Abstract
Changes in [Ca2+]i are a central step in platelet activation. In nonexcitable cells, receptor-mediated depletion of intracellular Ca2+ stores triggers Ca2+ entry through store-operated calcium (SOC) channels. Stromal interaction molecule 1 (STIM1) has been identified as an endoplasmic reticulum (ER)-resident Ca2+ sensor that regulates store-operated calcium entry (SOCE), but the identity of the SOC channel in platelets has been controversially debated. Some investigators proposed transient receptor potential (TRP) C1 to fulfil this function based on the observation that antibodies against the channel impaired SOCE in platelets. However, others could not detect TRPC1 in the plasma membrane of platelets and raised doubts about the specificity of the inhibiting anti-TRPC1 antibodies. To address the role of TRPC1 in SOCE in platelets, we analyzed mice lacking TRPC1. Platelets from these mice display fully intact SOCE and also otherwise unaltered calcium homeostasis compared to wild-type. Furthermore, platelet function in vitro and in vivo is not altered in the absence of TRPC1. Finally, studies on human platelets revealed that the presumably inhibitory anti-TRPC1 antibodies have no specific effect on SOCE and fail to bind to the protein. Together, these results provide evidence that SOCE in platelets is mediated by channels other than TRPC1.
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Introduction
Changes in [Ca2+]i play a central role in signaling processes in virtually all cells. In nonexcitable cells, such as platelets, the major Ca2+ entry pathway involves receptor-mediated release of Ca2+ from the sarcoplasmic/endoplasmic reticulum (SR/ER) which triggers Ca2+ influx through the plasma membrane (PM) by a process referred to as store-operated calcium entry (SOCE) [1]. Stromal interaction molecule (STIM) 1 has recently been identified as an ER-resident calcium sensor that activates store-operated calcium (SOC) channels in T cell lines [2–4] and mast cells [5]. In human T cells, the four transmembrane domain protein Orai1 (CRACM1) appears to be the predominant SOC channel [6, 7], but the C-terminal region of STIM1 may also interact with other SOC channel candidates such as transient receptor potential channels (TRPCs) 1, 2, and 4 [8]. We have recently shown that an activating EF hand mutant of STIM1 constitutively activates SOC channels in mouse platelets leading to macrothrombocytopenia and a bleeding phenotype [9]. While this indicates that STIM1-dependent SOCE is a major pathway of Ca2+ entry in platelets, the identity of the platelet SOC channel remains a matter of considerable debate. TRPC1, which is present in human platelets [10, 11] and murine megakaryocytes (detected on the mRNA level [12]) has been proposed as the major platelet SOC channel based on in vitro studies where a blocking antibody against the protein (obtained from Alomone Labs, Israel) caused impairment of SOCE stimulated by low doses of thrombin and the sarcoplasmic/endoplasmic reticulum calcium ATPase (SERCA) inhibitor thapsigargin (TG) [13]. These investigators reported that store depletion caused the de novo conformational coupling of IP3R type II in the stores with the TRPC1 channel suggested to be present in the plasma membrane [14, 15]. The same group further suggested that TRPC1 was present in lipid rafts and associated with TRPC4 and TRPC5, as was TRPC3 with TRPC6 associated [16]. Recently, another group also reported the expression of TRPC3 and TRPC4 [17]; however, other investigators were unable to detect TRPC3, TRPC4, or TRPC5 at the protein level, and the low levels of TRPC1 detected were found predominantly in the intracellular stores in contrast to TRPC6 which was strongly detected in the plasma membrane [18]. There is no reported detection of TRPC5 mRNA in platelets and megakaryocytes which questions the expression of this protein [11, 12] and doubts have been raised regarding the antibody used to detect TRPC4 [19]. There are further doubts raised regarding the specificity of the Alomone TRPC1 antibody used by the Rosado group with a reported lack of recognition of overexpressed hTRPC1 in heterologous systems [20] and another report stating that this antibody did not have any significant effect on Ca2+ entry induced by either TG or thrombin [21]. Recently, the de novo conformational coupling mechanism itself involving TRPC1 in Ca2+ entry has been questioned and a more prominent role for a Na+/Ca2+ exchanger working in reverse mode has been suggested after a possible Na+ entry event that may be mediated by TRPC1 [22]. In the light of these controversies and to address the role of TRPC1 in platelets directly, we analyzed TRPC1-deficient mice [23, 24]. We show that the lack of TRPC1 has no effect on Ca2+ store release and SOCE in platelets and does not influence their function in vitro or in vivo. Our findings on human platelets also indicate the absence of an interaction between TRPC1 and STIM1, suggesting that SOCE in platelets is mediated by channels other than TRPC1.
Materials and methods
Mice
Animal studies were approved by the local authorities (Bezirksregierung of Unterfranken). Generation of TRPC1 −/− mice has been described previously [23].
Chemicals and antibodies
Anesthetic drugs: medetomidine (Pfizer, Karlsruhe, Germany), midazolam (Roche Pharma AG, Grenzach-Wyhlen, Germany), and fentanyl (Janssen-Cilag GmbH, Neuss, Germany) and antagonists: atipamezol (Pfizer, Karlsruhe, Germany), flumazenil, and naloxon (both from Delta Select GmbH, Dreieich, Germany) were used according to the regulation of the local authorities. ADP (Sigma, Deisenhofen, Germany), U46619 (Alexis Biochemicals, San Diego, USA), thrombin (Roche Diagnostics, Mannheim, Germany), collagen (Kollagenreagent Horm, Nycomed, Munich, Germany), and TG (Molecular Probes) were purchased. Monoclonal antibodies conjugated to fluorescein isothiocyanate (FITC), phycoerythrin (PE), or DyLight-488 were from Emfret Analytics (Würzburg, Germany).
RNA isolation and RT-PCR
Platelet mRNA was isolated from 3 ml blood using Trizol reagent (Invitrogen, Karlsruhe, Germany). cDNA was synthesized using 1 μg platelet total mRNA and Super Script Reverse Transcriptase (Invitrogen, Karlsruhe, Germany) as described by the manufacturer. Gradient PCR was performed using TRPC1 and actin-specific primers.
Western blotting
TRPC1 was detected after immunoprecipitation of the protein from wild-type and TRPC1 −/− platelets as described previously [18]. TRPC1 was extracted by immunoprecipitation from platelet lysates using the polyclonal anti-XTRP-1 antibody (a generous gift from G. Barritt, Adelaide, Australia) previously demonstrated to recognize TRPC1 [20]. The immunoprecipitates were Western blotted using the TRPC1 recognizing monoclonal antibody 1F1 (a generous gift from Dr. L. Tsiokas, Oklahoma, USA).
Intracellular calcium measurements
Mouse platelet intracellular calcium measurements were performed as described [25]. Briefly, platelets isolated from blood were washed, suspended in Tyrode’s buffer without calcium, and loaded with Fura-2/AM (5 μM) in the presence of Pluronic F-127 (0.2 μg/ml; Molecular Probes) for 30 min at 37°C. After labeling, platelets were washed once and resuspended in Tyrode’s buffer containing 0 or 1 mM Ca2+. Stirred platelets were activated with agonists, and fluorescence was measured with a PerkinElmer LS 55 fluorimeter. Excitation was alternated between 340 and 380 nm, and emission was measured at 509 nm. Each measurement was calibrated using Triton X-100 and ethylene glycol bis(2-aminoethyl ether)-N,N,N′,N′-tetraacetic acid (EGTA). For the experiments with Stim1 Sax/+ mice and the respective controls, intracellular calcium measurements were performed by flow cytometry as described [9].
Platelet aggregation and flow cytometry
Washed platelets (200 μl with 0.5 × 106 platelets/μl) were analyzed in the presence of 70 μg/ml human fibrinogen. Transmission was recorded on a Fibrintimer 4 channel aggregometer (APACT Laborgeräte und Analysensysteme, Hamburg, Germany) over 10 min and was expressed in arbitrary units with buffer representing 100% transmission. Flow cytometry: Heparinized whole blood was diluted 1:20 and incubated with appropriate fluorophore-conjugated monoclonal antibodies for 15 min at room temperature and analyzed on a FACScalibur instrument (Becton Dickinson, Heidelberg, Germany).
Adhesion under flow conditions
Rectangular coverslips (24 × 60 mm) were coated with 0.2 mg/ml fibrillar type I collagen (Nycomed, Munich, Germany) for 1 h at 37°C and blocked with 1% bovine serum albumin (BSA). Heparinized whole blood was perfused as described [26]. Image analysis was performed off-line using the Metavue software (Visitron, Munich, Germany). Thrombus formation was expressed as the mean percentage of total area covered by thrombi.
Bleeding time
Mice were anesthetized and a 3-mm segment of the tail tip was removed with a scalpel. Tail bleeding was monitored by gently absorbing blood with filter paper at 20 s intervals without making contact with the wound site. When no blood was observed on the paper, bleeding was determined to have ceased. Experiments were stopped after 20 min.
Intravital microscopy of thrombus formation in FeCl3-injured mesenteric arterioles
Four-week-old mice were anesthetized, and the mesentery was exteriorized through a midline abdominal incision. Arterioles (35–60 μm diameter) were visualized with a Zeiss Axiovert 200 inverted microscope (×10) equipped with a 100-W HBO fluorescent lamp source, and a CoolSNAP-EZ camera (Visitron, Munich Germany). Digital images were recorded and analyzed off-line using the Metavue software. Injury was induced by topical application of a 3-mm2 filter paper saturated with FeCl3 (20%) for 10 s. Adhesion and aggregation of fluorescently labeled platelets (Dylight-488 conjugated anti-GPIX Ig derivative) in arterioles was monitored for 40 min or until complete occlusion occurred (blood flow stopped for >1 min).
Human platelet studies
Blood from volunteers who had denied taking any medication for 1 week was taken into one tenth volume 3.2% trisodium citrate according to local ethical guidelines and washed platelets prepared according to the methods described in detail previously [18]. Platelets labeled with Fura-2/AM were resuspended at 1.5 × 108 cells/ml and monitored for Ca2+ changes using a Cairn spectrofluorimeter (Cairn Research, Faversham, Kent, UK) with excitation at 340 and 380 nm and emission at 510 nm. Reagents were added at the time points described in the legends to the figures. Anti-TRPC1 antibody was from Alomone Labs (Israel) and Ank (raised to the intracellular first ankyrin domain of hTRPC1) was as previously characterized [18]. Where indicated, values represent the means±SEM with numbers of separate experiments indicated by [n].
For immunoprecipitation studies, washed platelets were resuspended at 1 × 109 cells/ml in a Tyrode medium containing 10 mM Hepes, 140 mM NaCl, 5 mM KCl, 1 mM MgCl2, 5 mM glucose, 0.42 mM NaH2PO4·H2O, 12 mM NaHCO3, 0.2 mM EGTA, 10 μM indomethacin, and 1 U/ml apyrase. Incubations were carried out in aggregation cuvettes at 37°C in the presence of 1 mM Ca2+, and cells were stimulated with either thrombin (1.25 U/ml), collagen-related peptide (CRP, 10 μg/ml), or TG (10 μM). After 1 min stimulation, incubations were stopped with equal volume Triton lysis buffer (containing 2% Triton, 2% sodium deoxycholate, 10 mM EGTA, 150 mM NaCl, 40 mM Tris pH 7.8, 5 μM pepstatin, 1 mM PMSF, 10 μg/ml aprotinin, 0.2 mg/ml soybean trypsin inhibitor, 10 μM E-64, 50 μM leupeptin, 1 mM sodium orthovanadate, 5 mM benzamidine, and 2.5 mM ethylene diamine tetraacetic acid). The lysates were centrifuged at 13,000×g for 5 min to remove insoluble material, and after preclearing with protein G sepharose, the STIM1 was immunoprecipitated using polyclonal anti-STIM1 antibody (ProSci, Poway, CA, USA) as described previously [18]. Immunoprecipitated STIM1 was detected by Western blotting using the monoclonal antibody GOK/STIM1 (BD Biosciences, Oxford, UK) and for association to TRPC1 with 1F1.
Results
RT-PCR revealed the presence of wild-type and mutant TRPC1 mRNA message in control and TRPC1 −/− platelets, respectively (Fig. 1a). Omission of exon 8 in the mutant mRNA message leads to a frame shift of the original reading frame and results in a STOP codon at positions 2 and 9 of exon 9 coding for the region downstream of the ion channel pore [23]. Consequently, the protein was detectable as an approximately 84 kDa band in wild-type but not mutant cells (Fig. 1b). Platelet count and the expression of different platelet surface glycoproteins (GP) were similar in wild-type and TRPC1 −/− animals (data not shown). Western blot analyses revealed unaltered expression of TRPC6 in the mutant platelets, excluding a compensatory upregulation of this channel (Fig. 1c). Platelets from TRPC6 −/− mice [27] served as a control. To estimate store content and SOCE in the cells, we performed intracellular Ca2+ measurements. Upon Ca2+ release from the ER, a conformational coupling between TRPC1 and the type II IP3 receptor has been proposed to happen, which in turn results in the opening of TRPC1—as SOC channel—and Ca2+ entry [14, 15]. To test this directly, we treated platelets with 5 μM TG (a selective inhibitor of the SERCA) in Ca2+-free buffer to empty the intracellular Ca2+ stores, and then added 1 mM Ca2+ to measure the extent of SOCE. Unexpectedly, neither the store content nor the amplitude of SOCE was different between wild-type and TRPC1 −/− platelets (Fig. 1d), demonstrating that TRPC1 is not required for TG-induced SOCE in platelets.
Agonist-induced platelet activation triggers the activation of phospholipase (PL) Cβ and/or PLCγ2, which hydrolyze phosphoinositol-4,5-bisphosphate (PIP2) to inositol-1,4,5-trisphosphate (IP3) and diacyl-glycerol (DAG). DAG mediates store-independent Ca2+ entry [28], whereas IP3 releases Ca2+ from the ER and in turn leads to SOCE [1]. To test Ca2+ responses to physiological agonists, we measured changes in [Ca2+]i upon platelet activation with thrombin—known to activate PLCβ through G protein-coupled receptors—and with CRP, which activates PLCγ2 through GPVI. Unexpectedly, both agonists evoked comparable Ca2+ responses in wild-type and TRPC1 −/− platelets (Fig. 1e,f).
We further investigated whether the lack of TRPC1 influences agonist-induced platelet activation in vitro. Flow cytometric analysis of integrin αIIbβ3 activation (JON/A-PE) and degranulation, determined as the surface expression of P-selectin, yielded indistinguishable results for TRPC1 −/− and control platelets in response to all tested agonists and agonist concentrations (Fig. 2a). Similarly, no differences in reactivity were noted between TRPC1 −/− and control platelets in standard aggregometry (Fig. 2b) and in a flow adhesion assay where whole blood was perfused over a collagen-coated surface at high shear rate (1,000 s−1). Wild-type and TRPC1 −/− platelets formed stable thrombi to the same extent and with the same kinetics (Fig. 2c).
Next, we analyzed the relevance of TRPC1 deficiency for platelet function in vivo in hemostasis and thrombosis [9]. Bleeding times after amputating the tail tip of wild-type and TRPC1 −/− mice were comparable (3.1 ± 1.1 min vs. 2.7 ± 1.9 min) (Fig. 3a). Similarly, the application of 20% FeCl3 on the exteriorized mesenteric arteries of TRPC1 −/− mice resulted in fast platelet adhesion and thrombus growth leading to irreversible vessel occlusion after 13.1 ± 3.0 min, which was comparable to the kinetics of thrombus formation and vessel occlusion observed in the control animals (15.1 ± 3.0 min; Fig. 3b,c).
Very recently, we have shown that the heterozygous expression of an activating EF hand mutant STIM1 (Stim1 Sax/+) constitutively activates SOC channels in murine platelets resulting in elevated basal [Ca2+]i, macrothrombocytopenia, and bleeding [9]. If TRPC1 was the SOC channel on the platelet surface that is regulated by STIM1, lack of the protein should rescue or at least ameliorate the phenotype of the Stim1 mutant platelets. To investigate this, we crossed the two mouse lines and studied their platelets. As shown in Fig. 4, the increase in basal [Ca2+]i and the resulting macrothrombocytopenia was not altered in TRPC1 −/−/Stim1 Sax/+ compared to Stim1 Sax/+ mice, clearly excluding TRPC1 as the major STIM1-regulated SOC channel on the platelet surface.
The above data in mouse platelets contrast with reports suggesting TRPC1 as the major SOC channel in human platelets on the basis of antibody-induced inhibition of Ca2+ entry using a commercial antibody raised to a predicted extracellular epitope of TRPC1 [13]. As there are also doubts regarding the specificity of this antibody [20], we decided to reexamine this effect. Human platelets were loaded with Fura-2/AM and [Ca2+]i measurements performed using 340/380 nm ratio fluorescence as previously described [18]. Figure 5a shows the effects of the incubation of platelets for 10 min with the commercial polyclonal anti-TRPC1 antibody (10 μg/ml final concentration, supplied in a phosphate buffered saline (PBS) vehicle containing 1% BSA and 0.05% sodium azide as preservative) previously reported to inhibit SOCE in human platelets [13]. As controls, water or 10 μg/ml of our previously characterized polyclonal Ank antibody, again in PBS containing 0.05% sodium azide, were used. The Ank antibody has been raised against an intracellular epitope of TRPC1 and does not recognize the protein in intact platelets [18]. Both antibodies showed no effect on Ca2+ release from stores, induced by either 0.25 U/ml thrombin or 200 nM TG. It is interesting to note that a similar reduction in the extent of Ca2+ entry was seen with both antibodies after the addition of 1 mM Ca2+. With 0.25 U/ml thrombin as the stimulatory agent, the Alomone antibody inhibited the peak height of Ca2+ entry by 30.2 ± 3.8% [mean±SEM, n = 4], the Ank antibody inhibited the peak height by 31 ± 4.5% [n = 3]. Using 200 nM TG as the agonist, the Alomone antibody inhibited the peak height by 17 ± 6.5% [n = 3], the Ank antibody inhibited the peak height by 15 ± 5.7% [n = 3], suggesting that this effect is not related to antibody recognition of a surface epitope of TRPC1. Furthermore, the inclusion of sodium azide (present in the vehicle of antibodies) for 10 min at 0.0007% final concentration caused no effect on Ca2+ release by either agonist but inhibited Ca2+ entry to a similar extent as the antibodies (with thrombin, 0.0007% sodium azide inhibited the peak height by 37.2 ± 5% [n = 3] and with TG, sodium azide inhibited the peak height by 15 ± 3.7% [n = 3]; fluorescence curves not shown for clarity). This suggests that the inhibition observed by the antibodies was due to the presence of sodium azide in the antibody preparations. Next, we performed Western blot analyses to test the specificity of the TRPC1 antibody, as other investigators have raised doubts about it [20]. In agreement with these reports, the Alomone anti-TRPC1 antibody failed to detect hTRPC1 overexpressed in QBI-293 cells, whereas a strong signal was obtained with the 1F1 antibody (Fig. 5b). This negative result was consistently obtained with at least three separate purchases of the Alomone antibody over a 3-year period.
Our studies using the TRPC1 −/−/Stim1 Sax/+ mutation in mouse platelets (Fig. 4) imply that STIM1 does not interact with TRPC1 in a functional capacity in mouse platelets. A recent report, again using the Alomone TRPC1 antibody, suggested that STIM1 interacts with TRPC1 in resting platelets and increases modestly upon activation of platelets with TG plus ionomycin [29]. We, therefore, investigated a possible interaction between STIM1 and TRPC1 in human platelets using our currently described antibodies. Washed platelets at 1 × 109 cells/ml were incubated with 1 mM Ca2+ in aggregometer cuvettes in the presence of thrombin (1.25 U/ml), CRP (10 μg/ml), or TG (10 μM) for 1 min followed by immunoprecipitation of STIM1 using a polyclonal antibody to STIM1 (ProSci, USA). The extractions were probed on Western blots for the presence of STIM1 (using the monoclonal GOK/STIM1 antibody) and for TRPC1 (using 1F1). Figure 6 shows a typical experiment repeated three times on separate occasions where STIM1 extraction is apparent in all incubations but there is no association to TRPC1 in either resting or stimulated platelets.
Discussion
STIM1 has been identified as the ER-resident Ca2+ sensor that activates SOC channels in T cells [2–4, 30], mast cells [5], and platelets [9]. However, while the identity of the SOC channel in human T cells [6, 7, 31] and mast cells [32] has been established as Orai1 (CRACM-1), the proposed function of TRPC1 as a major platelet SOC channel has been considerably debated [21, 33, 34]. TRPC1, which was the first mammalian TRPC channel to be identified, has probably been the most intensively studied and has had many functions ascribed to it including a role in SOCE or being a mechanosensitive channel (for review, see Beech [35]). However, with the exception of a role in salivary glands where TRPC1 is well-expressed [24], its physiological role in other tissues has remained elusive. In the current study, we demonstrate unaltered Ca2+ homeostasis and cellular activation in TRPC1 −/− platelets, clearly excluding a major role of this channel in SOCE in mouse platelets. Furthermore, we provide experimental evidence that some of the published data that had previously lead to the proposal of TRPC1 as a major SOC channel in human platelets may have been misleading due to the lack of specificity of reagents used.
Changes in [Ca2+]i are essential during cellular activation and are, therefore, tightly regulated. As platelets have to respond to vascular injury very rapidly, their signal transduction machinery is optimized for maximal activation within seconds including the rapid occurrence of maximal cytosolic Ca2+ levels upon agonist-induced stimulation [36–38]. This is perhaps best exemplified by the steep slope of Ca2+ entry after TG treatment of mouse or human platelets (Fig. 1d and Fig. 5a, respectively) which suggests it to be mediated by the activation of a highly abundant SOC channel. In agreement with this notion, STIM1, the principal regulator of SOCE, is highly expressed in platelets, even at higher relative density than in T cells [9]. In contrast, TRPC1 is expressed in both mouse (Fig. 1b) and human (not shown) platelets at extremely low levels, making it necessary to enrich the protein by immunoprecipitation for detection. Furthermore, it has previously been reported that most of the TRPC1 detected is not present in the plasma membrane of (human) platelets but is rather localized in intracellular stores, indicating it to perform functions other than SOCE [18]. In support of the latter, other investigators have also reported a widespread intracellular location for hTRPC1 overexpressed in HEK-293 cells [39]. In addition, others have suggested that TRPC1 alone is unable to increase whole cell currents in resting and carbachol-stimulated cells, suggesting that it may not fulfil a channel function but that it can form heteromers with TRPC4 and TRPC5 that are activated by Gq-coupled receptors rather than as SOC channels [40]. Furthermore, analysis of SOCs in freshly isolated smooth muscle cells from cerebral arteries or from thoracic aortas from wild-type and TRPC1 −/− mice revealed no difference, again suggesting an absence of a major role in SOCE [23]. In agreement with this, we found that TRPC1 deficiency does not have any effect on the kinetics and extent of TG-induced store depletion or subsequent SOCE or agonist-induced Ca2+ mobilization and entry in mouse platelets (Fig. 1d–f). Its absence in platelets has no measurable effect on platelet aggregation or secretion induced by any of the agonists examined (Fig. 2) nor on thrombus formation on a collagen-coated surface (Fig. 2c) or in a mesenteric arteriolar injury model utilizing ferric chloride where vessel occlusion is largely driven by thrombin stimulation of platelets and fibrin clot formation (Fig. 3). This data further suggests that the SOC channel in platelets comprises subunits other than TRPC1.
Platelets have been reported to express other TRPC isoforms and members of the TRPM subfamily [12]. Thus, a possibility exists that the function of TRPC1 may be compensated for by another TRP channel member. However, we consider this unlikely for the following reasons. Previous analysis of the TRPC1 −/− mouse vasculature suggested that there is no upregulation or downregulation of other TRPC channels [23], unlike the situation in TRPC6 −/− mice where TRPC3 levels are elevated [27]. We have found that levels of TRPC6 in wild-type versus TRPC1 −/− platelets are unchanged (Fig. 1c). Other members of the TRPC family (TRPC2, TRPC3, TRPC4, TRPC5, and TRPC7) have previously not been detected in mouse megakaryocytes from which platelets are produced [12] and are, therefore, unlikely to compensate for the absence of TRPC1 in this model system. Furthermore, with the exception of TRPC4 shown in endothelial cells [41], there is little evidence that any other TRPC channel is able to fulfil a SOCE role. In human platelets, TRPC4 expression has been detected and has been suggested to allow SOCE to be sensitive to alkalosis [17]. Although it is able to form heteromers with TRPC1 [39], its exact role in SOCE remains to be determined. Thus, there is little indication that another TRP channel compensates for the loss of the putative SOC activity of TRPC1 in the knockout platelets. We are convinced that, if a function for TRPC1 in platelet Ca2+ homeostasis was important, it would have been evident in at least one of the assays described in this study.
Although our results with mouse platelets do not fully exclude the possibility that species-specific differences might exist in the function of TRPC1 in platelets, we consider this to be unlikely for the following reasons. The proposal of TRPC1 as the major SOC channel in human platelets was largely based on the observation that a commercially available anti-TRPC1 antibody partially inhibited Ca2+ entry stimulated by low-dose thrombin and TG in those cells [14, 15]. However, in this study, we show that they have no specific effect on SOCE in human platelets and that the inhibition seen is not related to an antibody-recognized surface epitope but due to the presence of sodium azide in the preparations. In agreement with the studies of Ong et al. [20], we found that the Alomone TRPC1 antibody does not bind to hTRPC1 in a specific manner. Currently, we cannot rule out batch differences in the antibody preparations obtained from the manufacturer, but different purchases (different lot numbers) consistently yielded negative results over the last 3 years.
Our studies using the TRPC1 −/− Sax/+ mutation (Fig. 4) also imply that STIM1 does not interact with TRPC1 in a functional capacity in mouse platelets. The Sax mutation represents a constitutively active protein that is unable to sense the Ca2+ in intracellular stores and leads to the activation of the SOC channel resulting in increased basal cytosolic Ca2+ levels [9]. The observations in the Stim1 Sax/+ mouse model supports earlier studies in heterologous expression systems suggesting mutations in the EF hand domain to lead to constitutive activation of SOC channels [3]. If TRPC1 was the important entry channel or an important part of the channel complex linked to STIM1, then crossing the two mouse lines would have resulted in rescue of the Stim1 Sax/+ phenotype. That the TRPC1 −/−/Stim1 Sax/+ showed no difference compared to Stim1 Sax/+ mice confirms without doubt that TRPC1 plays no major role in SOCE in platelets. Using the antibodies described in our study, we failed to observe STIM1–TRPC1 interaction in human platelets at rest or upon stimulation with thrombin, CRP, or TG (Fig. 6) further supporting our other data showing a lack of effect of TRPC1 deficiency on platelet responses and suggesting it to be the same in human platelets. A recent study, again using the Alomone TRPC1 antibody, came to the conclusion that STIM1 interacts with TRPC1 in resting platelets and that a modest increase occurs upon stimulation with TG [29]. It was further reported that “electrotransjection” (electroporation at 4 kV/cm electric field) of a STIM1 antibody (GOK/STIM1) reduced SOCE, interaction of STIM1–TRPC1, and interaction of IP3R type II with TRPC1.
While it is very difficult to know all the reasons for the differences, use of different TRPC1 reagents may be partly responsible, and for reasons already described, we are not confident of their detection of TRPC1. The reported electroporation experiments [29] are also surprising. This technique was widely used in the 1980s by ourselves (K.S.A.) and other investigators to permeabilize the plasma membrane to allow free diffusion of small molecular size molecules (less than 1,000 Da) such as Ca2+, ATP, inositol, etc., but this technique did not allow diffusion of proteins [42–44]. It is, therefore, surprising that antibodies, which represent near globular structures of 150,000 Da, are reported to pass through the plasma membrane of electroporated platelets. If such a possibility exists, this would be accompanied by loss of cytosolic proteins and, with it, platelet integrity. Furthermore, the GOK/STIM1 antibody is known to recognize the N-terminal portion of STIM1 (amino acids 25–139) that houses the EF hand domain which is predicted to point into the lumen of the ER where Ca2+ binding occurs or to the outside if the STIM1 is plasma membrane-associated. If the electroporated GOK/STIM1 antibody is to have an effect, the antibody needs to penetrate into the lumen of the ER. With electroporation techniques, this is considered unlikely (see also Hughes and Crawford [43] and Authi et al. [44]).
Taken together, our results provide compelling evidence that TRPC1 is not a major SOC channel in platelets and further studies will be required to identify this channel in platelets. This will be of considerable importance as SOC channels in general and the platelet SOC channel in particular have been recognized as very attractive potential targets for pharmacological intervention.
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Acknowledgement
We would like to thank Sylvia Hengst for the excellent technical support. This work was supported by grant Ni556/7-1 and the SFB 688 from the Deutsche Forschungsgemeinschaft (DFG) (to B.N.). AA is supported by the Medical Research Council (UK), and KSA is supported by the British Heart Foundation.
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David Varga-Szabo and Kalwant S. Authi contributed equally to this article.
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Varga-Szabo, D., Authi, K.S., Braun, A. et al. Store-operated Ca2+ entry in platelets occurs independently of transient receptor potential (TRP) C1. Pflugers Arch - Eur J Physiol 457, 377–387 (2008). https://doi.org/10.1007/s00424-008-0531-4
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DOI: https://doi.org/10.1007/s00424-008-0531-4