Correspondence to Diane L. Barber: barber{at}itsa.ucsf.edu
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Introduction |
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Efficient chemotaxis entails two distinct but functionally linked components: directional sensing and polarity (Devreotes and Janetopoulos, 2003). Directional sensing, defined as the ability of a cell to perceive a signal and set up an initial internal asymmetry in the direction of the incoming signal, requires an asymmetric production of the lipid second messenger phosphatidylinositol 3,4,5-trisphosphate (PI(3,4,5)P3) but is independent of actin polymerization. Polarity reinforces internal asymmetries and translates them into relevant morphological changes to execute efficient movement toward chemoattractants. In contrast to directional sensing, localized actin polymerization, regulated predominantly by the localized activation of Rho family low molecular weight GTPases, is a conserved core determinant in cell polarity from yeasts to mammalian cells (Etienne-Manneville and Hall, 2002; Nelson, 2003). In chemotaxing neutrophils, actin polymerization at the leading edge of the cell acts in a positive feedback loop to reinforce localized production of PI(3,4,5)P3 and activation of the Rho family GTPase Rac (Weiner et al., 2002; Srinivasan et al., 2003), and in motile cells, including chemotaxing Dictyostelium cells, de novo actin polymerization is a predominant driving force for membrane protrusions or pseudopodia (Condeelis et al., 1990; Pollard and Borisy, 2003).
A long-speculated but poorly understood mechanism promoting de novo actin polymerization during cell movement is an increase in intracellular pH (pHi). Earlier work on the fertilization of sea urchin eggs (Begg and Rebhun, 1979) and the acrosomal reaction in Echinoderm sperm cells (Tilney et al., 1978) indicates that transient increases in pHi are necessary for actin polymerization and that artificially increasing pHi in the absence of external cues triggers F-actin formation. In Ascaris sperm cells, a pHi gradient that is higher at the front of the cell than at the rear is necessary for cell polarity and a leading edge assembly of cytoskeletal filaments (King et al., 1994; Italiano et al., 1999), even though motile Ascaris sperm cells lack actin and cytoskeletal filaments consist of bundled fibers of major sperm protein. In mammalian fibroblasts (Denker and Barber, 2002) and sperm cells (Wang et al., 2003), H+ efflux by plasma membrane isoforms of the Na-H exchanger, NHE, is necessary for directed migration and motility, respectively, although effects of NHE on actin polymerization have not been determined. In Dictyostelium cells, increases in pHi promote chemotaxis (Van Duijn and Inouye, 1991); however, the ion transport mechanisms regulating pHi homeostasis in Dictyostelium have not been clearly defined.
We now report that a Dictyostelium Na-H exchanger, DdNHE1, is necessary for cell polarity and chemotaxis in response to cAMP. DdNHE1 is developmentally expressed with chemotactic competence, is predominantly localized at the front of chemotaxing cells, and is necessary for cAMP-induced increases in pHi. In response to a gradient of cAMP, Ddnhe1-null (Ddnhe1) cells are unable to polarize, retain a rounded morphology, and extend pseudopodia around the cell periphery. Although Ddnhe1 cells retain directional sensing of cAMP, chemotaxis is impaired. Ddnhe1 cells lack an asymmetric localization of F-actin at the leading edge, and early and late phases of the biphasic increase in actin polymerization are attenuated compared with wild-type Ax2 cells. Stable expression of DdNHE1 in Ddnhe1 cells restores a polarized morphology, pseudopodia that are restricted to the leading edge, the kinetics of actin polymerization, and efficient chemotaxis. These findings demonstrate that DdNHE1 is necessary for chemotaxing Dictyostelium cells to regulate localized actin polymerization and to adopt a polarized phenotype.
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Results |
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Development of Ddnhe1 cells was not impaired, as indicated by similar expression in Ax2 and Ddnhe1 cells of developmentally regulated genes. Northern blot analysis confirmed that 6-h-stage Ddnhe1 cells expressed the cAMP receptor cAR1 and the G protein 2 subunit G
2 (Fig. 2 C), indicating that they retain the ability to sense the chemoattractant cAMP. Consistent with an established role for mammalian NHE1 in pHi homeostasis, DdNHE1 was necessary for steady-state pHi and for increased pHi in response to cAMP (Fig. 2 D). After 6-h starvation, Ax2 cells had a resting pHi of 6.58 ± 0.05 (n = 7) that increased to 7.14 ± 0.02 by 90 s with 2 µM cAMP. By 6 min, the pHi had returned to basal levels. In contrast, Ddnhe1 cells had a lower resting pHi of 6.48 ± 0.06 (n = 7) that increased to only 6.86 ± 0.07 with cAMP. Hence, DdNHE1 is a predominant, although not exclusive, determinant in the cAMP-induced increase in pHi. Stable expression of DdNHE1-HA in Ddnhe1 cells (Ddnhe1/DdNHE1) restored resting pHi to 6.63 ± 0.07 (n = 3). In response to cAMP, the pHi of 7.29 ± 0.13 in Ddnhe1/DdNHE1 cells was higher and sustained for longer than in Ax2 cells, possibly because DdNHE1, driven by the actin-15 promoter, was overexpressed.
Ddnhe1 cells lack polarity and have impaired chemotaxis
Although DdNHE1 is not necessary for the expression of developmentally regulated genes, chemotaxis in response to cAMP was markedly impaired in all the Ddnhe1 clones generated. Using time-lapse video microscopy to visualize movement of individual cells toward a point source of cAMP delivered by a micropipette, Ax2 cells rapidly developed an elongated, polarized morphology with a defined front in the direction of the point source of cAMP and pseudopodia that were restricted to the leading edge (Fig. 3, A and B; and Video 1, available at http://www.jcb.org/cgi/content/full/jcb.200412145/DC1). When the direction of the point source of cAMP was changed, Ax2 cells executed turns and retained the same leading and trailing edges characteristic of highly polarized cells (Fig. 3 C). In contrast, Ddnhe1 cells failed to adopt a polarized morphology in response to cAMP. They retained a rounded shape lacking a clear front and rear and extended pseudopodia around the entire cell (Fig. 3, A and B; and Video 2). In Ddnhe1/DdNHE1 cells, a polarized morphology and leading edge pseudopodia were restored (Fig. 3, A and B; and Video 3, available at http://www.jcb.org/cgi/content/full/jcb.200412145/DC1).
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Ddnhe1 cells have a sustained increase in membrane-associated PI(3,4,5)P3
cAMP induces a biphasic increase in the abundance of PI(3,4,5)P3 (Chen et al., 2003; Postma et al., 2003), correlating with the biphasic kinetics of actin polymerization. PI(3,4,5)P3 abundance was determined by using a reporter construct of a GFP-tagged pleckstrin homology (PH) domain of the cytosolic regulator of adenylyl cyclase (CRAC; GFP-PHCRAC). The PH domain of CRAC binds PI(3,4,5)P3 and has been used to determine the localization and abundance of PI(3,4,5)P3 in chemotaxing Dictyostelium cells (Parent et al., 1998; Chen et al., 2003; Postma et al., 2003). With a uniform concentration of 2 µM cAMP, Ax2 and Ddnhe1 cells both had biphasic increases in the abundance of membrane-associated (p100 fraction) GFP-PHCRAC (Fig. 6 A); however, there were marked differences. Although the maximal abundance of GFP-PHCRAC in the first phase was similar, in unstimulated Ddnhe1 cells there was significantly more membrane-associated GFP-PHCRAC and hence the fold increase was markedly less (1.2) compared with Ax2 cells (2.2). Additionally, although the kinetics of the second phase was similar, Ddnhe1 cells had markedly more membrane-associated GFP-PHCRAC at all time points.
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The ability of Ddnhe1 cells to acquire asymmetric localization of GFP-PHCRAC suggested DdNHE1 might act downstream of PI(3,4,5)P3 production by phosphatidylinositol 3 (PI3)kinases. This prediction was tested by determining cAMP-induced increases in pHi in the absence and presence of LY294002, which inhibits PI3-kinase activity. In Ax2 cells treated with 30 µM LY294002, the increase in pHi with cAMP was markedly attenuated (Fig. 6 C). In Ddnhe1 cells, the pHi response to cAMP was similar in the absence and presence of LY294002 (unpublished data). Hence, inhibition of PI3-kinase blocks DdNHE1-dependent, but not DdNHE1-independent, increases pHi in response to cAMP.
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Discussion |
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A rapid increase in actin filament assembly is the major driving force for directed cell motility (Condeelis et al., 1990; Pollard and Borisy, 2003). In response to chemoattractant, Dictyostelium cells have a biphasic increase in actin filament assembly (Chen et al., 2003; Park et al., 2004). In Ddnhe1 cells, the rapid (<10 s) first phase is markedly attenuated and the prolonged (30 to 180 s) second phase is largely absent. The first phase of actin polymerization may be essential for establishing morphological asymmetry, and Ddnhe1 cells never develop polarity, regardless of their distance from the chemoattractant source. Where actin polymerization is sustained determines the direction of cell movement, and DdNHE1, which localizes predominantly at the front of polarized cells, is also necessary for limiting F-actin assembly to the leading edge.
Several models have recently been proposed for how the first and second phases of actin polymerization are controlled (Chen et al., 2003; Mouneimne et al., 2004; Park et al., 2004; Sasaki et al., 2004). All models predict that the first phase is independent of PI(3,4,5)P3, and, consistent with this prediction, in Ddnhe1 cells when the first phase of actin polymerization is suppressed the abundance of membrane-associated PI(3,4,5)P3 is normal. In Dictyostelium cells, the first phase of actin polymerization is in part dependent on Rac1B (Park et al., 2004) and Ras proteins (Sasaki et al., 2004). Dictyostelium cells null for RacB have an actin polymerization profile similar to that of Ddnhe1 cells, including 60% decrease in the magnitude of the first phase and a markedly suppressed second phase (Park et al., 2004). In RacB-null cells, but not in Ddnhe1 cells, however, the basal abundance of F-actin is reduced compared with wild-type cells. Another distinction is that RacB-null cells exhibit only a small loss of polarity compared with the marked lack of polarity in Ddnhe1 cells. Dictyostelium Ras proteins also regulate the first phase of actin polymerization and polarity. Although Dictyostelium cells null for RasG have normal polarity and only slightly reduced F-actin in response to cAMP, expression of a dominant inactive DdRasG-S17N in RasG-null mutants to block activation of other Ras proteins results in loss of polarity and
30% reduction in the initial F-actin peak (Sasaki et al., 2004). The role of DdNHE1 in chemotaxis may be distinct from that of RacB or Ras because the phenotype of Ddnhe1 cells is similar to RacB-null cells in F-actin formation, but not in morphological polarity, and similar to RasG-null cells expressing DdRasG-S17N in loss of polarity, but not in the regulation of actin polymerization.
In mammalian cells, the first phase of actin polymerization is preceded by an increase in actin free barbed ends generated by the actin-severing protein cofilin (Mouneimne et al., 2004). Because the actin-severing activity of cofilin is pH-sensitive, cofilin is a possible candidate mediating pH-dependent effects of DdNHE1 on the first phase of actin filament assembly. Increased pHi is necessary to stimulate cofilin activity and to promote the recruitment of cofilin to the leading edge membrane of migrating cells (Bernstein et al., 2000; Bowman et al., 2000). In addition to cofilin, possible targets of DdNHE1-dependent increases in pHi include severin, an actin-severing and -capping protein of the pH-sensitive gelsolin family (Yin et al., 1990; Lamb et al., 1993), and hisactophilin, a pH sensor in Dictyostelium that nucleates actin filaments (Hanakam et al., 1996; Stoeckelhuber et al., 1996).
The second phase of actin polymerization is dependent on the abundance and localization of PI(3,4,5)P3, which are regulated by PI3-kinases and the PI3-phosphatase PTEN (Funamoto et al., 2002; Iijima and Devreotes, 2002). In pi3k1/2 cells and in cells treated with pharmacological inhibitors of PI3-kinases, the second phase of actin polymerization is suppressed but the first phase is retained (Funamoto et al., 2001; Chen et al., 2003). Consistent with previous papers that showed mammalian NHE1 may act downstream of PI3-kinases (Ma et al., 1994; Reshkin et al., 2000), the PI3-kinase inhibitor LY294002 completely blocks the DdNHE1-dependent increase in pHi in response to cAMP. Two predictions may explain why the second phase of actin polymerization is suppressed in Ddnhe1 cells despite increased PI(3,4,5)P3. DdNHE1 could act downstream of PI(3,4,5)P3 in a pathway regulating the second phase of actin polymerization, but, in contrast to a positive feedback loop suggested between actin polymerization and PI(3,4,5)P3 (Weiner et al., 2002; Srinivasan et al., 2003; Sasaki et al., 2004), increased pHi may act in a negative feedback mechanism to limit PI(3,4,5)P3 abundance. Alternatively, DdNHE1 regulates the second phase of actin polymerization independently of PI(3,4,5)P3.
Increased pHi is predicted to be an evolutionarily conserved mechanism necessary for cytoskeletal filament assembly and for motility (Tilney et al., 1978; Begg and Rebhun, 1979; Italiano et al., 1999). Protons do not directly regulate filament assembly (Tilney et al., 1978; Begg and Rebhun, 1979; Italiano et al., 1999) but likely act on pH-dependent filament-binding proteins, such as cofilin and gelsolin. In Dictyostelium cells, a pH-dependent increase in actin polymerization may be a developmentally regulated mechanism to control polarity because DdNHE1 is expressed in chemotactically competent cells but not in vegetative cells. In neutrophil-like HL60 cells, which are chemotactic only after differentiation, NHE1 is expressed in differentiated, but not in undifferentiated, cells (unpublished data). In fibroblasts (Denker and Barber, 2002) and epithelial cells (Klein et al., 2000), NHE1 also is necessary for directional migration but its expression at the plasma membrane is constitutive.
However, whether DdNHE1 regulates chemotaxis exclusively through increased H+ efflux or also by undetermined pH-independent actions remains to be determined. Independently of generating H+ efflux, mammalian NHE1 also anchors actin filaments by binding ERM (ezrin, moesin, and radixin) actin-binding proteins. Actin anchoring by NHE1, but not H+ efflux, is necessary for the bundling of actin stress fibers, localizing NHE1, and tethering actin filaments in specialized membrane domains (Denker and Barber, 2002). Although ERM proteins have not been identified in Dictyostelium, a GST-fusion protein containing the NH2-terminal FERM (protein 4.1 and ERM) domain of moesin binds directly to DdNHE1 (unpublished data), suggesting that binding of a FERM domaincontaining protein might maintain DdNHE1 at the cell front. We predict that the localization of NHE1 and DdNHE1 at the front of motile cells retains a leading edge H+ efflux that is necessary for cell polarity and directional movement.
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Materials and methods |
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Isolation of DdNHE1 and the generation of Ddnhe1 cells
Total RNA was isolated (QIAGEN; UC-100) from wild-type Ax2 cells (provided by C.J. Weijer, University of Dundee, Dundee, Scotland, UK), and RT-PCR was performed on chemotactically competent cells using primers designed to the NH2 and COOH termini of DdNHE1 (AA052201) (5'GGATCCATGAAATTGAACAAAAGTTATATATTAATAGTTG-3' and 5'GGGCCCTTAGTATGGGTAGTCGACTGGGTCGTAAGCACATCATTGGAGTGATGTTGGCTGTTATTG-3', respectively). The COOH terminus primer also contained an HA-epitope tag (underlined), and both primers contained restriction sites (NH2 terminus, BamHI; COOH terminus, SmaI) for cloning. The single PCR product obtained was cloned into the TOPO2.1 cloning vector and subcloned into pB17S, a Dictyostelium expression vector containing a neomycin resistance-conferring cassette, which was used in reconstituting DdNHE1-HA into Ddnhe1 cells.
To generate Ddnhe cells, Ax2 cells were electroporated (Howard et al., 1988) with 0.1 µg of linearized DNA consisting of a blasticidin resistance cassette (Bstr) excised from the Dictyostelium expression vector pUC118 (provided by C.J. Weijer) flanked by regions of DdNHE1. Three different constructs were used for three independent transformations, and individual clones were isolated from each transformation after selection with 10 µg/ml of Blasticidin. Two of the constructs consisted of the Bstr cassette inserted into partial DdNHE1 PCR products of two lengths (1 and 1.5 kb), and the third construct consisted of the Bstr cassette inserted into the 1.5-kb PCR product after excision of
200 bp of DdNHE1. Positive clones were identified by the absence of the DdNHE1 transcript from chemotactically competent cells (Fig. 2 A) and by the presence of a PCR product from genomic DNA by using a primer set consisting of one within the Bstr cassette and another within the genomic region near DdNHE1 (Fig. 2 B).
Surface biotinylation
Starved Ddnhe1/DdNHE1-HA cells and Ax2 cells expressing the PH domain of CRAC fused to GFP (PHCRAC:GFP; provided by P. Devreotes, Johns Hopkins University, Baltimore, MD) were labeled for 30 min on ice with 0.5 mg/ml of biotin in KK2 buffer (EZ-Link Sulfo-NHS-LC-Biotin; Pierce Chemical Co.). Cells were washed in ice-cold KK2 buffer three times and lysed with RIPA buffer (50 mM Tris-HCl, 150 mM NaCl, 1 mM EDTA, 1% NP-40, 0.5% deoxycholate, 0.1% SDS, and protease inhibitors, pH 7.5). Samples were cleared with protein GSepharose (170618-01; Amersham Biosciences) at 4°C. Supernatant was collected and incubated with anti-HA (1:250, 12CA5; Roche), anti-cAR1 (1:250; provided by C. Parent, National Cancer Institute, Bethesda, MD), or anti-GFP (1:250, J108; CLONTECH Laboratories, Inc.) antibodies in the presence of protein GSepharose at 4°C. Sepharose beads were washed three times in ice-cold RIPA Buffer, resuspended in loading buffer, and heated to 100°C for 5 min. Samples were subjected to 10% SDS-PAGE and transferred onto polyvinylidene difluoride membranes. Membranes were blocked with 5% milk and probed with HRP/Streptavidin (1:1000; Vector Laboratories). Data are representative of three independent cell preparations.
Northern blot analysis
Total RNA was isolated from Ax2 and Ddnhe1 cells before starvation and after 3 and 6 h of starvation in PB. 4 µg of total RNA was separated using gel electroporesis, transferred to nylon membranes (Hybond-N+; Amersham Biosciences), and probed with 32P-labeled cAR1 or G2 DNA probes. The membranes were stripped and reprobed for the ribosomal protein IG7 (provided by P. Schaap, University of Dundee) for loading control. Data are representative of Northern blots of two separate RNA preparations.
pHi measurements
pHi was determined in cells loaded with the pH-sensitive fluorescent dye 2',7'-bis-(2-carboxyethyl) 5- (and -6)-carboxyfluorescein (BCECF; Molecular Probes). During starvation of cells for 6 h, 5 µM BCECF was added for the final 30 min, 5 mM caffeine was added for the last 20 min, cells were washed once in PB, resuspended in PB containing 5 mM caffeine, and 5 x 105 cells were added to wells of a 96-well plate. Cells were allowed to attach for 5 min before removing excess cells and submerging the attached cells in 40 µl PB, pH 6.8, containing 5 mM caffeine. In parallel wells, 40 µl PB at pH 5.9, 6.8, and 7.0 containing 5 µM nigericin (Molecular Probes) was added to equalize intracellular and extracellular pH and calibrate fluorescence intensity to pHi. After 15 min, the fluorescence intensity was determined by using a SpectraMax Gemini XS Micro Plate fluorometer (Molecular Devices) at excitation wavelengths of 439 nm (H+-insensitive) and 490 nm (H+-sensitive) with an emission wavelength of 530 nm. A plot of the 490/439 nm ratios against the pH values of the buffers containing nigericin was used to generate a calibration curve from which pHi was determined. To determine pHi in response to cAMP, 2 µM was added to cells and the fluorescence intensity was determined at 45-s intervals. After 6 min, the fluorescence intensity at 439 and 490 nm was determined to confirm that fluorescence intensity at 439 remained constant. Determinations were performed in triplicate, and data were expressed as the mean ± SEM of the indicated independent cell preparations. Inhibition of PI3-kinases was achieved by incubating cells with 30 µM Ly294002 during the caffeine treatment.
Chemotaxis assays and cell tracking
For the analysis of individual cell movement, chemotactically competent cells were basalized for 20 min by adding 5 mM caffeine and then plated at a density of 103 cells/cm2 on nonnutrient 1% phosphate agar plates containing 5 mM caffeine. A micropipette containing 10 µM cAMP was placed next to cells, and images were captured every 30 s using a Spot LCD camera mounted on a microscope (model Axiovert S-100; Carl Zeiss MicroImaging, Inc.) with a 40x Hoffmann modulation objective and operated using Openlab software (Improvision). Cells were tracked using Openlab software, and their coordinates were plotted using Microsoft Excel software.
Phalloidin staining and immunolabeling of DdNHE1
Cells were submerged in PB, allowed to develop on plastic dishes for 8 h, and washed and fixed for 3 min in PB containing 3.7% glutaraldehyde/0.1% Triton X-100. The fixative was removed, and the cells were washed three times in PB. To visualize F-actin, cells were incubated in PB containing rhodamine phalloidin (Molecular Probes) for 1 h at RT. Cells were washed three times in PB and dried briefly, and a drop of Vectashield was added before a glass coverslip was placed over the cells.
For immunolabeling of DdNHE1, Ddnhe/DdNHE1-HA cells were fixed and washed as described in the previous paragraph, followed by blocking in PB containing 5% FBS for 30 min at RT. Cells were labeled for 1 h at RT with anti-HA antibodies (12CA5; Roche) at a dilution of 1:500 in PB containing 2% FBS. Cells were washed three times in PB and incubated at RT in PB containing FITC labeled antimouse IgG (Jackson ImmunoResearch Laboratories) for 1 h. Cells were washed three times in PB and allowed to dry briefly, and a drop of Vectashield was added before a glass coverslip was placed over the cells. Images were captured using an inverted confocal microscope (model LSM500; Carl Zeiss MicroImaging, Inc.) and three-dimensional projection images were generated using LSM software.
Actin polymerization assays
Starved cells basalized with 5 mM caffeine at a density of 2 x 107 cells/ml were stimulated with a uniform concentration of 2 µM cAMP for the indicated times and F-actin was determined as previously described (Steimle et al., 2001). Reactions were stopped by adding fixing buffer (100 mM MES, 5 mM EDTA, 10 mM MgCl2, and 1% Triton X-100, pH 6.8) and incubating for 15 min at RT. Samples were centrifuged for 5 min at 14,000 rpm, the supernatant removed, and cell pellets resuspended in sample loading buffer and boiled for 10 min. Samples were separated by 12% SDS-PAGE, proteins stained with Coomassie blue, and the predominant band, which was actin, quantified by using National Institutes of Health (NIH) image analysis software. Results were expressed as the mean ± SEM of three or more independent experiments.
Membrane-associated PHCRAC:GFP
Ax2 cells and Ddnhe1 cells were transformed with the reporter construct PHCRAC:GFP, which binds PI(3,4,5)P3. Chemotactically competent cells were basalized in 5 mM caffeine and washed two times in PB before stimulation with 2 µM cAMP for the indicated times. Ice-cold buffer (EDTA and Tris HCl, pH 8.0) was added and the cells were sonicated three times for 5 s each time. A postnuclear supernatant fraction was collected (total fraction) and centrifuged at 100,000 g for 20 min at 4°C to obtain particulate (p100) and soluble (s100) fractions. Samples were separated by 10% SDS-PAGE, transferred onto polyvinylidene difluoride membranes, blocked with 5% milk, and probed with anti-GFP monoclonal mouse antibodies (J108; CLONTECH Laboratories, Inc.). Intensity of the bands was determined by using NIH image analysis software, and results were expressed as the mean ± SEM of five independent experiments.
Directional sensing was determined in cells expressing PHCRAC:GFP and starved for 6 h. Cells were treated with 5 mM caffeine and latrunculin (1 µM) for 20 min and plated onto nonnutrient 1% agar plates containing latrunculin and caffeine. Fluorescence images were acquired before (5 s) and after (+5 s) placing a needle containing 10 µM cAMP at a distance of 20 µm from the cell. Intensity of GFP fluorescence at the perimeter was determined using NIH image software, normalized to maximal fluorescence, and expressed as previously described (Janetopoulos et al., 2004) by plotting intensity as a function of the percent of the perimeter. Data represent the mean ± SEM of four cells from two independent cell preparations.
Online supplemental material
Time-lapse video microscopy (Fig. 3) of 6 h starved cells (Ax2, Ddnhe1, and Ddnhe1/DdNHE1) chemotaxing toward a pipette tip containing 10 µM cAMP is shown in Videos 1, 2, and 3, respectively. Images were captured at 30-s time intervals using a Spot LCD camera mounted on a microscope (Axiovert S-100; Carl Zeiss MicroImaging, Inc.) with a 40x Hoffmann modulation objective and operated using Openlab software (Improvision). Captured images were compiled into a QuickTime movie using Sorenson Video Compressor software. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200412145/DC1.
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Acknowledgments |
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This work was supported by National Institutes of Health grant GM58642 and an award from the Sandler Program in Basic Sciences. This investigation was conducted in a facility constructed with support from Research Facilities Improvement Program grant C06 RR16490 from the National Center for Research Resources, National Institutes of Health.
Submitted: 22 December 2004
Accepted: 10 March 2005
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