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a Section of Cell and Developmental Biology and Center for Molecular Genetics, University of California at San Diego, La Jolla, California 92093
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) q4 G+ }" Z/ T2 @Correspondence to: Richard A. Firtel, Center for Molecular Genetics, Rm. 225, University of California at San Diego, 9500 Gilman Dr., La Jolla, CA 92093-0634. Tel:(858) 534-2788 Fax:(858) 534-7073 E-mail:rafirtel@ucsd.edu.
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7 v# \. E/ Z9 S `% \Abstract, S/ s& \& I0 N1 {# @4 O5 H
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We show that cells lacking two Dictyostelium class I phosphatidylinositol (PI) 3' kinases (PI3K and pi3k1/2-null cells) or wild-type cells treated with the PI3K inhibitor LY294002 are unable to properly polarize, are very defective in the temporal, spatial, and quantitative regulation of chemoattractant-mediated filamentous (F)-actin polymerization, and chemotax very slowly. PI3K is thought to produce membrane lipid-binding sites for localization of PH domain–containing proteins. We demonstrate that in response to chemoattractants three PH domain–containing proteins do not localize to the leading edge in pi3k1/2-null cells, and the translocation is blocked in wild-type cells by LY294002. Cells lacking one of these proteins, phdA-null cells, exhibit defects in the level and kinetics of actin polymerization at the leading edge and have chemotaxis phenotypes that are distinct from those described previously for protein kinase B (PKB) (pkbA)-null cells. Phenotypes of PhdA-dominant interfering mutations suggest that PhdA is an adaptor protein that regulates F-actin localization in response to chemoattractants and links PI3K to the control of F-actin polymerization at the leading edge during pseudopod formation. We suggest that PKB and PhdA lie downstream from PI3K and control different downstream effector pathways that are essential for proper chemotaxis.% _: j. y8 l# X
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Key Words: Dictyostelium, PH domain, actin polymerization, chemotaxis, PI3 kinase, G+ x8 E: x6 z2 y% n' U1 y
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Phosphatidylinositol (PI)1 3' kinase (PI3K) is a regulator of cell growth and survival in higher eukaryotes (Leevers et al. 1999 ; Rameh and Cantley 1999 ; Vanhaesebroeck and Waterfield 1999 ). Activation of PI3K produces the membrane-soluble products PI 3,4,5-triphosphate (PIP3) and PI 3,4-bisphosphate (PIP2), resulting in the membrane localization and activation of downstream effectors. In mammalian cells, the PI3K effector protein kinase B ( or Akt) inhibits apoptosis, regulates GSK3 and cell metabolism, and posttranscriptionally regulates gene expression (Cross et al. 1995 ; Datta et al. 1997 ; Cardone et al. 1998 ; Brunet et al. 1999 ; Gold et al. 1999 ; Kennedy et al. 1999 ; Osada et al. 1999 ; Tang et al. 1999 ). In Caenorhabditis elegans, PI3K and PKB control dauer larval formation; in Drosophila, PI3K regulates cell size (Paradis and Ruvkun 1998 ; Weinkove et al. 1999 ). Furthermore, PI3K regulates chemotaxis in different classes of leukocytes (Dunzendorfer et al. 1998 ; Vanhaesebroeck et al. 1999 ; Hirsch et al. 2000 ; Li et al. 2000 ; Sasaki et al. 2000 ).6 q% `( ?4 }9 }: h* \
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Dictyostelium contains three class I PI3Ks (Zhou et al. 1995 ). Two, PI3K1 and PI3K2, are genetically redundant and most closely related to the mammalian class IA PI3K p110 (Vanhaesbroeck et al. 1997 ). The third, PI3K3, is most closely related to PI3K. (The Dictyostelium PI3Ks were originally called DdPI3K1, DdPI3K2, and DdPI3K3 , but the names were shortened to PI3K1, PI3K2, and PI3K3 .) Disruption of PI3K1 and PI3K2 (pi3k1/2-null cells, previously called ddpi3k1/pi3k2) results in cells that are small, grow slowly (Zhou et al. 1995 ), have an aberrant cell structure, are poorly polarized, and are defective in endocytosis (Buczynski et al. 1997 ). In addition, these cells exhibit an aggregation defect that suggests they do not chemotax effectively (Zhou et al. 1998 ), which is consistent with the requirement of PI3K for chemotaxis in mammalian cells (Dunzendorfer et al. 1998 ; Vanhaesebroeck et al. 1999 ; Hirsch et al. 2000 ; Li et al. 2000 ; Sasaki et al. 2000 ) but in conflict with results reported previously by Buczynski et al. (1997). Disruption of Dictyostelium PI3K3 has no observable phenotype, although studies suggest that a double knockout of PI3K3 with either PI3K1 or PI3K2 is lethal (Zhou et al. 1995 ), implying that basal PI3K activity is essential for cell growth in Dictyostelium.
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Studies on Dictyostelium PKB, a PI3K effector, suggest PI3K function is required for cell polarity and proper chemotaxis (Meili et al. 1999 , Meili et al. 2000 ). Dictyostelium PKB is rapidly and transiently activated in response to chemoattractants via a receptor-mediated, PI3K–dependent pathway. When placed in a chemoattractant gradient, pkbA-null cells do not polarize and move very slowly. Although wild-type cells produce pseudopodia almost exclusively from the leading edge, pkbA-null cells produce multiple pseudopodia simultaneously in all directions. The PKB PH domain rapidly and transiently translocates to the plasma membrane upon chemoattractant stimulation and is found at the leading edge in chemotaxing cells. The kinetics of membrane translocation and kinase activity suggest a causal relationship between membrane localization of PKB and its activation (Meili et al. 1999 ) and are consistent with results in mammalian cells (Andjelkovic et al. 1997 ). Chemoattractants stimulate PKB activity in mammalian cells (Tilton et al. 1997 ), and the pleckstrin homology (PH) domain of mammalian PKB exhibits a similar chemoattractant-regulated membrane localization in neutrophils (Servant et al. 2000 ). These results suggest that these basic mechanisms are conserved between mammalian and Dictyostelium cells and that PKB may be a key regulator of cell polarity and chemotaxis in leukocytes. PI3K1 and PI3K2 are required for PKB activation, indicating PI3K is required for chemotaxis in Dictyostelium, and results suggesting pi3k1/2-null cells chemotax more rapidly than wild-type cells are incorrect (Buczynski et al. 1997 ).4 f9 M/ F9 z& x% X
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The analyses of several PH domain–containing proteins in Dictyostelium and mammalian cells indicate a broad role for PI3K in regulating localized responses at the leading edge of chemotaxing cells (Parent et al. 1998 ; Meili et al. 1999 ; Servant et al. 2000 ). We and others have proposed that a localized activation of PI3K at the leading edge leads to the formation of PI(3,4,5)P3- and PI(3,4)P2-enriched lipid domains that function as docking sites for diverse PH domain–containing proteins, resulting in an enrichment of these proteins, localized responses, the formation of a new pseudopod, and directed cell movement (Parent and Devreotes 1999 ; Firtel and Chung 2000 ; Rickert et al. 2000 ). Here, we characterize the role of PI3K in chemotaxis through a detailed analysis of the phenotypes of pi3k1/2-null cells, wild-type cells treated with the PI3K inhibitor LY294002, and a new PI3K effector. Our findings support the model presented above for PI3K function and provide a new linkage between PI3K, actin polymerization, and chemotaxis that is independent of the activation of PKB.. {! t+ B; C# k+ _/ q+ O
) _# S/ P+ o6 T0 tMaterials and Methods2 I$ A7 i6 m, `3 v3 v/ Q
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6 [" y1 z4 Z5 M$ k% o6 EDictyostelium cells, strain KAx-3, were grown in axenic HL5 medium and transformed by electroporation. For gene disruptions, we selected cells in the presence of blasticidin. We observed morphology by plating washed exponentially growing cells on nonnutrient agar plates (Ma et al. 1997 )./ z1 `8 k9 v) n# d3 ~ v
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Because of concerns about the original pi3k1/2-null strain, we remade the strain in the KAx-3 background. It is designated GMP1., N/ p" s' ]" g8 U) g
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Constructs
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- t% B. z2 t7 OWe generated a phdA knockout construct by inserting the blasticidin resistance cassette into the XbaI and BamHI sites of a PH domain–containing protein A (PhdA) ORF inserted in pSP72. For PhdA–green fluorescent protein (GFP) fusion protein expression, PhdA was amplified by PCR, ligated to a GFP fragment, and cloned into the expression vector EXP-4( ). A mutant, PhdAR41C, was generated using PCR. Successful mutagenesis was confirmed by sequencing.4 g' L4 h$ n2 J# r# L
& O) u0 b! D9 A5 o$ E: OChemotaxis and Image Acquisition
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The analyses of chemotaxis towards cAMP and global responses to cAMP were done as described previously (Chung and Firtel 1999 ) and analyzed with the DIAS program (Soll and Voss 1998 ). We performed folate chemotaxis on starved cells grown in association with Klebsiella aerogenes using a Dunn chamber with 5 μM folate.
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Quantitation of membrane or cortical localization of GFP fusion of PH domain–containing proteins and GFP-coronin in wild-type cells represents the averages of at least five cells from at least three separate experiments. We measured the intensity of cortical GFP by line scanning with Metamorph software. The level of cortical GFP was calculated by dividing intensity before stimulation (E0) by intensity at each time point (E) after subtraction of basal intensity (Moniakis et al. 2001 ).. r: k9 B# _! i) N# ^, E/ s
1 M+ C4 y9 }, I7 \: wWe added LY294002 to a final concentration of 30 μM 10 min before the addition of cAMP for biochemical assays, real time recording of chemotaxis toward the micropipette or translocation of GFP fusion proteins. No differences were observed if the drug was added either 30 or 60 min before stimulation.
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Biochemical Assays- T4 v% E) `- D. M* I
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We measured the amount of F-actin in response to cAMP stimulation using TRITC phalloidin as described (Chung et al. 2000 ). The values are the averages of at least three separate experiments. We assayed guanylyl cyclase using the cGMP assay kit (Amersham Pharmacia Biotech) (Ma et al. 1997 ). PKB activity was measured as described (Meili et al. 1999 ). Adenylyl cyclase was measured by C. Parent (Parent and Devreotes 1995 ).3 q( q8 M2 Z6 {) R( c% E( Z: U
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To measure the in vitro translocation of PhdA, cells expressing PhdA–GFP were pulsed with cAMP and treated with caffeine as described previously (Chung et al. 2000 ), resuspended at 8 x 107 cells/ml in 5 mM NaPO4 buffer containing 2 mM MgSO4, and filter lysed using Nuclepore filters in the presence or absence of 40 μM GTPS and 1 μM cAMP. We incubated the cell lysates for 5 min on ice. To stop the reaction, we added 1 ml of ice-cold phosphate buffer. Membrane fractions were collected by centrifugation for 1 min at 15,000 g and subjected to immunological detection of PhdA–GFP by using anti-GFP antibody (BABCO). In separate experiments, the cells were lysed in the presence of 40 μM GDP?S or in the presence of 40 μM GTPS and 12.5 μM LY294002.
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pi3k1/2-null Cells Exhibit Aberrant Chemotaxis0 @6 z" ]1 h& W: Y! _' C
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The analyses by Zhou et al. (1998) on pi3k1/2-null cells and Meili et al. (1999, 2000) on pkbA-null cells suggest that PI3K is required for proper cell polarity and chemotaxis. Since these results conflict with previously published results on pi3k1/2-null cells, which suggest that pi3k1/2 cell chemotax more rapidly than wild-type cells (Buczynski et al. 1997 ), we have undertaken a detailed analysis of chemotaxis of pi3k1/2-null cells using more current experimental technologies and analysis methods.
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3 ] C1 a8 b$ K5 f6 e8 xFig 1 shows an analysis of the ability of pi3k1/2-null cells (strain GMP1; see Materials and Methods) to chemotax towards a micropipette containing the chemoattractant cAMP. These cells are poorly polarized (not elongated) and move very slowly compared with wild-type cells, as illustrated by the number of cells that move toward the micropipette tip over a period of time. This phenotype is similar to that of pkbA-null cells and consistent with the conclusion that PKB lies downstream from PI3K (Meili et al. 1999 ). We quantitated the chemotaxis parameters of the pi3k1/2-null cells, including cell shape and directionality of cell movement (an indicator of chemotaxis efficiency), using the DIAS computer software program (Soll and Voss 1998 ). This analysis indicates that pi3k1/2-null cells are more rounded and move more slowly than wild-type cells and produce pseudopodia randomly along the sides of the cells rather than predominantly at the leading edge, as do wild-type cells (Fig 1 and Table 1). As a result, the cells chemotax very inefficiently with low directionality (Table 1). Expression of PI3K in pi3k1/2-null cells complements the growth and developmental phenotypes of this strain (Zhou et al. 1995 ).
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H. R; l# G0 R3 v/ T6 Q7 X+ QFigure 1. Time-lapse recording of chemotaxis of wild-type and pi3k1/2-null cells. (A) After pulsing with cAMP, cells were transferred to glass-bottomed dishes and allowed to adhere to the bottom. A needle filled with 150 μM cAMP was placed on the bottom and is visible in the images. The movement of wild-type cells, pi3k1/2-null cells, pi3k1/2-null cells expressing PI3K1, or wild-type cells plus 30 μM LY294002 toward the cAMP source was recorded (Chung and Firtel 1999 ). Zero- (0; when the micropipette was inserted) and 20-min time points are shown. The insets show an enlargement of representative cell(s). (B) DIAS computer analyses. See Table 1 for the numerical analysis. (C) Chemotaxis to folate in a Dunn chamber. Superimposed images at 1-min intervals depict the movement of these strains and give an indication of the chemotaxis efficiency. The graphs plot the change of direction ofthe leading edge relative to the cell's centroid.2 a& b7 x. a. N6 g; c
1 Y: L/ \9 z7 X/ G& Y& STable 1. DIAS Analysis of Chemotaxis
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Since the ability of cells to respond to extracellular cAMP is developmentally regulated, we wanted to ensure these cells were competent to respond to extracellular cAMP. RNA blot analysis revealed that the level of expression of the cAMP receptor cAR1 in response to pulses of cAMP was only slightly lower than that of wild-type cells and well within the range of other responsive cell types (data not shown). Dictyostelium has a PKB and a related kinase, PKBR-1, that differs from PKB in that it lacks a PH domain and is constitutively membrane localized via myristoylation (Meili et al. 2000 ). Like PKB, PKBR-1 kinase activity is stimulated in response to cAMP; however, unlike the activation of PKB the activation of PKBR-1 is not inhibited by the PI3K inhibitor LY294002 (Meili et al. 2000 ). We found that PKBR-1 activation is normal in both the level of kinase activity and its kinetics in pi3k1/2-null cells, indicating that pi3k1/2-null cells exhibit some normal cAMP-mediated responses and the cells are not generally unresponsive.9 N9 C" V& a% w4 i
' O4 `4 Y6 Z. @+ m8 jTo support our conclusions that PI3K plays a key role in chemotaxis and to eliminate possible concerns that pi3k1/2-null cells may be less developmentally competent to respond to the chemoattractant cAMP, we examined the effect of treatment of aggregation-stage cAMP-responsive wild-type cells with the PI3K inhibitor LY294002 on chemotaxis. For these experiments, we used a concentration of 30 μM of the drug, which we demonstrate to be the lowest concentration that effectively inhibits translocation of PH domains to the plasma membrane in response to chemoattractant stimulation and PKB activation (Meili et al. 1999 , Meili et al. 2000 ; see below, Fig 4 C) (note, this concentration varies with the lot of LY294002). As shown in Fig 1 and Table 1, these cells have polarity and chemotaxis defects similar to those of pi3k1/2-null cells. One noticeable difference is that LY294002-treated wild-type cells display fewer changes in the direction of cell movement than pi3k1/2-null cells and, for the most part, are more rounded and produce fewer pseudopodia. This difference may be due to the level of inhibition of the PI3K pathways by the drug, which presumably inhibits all three PI3Ks (Meili et al. 1999 , Meili et al. 2000 ). To test this possibility, we examined the chemotaxis behavior of pi3k1/2-null cells treated with LY294002. These cells exhibited phenotypes more severe than those of pi3k1/2-null cells and similar to those of LY294002-treated wild-type cells (Table 1).
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Figure 2. Changes in F-actin in pi3k1/2-null cells in response to chemoattractant stimulation. (A) F-actin levels in wild-type, pi3k1/2-null cells, and wild-type cells plus 30 μM LY294002 after cAMP stimulation. The F-actin content was determined as described previously (Chung et al. 2000 ). (Wild-type cells treated with 10 μM LY294002 showed little effect on changes in F-actin; 30 and 60 μM had similar effects; 90 μM had a slightly greater effect .) (Ba) Cells expressing GFP-coronin were globally stimulated with saturating (μM) levels of cAMP. Changes in the localization of GFP-coronin, as determined by fluorescence, were followed as described in Materials and Methods. (Wild-type cells treated for 10 min with LY294002 are round in the absence of a cAMP gradient.) (Bb) Kinetics of GFP-coronin translocation to the membrane after cAMP stimulation. Intensity of fluorescence on the membrane was measured using Metamorph software. Graph shows increase fold calculated by dividing intensity before stimulation (E0) by intensity at each time point (E). (Bc) Intensity profiles of images in Ba. (Ca) Translocation of coronin in response to changes in the position of the micropipette containing cAMP. Placing the tip of a micropipette filled with 150 μM cAMP near the cell causes the accumulation of GFP-coronin at the edge of the cell closest to the tip and the formation of a new pseudopod. Changing the position of the tip to the opposite side results in the formation of new pseudopodia enriched in GFP-coronin and a retraction of the old pseudopod. Asterisks indicate the position of the micropipette. Open arrow indicates retracting pseudopod; white arrow indicates new pseudopod. (Cb) Kinetics of translocation of coronin. The graph shows fold increase calculated by dividing intensity before stimulation (E0) by intensity at each time point (E).7 I1 K9 O6 _0 [! k- F% l: r
" C7 q* r+ ?7 yFigure 3. Development morphology of PhdA mutant strains and deduced amino acid sequence of PhdA. (A) phdA-null cells form smaller aggregates. (B) Developmental expression pattern of PhdA. Total RNAs were isolated at the time indicated from wild-type and phdA-null cells and subjected to Northern blot analysis. White and open arrows indicate the 2.2- and 1.0-kb transcripts of PhdA, respectively. The bottom panel shows the expression pattern of cAMP receptor cAR1. (C) Sequence comparison of PhdA and CRAC (Insall et al. 1994 ). Asterisks indicate the sites of mutations used in this study. (D) Comparison of the PH domain of PhdA with other PH domains from Dictyostelium.
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/ Z! S0 w% \4 ]; T' j! k n2 hFigure 4. Translocation of PhdA–GFP in response to cAMP stimulation. (A) Global stimulation of cells by dropping cAMP solution. Wild-type cells expressing the PhdA–GFP fusion protein exhibit translocation of the protein to the cell membrane (top). In contrast, PhdA–GFP expressed in pi3k1/2-null cells distributes uniformly throughout the cell after stimulation with cAMP (middle). Wild-type cells expressing PhdAR41C–GFP fusion protein exhibit no translocation of the protein after stimulation (bottom). (B) Accumulation of PhdA–GFP at the leading edge of migrating cells. Wild-type cells migrating toward cAMP source show a distinct localization of PhdA–GFP at the leading edge (top); pi3k1/2-null cells do not (middle). PhdAR41C–GFP in migrating wild-type cells localizes uniformly (bottom). Asterisks indicate the position of the tip of the micropipette containing the cAMP solution. (C) Dose–response curves of LY294002 inhibition of PhdA–GFP translocation to the plasma membrane. (D) In vitro translocation of PhdA–GFP by GTPS (as described in Materials and Methods). Membrane fractions were collected by centrifugation and PhdA–GFP was subjected to immunological detection using an anti-GFP antibody.
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Dictyostelium cells also chemotax to folic acid, a response that is maximal shortly after starvation in cells grown on bacteria (Varnum and Soll 1981 ). However, the chemotaxis response is not as robust as that to cAMP during the aggregation stage, and the response is maximal at much higher concentrations of ligand (1–10 μM). Because of this, cells do not chemotaxis effectively to folate emitted from a micropipette, possibly because of the inability to establish an appropriate chemoattractant gradient, but they do chemotax effectively to folate in a Dunn chamber (Insall, R., personal communication). Analysis of bacterially grown wild-type and pi3k1/2-null cells revealed that wild-type cells chemotax with a directionality of 0.84 ± 0.05, whereas pi3k1/2-null cells chemotax with a directionality of only 0.38 ± 0.18 (Fig 1 C). The results demonstrate definitively that pi3k1/2-null cells exhibit chemotaxis defects to two chemoattractants at different stages of development. These results expand on those of Zhou et al. (1998) but disagree with those of Buczynski et al. (1997); the reason for the discrepancy between the present and previous findings on pi3k1/2-null cells is unknown.7 w, x: D6 G6 J% i
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pi3k1/2-null Cells Exhibit Defects in Chemoattractant-mediated Actin Polymerization
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When cells are rapidly bathed in the chemoattractant cAMP, which simultaneously activates all receptors on the cell surface, wild-type Dictyostelium cells exhibit a transient 2.2-fold increase in the level of F-actin that peaks 5 s after cAMP addition (Carboni and Condeelis 1985 ; Condeelis and Hall 1991 ). pi3k1/2-null cells exhibit a reduced basal level of F-actin (zero time point), and the chemoattractant-mediated F-actin assembly is reduced significantly compared with that of wild-type cells (Fig 2 A). The level of F-actin stays elevated for a longer period of time, 30 s after stimulation, whereas the level of F-actin in wild-type cells returns to prestimulation levels in that time. Wild-type cells pretreated with LY294002 display a pattern and level of cAMP-stimulated F-actin similar to those of pi3k1/2-null cells but with a higher basal level of F-actin (Fig 2 A). The dose–response curve of LY294002 inhibition of F-actin assembly is very similar to that of PH domain translocation (data not shown; see Fig 4 C).1 ]1 [+ Q ?+ O) O
0 _% }! O9 X( PAlthough these experiments quantitate F-actin polymerization in response to global stimulation, they do not provide an accurate measurement of the kinetics of new F-actin polymerization during pseudopod formation or the ability of cells to spatially respond to changes in the direction of a chemoattractant gradient. Such changes can be dynamically visualized in chemotaxing cells using a GFP fusion of the F-actin–binding protein coronin (Gerisch et al. 1995 ). When wild-type cells expressing GFP-coronin are given a global stimulation, GFP-coronin becomes uniformly localized to the cell cortex (Fig 2 Ba), as expected from the analysis of F-actin localization and previous results using this reporter (Gerisch et al. 1995 ). We quantitated the kinetics of this response by measuring the increase in fluorescence across the plasma membrane. In wild-type cells, GFP-coronin translocation peaks at 5 s, similar to the kinetics of F-actin assembly measured biochemically (Fig 2 Bb). In contrast, the increase is reduced in pi3k1/2-null cells (cells expressed GFP-coronin at a similar level as determined by the fluorescence of unstimulated cells) and the kinetics are extended (Fig 2 Bb), similar to our observations in the actin polymerization assays. Wild-type cells treated for 10 min with LY294002 become very rounded, exhibiting a loss of polarity (Chung et al. 2001 ). When stimulated with cAMP, these cells show kinetics of cortical GFP-coronin that are very similar to those of pi3k1/2-null cells, consistent with PI3K being required for this process.9 Z, ~3 n. ^+ P& L: J" s
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To study the ability of cells to form a new pseudopod, we placed GFP-coronin–expressing cells in a chemoattractant gradient and examined the subcellular localization of the fluorescent signal as the cells moved towards the micropipette. As demonstrated previously, GFP-coronin localizes to the cortex of the leading edge in wild-type cells (Gerisch et al. 1995 ; Fig 2 C). When we move the micropipette to a new position relative to the cell, the old pseudopod rapidly retracts and a new one forms proximal to the new cAMP source with a half-maximal response at 10 s. With the retraction of the old pseudopod, there is a concomitant loss of GFP-coronin from this site on the cell and an enrichment of GFP-coronin at the position of the new pseudopod (Gerisch et al. 1995 ). Phalloidin staining indicates that the GFP-coronin signal colocalizes with F-actin formation (data not shown). In pi3k1/2-null cells, the kinetics of the formation of a new pseudopod and the loss of the old pseudopod were also delayed, with the half-maximal response for the formation of the new pseudopod occurring at 24 s and a delay in the initial response (Fig 2 C). In addition, the kinetics of the loss of the old pseudopod, as determined by the loss of GFP-coronin signal, were significantly slower in pi3k1/2-null cells. This aspect of the phenotype cannot be readily quantified but is observable by examining the intensity of fluorescence in time-lapse pictures (Fig 2 C). Similar experiments in LY294002-treated wild-type cells showed a very delayed response that exhibited a much greater cell-to-cell variability in the kinetics (Fig 2 C). These results are consistent with a requirement for PI3K in the proper spatiotemporal regulation of F-actin localization in response to chemoattractants.9 [' {& {# e8 l t N
, e# c8 @; `6 o) x8 `5 AIdentification of the Gene Encoding PhdA, a New PH Domain–containing Protein Required for Aggregation- Q' j1 I0 c/ O, D" B5 |/ |$ j
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As the growth and aggregation phenotypes of the pi3k1/2-null cells are more severe than those of PKB (pkbA)-null cells, we expect that other PI3K effectors were required for chemotaxis in addition to PKB. As in the model outlined in the Introduction, such proteins might contain a PH domain.
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' A' \+ K2 s0 R1 ?% \3 ~+ rA new gene, PhdA, was identified in a genetic screen for mutant strains with developmental defects (strain DG1093; http://www-biology.ucsd.edu/others/dsmith/REMIgenes2000.html). The developmental phenotype suggested that phdA-null cells exhibit aggregation and, potentially, chemotaxis defects. An independently derived phdA-null strain was created by homologous recombination and used for the described experiments (see Materials and Methods). When plated for development, phdA-null cells form very small aggregates and fruiting bodies similar to the phenotype of mek1-null cells, which are defective in chemotaxis (Ma et al. 1997 ). The phdA-null strain developmental phenotypes are complemented by expressing PhdA or a PhdA–GFP fusion protein from the constitutive Actin 15 promoter (Fig 3 A; data not shown).1 B: G1 c& b5 O% J/ \' S+ v
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The derived PhdA ORF encodes a 284–amino acid protein with an NH2-terminal PH domain and a short novel COOH-terminal domain (Fig 3 C; sequence data available from GenBank/EMBL/DDBJ under accession no. AF080677). The PH domain shares homology with the PH domains of PKB and Ca2 release-activated Ca2 (CRAC), a cytoplasmic protein required for receptor-mediated adenylyl cyclase activation in Dictyostelium (Insall et al. 1994 ). BLAST analysis indicates that the PhdA COOH terminus is novel, but very weak homology is observed in a one-to-one comparison with the COOH terminus of CRAC, suggesting that PhdA and CRAC may be distantly related. PhdA expresses two distinct transcripts, a larger one expressed during growth and early development and a smaller transcript induced during mound formation (Fig 3 B).* X' t$ H% i1 _5 F- `
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PhdA Translocates to the Leading Edge via a PI3K–dependent Pathway
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The presence of a PH domain related to those in PKB and CRAC suggests that PhdA may also translocate to the plasma membrane in response to a global stimulation by cAMP and to the leading edge in chemotaxing cells. To examine this, we used a PhdA–GFP fusion protein and performed time-lapse videomicroscopy.6 e. s/ J* i/ Q( f# @- \
; Q- l6 Y6 T N9 Q7 kIn unstimulated cells, PhdA–GFP exhibits a uniform distribution throughout the cell. In response to global stimulation, there is a rapid and transient translocation of PhdA–GFP from the cytosol to the plasma membrane, peaking at 5 s, with the protein disassociating by 12 s (Fig 4A and Fig C). Moreover, when we place cells in a cAMP gradient, PhdA–GFP localizes to the leading edge (Fig 4 B). These behaviors are similar to those of CRAC–GFP and PKB PH domain–GFP fusions (Parent et al. 1998 ; Meili et al. 1999 ). We then assessed the role of PI3Ks in these responses. Fig 4A and Fig B, show that neither global stimulation nor directional stimulation (gradient of cAMP) lead to the translocation of PhdA–GFP from the cytosol to the plasma membrane in pi3k1/2-null cells, suggesting that the membrane localization is dependent on PI3K activity. To confirm this conclusion, we pretreated aggregation-competent wild-type cells expressing PhdA–GFP with various concentrations of LY294002 and examined the ability of cAMP to stimulate PhdA–GFP translocation. A slight delay in the response is seen with 10 μM LY294002; a concentration 30 μM results in complete inhibition (Fig 4A and Fig C).
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To examine whether the requirement of PI3K for PhdA translocation is a general property of PH domains known to translocate to the plasma membrane in response to chemoattractant signaling, we performed a similar set of experiments in wild-type cells treated with LY294002 using GFP fusions of the PH domain of PKB and CRAC (Parent et al. 1998 ; Meili et al. 1999 ). In both cases, we observed the same dose-dependent inhibition of translocation of these GFP fusion proteins as we did with PhdA (data not shown). These results suggest that PI3K is required to regulate the transient chemoattractant-mediated membrane localization of this class of PH domain–containing proteins.
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To further examine the role of PI3K and other upstream pathways on PhdA translocation, we employed an in vitro translocation assay (Lilly and Devreotes 1995 ; Parent et al. 1998 ). Wild-type cells expressing PhdA–GFP were lysed in the presence or absence of GTPS or GDP?S and incubated. The reaction was stopped, and the membrane fraction was processed for Western blot analysis using an anti-GFP antibody. Fig 4 D indicates that PhdA–GFP translocates to the particulate plasma membrane–containing fraction when the cells are lysed in the presence of GTPS but not GDP?S. This GTPS-dependent translocation is blocked when the lysates are preincubated with LY294002 in a dose-dependent fashion, indicating that the translocation is PI3K dependent (Fig 4 D; data not shown).
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" n3 \/ ^0 M' _/ E. mIt was demonstrated previously that a conserved Arg residue within PH domains is required for PI(3,4,5)P3 binding (Fukuda et al. 1996 ; Salim et al. 1996 ; Hyvonen and Saraste 1997 ; Isakoff et al. 1998 ). Mutation of this Arg (Arg25)Cys in the Akt1 PH domain or Arg28Cys in Btk abrogates the binding of these PH domains to PI(3,4,5)P3. Although PhdA–GFP completely restores the developmental defects of phdA-null cells, PhdA–GFP with an equivalent mutation (PhdAR41C–GFP) expressed at comparable levels does not complement phdA-null cells (data not shown). Moreover, PhdAR41C–GFP does not translocate to the plasma membrane or leading edge on global or directional chemoattractant stimulation (Fig 4A and Fig B) nor does it bind membrane fractions from GTPS-treated cell lysates (Fig 4 D). These results indicate that the PH domain is integral to PhdA function and further support the conclusion that PI3Ks, presumably functioning through the formation of PI(3,4,5)P3 and/or PI(3,4)P2, mediate PhdA membrane translocation.1 J* ~) t: m% o) r) L* t
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phdA-null Cells Are Defective in Chemotaxis: w8 B. O' ~$ A% x: P3 z' k
9 E6 i" D0 r7 TThe small aggregate size produced by phdA-null cells, which is similar to that of mek1-null cells (Ma et al. 1997 ), suggests that PhdA might be required for chemotaxis. Time-lapse videomicroscopy of cells plated as a monolayer on nonnutrient agar shows that after 3 h of starvation, wild-type cells form discernible discrete domains with aggregation centers, which act as oscillators for the initiation of waves of the chemoattractant cAMP (Fig 5 A). These waves move outward from the center and control the inward chemotaxis of cells, leading to the formation of a multicellular organism (Siegert and Weijer 1991 ) and can be "visualized" through the changes in cell shape resulting from cytoskeletal reorganizations. At 3.5–4 h, wild-type cells start to chemotax inward, forming large discrete mounds by 6–7 h. In contrast, phdA-null cells display a more random pattern with multiple, smaller, and less distinct aggregation centers (Fig 5 B). Chemotaxis is initiated at 4 h, but instead of cells moving to a small number of discrete centers random wave patterns persist, and the cells appear to randomly coalesce into ill-formed, asymmetric aggregates (see image at 5:40 h), which eventually break up into small distinct aggregates (7:00-h image). In contrast to wild-type cells, no aggregation streams are observed.4 g$ \5 }5 W" o4 M0 K
7 r! j p9 K5 Y1 ?% a: \( b7 V; }; AFigure 5. Time-lapse phase–contrast microscopy of wild-type and phdA-null cells during aggregation. Log-phase cells were washed and plated as a monolayer on nonnutrient agar plates, and aggregation was recorded as described previously (Ma et al. 1997 ). (A) Wild-type cells. White arrows indicate aggregation centers. Black arrows mark the outer limits of the aggregation domain. (B) phdA-null cells. phdA-null cells show a random wave pattern with multiple and less distinct aggregation centers from 4:00 to 5:40 h. Although wave patterns are observed, the cells form aberrant aggregates that break up into small distinct ones at 7:00 h.+ W9 {$ ~7 H7 A0 h8 K% E0 ^: W
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Further analysis demonstrates that the aggregation defect observed in phdA-null cells is caused by a defect in chemotaxis. We find that phdA-null cells chemotax more slowly and make significantly more changes in direction than wild-type cells (Fig 6a and Fig c, and Table 1). Analysis of cell shape revealed morphological differences between phdA-null and wild-type cells. Wild-type cells are more elongated (polarized) than phdA-null cells (Table 1) and have a round fairly smooth pseudopod/lamellipod at the leading edge. In contrast, the leading edge of phdA-null cells consists of multiple small projections or fingers that change with time (Fig 6 B). Analysis of random motility (in the absence of a chemoattractant gradient) by DIAS revealed no significant differences between wild-type and phdA-null cells (data not shown), suggesting that PhdA may regulate pseudopod formation during chemotaxis.2 {1 i3 _7 m# _
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Figure 6. Chemotaxis of PhdA mutant strains to a cAMP source. (A) Chemotaxis of phdA-null cells to a micropipette filled with cAMP (see legend to Fig 1; the wild-type panels are the same as those in Fig 1 and are added as a comparison). Wild-type cells expressing PhdAR41C partially phenocopy the phdA-null phenotype. (B) Leading edge of the phdA-null cell. The leading edge of a migrating wild-type cell is smooth, but the phdA-null cell forms multiple spike structures at the leading edge. Wild-type cells expressing PhdAR41C exhibit similar projections. Arrows indicate leading edge protrusions. (C) DIAS computer analyses of phdA mutants (see legend to Fig 1). phdA-null cells exhibit more changes of direction than wild-type cells. Wild-type cells expressing PhdAR41C exhibit a reduction in elongation and movement and an increase in the change of direction as phdA-null cells.
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! l. C( G/ J: M2 i' e+ ETo ensure that phdA-null cells are developmentally competent to respond to the cAMP signal, we examined the expression of two aggregation-stage developmental markers: the cAMP receptor cAR1 and the cell adhesion molecule contact sites A. Northern blot analysis revealed that phdA-null cells exhibit normal expression of both genes (Fig 3 B; data for contact site A not shown). In addition, we measured the cAMP-mediated activation of adenylyl cyclase in phdA-null cells and observed that phdA-null and wild-type cells exhibit indistinguishable levels of adenylyl cyclase activity (data not shown), indicating the phdA-null cell aggregation defects are not due to an inability to relay the chemoattractant signal.- \4 g1 |+ k. \ H
+ Y4 r* S7 [& S) d% K* C" vphdA-null Cells Are Defective in the Kinetics and Level of Actin Polymerization! L2 U7 X: m A2 D: e% n+ F3 H
% ~# x# w. G/ [- vBecause of the chemotaxis phenotypes exhibited by phdA-null cells, we investigated whether these cells exhibit defects in F-actin polymerization. Upon global stimulation with cAMP, phdA-null cells exhibit kinetics of F-actin polymerization that are similar to those of wild-type cells (within the limits of this assay); however, the level of F-actin is reduced, although not to the extent observed in pi3k1/2-null cells (Fig 7 A). Like pi3k1/2-null cells, the basal level of F-actin in unstimulated cells is reduced. As a control, we examined the kinetics and level of F-actin in pkbA-null cells, which were indistinguishable from those of wild-type cells (Fig 7 A), suggesting that differences between wild-type and phdA-null cells are not due to any mutation in a PI3K effector.
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5 {5 g! V4 ^" hFigure 7. Regulation of F-actin in phdA-null cells. (A) F-actin levels in wild-type cells, phdA-null cells, wild-type cells expressing PhdAR41C, phdA-null cells expressing PhdA, and pkbA-null cells after cAMP stimulation. See the legend to Fig 2 for details. (B) Kinetics of GFP-coronin translocation in phdA-null cells (see legend to Fig 2). The asterisks indicate the position of the micropipette containing the chemoattractant. The black arrow indicates the retracting pseudopod, and the white arrow indicates the new pseudopod. The data for wild-type and pi3k1/2-null cells are taken from Fig 2. The graph represents an averaging of five cells from the same experiment. The experiment was repeated several times on the same day and three different times on different days; all experiments produced comparable results. (C) cAMP-mediated PKB kinase activity. PKB activity was tested according to Meili et al. (1999). PKB protein levels were determined in these samples using Western blot analysis (Meili et al. 1999 ).: M2 w; ^2 f ~( i) h" B- W
# i- b. X' @2 ^3 s; k* KWe then used GFP-coronin to examine the spatial regulation of chemoattractant-mediated F-actin accumulation. Upon global stimulation, phdA-null cells exhibit a small but reproducible shift of the curve with a peak at 7 s, compared with 5 s for wild-type cells (data not shown). When we examined the ability of phdA-null cells to retract an old pseudopod and form a new one when the micropipette is moved, we observed that the response was significantly delayed in phdA-null cells, with the half-maximal response occurring at 20 s and a delay in the initiation of the response (Fig 7 B), similar to observations in pi3k1/2-null cells (Fig 2 and Fig 7 B). The kinetics of loss of the old pseudopod, as determined by the loss of GFP-coronin, were also significantly slower in phdA-null cells. This suggests that both phdA-null and pi3k1/2-null cells have a defect in the ability of cells to establish a new pseudopod and in the spatiotemporal regulation of F-actin assembly.
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/ y( m! G' T1 I1 z. i' y7 u- |5 SPhdA Is Not Required for PKB Activation or Myosin Assembly2 \( u* Z4 u6 {6 v% [
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To examine the possible genetic interaction of PhdA with PKB, we measured the chemoattractant-mediated activation of PKB activity and PKB expression level in phdA-null cells. phdA-null cells exhibit an enhanced activation of PKB kinase activity in response to cAMP (Fig 7 C). The kinetics of PKB activation and adaptation and PKB expression levels are similar to those of wild-type cells, suggesting that the chemotaxis defect of phdA-null cells is not due to a problem in the chemoattractant-mediated activation of PKB. The increased activation of PKB could be due to a change in the kinetics and/or to the extent of the localization of the subclass of PH domain that responds to the activation of PI3K; for example, the loss of PhdA might reduce competition for a limiting number of PH domain–binding sites at the leading edge, resulting in an increase in PKB activation. To examine this, we tested the kinetics of localization of CRAC-GFP, the PKB PH domain–GFP fusion, and a GFP fusion of a mutant PhdA that is able to translocate but not complement the phdA-null phenotype (PhdAD272G,E283K–GFP, see below) expressed in phdA-null cells. All three GFP PH domain protein fusions exhibit the same kinetics of translocation in response to global stimulation and in a relocalization assay in which the position of the micropipette is changed within the limits of these assays (data not shown). Our data suggest that the increased level of PKB activation in phdA-null cells is not due to a loss of competition of PH domains for limiting PI(3,4,5)P3 and/or PI(3,4)P2. Furthermore, phdA-null cells expressing PhdAD272G,E283K–GFP exhibit a level of PKB activation between those of phdA-null and wild-type cells (Fig 7 C). To determine if increased PKB activity results in chemotaxis defects similar to those of phdA-null cells, we examined chemotaxis of wild-type cells overexpressing PKB (Meili et al. 1999 ). These cells exhibit essentially wild-type chemotaxis (Table 1), indicating that the increased PKB activation in phdA-null cells does not underlie the phdA-null chemotaxis defects. Since the chemotaxis defects of phdA and pkbA-null cells are distinct, we suggest that PhdA and PKB regulate different effector pathways downstream from PI3K.7 ~0 ]; ?/ K8 X/ t* B x. i; H" a& v
) @9 J+ `5 X% u: G$ jWe examined two other pathways required for chemotaxis: chemoattractant stimulation of guanylyl cyclase and myosin II assembly, which is required for cortical tension and retraction of the posterior cell body (Wessels et al. 1988 ). Cyclic GMP is a second messenger that regulates chemotaxis (van Haastert and Kuwayama 1997 ). Guanylyl cyclase is rapidly stimulated in response to cAMP in wild-type cells, with levels of cGMP peaking at 10 s (Mato et al. 1977 ). phdA-null cells exhibit an 30% decrease in receptor-mediated cGMP production (data not shown). This effect alone might not cause the observed chemotaxis defect of the phdA-null cells. Examination of cells expressing myosin II–GFP (Moores et al. 1996 ) indicated a similar posterior localization of myosin II–GFP in chemotaxing wild-type and phdA-null cells (data not shown). Moreover, the level of assembled myosin II was the same in phdA-null and wild-type cells (data not shown), suggesting that PhdA does not regulate myosin II.
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PhdA May Function as an Adaptor Protein
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Other than the PH domain, the sequence of PhdA provides little insight into how it might function. PhdAR41C does not localize to the plasma membrane and does not complement the null cell. If PhdA were to function by localizing components required for chemotaxis to the leading edge, we reasoned that PhdAR41C might act as a dominant negative form when expressed in wild-type cells by sequestering these components in the cytosol. As shown in Fig 6 and Table 1, the expression of PhdAR41C in wild-type cells leads to chemotaxis defects that are similar to but less severe than those of phdA-null cells. This dominant interfering phenotype of PhdAR41C supports a model in which PhdA might function as a docking site for other proteins at the leading edge. If this were the case, point mutations in the COOH-terminal domain might abrogate PhdA function but not alter its membrane localization. We identified a PhdA mutant carrying two point mutations in the COOH-terminal domain (PhdAD272G,E283K) resulting from PCR amplification. A PhdAD272G,E283K–GFP fusion translocates to the plasma membrane, but neither this fusion nor PhdAD272G,E283K without the GFP tag complements the null phenotype, indicating that the COOH-terminal domain and a functional PH domain are essential for PhdA function (data not shown). These results are consistent with our model in which PhdA functions as a docking site for cellular proteins that must assemble at the leading edge in response to chemoattractant signals.$ F6 B: u+ r& P D
. o0 K+ v$ Y0 L6 q, dWe expanded these studies to examine whether wild-type cells expressing PhdAR41C exhibit an elevated level of PKB activation similar to that seen in phdA-null cells. Fig 7 C indicates that PhdAR41C-expressing cells have an elevated PKB activation. This was not observed when PhdAD272G,E283K was expressed in wild-type cells (data not shown).; i( f* X* G* x& J# B
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Discussion- M; C# e @* |% M
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PI3K Is Required for Cell Polarity, Actin Polymerization, and Proper Chemotaxis
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) Y' q& A$ j O6 |! [5 {6 C6 U/ kWe undertook a more detailed analysis of the role of PI3K1 and PI3K2 (Zhou et al. 1995 ) in regulating chemotaxis. We find that pi3k1/2-null cells are poorly polarized, move more slowly than wild-type cells, and make large numbers of random turns that result from the simultaneous protrusion of multiple pseudopodia from the cells. The observed cell polarity phenotypes of the pi3k1/2-null cells are consistent with those of cells lacking PKB, a PI3K effector that is not activated in response to the chemoattractant cAMP in pi3k1/2-null cells (Meili et al. 1999 ). In addition, we demonstrate that pi3k1/2-null cells are defective in regulating chemoattractant-mediated actin polymerization. All of these defects were reproduced when cAMP-responsive wild-type cells were treated with the PI3K inhibitor LY294002. As the level of F-actin polymerization is normal in pkbA-null cells, we suggest that the actin polymerization defect is due to a PI3K effector other than PKB. pi3k1/2-null cells are unable to properly spatially regulate F-actin assembly and thus to properly extend F-actin–enriched pseudopodia in the direction of the chemoattractant source, which leads to chemotaxis defects and an inability to efficiently respond to changes in the direction of the chemoattractant gradient. We obtained similar results with wild-type cells treated with LY294002, suggesting that the chemotaxis phenotypes of the pi3k1/2-null cells probably result from a requirement for PI3K in chemotaxis rather than a developmental defect of pi3k1/2-null cells that renders them less responsive to cAMP, although we cannot exclude the possibility of some pleiotrophic developmental abnormalities resulting from disruption of PI3K1 and PI3K2. We were unable to examine the phenotypes of double knockouts of PI3K1 or PI3K2 and the third Dictyostelium class I PI3K (PI3K3). Thus, we do not know the cellular function of PI3K3, although we expect that some of the differences between pi3k1/2-null cells and wild-type cells treated with LY294002 may be the result of inhibiting all three PI3Ks with the drug.
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' r8 X+ A+ J$ }& p+ x x; B z4 TThe Analysis of PhdA Defines a New Subset of Chemotaxis Pathways Regulated by PI3K
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Our analysis of phdA-null cells provides a further understanding of the molecular mechanisms by which PI3K regulates chemotaxis. PhdA, like PKB, localizes to the leading edge of chemotaxing cells, a process that is PI3K dependent and necessary for both PhdA and PKB to function. However, the phenotypes of the phdA and pkbA-null strains indicate that the two proteins have distinct cellular functions: pkbA-null cells have a severe loss of cell polarity, whereas phdA-null cells exhibit almost normal cell polarity but are defective in the spatiotemporal regulation of actin assembly. phdA-null cells normally localize myosin II in the posterior of cells, whereas myosin II assembly is abrogated in pkbA-null cells (Chung and Firtel 1999 ; Chung et al. 2001 ). These studies suggest that PI3K regulates chemotaxis by controlling at least two effector pathways, one through PhdA and one through PKB.
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1 b# D9 U5 A( nphdA-null Cells Exhibit an Abnormal Pattern of F-Actin Assembly6 \2 w! T& D# g. N
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The F-actin assembly defect in phdA-null cells is different from those defined for mutations affecting Rho family proteins. Dominant negative Rac1 blocks cell polarity, chemotaxis, and F-actin assembly in chemotaxing macrophage and Dictyostelium cells (Allen et al. 1998 ; Chung et al. 2000 ). Although phdA-null cells do not chemotax effectively, they polarize and produce a pseudopod at the leading edge in the direction of the chemoattractant source significantly better than cells in which the Rac1 GTP exchange is blocked or inhibited. We view the 30% reduction in chemoattractant-mediated F-actin polymerization in phdA-null cells as an indicator of the potentially more significant defect in the ability to respond to changes in the direction of the chemoattractant gradient, including localized F-actin assembly required to form a new pseudopod. Using GFP-coronin as an in vivo real time reporter of the distribution and subcellular localization of F-actin formation, we observe a significant delay in the retraction of the old pseudopod and production of a new pseudopod. We interpret these changes to result from a delay in the F-actin response, although we cannot exclude the possibility that another component of the pathway leading to coronin localization may be affected in phdA or pi3k1/2-null cells. Since a pseudopod is formed by the polymerization of F-actin at the leading edge (Weiner et al. 1999 ), this delay in pseudopod formation is in agreement with the delay in coronin localization and may underlie the phdA chemotaxis defects. Another difference between wild-type and phdA-null cells is that phdA-null cells produce a pseudopod by extending multiple finger-like projections, possibly a result of the F-actin defect. Receptor-mediated activation of adenylyl cyclase and aggregation-stage gene expression are normal, suggesting that PhdA function during aggregation is restricted to the chemotaxis pathway. The defect in F-actin polymerization and subcellular localization is more severe in pi3k1/2-null cells than in phdA-null cells. One possible explanation is that additional PI3K effectors are required for the regulation of F-actin assembly.
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PhdA Lies Downstream from PI3K and May Function as an Adaptor Protein+ K! P9 A! Y) ]2 j) T
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PhdA, PKB, and CRAC all contain a PH domain and translocate to the plasma membrane in response to cAMP stimulation. We present evidence suggesting that this translocation takes place in response to the activation of PI3K and the production of PI(3,4,5)P3 and/or PI(3,4)P2: the translocation is absent in pi3k1/2-null cells; a point mutation in the PH domain (PhdAR41C) blocks the translocation; the translocation requires the function of PI3K1 and PI3K2; and the PI3K inhibitor LY294002 blocks in vivo and GTPS-mediated in vitro translocation. We suggest that in chemotaxing cells, PI3K is preferentially activated at the leading edge, which results in the localized response. Our experiments using a point mutation in the PhdA PH domain suggest that PhdA must translocate to the plasma membrane to function properly. Parallel studies with PKB in Dictyostelium carrying a similar Arg mutation in the PH domain reveal that translocation of the protein to the plasma membrane is required for PKB activation and function (Meili et al. 2000 ).+ T& c/ M' ^2 c7 w! n r# W
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How does PhdA regulate the actin response? We suggest that PhdA functions as an adaptor protein required to mediate responses leading to pseudopod formation at the leading edge. This model is supported by our observation that PhdA carrying a point mutation in the PH domain, which does not translocate, functions as a dominant interfering protein in wild-type cells. Moreover, point mutations in the COOH-terminal domain abrogate PhdA function without affecting its membrane localization, indicating that this domain is required for PhdA function. We propose that the PhdA COOH-terminal domain binds signaling components, possibly those regulating actin assembly, that are required for chemotaxis and localizes them to the leading edge. Expression of PhdAR41C in wild-type cells would inhibit chemotaxis by binding to and sequestering in the cytosol the proposed signaling components. Expression of PhdAR41C in wild-type cells results in an increased PKB activation with phenotypes similar to those of phdA-null cells. PhdA may modulate PKB activation/adaptation, but we do not know if this is direct or indirect. Regardless, we do not think this effect of PhdA is crucial to its role in controlling chemotaxis. Since phdA-null cells can polymerize actin and move, albeit slowly, we suggest that these pathways are not completely abrogated in phdA-null cells and can function, although less efficiently, without PhdA.
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Our in vitro analysis indicates involvement of the GTP-bound form of G proteins in mediating PhdA translocation, but we do not know which G proteins are required. The heterotrimeric G protein associated with the cAMP receptor (G2/?) is required for PKB activation (Meili et al. 1999 ), and a point mutation in the PI3K1 Ras-binding site abrogates the ability of PI3K1 to complement pi3k1/2-null cells with respect to activation of PKB (Meili, R., S. Funamoto, and R.A. Firtel, unpublished observations). Both G2 and Ras may also be required for PhdA translocation in vivo, although we cannot exclude involvement of other G proteins.: K& ]$ b: ?8 W) R1 ~8 p
' I4 s+ x0 J4 f8 u6 HOur work is consistent with the model that the key function of PI3K is to provide binding sites (PIP3 and/or PIP2) for the localization of these proteins to the plasma membrane. The inability of myr-tagged proteins (PhdA and PKB), which localize uniformly along the whole plasma membrane, to complement the null phenotypes is consistent with a model in which the proteins must localize to the leading edge to properly function; the uniform distribution of membrane-localized PhdA may impair chemotaxis by not localizing the response to the leading edge. The observations that mammalian PKB is activated in response to chemoattractants, a mammalian PKB PH domain–GFP fusion localizes to the leading edge in chemotaxing neutrophils, and mammalian PKB is not activated in pi3k-null cells (see Introduction) suggest that the role of PKB in Dictyostelium chemotaxis may be conserved in mammalian cells. Although PhdA does not have a direct homologue in other systems, the requirement for multiple, coordinated, localized effector responses, including actin polymerization and coronin function, at the leading edge in eukaryotic chemotaxing cells suggests that other PH domain–containing proteins with similar functions exist in metazoans, and PI3K provides binding sites for the localization and activation of these proteins.
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! z; M4 D$ A8 e- c0 JFootnotes% W- J+ Y5 z+ r& R' V7 n/ ?# M
. `2 m% I7 V$ k4 }* t: E3 f) J9 U1 Abbreviations used in this paper: CRAC, Ca2 release-activated Ca2 ; GFP, green fluorescent protein; PH, pleckstrin homology; PhdA, PH domain–containing protein A; PI, phosphatidylinositol; PI3K, PI 3'-kinase; PI (3,4,5)P3, PI 3,4,5-triphosphate; PI (3,4)P2, PI 3,4-bisphosphate; PKB, protein kinase B.
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Acknowledgements
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We thank Carole Parent for graciously performing the adenylyl cyclase assays and allowing us to use these data, N. Iranfar and W. Loomis for the PhdA restriction enzyme–mediated integration mutant, Firtel laboratory members for helpful suggestions, and Jennifer Roth for critical reading of the manuscript.
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% G4 N' r4 F/ z+ k' N- T2 F, j1 RS. Funamoto was supported in part by a Japanese Society for the Promotion of Science Research Fellowship for Young Scientists. This work was supported by U.S. Public Health Service grants to R.A. Firtel.Revised: 20 March 2001References; q/ w" c2 F" L3 [8 ~
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5 S/ U# |* P6 x7 r5 w- |Brunet, A., Bonni, A., Zigmond, M.J., Lin, M.Z., Juo, P., Hu, L.S., Anderson, M.J., Arden, K.C., Blenis, J., and Greenberg, M.E. 1999. Akt promotes cell survival by phosphorylating and inhibiting a forkhead transcription factor. Cell 96:857-868.& u2 T( B' t5 I, @+ z4 E
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