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Vol. 14, Issue 5, 1900-1912, May 2003
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* Departement des Maladies Infectieuses, Centre National de la Recherche
Scientifique Unité Mixte Recherche 8104, Institut Cochin, 75014 Paris,
France;
Laboratoire de Physiologie de la reproduction ESA 7080, Centre National de la
Recherche Scientifique/Institut National de la Recherche Agronomique, 75005
Paris, France;
Laboratoire des venims, Institut Pasteur, 75015 Paris, France; and
Laboratoire de Signalisation Immuno-Parasitaire, Unité de Recherche
Associée Centre National de la Recherche Scientifique 1960, Institut
Pasteur, 75015 Paris, France
Submitted August 5, 2002;
Revised January 10, 2003;
Accepted January 16, 2003
Monitoring Editor: David Drubin
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ABSTRACT |
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 TOP ABSTRACT INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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INTRODUCTION |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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). To date, no vaccine or sterilizing drugs are available
against these microorganisms.
Apicomplexan parasites display different life cycle forms and alternate
between extra- and intracellular locations in their hosts. Extracellular
stages are usually polarized cells called zoites, which not only invade host
cells but also are highly motile. Zoite motility is a substrate-dependent, but
unique type of locomotion (Russell and
Sinden, 1981; King,
1988). Most eukaryotic cells that move on a solid substrate crawl
by extending protrusions at their leading edge that adhere to substrate and by
retracting the protrusions the cells move forward
(Heidemann and Buxbaum, 1998;
Small et al., 2002).
In stark contrast, apicomplexan zoites glide on the substrate, without
changing their shape. Forward gliding is thought to result from secretion of
substrate-binding factors at the parasite anterior pole, followed by their
redistribution to the posterior pole. Gliding is exceptionally rapid, 
1
to 20 µm/s in vitro (Preston and King,
1996). This is 1 to several order(s) of magnitude faster than the
speed of the most rapid crawling cells, such as keratocytes
(Small et al., 1999),
amoebae (Van Duijn and Inouye,
1991), and polymorphonuclear cells
(Mitchinson and Cramer,
1996).
Host cell invasion by apicomplexan zoites is a highly dynamic process,
lasting only a few seconds (Morisaki
et al., 1995). The apical tip of the parasite attaches to
host cell receptors and the host cell-parasite junction is then translocated
from the anterior to the posterior pole of the zoite, making the parasite move
into the nascent parasitophorous vacuole formed by invagination of the host
cell plasma membrane (Aikawa et
al., 1978).
Numerous parasite surface molecules have been described in apicomplexan
zoites (Boothroyd et al.,
1998), and some have been proposed to act as parasite adhesins
(Soldati et al.,
2001). Recently, a family of transmembrane proteins (MICs), stored
in the secretory apical organelle called micronems and conserved in the
Apicomplexa phylum has emerged as central to both gliding and invasive
capacities (Sultan et al.,
1997; Kappe et al.,
1999). These proteins are thought to link the extracellular
ligands that are used for parasite traction to a motor system in the parasite
(Ménard, 2001).
Although what provides the force for zoite motility and cell invasion
remains unknown, actin polymerization in the parasite plays a central role.
The use of drugs that interfere with actin polymerization has provided
evidence for the importance of actin dynamics in the parasite during both
gliding and cell invasion in Apicomplexa
(Miller et al., 1979;
Poupel and Tardieux, 1999;
Shaw and Tilney, 1999). In
T. gondii tachyzoites, selection of mutants that are resistant to
cytochalasins demonstrated that parasite and not the host cell actin
polymerization is important for parasite entry into the host cell
(Dobrowolski and Sibley,
1996). A role for myosin motor(s) has been suggested by
Dobrowolski et al.
(1997), and recent
characterization of TgMyoA provided evidence that it contributes to the zoite
motile force (Herm-Götz et
al., 2002; Meissner
et al., 2002).
Besides myosins (Heintzelman and
Schwartzman, 1997), a few actin-binding factors have been
identified in T. gondii. A homolog of the actin depolymerizing
factor/cofilin has been cloned (Allen
et al., 1997). In tachyzoites, we identified Toxofilin as
an actin-binding protein. Toxofilin was purified in a complex with actin
monomers at a 1:1 stoichiometry and shown to regulate association of actin
monomers as well as elongation of actin polymers
(Poupel et al.,
2000). Herein, we report that Toxofilin controls most of the
parasite G-actin that is known to form >95% of the actin pool,
demonstrating that Toxofilin regulation is key to actin dynamics. We identify
and characterize two counteracting Toxofilin regulatory molecules and provide
evidence that these contribute to Toxofilin properties on actin dynamics both
in vitro and in vivo.
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MATERIALS AND METHODS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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). Fresh
tachyzoites (5 x 107 in 1 ml) were exposed to the
cell-permeant kinase inhibitor
5,6-dichloro-1-
-D-ribofuranosylbenzimidazole (DRB; 62.5, 125,
and 250 µM) or to the solvent (ethanol) (90 min, 37°C) and then
incubated with subconfluent HeLa cells. In one control experiment, DRB was
added only during the invasion assay (30 min). Intracellular and extracellular
parasites were labeled as described previously
(Poupel and Tardieux, 1999).
For the gliding assay, glass chamber slides were coated by incubation in 50%
fetal bovine serum diluted in phosphate-buffered saline (PBS) (1 h, 37°C)
followed by rinsing in PBS. Freshly harvested untreated or DRB-treated (250
µM, 90 min, 37°C) tachyzoites were resuspended in PBS (107
in 1 ml) and observed by time-lapse videomicroscopy by using an Axiovert
equipped with a temperature-controlled stage (Carl Zeiss, Jena, Germany).
Images were collected under low-light illumination by using an intensified
charge-coupled device camera (Cool snap HQ; Princeton Scientific Instruments,
Monmouth Junction, NJ) at 63x magnification.
Exposure of Tachyzoite to [32P]Orthophosphate and
Toxofilin Immunoprecipitation
Parasites (5 x 108) were incubated in phosphate free
buffer (10 mM Tris-HCl, pH 7.4, 150 mM NaCl, 5 mM KCl, 5 mM MgCl2,
1.6 mM CaCl2, 0.5% glucose, 0.1% bovine serum albumin) with 250
µCi/ml of orthophosphoric acid (specific activity of 8.8 x
109 Ci/mmol; PerkinElmer Life Sciences, Boston, MA) (120 min,
37°C). Tachyzoites were lysed in 0.4 ml of (30 mM Tris-HCl, pH 7.4, 150 mM
NaCl, 1 mM EGTA, 0.5% Triton X-100, 0.5% Nonidet P-40, 25 mM NaF, 150 µM
orthovanadate, 3 mM NaPO4, 1 mM dithiothreitol, 0.5% [vol/vol] protease
inhibitor stocks). The supernatant (20 min, 20,000 x g,
4°C) was precleared on protein A-Sepharose (Pharmacia AB, Uppsala, Sweden)
(1 h, 4°C). This supernatant does not contain F-actin because we have
previously shown that extraction of the very few tachyzoite actin filaments
required special conditions including jasplakinolide-containing buffer
(Poupel and Tardieux, 1999).
The unbound fraction was successively incubated with Toxofilin antibodies
(overnight, 4°C) and with protein A-Sepharose (2 h, 23°C). Eluates in
SDS-PAGE sample buffer were subjected to 12.5% acrylamide gel electrophoresis.
Gels were dried and scanned for their radioactivity.
Western Blot Analysis
Western blots were performed as described in Poupel and Tardieux
(1999). The antibodies used
were affinity-purified rabbit anti-Toxofilin, rat anti-Toxofilin (1:5000), and
rabbit anti-T. gondii actin antibodies (1:4000). The horseradish
peroxidase-conjugated second antibody was used at 1:10000 (Jackson
Immunoresearch Laboratories, West Grove, PA) (1 h, 23°C). Cross-reactive
proteins were visualized using the ECL system (Pierce Chemical, Rockford,
IL).
Production of rToxofilin for Use as a Substrate of
Kinases/Phosphatases
We used the vector pGEX6-P3 (Pharmacia AB) containing the Toxofilin
encoding cDNA to prepare rToxofilin as described in Poupel et al.
(2000), but we replaced
sarcosyl with N-tetradecyl-N,N-dimethyl-3
ammonio-1-propanesulfonate (0.5% wt/vol) (Sigma-Aldrich, St. Louis, MO) in the
lysate buffer. Soluble rToxofilin was immunoprecipitated with anti-Toxofilin
antibodies (overnight, 4°C) and recovered on protein A dynabeads (2 h,
23°C) (Dynal Biotech, Oslo, Norway) before the kinase/phosphatase
assay.
Identification and Cloning of T. gondii Type 2C
Phosphatase (PP2C)
Native Gel and Peptide Microsequencing. After native
electrophoresis (Poupel et al.,
2000), the gel slice containing the 36-kDa actin-binding
protein was subjected to tryptic digestion (30°C, 18 h, 0.3 mg of trypsin
in 0.1 M Tris-HCl, pH 8.6, 0.01% [vol/vol] Tween 20), and the peptides were
recovered by high-performance liquid chromatography (HPLC). The sequencing of
two peptides gave, respectively, VFDGTVGDFA(Q)ENV and NQSADNITAMTVFFK. The
latter was found in one clone from the T. gondii database of
expressed sequence tags (TgESTzy48A06.r1, November 1999) (WashU-Merk
Toxoplasma EST project; Ajioka et
al., 1998).
cDNA library screening and DNA sequencing: the oligonucleotide with the sequence: 5'-AGTGCAGACAACATTACTGCGATG-3' corresponding to part of one peptide microsequence (SADNITAM) was used as the up stream primer, whereas 5'-AGACACACCAAGAATCTCGTC-3' was chosen as the downstream primer in the TgESTzy48A06.r1clone. After polymerase chain reaction (PCR) amplification, the 207-base pair fragment was 32P labeled (Megaprime kit; Amersham Biosciences, Amersham, United Kingdom) and used to screen a T. gondii tachyzoite cDNA library (kindly provided by J.W. Ajioka, University of Cambridge, Cambridge, United Kingdom). The entire nucleotide coding sequence has been deposited at the European Molecular Biology Laboratory nucleotide sequence database (AJ315476 [GenBank] ).
Production of a Thioredoxin-Hispatch Tg PP2C and Biochemical
Characterization
Recombinant TgPP2C was prepared by PCR amplification of a full-length
TgPP2C encoding cDNA, by using primers introducing an EcoRI
restriction site in 5' and a XbaI restriction site in 3'
(upper strand, 5'-GCCGAATTCCCATGAAGTCCTCTGCTGAAATTAG-3'; lower
strand, 5'-GCCTCTAGACTAATCAGTCTTCTTGAAGAACACTG-3'). The amplified
fragment was cloned into the pThioHis B vector (Invitrogen, Carlsbad, CA).
After induction of protein expression (0.1 mM isopropyl
-D-thiogalactoside, 2 h, 37°C), the fusion protein was
purified on a nickel column (Probond; Invitrogen) followed by a
phenylarsineoxide-agarose column (Thiobond; Invitrogen). Eluates were dialyzed
against buffer A (10 mM Tris-HCl, pH 7.5, 150 mM NaCl) and stored aliquoted at
–80°C. The phosphatase activity of the rPP2C was verified using
32P-labeled casein in presence of PP1/PP2A-sensitive inhibitor
okadaic acid (OA, 1 µM) or 10 mM EDTA as well as in presence of
MgCl2.
Tachyzoite Cytosol Preparation and Heparin Chromatography
Cytosol. Cytosol was prepared from 109 frozen
tachyzoites as described previously
(Poupel et al., 2000)
but in kinase buffer (buffer A supplemented with 10 mM MgCl2, 1 mM
dithiothreitol, 0.2% [vol/vol] protease inhibitor stocks). In some
experiments, cytosols were depleted in PP2C by incubation with 2 µg of the
affinity-purified polyclonal anti-T. gondii PP2C antibodies and then
with protein A-Sepharose. Control cytosol precleared on protein A-Sepharose
and PP2C-depleted cytosol were then subjected to kinase assay.
Heparin Chromatography. A cytosol from 109 parasites was precleared on Sepharose CL-4B and chromatography performed on heparin Sepharose CL-4B (Pharmacia AB) (1 h, 4°C). After several washes, the heparin-bound proteins were eluted in 10 mM Tris-HCl, pH 7.5, 0.5 M NaCl. The eluate was dialyzed against kinase buffer before the kinase assay.
Kinase and Phosphatase Assays
Kinase Reaction on rToxofilin. Two micrograms of
immobilized rToxofilin was incubated with a tachyzoite cytosol prepared from 2
x 108 (100 µl) and precleared on protein A dynabeads. The
reaction was started by adding 100 µM Na2NTP and 10 µCi of
the same [
32P]NTP (ATP, 3000 Ci/mmol; GTP, 6000 Ci/mmol;
PerkinElmer Life Sciences) (15 min, 30°C). After washes, rToxofilin and
bound proteins were eluted in SDS-PAGE sample buffer before electrophoresis
and radioactivity scan (PhosphorImager; Amersham Biosciences, Sunnyvale, CA).
To characterize the rToxofilin kinase(s) five types of reagents were used: 1)
[32P]GTP as a unique phosphate source; 2) pharmacological
inhibitors such as heparin (20 µg/ml; Sigma-Aldrich), DRB (100 µM),
chrysin (100 µM; Sigma-Aldrich), emodin (100 µM; Sigma-Aldrich), or
staurosporine (10 µM; Calbiochem, San Diego, CA); 3) heparin chromatography
eluate and the corresponding unbound fraction; 4) purified human recombinant
CKII (
dimer or tetramer, 250 ng) (gift from C. Cochet,
INSERM 4244, Grenoble, France); and 5) a standard CKII peptide substrate
(Upstate Biotechnology, Lake Placid, NY).
Kinase Reaction on Tachyzoite Cytosol. Control and
PP2C-immunodepleted cytosols were incubated with 100 µM Na2 ATP
and 10 µCi of [32P]ATP (15 min, 30°C). Kinase
reactions were stopped by addition of SDS-PAGE sample buffer and analyzed by
SDS-PAGE followed by radioactivity scan.
Phosphatase Reaction on rToxofilin. The purified rPP2C was added (5 or 20 µg) during or after the kinase assay. In some control experiments, 1 unit of a recombinant fragment of rabbit catalytic type 1 phosphatase (Upstate Biotechnology) was replacing rPP2C. In experiments where the phosphatase assay was performed on Ser53phosphorylated rToxofilin, the latter was incubated with cytosol supplemented with 10 mM MgCl2, 2 mM EDTA or a combination of 10 mM MgCl2 and 2 µM OA. Eluates containing rToxofilin were treated as described for the kinase assay.
Enzymatic Digestion of 32P-labeled rToxofilin, HPLC, and
Covalent Sequencing
rToxofilin (10 µg) was phosphorylated using either a tachyzoite cytosol,
an eluate after heparin chomatography, or a purified human casein kinase II.
After SDS-PAGE, phosphorylated rToxofilin was excised as a band from the gel
and incubated with 0.4 µg of endolysine-C in 50 mM Tris-HCl, pH 8.6, 0.01%
(vol/vol) Tween 20 (1 h, 35°C). The peptides were separated by HPLC and
eluted with a 20–70% acetonitrile, 0.1% trifluoroacetic acid gradient.
The radioactivity contained in each collected fraction was measured using a
Cerenkov counter. Radioactive peptides were covalently fixed to Sequelon AA
filter (Millipore, Bedford, MA) and sequenced in a 494 sequencer (Applied
Biosystems, Foster City, CA).
Cloning, Expression, and Purification of Recombinant T.
gondii Casein Kinase II Catalytic Subunit
Using the EST (GenBank accession no. BM 189807) and the contigs TGG_ 3802
and TGG_2216, we reconstituted an open reading frame consistent with the
CKII protein sequence. Indeed, alignment of the translated sequence
with known CKII proteins from related organisms, including
Theileria parva (GenBank accession no. M92084
[GenBank]
) and higher organisms
confirmed that the reading frame was encoding a CKII protein. The
reverse primer 5'-GAACTCCGCAAGACCCCAGTCG-3' was used in a reverse
transcription reaction containing 30 U of avian myeloblastosis virus reverse
transcriptase (Finnzymes) under conditions specified by the supplier except
that the reaction was carried out on 3 µg of RNeasy kit (QIAGEN, Valenica,
CA)-purified parasite mRNA. Reverse transcriptase product was amplified using
PCR with the same reverse primer and the forward primer
5'-CGAGTACTGGGACTACGAGAAC-3'. The PCR product was cloned into
pCRT7/CT-TOPO vector (Invitrogen) and verified by nucleotide sequencing. After
induction of protein expression (1 mM isopropyl
-D-thiogalactoside, 2 h, 37°C), the fusion protein was
purified on a nickel column (Probond; Invitrogen) and the imidazole eluate was
dialyzed against 10 mM Tris-HCl, pH 7.5, 150 mM NaCl, 10 mM MgCl2
(2 h, 4°C). It was readily tested in kinase assay with a synthetic
Toxofilin peptide encompassing Ser53 by using the CKII assay kit
(Upstate Biotechnology). Bacteria that did not carry plasmid were treated
similarly to get a control of bacterial kinase activity on the Toxofilin
peptide.
Site-directed Mutagenesis on rToxofilin
Using the Quickchange site-directed mutagenesis kit (Stratagene, La Jolla,
CA), we introduced a single amino acid mutation in rToxofilin replacing serine
at position 53 by alanine by using the following primers:
5'-GGAAGATTCGAGGCTGGAGACGAAG-3' and
5'-CTTCGTCTCCAGCCTCGAATCTTCC3' or by glutamic acid by using
5'-GGAAGATTCGAGGAGGGAGACGAAG-3' and
5'-CTTCGTCTCCCTCCTCGAATCTTCC. Positive bacterial clones were verified by
nucleic sequencing. rToxofilin mutants (S53A and S53E) were prepared as for
wild-type rToxofilin (WT) and subjected to kinase assay.
Ectopic Expression of Green Fluorescent Protein (GFP)-WT and Mutant
Toxofilin Fusion Proteins in Fibroblastic Cells
Fibroblastic cell line derived from African green monkey kidney (CV1 line)
was transfected with the plasmids encoding GFP-WT, GFP-S53A, or S53E
Toxofilin. F-actin was visualized as described in Poupel et al.
(2000). The samples were
examined under an Axiovert (Carl Zeiss). Images were acquired and analyzed
using a charge-coupled device coolsnap HQ camera and the MetaMorph imaging
system.
Surface Plasmon Resonance Experiments
They were performed at 25°C using a Biacore 2000 system (Biacore AB,
Uppsala, Sweden). rToxofilin S53E and WT were covalently coupled via
primary amino groups on CM5 sensor chips surface
(Faure et al., 2000).
The surface plasmon resonance signals for immobilized Toxofilin on two
different flow cells were found to be 1400 pg ·
mm–2 for S53E and 1960 pg ·
mm–2 for WT. The interaction between G-actin and
the chip-immobilized Toxofilin was studied by injecting dilutions of G-actin
(25–400 µg/ml, 2 min, 10 µl/min flow rate). The kinetic constants
kon and koff for the interaction of
G-actin with immobilized Toxofilin were calculated using Biacore BIAEVALUATION
3.1 software (Schuck,
1997).
|
RESULTS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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). To further evaluate whether Toxofilin is a major player in
actin dynamics in T. gondii, we first asked whether Toxofilin bound
most of the parasite G-actin. For this, we immunoprecipitated Toxofilin from
the precleared tachyzoite cytosol by using anti-Toxofilin antibodies and
probed the nonprecipitated material with anti-Toxofilin and anti-actin
antibodies. As shown in Figure
1, immunoprecipitation of Toxofilin (lane b) efficiently depleted
Toxofilin as well as most of G-actin (lane c) from the tachyzoite cytosol
(lane a). Similar results were obtained when DNAse 1 chromatography was
performed (Poupel et al.,
2000), whereas preimmune sera did not precipitate Toxofilin or
actin (our unpublished data). This showed that most G-actin is complexed to
Toxofilin in the tachyzoite cytosol, and thus suggested that Toxofilin may
play a key role in parasite actin dynamics.
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We previously reported that an additional and less abundant 36-kDa
polypeptide copurified with the actin–Toxofilin complex isolated in
native gels (Poupel et al.,
2000). Large amounts of the complex were prepared and the
36-kDa polypeptide was subjected to tryptic digestion and the peptide
sequence was derived. Based on these amino acids, a DNA probe was synthesized
and a T. gondii cDNA library screened and 12 positive clones
corresponding to the same gene selected. This gene encodes a 331 amino acid
polypeptide, with a theoretical isoelectric point of 5.44 and expected
molecular mass of 36.81 kDa. It is homologous to a variety of eukaryotic type
2C serine-threonine phosphatases (PP2C), including those from closely related
protozoans (Figure 2). PP2Cs
form a distinct group among the serine/threonine protein phosphatases that are
known to display 11 conserved motifs scattered along the catalytic domain,
with eight perfectly conserved amino acid residues that serve as a PP2C
signature in both eukaryotes and prokaryotes
(Shi et al., 1998)
(Figure 2). Among these, it has
been proposed that Asp residues (45, 67, 273, and 318), together with Glu-44
and Gly-68, coordinate the active site metal ions
(Das et al., 1996).
Indeed, PP2Cs are defined by their Mn2+ or
Mg2+ ion dependence and their insensitivity to
pharmacological agents blocking the other serine threonine phosphatase groups
(Cohen, 1989). Of note, as
described for bacteria (Obuchowski et
al., 2000), but not for P. falciparum, T. gondii
PP2C sequence lacks His69 within the conserved motif DGH (motif II), a residue
that has been shown to be critical for mouse PP2C activity in vitro
(Kusuda et al.,
1998).
|
Next, the functional activity of the Toxofilin-associated PP2C was assessed: when 32P-labeled casein was incubated with the Toxofilin immunoprecipitate, 3.14 ± 0.16 pmol of phosphocasein were dephosphorylated after a 90-min incubation at 30°C (three separate experiments). To check whether the phosphatase activity found in the Toxofilin immunoprecipitate was selective for type 2C the 32P-casein dephosphorylation assay was performed in the presence of OA, a potent inhibitor of type 1 and type 2A phosphatases. Incubation with OA up to 1 µM did not affect dephosphorylation of phosphocasein, whereas the presence of magnesium was required (our unpublished data). The PP2C activity associated with the Toxofilin immunoprecipitate was estimated as 0.3% of the total PP2C activity measured in cytosol.
Toxofilin Is Phosphorylated In Vivo and In Vitro
To analyze the relevance of the association of PP2C with Toxofilin, we
investigated whether Toxofilin is phosphorylated both in vivo and in vitro.
Therefore, tachyzoites were incubated with [32P]orthophosphate and
Toxofilin was immunoprecipitated using rabbit anti-Toxofilin antibodies. As
shown in Figure 3A, the
immunoprecipitate contained a 32P-polypeptide of the apparent size
of Toxofilin that was recognized by rat polyclonal anti-Toxofilin antibodies
(bottom). Furthermore, we incubated immobilized rToxofilin with the tachyzoite
cytosol in presence of [32P]NTP. As shown in
Figure 3B (lane a), rToxofilin
was readily detected after SDS-PAGE and Coomassie staining. Gel
autoradiography indicated that a major 32P signal comigrated with
rToxofilin (lanes b and c). No 32P signal was detected comigrating
with rToxofilin when the assay was performed in the absence of rToxofilin
(lane d). This indicated that rToxofilin is phosphorylated under these in
vitro conditions.
|
Toxofilin Is Phosphorylated by a CKII-like Parasite Kinase Activity
and by Human CKII
We then attempted to identify the type of kinase activity that
phosphorylates Toxofilin by using a variety of kinase inhibitors. Six putative
phosphorylation sites were recognized in Toxofilin sequence by using the
PROSITE software, among which three were consensus sites for CKII
(23TASE, 53SGDE, and 165TLLE). We found that
staurosporine, one of the most potent specific inhibitors of serine/threonine
protein kinases that remains poorly effective on CKII
(Meggio et al.,
1995), did not significantly inhibit rToxofilin phosphorylation by
the parasite cytosol (Figure
3B, lane j), compared with the control (lane f). Various
inhibitors of CKII have been described, such as glycosaminoglycan heparin
(O'Farrell et al.,
1999), the nucleotide analog DRB, chrysin, and emodin. Chrysin and
DRB are thought to specifically inhibit CKII activity
(Shugar, 1994;
Critchfield et al.,
1997), whereas emodin inhibits CKII, but is poorly effective on
other serine/threonine protein kinases
(Battistutta et al.,
2000). When the tachyzoite cytosol was incubated with any of the
CKII inhibitors before the phosphorylation assay, the level of rToxofilin
phosphorylation was markedly decreased
(Figure 3B, lanes e and
g–i).
CKII can use both GTP and ATP as phosphate donor
(Allende and Allende, 1995). In
agreement with the involvement of a CKII-like activity in Toxofilin
phosphorylation, rToxofilin was efficiently phosphorylated in our assay
performed with GTP (Figure 3B,
lane c). CKII activity is also defined by its lack of dependence on second
messengers such as cyclic nucleotides or calcium, which are important for the
activity of calcium-calmodulin–dependent protein kinases or
cAMP/cGMP-dependent kinases (Guerra et
al., 1999). We found that rToxofilin phosphorylation did not
depend on cyclic nucleotides or calcium (our unpublished data). Heparin
chromatography has been used extensively for CKII purification in a variety of
systems (Litchfield et al.,
1990a). Therefore, we subjected the tachyzoite cytosol to heparin
Sepharose chromatography and tested whether the eluate could phosphorylate
rToxofilin. As shown in Figure
3C, it contained most of the rToxofilin kinase activity (lane b),
whereas the flow-through material was markedly depleted in rToxofilin kinase
activity (lane c). In addition, when heparin was added to the eluate before
the assay, rToxofilin phosphorylation was significantly diminished (lane d).
As a control, when the assay was performed with the eluate, but in the absence
of rToxofilin no 32P signal was detected at the size of rToxofilin
(lane e). We next asked whether purified human CKII could phosphorylate
rToxofilin. CKII is a heterotetramer composed of two catalytic subunits
( or ') associated with two regulatory subunits (
and '). We observed in vitro that the catalytic subunit
(lane f), as well as the tetramer 22 (lane
g) of human CKII phosphorylated rToxofilin. At equimolar concentration, the
22 tetramer induced higher levels of
phospho-transfer onto rToxofilin than the 2 dimer, which is
in agreement with the known enhancing/stabilizing role of subunit on
the subunit kinase activity
(Meggio et al.,
1992). Acidic synthetic phosphopeptides have proven to be useful
tools for isolating CKII, or CKII-like activities
(Litchfield et al.,
1990b). Therefore, we tested whether the CKII consensus substrate
RRRDDDSDDD could be a target for the parasite cytosol and for the parasite
fraction eluted of heparin Sepharose. By using similar concentrations of total
proteins, the parasite cytosol exhibited a moderate kinase activity on the
peptide, whereas the heparin eluate was 5–10 times more active in
catalyzing 32P transfer to the substrate
(Figure 3D). Addition of a
protein kinase A cocktail inhibitor (Upstate Biotechnology) to the
kinase-containing fraction did not significantly change the amount of
32P transfer to the CKII peptide (our unpublished data), indicating
that a potential parasite protein kinase A activity is not responsible for the
phosphorylation of the CKII peptide substrate. These results demonstrate that
the kinase activity enriched in the heparin eluate can catalyze phosphate
transfer to a consensus CKII peptide. Together, these data strongly suggest
that a tachyzoite CKII-like activity is the major source of Toxofilin
phosphorylation.
CKII-like Kinase and PP2C Control Ser53 rToxofilin
Phosphorylation
To identify the Toxofilin phosphorylation site(s), we incubated rToxofilin
with [32P]ATP in the presence of either the
Toxofilin-kinase–enriched eluate, or purified human CKII. From all the
rToxofilin peptides generated after endolysine digestion, only one contained
detectable amounts of radioactivity. This peptide was then subjected to
covalent sequencing, which allowed the detection of significant radioactive
counts only associated to Ser53
(Table 1).
|
Therefore, these data strongly suggest that Ser53 of rToxofilin is the target for both a T. gondii CKII-like kinase and a human CKII
First, to confirm that Toxofilin Ser53 is a substrate for T.
gondii CKII, we attempted to clone and express recombinant T.
gondii CKII before performing kinase assays. Using both an EST
(TgEST BM189807
[GenBank]
) and contigs (TGG_3802 and TGG_2216), we cloned and sequenced
the CKII catalytic site, which is shown aligned with other known CKIIs
(Figure 4A). Of note, T.
gondii CKII displays 29% identity to human CKII and only
28% identity with CKII of the related parasite Theileria parva
(Figure 4A). After expression
and semipurification of the CKII recombinant polypeptide, CKII kinase
assays were performed using a synthetic peptide derived from the Toxofilin
sequence that contains Ser53 (RFESGDEG). As shown in
Figure 4B, recombinant
T.gCKII catalyzes 32P transfer onto the Toxofilin peptide,
as does human recombinant CKII, whereas, in contrast, no transfer was observed
with the control bacterial lysate.
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Second, we checked whether Toxofilin Ser53 is important for
rToxofilin activity. To this end, we constructed rToxofilin mutants in which
Ser53 was replaced by either an alanine residue (S53A) or by a
glutamic acid residue (S53E). As shown in
Figure 5, [32P] incorporation into S53A rToxofilin was greatly
decreased after incubation with either the purified recombinant human CKII
(lane b) or the Toxofilin kinase-enriched fraction (lane e), compared with the
wild-type rToxofilin. As expected, 32P incorporation into
S53E rToxofilin was equally reduced by both source of kinases (lanes c and f).
Indeed, although glutamic acid mimics a constitutively active phosphorylated
state, it is not a phosphate acceptor. These data confirm that
Ser53 is the major site of Toxofilin phosphorylation by a CKII-like
kinase, but because we observed a very faint 32P signal in the
mutants, CKII might also weakly phosphorylate other sites.
|
We then asked whether Toxofilin-bound PP2C dephosphorylates Toxofilin. To this end, a ThioHis-PP2C fusion protein (rPP2C) was produced, and its phosphatase activity was assayed on rToxofilin. We found that rToxofilin phosphorylation was markedly decreased upon addition of purified rPP2C in the kinase assay and the effect was dose dependent (Figure 6A, lanes c and d). In contrast, addition of purified human PP1 did not decrease rToxofilin phosphorylation by the cytosolic fraction (Figure 6A, lane b). We also compared phosphorylation of cytosolic proteins by using either the native cytosol or the PP2C-immunodepleted cytosol. As shown in Figure 6B, several cytosolic proteins displayed higher phosphorylation levels in the absence, compared with the presence of PP2C (compare lanes b and a). Interestingly, the major hyperphosphorylated protein comigrated with Toxofilin (Figure 6C). These data demonstrate that T. gondii endogenous and recombinant PP2C dephosphorylates Toxofilin and rToxofilin, respectively. To test whether native PP2C directly dephosphorylates Toxofilin on Ser53, phosphorylated rToxofilin was produced using human CKII and subsequently incubated with the cytosol. As shown in Figure 7A, Ser53-phosphorylated rToxofilin was dephosphorylated by the cytosol (lane b). In contrast, rToxofilin remained phosphorylated in control buffer (lane a). Furthermore, we found that the phosphatase activity contained in the cytosol required magnesium (lanes b and c) and was insensitive to OA (lane d). These data provide strong evidence that Ser53 dephosphorylation is induced by a selective type 2C phosphatase activity, and not by type 1 or type 2A phosphatases. Finally, to address the question of a potential parasite cofactor for PP2C, we compared the efficacy of rPP2C and endogenous PP2C on dephosphorylation of Ser53. Ser53 phosphorylated rToxofilin was incubated with either buffer, rPP2C or the cytosol, by using the same amount of magnesium-dependent phosphatase activity from both sources. We found that the cytosol contained a specific activity 13 fold higher than the same volume of rPP2C. As illustrated in Figure 7B, under these conditions, rToxofilin remained phosphorylated in presence of buffer (lane a). In contrast, rToxofilin was dephosphorylated by the rPP2C (lane b) and by the cytosol (lane c), but to a much greater extent upon exposure to cytosol. These data raise the question of incomplete folding of the rPP2C, compared with the native molecule. In spite of this possibility, rPP2C was very efficient when added to the cytosol (Figure 6A) and this suggests that a cytosolic cofactor might optimize its phosphatase activity.
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Ser53 Is the Major Site of Toxofilin Phosphorylation and
Is Important for Toxofilin Function In Vitro as In Vivo
To best visualize the effect of Ser53 substitution on
actin dynamics, we used a fibroblastic cell line (CV1) known to display
abundant actin stress fibers. As previously described for transfected
epithelial HeLa cells (Poupel et
al., 2000), ectopic expression in CV1 cells of wild-type
GFP-Toxofilin induced a profound disorganization of actin filament with a
major breakdown of actin stress fibers
(Figure 8, bottom left). CV1
cells expressing either GFP-Toxofilin S53A or GFP-Toxofilin S53E exhibited
extremely opposite phenotypes, because the former displayed significant
amounts of actin stress fibers (Figure
8, top right, see white arrows), whereas the latter displayed a
dramatic loss of actin stress fibers
(Figure 8, bottom right). These
data showed that Ser53, and presumably its phosphorylation state in
vivo, are implicated in the control of Toxofilin properties on actin dynamics.
To check whether the effect of Toxofilin Ser53 substitution on
actin dynamics in vivo could reflect a modification in Toxofilin-actin binding
properties in vitro, we used the Biacore technique. This allowed us to compare
the kinetic parameters of G-actin binding to unphosphorylated Ser53
Toxofilin (WT) and to the phosphorylated state of Toxofilin (S53E). As
illustrated in Table 2, G-actin
binds to WT with an association rate constant (kon)
threefold increased compared with Ser53E and a dissociation rate constant
(koff) fourfold decreased, leading to a 14-fold increase
in Kdapp. Therefore, these data suggest a potential role
for phosphorylation on Ser53 in the Toxofilin-G–actin
interaction.
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CKII Inhibitor DRB Decreases Invasion of T. gondii
Tachyzoites into Mammalian Cells
Because DRB inhibits rToxofilin phosphorylation in vitro and because it has
been characterized as a cell-permeant molecule, we tested whether DRB
treatment could affect tachyzoite motile properties. We exposed parasites to
DRB and assessed their gliding activity as well as their invasiveness to host
cells. When untreated parasites were added to serum-coated glass and observed
by phase contrast videomicroscopy, a majority displayed typical circular
forward gliding motility (Figure
9A, top), whereas DRB-treated parasites did not move forward,
although bending and twirling were still frequently seen
(Figure 9A, bottom). Regarding
parasite invasiveness, when DRB-treated parasites were incubated with HeLa
cells in presence of the drug, their invasive capacities were significantly
impaired in a dose-dependent manner (Figure
9B). In contrast, when parasites were exposed to the highest
concentration of DRB (250 µM) only during the invasion assay, no loss of
parasite invasiveness was detected, which excludes that reduced invasion is
due to an effect of DRB on the host cells. In addition,
Figure 9C shows that the
average number of tachyzoites within an infected cell decreases with
increasing concentrations of DRB. As assessed using ethidium bromide and
calcein (Molecular Probes), DRB-treated parasites were alive and did not
display any plasma membrane damage (our unpublished data). Together, these
results suggest that a parasite CKII activity is required for tachyzoite
motile properties.
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DISCUSSION |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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),
whereas F-actin could be detected biochemically under special conditions
(Poupel and Tardieux, 1999).
The only molecule that has been found to bind actin in Apicomplexa, apart from
myosins, is Toxofilin, a protein with no homolog in the database. Toxofilin
binds G-actin both in vivo and in vitro and caps barbed-end actin filaments
(Poupel et al.,
2000). This study describes how Toxofilin properties are
regulated.
Toxofilin Is Phosphorylated by a CKII Kinase
CKII is a highly conserved serine/threonine protein kinase found in all
eukaryotes examined so far that catalyzes phosphate transfer onto a large
number of proteins (Allende and Allende,
1995). CKII activity has already been involved in processes that
require actin recruitment, such as the formation of cell-cell adherens
junctions (Lickert et al.,
2000). More directly, muscle actin has been shown to selectively
inhibit CKII kinase in vitro in a dose-dependent manner
(Karino et al.,
1996). Several lines of evidence indicate that a CKII-like
activity phosphorylates Toxofilin in T. gondii. First, the phosphate
source for Toxofilin phosphorylation by the parasite cytosolic kinase may be
either ATP or GTP nucleotides. Second, the parasite kinase activity is
inhibited in the presence of CKII inhibitors such as soluble heparin, DRB,
chrysin, and emodin at doses usually active in vitro. Third, Toxofilin
phosphorylation is insensitive to staurosporine, a broad-spectrum
serine/threonine kinase inhibitor, or to second messengers, such as calcium
and cyclic nucleotides, features that characterize a CKII-like kinase
activity. Finally, as expected for a CKII activity, the Toxofilin kinase
activity could be recovered by heparin chromatography. The purified activity
catalyzed 32P incorporation into both recombinant Toxofilin and a
synthetic peptide acting as a consensus substrate for mammalian CKII.
In agreement with these data, we cloned in Toxoplasma a cDNA sequence
displaying significant similarities to CKII from both apicomplexan
parasites and higher eukaryotes, confirming the sequence as a bona fide
CKII. In P. falciparum, at the time of this study, eight
contigs in the genome database (chr2_11953, chr3_3P8, chr7_000012,
chr7_000106, chr8_000118, chr11_1, chr12_1, and chr13_1000007; Plasmo
database, June 2002) display a high degree of sequence similarity with
CKII from other eukaryotes. In T. parva and T.
annulata, CKII has been already cloned and characterized
(Ole-MoiYoi et al.,
1992). Importantly, the recombinant T. gondii CKII
polypeptide successfully catalyzed 32P transfer onto a Toxofilin
synthetic peptide encompassing the serine residue that we characterized as
phosphate acceptor.
Toxofilin Is Dephosphorylated by a PP2C-like Phosphatase
PP2Cs have been mostly implicated in a variety of cell types, in the
control of cyclin dependent-kinase Cdk2
(Chen et al., 1999),
as well as a number of mitogen-activated protein kinases
(Hanada et al.,
2001). PP2C has also been connected to actin dynamics. For
example, in Arabidopsis thaliana and Commelina communis, the
ABI1 and ABI2 PP2Cs contribute to the absidic acid-induced actin filament
reorganization observed during stomatal closure
(Merlot et al.,
2001). In addition, human platelet PP2C dephosphorylates moesin in
vitro, affecting its binding to F-actin
(Huang et al., 1999).
In P. falciparum, an unusual PP2C has been cloned that carries two
successive catalytic domains and requires dimerization for optimal activity
(Mamoun et al.,
1998). One potential substrate of the P. falciparum PP2C
is the elongation factor 1 (Mamoun
and Goldberg, 2001).
We have shown herein that the 36.8-kDa component of the
Toxofilin–actin complex is a PP2C type phosphatase: the corresponding
amino acid sequence displays the eight critical amino acid residues conserved
in all members of the PP2C family. In addition, we have shown that Toxofilin
is selectively dephosphorylated by endogenous or recombinant PP2C, but not by
human PP1 that has been shown to be active on several T. gondii
molecules (Delorme et al.,
2002).
Toxofilin Ser53 Is the Site for Regulation and Control of
Actin Dynamics by PP2C and CKII In Vivo
The phosphorylation site on Toxofilin was mapped at
Ser53 by using a kinase assay with heparin eluate, or
human CKII as source of kinase. This residue lies within a CKII
phosphorylation consensus site, ES53GDEG, which contains the
canonical D at +2 and E at +3 (Songyang
et al., 1996). Furthermore, in vitro 32P
incorporation in S53A, or S53E Toxofilin mutants was markedly inhibited using
either the parasite heparin-bound eluate, or the human CKII. Interestingly, a
PP2C activity present in the parasite cytosolic fraction dephosphorylates
Ser53-phosphorylated Toxofilin more efficiently than recombinant
PP2C. This may suggest that other isoforms of PP2C might be expressed and
efficient at dephosphorylating Toxofilin. It might also be that a cytosolic
molecule modulates PP2C activity on Toxofilin and no such regulatory molecule
have been yet described for PP2Cs in other eukaryotic systems. If selectivity
to Toxofilin and potentially to other parasite PP2C substrates is conferred by
partner(s), these might become potential drug targets.
In vivo, the Ser53 residue seems key to the function of
Toxofilin on actin assembly/disassembly. Indeed, upon expression of WT
Toxofilin in fibroblasts, we observed that most of the actin stress fibers had
disassembled, an observation similar to what we previously reported upon
expression in epithelial cells. In these cells, the GFP-WT Toxofilin, but not
the GFP alone, is found phosphorylated (our unpublished data) but presumably,
not all the WT Toxofilin is. In contrast, the whole population of S53E
Toxofilin behaves like phosphorylated and in terms of phenotype, its
expression induced an even more striking disorganization of actin stress
fibers. However, the Toxofilin-Ser53E mutant protein may not necessarily
behave in exactly the same way in vitro or in cells. In contrast, expression
of the S53A Toxofilin-GFP fusion did not significantly affect actin stress
fiber organization. In addition, our in vitro study using the Biacore system
confirmed these results by showing that the stability of the
actin–Toxofilin complex depends on the phosphorylation status of
Ser53. The phosphorylation of Ser53 on Toxofilin
decreased the affinity for G-actin and if we extrapolate this to the in vivo
situation observed in fibroblasts, we may speculate that the massive
disorganization of actin stress fibers triggered by S53E Toxofilin results
more from an effect on F-actin. We have shown that Toxofilin caps actin
filaments (Poupel et al.,
2000), and we have data characterizing a Toxofilin severing
activity on F-actin (our unpublished data). Finally, using time-lapse
videomicroscopy, we bring evidence that the parasite CKII activity is required
for both gliding and host cell invasion, because DRB treatment that strongly
inhibited rToxofilin phosphorylation in vitro also impaired tachyzoite
gliding.
A connection between CKII and PP2C has been recently suggested in the
microplasmodia Physarum polycephalu. First, De Corte et al.
(1996) reported that fragmin
could be phosphorylated in vitro by a CKII-type enzyme without modifying
fragmin properties. Second, a large 46-kDa type 2C phosphatase that
dephosphorylates CKII phosphorylated-fragmin has been described previously
(Waelkens et al.,
2000). Nonetheless, neither CKII nor PP2C regulators were detected
associated with the actin–fragmin complex.
Our study shows that Toxofilin's properties on actin are mediated by
phosphorylation of Ser53 residue through a balance between the
counteracting T. gondii CKII kinase and PP2C phosphatase
activities. Although the intrinsic properties of actin seem well conserved
among "lower and higher" eukaryotes and are central to both cell
crawling and gliding motility, it is noteworthy that the phylum of
apicomplexan has selected unique mechanisms underlying the speed and the
nature of their gliding motion. Such unique mechanisms could integrate
transient interactions between Toxofilin, actin, and signaling molecules.
Future dissection of the phosphate flux onto Toxofilin within parasites will
provide clues on the spectacular dynamic character of actin in these
cells.
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ACKNOWLEDGMENTS |
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TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
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Footnotes |
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Corresponding author. E-mail address: tardieux{at}cochin.inserm.fr.
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W. Daher, G. Oria, S. Fauquenoy, K. Cailliau, E. Browaeys, S. Tomavo, and J. Khalife A Toxoplasma gondii Leucine-Rich Repeat Protein Binds Phosphatase Type 1 Protein and Negatively Regulates Its Activity Eukaryot. Cell, September 1, 2007; 6(9): 1606 - 1617. [Abstract] [Full Text] [PDF]
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P. J. Bradley, C. Ward, S. J. Cheng, D. L. Alexander, S. Coller, G. H. Coombs, J. D. Dunn, D. J. Ferguson, S. J. Sanderson, J. M. Wastling, et al. Proteomic Analysis of Rhoptry Organelles Reveals Many Novel Constituents for Host-Parasite Interactions in Toxoplasma gondii J. Biol. Chem., October 7, 2005; 280(40): 34245 - 34258. [Abstract] [Full Text] [PDF]
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