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r1,2Correspondence to Lydia Tabernero: lydia.tabernero{at}man.ac.uk; or Keith R. Matthews: keith.matthews{at}ed.ac.uk
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The life cycle of T. brucei is divided between a mammalian host and the tsetse fly (Matthews, 2005). In mammals, the parasite population consists of proliferative slender cells and nonproliferating stumpy forms, which are arrested in G1/G0 (Matthews et al., 2004). The transition between these forms occurs in response to a parasite-derived signal in the bloodstream (Vassella et al., 1997), resulting in an accumulation of stumpy forms. This optimizes parasite transmissibility because stumpy forms are preadapted for uptake into the tsetse fly (Engstler and Boshart, 2004). In particular, they have up-regulated certain metabolic activities in preparation for life in the fly and are more resistant to proteolytic attack and pH fluctuations (Sbicego et al., 1999; Nolan et al., 2000). In the tsetse, stumpy forms differentiate to procyclic forms, a transition that can be efficiently reproduced in culture by cis aconitate and a reduction of temperature (Ziegelbauer and Overath, 1990). Once stimulated to differentiate, stumpy forms embark on a precisely programmed developmental pathway involving changes in cell morphology, metabolic activity, surface antigen expression, and gene expression. Importantly, the generation of stumpy forms in the bloodstream represents an irreversible commitment to differentiate; stumpy forms not taken up in a fly blood meal ultimately degenerate in the bloodstream (Turner et al., 1995).
In higher eukaryotes, tyrosine phosphorylation is a well-characterized mechanism for regulating cell growth and differentiation, as well as many other aspects of cell life (Neel and Tonks, 1997; Tonks, 2003). However, less is known about tyrosine phosphorylation events in lower eukaryotes and prokaryotes. For example, in bacteria, protein tyrosine phosphorylation is a rare occurrence and yet tyrosine phosphatases are essential for infection and survival of pathogenic species like Salmonella, Yersinia, or Mycobacterium (Black et al., 2000; Lin et al., 2003; Singh et al., 2003). Kinetoplastid parasites such as Trypanosoma spp. and Leishmania spp. occupy an interesting evolutionary niche, being unicellular organisms and among the most diverged representatives of the eukaryotic world. Although intracellular signaling events have not yet been described in detail for these organisms, it is likely that tyrosine phosphorylation will also play a role in cellular processes as in higher eukaryotes. Supporting this, there is evidence that several proteins are phosphorylated on tyrosine residues in kinetoplastids (Parsons et al., 1991; Cool and Blum, 1993) presumably through the activity of dual-specificity protein kinases, as kinetoplastid genomes do not encode any recognizable tyrosine-specific kinases (Parsons et al., 2005). Tyrosine phosphatase activity also shows marked differences among different life cycle stages in both T. brucei and T. cruzi (Bakalara et al., 1995a).
From the precedent in higher eukaryotes, it is likely that phosphotyrosine phosphatases will be also relevant in the control of cell growth and development in kinetoplastids. Supporting this idea, it was recently reported that the heterologous expression of the human PTP1B gene in Leishmania, together with the inhibition of tyrosine kinases, promoted partial differentiation from promastigote to amastigote forms (Nascimento et al., 2003). Here, we demonstrate that the activity of a T. brucei protein tyrosine phosphatase, TbPTP1, exhibits a pivotal function in parasite differentiation. Biochemical characterization of the enzyme demonstrates that it is a tyrosine-specific phosphatase whose enzymatic activity is regulated by pH and changes in its oxidation state. Importantly, when TbPTP1 activity is inhibited by RNAi or biochemically, differentiation to procyclic forms occurs spontaneously in the absence of any exogenous trigger. This response is restricted to a subset of bloodstream cells, which we propose are those already committed to differentiation. Supporting this, tyrosine phosphatase inhibition in a homogeneous population of stumpy forms triggers synchronous, efficient, and complete differentiation to proliferative procyclic forms. These data reveal that a tyrosine phosphatase activity is a key molecular regulator of the initiation of trypanosome differentiation, providing a potential pharmacological target to restrict parasite transmissibility and virulence.
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Previous evidence that protein phosphatase activities were differentially regulated during the trypanosome life cycle (Bakalara et al., 1995b) prompted us to examine the developmental mRNA expression profile of TbPTP1 by Northern blotting. Total RNA was prepared from monomorphic bloodstream slender forms, bloodstream stumpy forms, and in vitro–cultured procyclic forms. This revealed that the TbPTP1 mRNA was expressed in all stages examined, although up-regulated in stumpy forms (1.5–3-fold), which was somewhat variable between samples (Fig. 1 A). To relate mRNA expression to that of the protein, an anti-peptide antibody was raised against the sequence N-AMKQKRFGMVQRLEQ-C from the amino acid sequence at position 265–279 in TbPTP1. When reacted against lysates derived from isogenic monomorphic slender and stumpy forms of T.b. rhodesiense EATRO 2340 and procyclic forms of T. brucei Lister 427, approximately equal expression of TbPTP1 protein was detected. TbPTP1 expression was also analyzed during synchronous differentiation of bloodstream stumpy forms to procyclic forms. This revealed no transient changes in the protein expression levels of TbPTP1 during the events of differentiation (Fig. 1 B). Finally, analysis of the subcellular localization of TbPTP1 by differential detergent extraction revealed that TbPTP1 associated predominantly with the cytoskeletal fraction in bloodstream forms (Fig. 1 C). Although no association with any discrete structure (e.g., the flagellum) could be detected (Fig. S1, available at http://www.jcb.org/cgi/content/full/jcb.200605090/DC1), a cytoskeletal association for TbPTP1 matches the distribution of several tyrosine phosphatases characterized in other organisms (Howard et al., 1993; van Ham et al. 2005). This compartmentalization is believed to contribute to their substrate specificity.
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Other distinct motifs were also identified in the trypanosomal PTP1s, generating a total of four trypanosome-specific motifs in the catalytic region (Fig. 2, T1–T4). These are as follows: T1 at position 55–63, "LANEXTIYP"; T2 at position 165–167, "EVD"; T3 at position 239–244, "LIGAYA"; and T4 at position 290–295, "RLGV (D/S) (I/V)." In addition, two other motifs have been identified in the precatalytic (Pc) region: PcT1 "R (M/L)QREFXQLQ" at position 20–29 and PcT2 "ENPRXI (D/N)FTTSL" at position 32–43. These precatalytic motifs are well conserved in all members of the T. brucei clade (T. brucei, T. congolense, and T. vivax) and less conserved in T. cruzi. A BLAST search failed to identify any of these motifs in other proteins, indicating that they are unique to the trypanosomal PTP1 family. We hypothesize that these trypanosome-specific motifs may be relevant to regulation of TbPTP1 or molecular recognition of other cellular targets.
The activity of TbPTP1 is regulated by reversible oxidation in vitro
Having identified TbPTP1 as a putative tyrosine phosphatase, it was important to characterize its enzymatic activity profile and substrate specificity. For this, recombinant protein was produced for the wild-type protein and for two TbPTP1 mutants, one for the putative catalytic cysteine, Cys 229 (in the P-loop) and one for the catalytic Asp 199 (in the WPD loop). The catalytic mutants of TbPTP1 were generated by mutating Cys 229 to serine (C229S) and Asp 199 to alanine (D199A). The wild-type enzyme and mutant enzymes were expressed as His6-tagged fusions and purified to >95% homogeneity. After removal of the His tag by enterokinase digestion, multiangle light scattering analysis of the enzyme showed that TbPTP1 behaves as a monomeric protein in solution, with a determined mass of 35,140 D.
The phosphatase activities of the purified recombinant wild-type, D199A, and C229S enzymes were assayed using various concentrations of p-nitrophenylphosphate (pNPP), a widely used substrate of tyrosine phosphatases. The pH profile analysis of pNPP dephosphorylation demonstrated that the wild-type enzyme has the highest specific activity at pH 6.0 (Fig. 3 A), in agreement with the fact that PTPs in general have optimal enzymatic activities at low pH values. The mutant enzyme D199A showed low activity (5–8% of the wild type), and the C229S mutant enzyme was totally inactive under any assay condition and substrate concentration tested (unpublished data). This confirms our predictions from the sequence analysis and demonstrates that both residues, Cys 229 and Asp 199, are essential in the mechanism of catalysis of TbPTP1, matching their orthologues in mammalian PTPs. Steady-state kinetic analysis of the wild-type enzyme yielded a Vmax value of 0.12 mM min–1 and a kcat/Km of 3.57 mM–1 x s–1 for the dephosphorylation of pNPP. Addition of 2 mM of DTT had a marked effect on the catalytic rate, increasing the Vmax by threefold and the kcat/Km by 14-fold (Fig. 3 B and Table S1, available at http://www.jcb.org/cgi/content/full/jcb.200605090/DC1), consistent with previous observations suggesting that the catalytic cysteine needs to be in a reduced state for efficient nucleophilic attack of the substrate (Denu and Tanner, 1998). To investigate whether redox events (Denu and Tanner, 1998; Salmeen et al., 2003; van Montfort et al., 2003) could influence the enzymatic activity of TbPTP1, we performed a time course activity assay using increasing amounts of the oxidizing agent, hydrogen peroxide (H2O2). Fig. 3 C shows that after 10 min of incubation, the addition of 0.25 mM H2O2 completely inactivated TbPTP1 and 0.025 and 0.1 mM H2O2 reduced the enzyme activity by 37 and 58%, respectively. Importantly, the enzymatic activity of the inactive TbPTP1 toward pNPP was completely restored after 5 min of incubation with 10 mM DTT. These experiments indicate that TbPTP1 is sensitive to reversible redox regulation, consistent with several characterized mammalian PTPs (Denu and Tanner, 1998).
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TbPTP1 ablation induces spontaneous differentiation to procyclic forms in a subset of bloodstream forms
To initiate a functional analysis in vivo, TbPTP1 was targeted in cultured bloodstream forms by RNAi. The TbPTP1 coding region was inserted into the vector pZJM (Wang et al., 2000) between two opposing T7 RNA polymerase promoters and transfected in to the "single marker" bloodstream line, which expresses T7 RNA polymerase (Wirtz et al., 1999). This results in TbPTP1 double-stranded RNA expression, thereby invoking RNAi. We successfully generated several viable cell lines, although in only one case was effective ablation of TbPTP1 mRNA and loss of protein observed, and this generated a subtle growth phenotype (Fig. S2, available at http://www.jcb.org/cgi/content/full/jcb.200605090/DC1). During phenotypic characterization of this cell line, we observed that a small proportion (2–12%) of cells spontaneously differentiated to procyclic forms despite maintenance of the cells in bloodstream form culture conditions (HMI-9 culture medium at 37°C). This phenotype manifested itself as the presence of cells in the population that stained strongly with antibodies specific for both EP and GPEET (Fig. 5 A) procyclin (Roditi and Clayton, 1999).
Significantly, this did not represent loss of procyclin gene expression control alone (as can be observed at a frequency of up to 0.1% in wild-type bloodstream populations); analysis of the procyclin-stained cells indicated that they also exhibited characteristic procyclic-form morphology, with their mitochondrial genome (kinetoplast) being positioned away from the cell posterior (Matthews et al., 1995; Fig. 5 B). They also expressed the procyclic stage–specific cytoskeletal antigen CAP5.5 (Hertz-Fowler et al., 2001; unpublished data). Unfortunately, the differentiation phenotype was rapidly unstable and thus difficult to maintain in culture, with the proportion of differentiated cells decreasing in successive passages, even in the absence of induction.
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Initially, we assayed BZ3-induced differentiation in pleomorphic slender cells derived from a rodent infection. This resulted in an 
7% differentiation after 24 h, consistent with the response of cultured monomorphic cells (Fig. S3, available at http://www.jcb.org/cgi/content/full/jcb.200605090/DC1). Thereafter, trypanosome populations highly enriched for stumpy forms were harvested from a mouse infection, and these cells were exposed either to 150 µM BZ3, 6 mM cis aconitate, or 0.3% vol/vol DMSO (used to solubilize BZ3). In all cases, the cells were then maintained in bloodstream-form culture conditions (37°C in HMI-9) over a period of 24 h, conditions that are compatible with both efficient differentiation of cis aconitate–stimulated cells (Matthews and Gull, 1997) and maintenance of the viability of undifferentiated stumpy forms. Samples were harvested at various time points and analyzed for the expression of EP procyclin by immunofluorescence and for morphological differentiation by quantitative analysis of the kinetoplast–posterior dimension in each cell population. Figs. 8 and 9 demonstrate the remarkable result of this analysis: stumpy populations differentiated to procyclic forms synchronously and efficiently when exposed to BZ3, with the kinetics of this being equivalent to cells exposed to cis aconitate (Matthews and Gull, 1994).
Thus, by 6 h in 150 µM BZ3, >70% of cells were EP procyclin positive (Fig. 8 A), and by 24 h the kinetoplast–posterior dimension had increased from 1 µm (equivalent to that seen in bloodstream forms) to 5 µm (equivalent to that in procyclic forms; Matthews et al., 1995; Fig. 8 B). In contrast, cells exposed to DMSO alone remained as bloodstream stumpy forms and showed no evidence of differentiation to procyclic forms (Fig. 9 A). Moreover, by 24 h, differentiated cells in the 150 µM BZ3–treated population were undergoing cell division as differentiated procyclic forms and had induced expression of the procyclic stage–specific cytoskeletal protein CAP5.5 (Matthews and Gull, 1994; Hertz-Fowler et al., 2001; Fig. 9, B and C). We conclude that inhibition of TbPTP1 stimulates committed bloodstream-form trypanosomes to differentiate to procyclic forms in the absence of any previously described trigger for this process.
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Discussion |
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When expressed as a recombinant protein, TbPTP1 preferentially dephosphorylated phosphotyrosine substrates and was inhibited in vitro by sodium orthovanadate, a known tyrosine-specific phosphatase inhibitor. Moreover, the enzyme was regulated by reversible oxidation and mutation of the predicted essential catalytic residues C229 and D199 resulted in proteins with either severely impaired enzymatic activity (D199A) or total inactivity (C229S). Together, these results confirm the assignment of TbPTP1 as a phosphotyrosine-specific phosphatase. This contrasts with previously reported phosphatases in T. brucei, for which our sequence analysis failed to find any of the conserved PTP-specific motifs or any homology to the classical PTPs (Bakalara et al., 2000). Thus, TbPTP1 is to our knowledge the first report of a cloned gene encoding a bona fide nonreceptor tyrosine-specific phosphatase in these organisms.
The biological function of TbPTP1 was investigated by two experimental approaches: gene-specific RNAi and using a cell-permeable PTP1B-specific inhibitor in vivo. The first approach implicated TbPTP1 in life cycle regulation, with spontaneous differentiation being observed in a subset of cultured bloodstream-form cells. However, this phenotype was unstable, and the proportion of differentiated cells was reduced to wild-type levels with continued culture of the parasites whether cells were induced or not. This is not surprising, as transfection procedures and continued passage at 37°C in bloodstream-specific culture media would quickly select against populations that generate procyclic forms. Moreover, other functions of TbPTP1 in proliferative bloodstream forms cannot be excluded. Therefore, we also analyzed the effect of a recently characterized cell-permeable allosteric inhibitor of PTP1B, a benzabromarone derivative (Wiesmann et al., 2004). This inhibitor prevents the closure of the WPD loop of PTPs, therefore keeping the enzyme in a catalytically inactive form. We demonstrated that this inhibitor was effective against TbPTP1, but not against the human low molecular weight PTP (LMWPTP) or a dual-specificity phosphatase. Analysis of the phosphatase complement of the complete T. brucei genome identified only two putative proteins with an intact WPD loop motif and predicted tyrosine phosphatase activity. One of these is TbPTP1, and we have confirmed its BZ3 sensitivity here. The second enzyme, which we term TbPTP2 (Tb11.01.5450), is not likely to contribute to the observed differentiation phenotype, as RNAi against this enzyme does not elicit differentiation of bloodstream forms (unpublished data). Although we cannot exclude other potential uncharacterized targets in trypanosomes, the compatible phenotypes resulting from genetic and pharmacological inhibition of TbPTP1 implicate this enzyme as being responsible for the differentiation phenotype. Moreover, specificity of the response was further supported by the enhanced differentiation observed in BZ3-treated cells expressing the dominant-negative D199A mutant of TbPTP1.
Only a small subset of bloodstream-form cells in asynchronous in vitro cultures were stimulated to differentiate to procyclic forms by BZ3. However, the most striking observation was the effect of this inhibitor on uniform populations of stumpy forms. Here, treatment with the PTP1B inhibitor resulted in efficient differentiation to procyclic forms. We observed that stage-regulated protein expression (EP procyclin; CAP5.5), kinetoplast repositioning, and cell cycle progression all occurred with equivalent efficiency and on the same time scale as cells treated with cis aconitate, an established trigger for trypanosome differentiation. We interpret the differentiation of the small proportion of cells in bloodstream cultures as the response of the subset of cells in this population, which have entered division arrest or committed to other early events in stumpy formation, before morphological transformation. We previously referred to these cells as stumpy* forms (Tasker et al., 2000).
In Fig. 10, we present a model for the role of TbPTP1 in the control of bloodstream to procyclic differentiation. In this model, bloodstream parasites commit to stumpy formation and become competent (stumpy*) to differentiate to procyclic forms. However, they are held arrested in this state in the bloodstream by the action of TbPTP1. Then, upon uptake by the tsetse fly, this inhibition is removed and the parasites progress unhindered to procyclic forms, progressing through a highly programmed developmental pathway in which cellular events occur on a predetermined pathway and time scale. This model has two important implications. First, it supports the concept that proliferative slender cells are not competent to differentiate to procyclic forms unless they commit to the early events of stumpy formation, in particular, cell cycle arrest. Also, it suggests that the default pathway for stumpy forms is to differentiate directly to procyclic forms and that this differentiation is inhibited in the bloodstream by the action of TbPTP1. In other words, differentiation primarily results from release of the "brake," rather than application of the "accelerator." This scenario is compatible with the role of PTP1 in Dictyostelium slug development, where removal of a PTP1 precipitates accelerated differentiation via cell aggregation (Howard et al., 1992).
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The proposed role of TbPTP1 in preventing inappropriate differentiation of stumpy forms in the mammalian bloodstream is essential for transmissibility of the parasite. If not strictly controlled, the progression to procyclic forms would result in rapid death of the stumpy population in the bloodstream because of either the activation of complement by the alternative pathway (killing cells that have lost the variant surface glycoprotein) or the generation of antibodies to invariant procyclic surface antigens. This makes TbPTP1 a key component of the regulation of the trypanosome life cycle and hence a potentially important pharmacological target for controlling trypanosome transmission, for example, in epidemic foci involving intensive human–human or human–livestock transmission. If coupled with factors to promote stumpy formation, targeting TbPTP1 may also help limit parasite virulence and promote trypanosome clearance. There is intense interest in the development of PTP1B inhibitors in the pharmaceutical industry because of the importance of these enzymes in diabetes and obesity (Ukkola and Santaniemi, 2002; Zhang and Lee, 2003), and we are currently investigating the opportunity for piggyback strategies to target kinetoplastid PTPs. Significantly, the presence of trypanosome-specific motifs in this enzyme offers the potential for developing inhibitors with specificity for the parasite enzyme with respect to their mammalian counterparts.
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Materials and methods |
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Parasite growth and differentiation
Parasite lines used were T.b. rhodesiense EATRO 2340 GUP2965 (monomorphic slender forms) or, for stumpy generation, the isogenic pleomorphic line GUP2962 (Matthews and Gull, 1994). For RNAi analyses, T.b. brucei Lister 427 single-marker cells were used (a gift from G. Cross, Rockefeller University, New York, NY; Wirtz et al., 1999), whereas established procyclic forms were T.b. brucei Lister 427.
For BZ3 inhibition assays, cells in HMI-9 medium (Hirumi and Hirumi, 1989) at 37°C were exposed to DMSO, PTP1B inhibitor BZ3, or 6 mM cis aconitate. Samples were assayed by immunofluorescence at room temperature using antibody to EP procyclin (diluted 1:500 in PBS; Cedar Lane Laboratories), antibody to GPEET (diluted 1:200; a gift from I. Roditi, University of Bern, Bern, Switzerland), or the procyclic form cytoskeletal protein CAP5.5 (undiluted hybridoma supernatant; a gift from K. Gull, University of Oxford, Oxford, England; Hertz-Fowler et al., 2001). Secondary antibodies used were goat anti–mouse (EP procyclin; CAP5.5) or –rabbit (GPEET procyclin) conjugated to either FITC (1:50; Sigma-Aldrich) or Alexa 488 (1:200; Invitrogen). Slides were stained with 1 µg/ml DAPI and mounted in MOWIOL (Harlow Chemical Co.). Morphometric measurements of kinetoplast repositioning used Scion Image 1.62. Images were captured using a Cohu charged-coupled device camera attached to an Axioscope 2 (Carl Zeiss MicroImaging, Inc.) using either Plan Neofluar 63x (1.25 NA) or Plan Neofluar 100x (1.30 NA) phase-contrast objectives. Images were processed using Photoshop CS (Adobe).
DNA cloning
A 595-bp fragment related to PTPROt (Aguiar et al., 1999) formed part of the sheared T. brucei strain TREU 927/4 genomic DNA clone 18E19 (available from GenBank/EMBL/DDBJ under accession no. AQ649023). Oligonucleotides were designed to the 5' (TbPTP A; 5'-CATCAACCTCGTACGACG-3') and 3' (TbPTP B; 5'-CAAGCCATACAATAATTG-3') ends of the gene fragment, and were these used in independent amplifications with primers specific for the spliced leader sequence or polyA tail to amplify the gene in two overlapping halves from cDNA. The sequence of the full gene was verified after completion of the trypanosome genome sequence.
Northern and Western blotting
RNA preparation and Northern blotting was performed as described by Tasker et al. (2000) using a digoxygenin-labeled TbPTP1-specific riboprobe (Roche). Stumpy cell fractionation used the Qproteome kit (QIAGEN) with each fraction being probed with antibodies to 
-tubulin (cytoskeletal fraction; a gift from K. Gull), cytosolic PGK (cytosol; a gift from P. Michels, Université Catholique de Louvain, Brussels, Belgium), and BiP (membrane and organelles; a gift from J. Bangs, University of Wisconsin, Madison, WI) as controls. For detection of TbPTP1, an anti-peptide (NH2-AMKQKRFGMVQRLEQ-COOH) antibody was raised in rabbits and affinity purified against the immunogen (Eurogentec). Preimmune serum detected no trypanosome protein. Western blotting was performed according to Tasker et al. (2000).
RNAi and ectopic expression for TbPTP1 and mutants
TbPTP1 transcript ablation in bloodstream forms was achieved by cloning the TbPTP1 coding sequence into pZJM (Wang et al., 2000), which was then linearized by NotI digestion and transfected as previously described. Transformants were selected with 2.5 µg/ml phleomycin. Ectopic overexpression of TbPTP1 and D199A mutants used the trypanosome expression vector pHD451.
Phosphatase assays using phosphosubstrates
Dephosphorylation of phosphosubstrates was detected by measuring the release of inorganic phosphate with the malachite green detection system according to the manufacturer's protocol (Protein tyrosine phosphatase assay kit; Sigma-Aldrich). Reaction mixtures (50 µl) contained 5–10 µg of purified TbPTP1 with concentrations from 0.01 to 0.2 mM of phosphopeptides in 50 mM Hepes and 150 mM NaCl, pH 7.0. Reactions were incubated at 37°C for 15–30 min and quenched by adding of 50 µl of malachite green reagent. After 15 min of further incubation at room temperature, the absorbance of the samples were measured at 620 nm in a microplate reader (Opsys MR; Dynex Technologies), with released inorganic phosphate being determined using a phosphate standard curve. The specific activity is defined as pmoles of inorganic phosphate released in a minute per milligram of protein. Kinetic constants Km and Vmax were calculated using the Lineweaver-Burke plot of the reciprocal initial velocity versus the reciprocal concentration of substrates. See the supplemental text (available at http://www.jcb.org/cgi/content/full/jcb.200605090/DC1) for information about protein expression constructs and recombinant protein purification.
Phosphatase assays using pNPP
Enzyme activity was measured by monitoring TbPTP1 (5–20 µg) catalyzed hydrolysis of pNPP to p-nitrophenol (Zhang and Van Etten, 1990). A final concentration of 20 mM pNPP was present in the assay. The pNPP assay buffer was 50 mM Tris, 50 mM bisTris, and 100 mM Na acetate, pH 5–7.5. Each reaction (400 µl) was performed in triplicate, being incubated at 37°C for 15 min and quenched by adding 500 µl of 1 M NaOH. The concentration of released p-nitrophenol, determined at 405 nm, was converted to millimolar units using a millimolar extinction coefficient of 18.0 mM–1 cm–1.
Reversible inactivation of TbPTP1 by H2O2
The assays (120 µl) contained 60 µg of TbPTP1 and 0–0.25 mM H2O2 in 50 mM Hepes, pH 7.0, and 150 mM NaCl. Reactions, initiated by addition of H2O2, were incubated at room temperature. After 15 min, 10 mM DTT was added. 20-µl samples removed at 0, 5, 10, 15, 20, 30, and 40 min were assayed for residual activity using pNPP as substrate.
Online supplemental material
Table S1 shows kinetic constants for the hydrolysis of phosphosubstrates by TbPTP1. Fig. S1 shows immunofluorescence localization of ectopically expressed TbPTP1. Fig. S2 shows growth kinetics, RNA, and protein expression of the TbPTP1 RNAi line and the response of the TbPTP RNAi line to pCPTcAMP. Fig. S3 shows BZ3 response of pleomorphic slender cells. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200605090/DC1.
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Acknowledgments |
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This work was supported by Wellcome Trust grant 068793 and by Wellcome Trust Programme grant 073358 to K.R. Matthews.
Submitted: 15 May 2006
Accepted: 19 September 2006
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References |
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