (Figure 1)(Wessels et al., 1992). We, therefore, next tested whether regA cells responded normally to the temporal dynamics of a naturalwave by simulating temporal waves in a round chamber in whichspatial gradients of cAMP are not established (Varnum et al.,1985; Varnum-Finney et al., 1987a). We found that mutant cellscould distinguish between an increasing versus decreasing temporalgradient of cAMP and adjusted their velocity accordingly, mostnotably through a positive chemokinetic response in the frontof the wave. However, a comparison of the centroid tracks of cellsin these perfusion experiments showed that regA cells made many more turns than wild-type cells and moved chaoticallyduring the increasing phases of the waves. Therefore, althoughthe chemokinetic response was intact, chemotaxis wasaberrant.

RegA Is Necessary for Suppressing Lateral Pseudopod Formation in Increasing Temporal Gradients of cAMP

The reason that regA cells failed to show persistent movement in the increasing phase of a temporal wave of cAMP became obviouswhen cells were viewed at higher magnification. While Ax4 cellsexposed to an increasing temporal gradient of cAMP suppressedlateral pseudopod formation, regA mutant cells did not. The frequency of lateral pseudopod formationwas fivefold higher in mutant cells than in wild-type cells. Sucha defect would have severe consequences during natural aggregation.Normal cells select a direction at the beginning of a wave thenmove for $>=$ 1 min in a relatively blind manner toward the aggregationcenter in the front of the wave, primarily because lateral pseudopodformation is suppressed by the increasing temporal gradient ofcAMP (Figure 1) (Wessels et al., 1992). During the peak and thedecreasing phase of a wave, they make no net progress in any direction(Wessels et al., 1992). Therefore, the net progress of cells towardthe aggregation center is accomplished in the limited period inthe first two-thirds of a wave of cAMP (Wessels et al., 1992).The suppression of lateral pseudopod formation that occurs immediatelyafter the directional decision appears to be essential for directionaltranslocation toward the aggregation center. Loss of that capacityin regA cells makes them veer off course and disruptsaggregation.

Mechanism of Lateral Pseudopod Suppression

Several cytoskeletal elements have been demonstrated to affect the frequency of lateral pseudopod formation (Wessels et al.,1988; Wessels and Soll, 1990; Wessels et al., 1991; Titus et al.,1992; Wessels et al., 1996). The most dramatic of these is myosinII. Deletion of the myosin II heavy chain gene, mhcA, (DeLozanneand Spudich, 1987; Manstein et al., 1989) or the inhibition ofthe expression of mhcA by an antisense construct (Knecht and Loomis,1987) resulted in the loss of polarity and the extension of pseudopodsat equal frequency around the cell perimeter (Wessels et al.,1988; Wessels and Soll, 1990). Because lateral pseudopod formationwas normally suppressed in the posterior half of a crawling cell(Varnum-Finney et al., 1987a, b) and myosin II had been demonstratedto be localized there (Yumura and Fukui, 1985), the behavioralphenotype of mhcA null mutants was interpreted to indicate thatmyosin II localized in the cell cortex played a direct role inthe suppression of lateral pseudopod formation (Wessels et al.,1988; Spudich, 1989; Wessels and Soll, 1998). Several additionalobservations supported this interpretation. First, it was demonstratedthat mhcA null mutant cells exhibited a decrease in cortical tension(Pasternak et al., 1989). Second, conversion of the three mappedthreonine phosphorylation sites in the myosin II heavy chain tailto alanines in mutant 3XALA resulted in myosin overassembly (Luck-Vielmetteret al., 1990; Egelhoff et al., 1993), increased cortical tension(Egelhoff et al., 1996), and the abnormal bifurcation of anteriorpseudopods during chemotaxis, presumably as a result of increasedcortical tension (Stites et al., 1998). Since phosphorylationleads to the dissociation of myosin II filaments in vitro (Kuczmarskiand Spudich, 1980; Cote and McCrea, 1987; Ravid and Spudich, 1989),it was suggested that in a normal crawling cell, carefully orchestratedphosphorylation-dephosphorylation of myosin II leads to the disassembly-reassembly,respectively, of myosin II necessary for relocalization in theprocess of cellular translocation and turning. The movement ofmyosin II into the cortex, where it polymerizes into thick filamentsthat generate cortical tension (Pasternak et al., 1989), mustbe a delicately regulated, cyclical, and localized event thatinvolves the activation of specific kinases and phosphorylasesof both myosin heavy chain and light chain (Tan et al., 1992).Our data suggest that RegA may be an essential component in theregulation of this balance in response to temporal gradients ofcAMP.

Since RegA is not necessary for reading the direction of a spatial gradient or recognizing a temporal gradient of cAMP, onecan assume that the changes in the concentration of intracellularcAMP effected by the deactivation and reactivation of RegA phosphodiesteraseactivity in the front and back, respectively, of a natural waveare not involved. However, since RegA is essential for suppressinglateral pseudopod formation in response to an increasing temporalgradient of cAMP, one can assume that the periodic changes inintracellular cAMP that result from oscillations in the networkthat controls RegA activity are coupled to changes in the cellcortex. The myosin II staining experiments that we have performeddemonstrate that regA plays a role in regulating the corticallocalization of myosin II in the front of a temporal wave of cAMP.The high level of myosin II localization in the cell cortex posteriorto the leading edge of an Ax4 amoeba responding to an increasingtemporal gradient of cAMP, and the concomitant suppression oflateral pseudopod formation suggest that the high level of corticaltension generated by the localization of myosin II acts as a suppressorof lateral pseudopod formation. The severe reduction in corticallocalization in reg cells in the front of a temporal wave of cAMP demonstrates thatRegA plays a direct role in regulating the disassembly-assemblyof myosin II leading to cortical localization in response to anincreasing temporal waves of cAMP. Since RegA appears to be themajor regulator of intracellular cAMP, which in turn regulatesthe level of PKA activity (Wang and Kuspa, 1997; Loomis, 1998;Aubry and Firtel, 1999), it is reasonable to suggest that RegAfunctions through PKA to regulate myosin localization throughphosphorylation. Although the pathway from PKA to relevant myosinII kinases has not been elucidated, recent evidence suggests thatPAKa, a p21-activated Ser/Thr protein kinase, functions as aninhibitor of myosin heavy chain kinase (Chung and Firtel, 1999).The deletion of PAKa has been demonstrated to affect the directionof cellular translocation and to affect the suppression of lateralpseudopod formation in a chemotactic gradient, effects that arequite similar to those resulting from the deletion of RegA. Thesteps in the pathway beginning with RegA and ending in the phosphorylation/dephosphorylationof myosin II must now beidentified.

	ACKNOWLEDGMENTS

The authors are indebted to J. Swails for help in assembling the manuscript. The research was supported by National Institutesof Health grants HD-18577 (D.R.S.) and GM52359 (A.K.), and byNational Science Foundation grant No. 9728463 (W.F.L.). The authorsacknowledge use of the W.M. Keck Dynamic Image Analysis Facilityat the University of Iowa funded by the W.M. KeckFoundation.

	FOOTNOTES

Correspondingauthor.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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