TRPC Channels in SOCE Scenario: Comparison
Please note this is a comparison between Version 2 by Vivi Li and Version 1 by Juan Antonio Rosado.

Transient receptor potential (TRP) proteins form non-selective Ca2+ permeable channels that contribute to the modulation of a number of physiological functions in a variety of cell types. Since the identification of TRP proteins in Drosophila, it is well known that these channels are activated by stimuli that induce PIP2 hydrolysis. The canonical TRP (TRPC) channels have long been suggested to be constituents of the store-operated Ca2+ (SOC) channels; however, none of the TRPC channels generate Ca2+ currents that resemble ICRAC. STIM1 and Orai1 have been identified as the components of the Ca2+ release-activated Ca2+ (CRAC) channels and there is a body of evidence supporting that STIM1 is able to gate Orai1 and TRPC1 in order to mediate non-selective cation currents named ISOC. STIM1 has been found to interact to and activate Orai1 and TRPC1 by different mechanisms and the involvement of TRPC1 in store-operated Ca2+ entry requires both STIM1 and Orai1. In addition to the participation of TRPC1 in the ISOC currents, TRPC1 and other TRPC proteins might play a relevant role modulating Orai1 channel function. 

  • TRPC1
  • STIM1
  • Orai1
  • calcium influx
  • store-operated Ca2+ entry (SOCE)

1. Introduction

The relevance of Ca2+ influx in cellular physiology was revealed by Ringer in the early 1880s [1] and was almost a century later when store-operated Ca2+ entry (SOCE), also known as capacitative Ca2+ entry, was identified [2] (Figure 1). SOCE is a singular mechanism for Ca2+ influx as it is activated by discharge of the intracellular agonist-sensitive Ca2+ stores unlike other Ca2+ entry pathways activated by physical changes of the plasma membrane (PM) or direct chemical stimulation of the channels. A number of store-operated currents with different biophysical properties have been described; among them, the first identified and best characterized one is the highly Ca2+ selective Ca2+ release-activated Ca2+ current (ICRAC). ICRAC is a non-voltage activated, inwardly rectifying, current initially described in mast cells upon depletion of the intracellular Ca2+ pools by means of stimulation with inositol 1,4,5-trisphosphate (IP3), ionomycin, or excess of EGTA [3]. As mentioned before, ICRAC is not the only store-operated current and a variety of store-operated currents grouped under the term ISOC have been reported in different cell types, which differ from ICRAC in several biophysical features (see Table 1), including that ISOC are not selective for Ca2+ and exhibit greater conductance than ICRAC (for a review, see [4]). Since the identification of SOCE, two main issues attracted considerable attention and interest: (1) the molecular basis of the communication between the intracellular Ca2+ stores and the channels in the PM and (2) the nature of the store-operated channels.
Figure 1. Milestones in the characterization of Ca2+ entry. In the early 1880s, Ringer revealed the functional role of Ca2+ entry in heart contraction. About a century later, store-operated Ca2+ entry (SOCE) was discovered and, by that time, transient receptor potential (TRP) channels were identified, first in Drosophila and then in mammals. In 2005 and 2006 STIM1 and Orai1, the key components of the Ca2+ release-activated Ca2+ (CRAC) channels, were identified, and canonical TRP (TRPC) channels were found to participate in a non-selective store-operated current together with STIM1 and Orai1. The model represents two alternatives for the involvement of TRPC in the store-operated channels.
Table 1. Biophysical features of store-operated Ca2+ channels. Notes: STIM1 CMD: STIM1 calcium modulating domain; DVF: divalent-free solution; n/d: not determined; STIM1 SOAR: STIM1Orai1-activating region.
  Orai1 Channels Ora1-TRPC Channels References
Current Voltage (I–V) profile Inwardly rectifying Inwardly rectifying [20,21,22][5][6][7]
Positive reversal potential ~ + 50 mV Positive reversal potential

0 to ~ + 10 mV
Permeability and Selectivity Ca2+ K+, Na+, Cs+, Ca2+ and Ba2+ [4,23][4][8]
Low to Cs3+  
Conduct Na+, Li+ and K+ in DVF solutions  
Activation Store depletion via STIM1 SOAR region Store depletion via STIM1 SOAR and polibasic C-terminus regions [24,25][9][10]
Endogenous current size 0.1–0.2 pA/pF at −100 mV   [26][11]
Fast Inactivation Ca2+ n/d [27,28][12][13]
STIM1 CMD
Orai1 68–91 aa
Orai1 137–173 aa
Slow inactivation Mitochondria n/d [29,30,31][14][15][16]
STIM1 390–391 aa
SARAF
Inhibitors 2-APB (30–50 µM) n/d [32,33,34,35,36,37][17][18][19][20][21][22]
La3+ and Gd3+ (100 µM)
Low pH = 6.7
Synta 66
GSK-7975A

GSK-5503A
AnCOA4 (~5 µM)
Back to 1969, Cosens et al. identified a spontaneous Drosophila mutant with altered electroretinogram [5][23] that was attributed to a mutation of the so called transient receptor potential (TRP) channel that resulted in transient, rather than sustained, light-dependent depolarization of the photoreceptors upon Na+ and Ca2+ entry [6][24]Drosophila TRP and its homologue TRPL were characterized as Ca2+ permeable channels activated downstream of phospholipase C [7][25]. In 1995, two separate groups identified the first human homolog of the Drosophila TRP channel, TRPC1 [8,9][26][27]. After the characterization of TRPC1, a number of homologs were identified in mammalian cells and grouped into six subfamilies: TRPC (canonical) comprising seven members (TRPC1-TRPC7), TRPV (vanilloid) including subtypes TRPV1 to TRPV6, TRPM (melastatin), which comprises eight members (TRPM1-TRPM8), TRPA (ankyrin) consisting of only one member TRPA1 and TRPP (polycystin) as well as TRPML (mucolipin) comprising three members each (revised in [10,11][28][29]).
The basic structure of TRP channels consists of six transmembrane helical domains (TM1 through TM6) with a loop between TM5 and TM6 forming the channel pore and N- and C-terminal regions located in the cytosol. TRP channels are thought to tetramerize to form a 24-helix functional protein complex. Mammalian TRP channels exhibit different functional domains, including a variable number of N-terminal ankyrin repeats present in TRPC, TRPV and TRPA that is involved in protein-protein interaction (revised in [10,12,13][28][30][31]). Remarkably, three members of the TRPM subfamily contain a catalytic kinase domain in the C-terminal region and TRPC and TRPM channels exhibit a conserved TRP domain adjacent to TM6, containing a highly conserved sequence named TRP box, involved in signal transduction coupling and channel gating [14][32]. In addition, a number of mammalian TRP members contain N- and/or C-terminal coiled-coil domains that play an important role in channel multimerization [15][33] as well as the interaction of TRPC channels with the endoplasmic reticulum (ER) Ca2+ sensor STIM1 [16][34]. TRPC members contains a C-terminal calmodulin (CaM)- and inositol 1,4,5-trisphosphate receptor (IP3R)-binding (CIRB) site, which participates in the regulation of TRPC channel function [17,18][35][36].
TRP channels are mostly non-selective cation channels that are permeable to both monovalent and divalent cations with Ca2+ to Na+ permeability ratios ranging from 0.01 to over 100 [19][37]. The pore-forming TM5–TM6 loop has been reported to be highly conserved among all TRP members, and contains several hydrophobic residues at the beginning of the channel pore. TRP channel gating occurs in response to a variety of physical and chemical stimuli and leads to both rises in cytosolic Ca2+ concentration and membrane depolarization, which, in turn, activate a number of cellular functions. TRP-induced membrane depolarization might also decrease the driving force for Ca2+ influx through other channels (see Section 3).
Since the identification of the mammalian TRP channels, a considerable attention has been focused on the role of TRPC1 and other TRPC channels as candidates to conduct Ca2+ influx during SOCE.

2. TRPC Channels in the STIM1–Orai1 Scenario

A new scenario emerged in the study of SOCE after the identification of Orai1 and Stim1 as the key components of the CRAC (Ca2+ release-activated Ca2+ channels). STIM1 was identified as the Ca2+ sensor in the ER which communicates the Ca2+ content of the stores to the channels in the plasma membrane, while Orai1 was identified as the pore subunit of the CRAC channel in the plasma membrane [38,39,40,41][38][39][40][41]. The expression of splice variants of STIM1 and Orai1 with functional and biophysical differences have been demonstrated in mammalian cells. STIM1L, a longer splice variant of STIM1 described in adult human muscle fibers, displays a fast full SOCE activation compared to STIM1 [42]. Regarding to Orai1, two different variants generated by alternative translation initiation, Orai1α and Orai1β, have been shown to drive ICRAC and ISOC currents [43,44][43][44]. In addition to these variants, mammalian cells also express other STIM and Orai isoforms involved in the generation of ICRAC currents. STIM2 is a more sensitive ER Ca2+ sensor than STIM1, but it promotes a weaker CRAC channel activation [45]. Three variants of STIM2, (STIM 2.1, STIM2.2, and STIM2.3) with different roles in the modulation of SOCE have been identified. While STIM2.1 has been described to play an inhibitory role, STIM2.2 has been shown as an activator of SOCE. The function of the STIM2.3 variant still remains unclear [46,47][46][47]. Orai2 and Orai3 proteins have also been shown to drive ICRAC currents after depletion of the intracellular stores [48,49,50][48][49][50] and their regulation and physiological role are less known as compared to Orai1. Therefore, it is currently widely established that the Orai-STIM complex, mainly Orai1-STIM1, constitutes the highly selective CRAC channel. TRPC1 was the first candidate proposed as SOC channel in Chinese hamster ovary cells [51] and monkey COS cells [52] by the expression of TRPC1A, a splice variant of TRPC1, and the expression of a full-length cDNA encoding human TRPC1, respectively. In both cases, the consequence was an increased SOCE after depletion of the intracellular Ca2+ stores. Later, the role of TRPC1 as the SOC channel was confirmed using different approaches in a large number of human cells, including submandibular gland cells [53], endothelial cells [54] and platelets [55], among others. However, the involvement of TRPC channels in SOCE has long been controversial with different studies providing evidence against a functional role of TRPC channels in SOCE. For instance, overexpression of TRPC channels, including TRPC3 [56[56][57],57], has been found to induce non-capacitative Ca2+ entry downstream of phospholipase C in a variety of cell models. A major problem for the involvement of TRPC channels in SOCE is that these channels cannot reproduce the biophysical properties of ICRAC. Nevertheless, as ICRAC is not the only store-operated Ca2+ current, this observation does not rule out the possibility that TRPC channels also participate in SOCE under certain scenarios, such as the assembly with the STIM1-Orai1 complex. In the new STIM1-Orai1 scenario for SOCE, it was soon reported that both proteins together with TRPC1 are assembled to form a dynamic STIM1-Orai1-TRPC1 ternary complex that drives the ISOC current [22,58,59,60][7][58][59][60]. Upon store depletion, STIM1 activation promotes its oligomerization and translocation to the ER-PM junctions where it binds Orai1 [58,59][58][59] and TRPC1 [59,61,62][59][61][62] in lipid rafts domains, gating both Ca2+channels [63,64][63][64]. STIM1 mediates Orai1 activation by the interaction of the cytosolic STIM1-Orai1 activation region (SOAR) of STIM1 [24][9] with two STIM1-bindings sites located at the C- and N-termini of Orai1 [65,66,67][65][66][67]. The SOAR region is also required for STIM1-TRPC1 interaction; however, it is not sufficient to activate TRPC1 [24][9]. The activation of TRPC1 requires electrostatic interaction between highly positively charged lysines (684KK685) located in polybasic lysine-rich domain (K-domain) of the STIM1 C-terminus with the conserved, negatively charged, aspartate residues in TRPC1 (639DD640) and equivalent residues in other TRPC channels [25][10]. However, there is no evidence about the domains of Orai1 and TRPC1 involved in their interaction, suggesting that TRPC1-Orai1 binding could be indirectly mediated by STIM1 or still unidentified adaptor proteins [68,69][68][69]. The first evidence of the dynamic assembly of the STIM1-Orai1-TRPC1 ternary complex was found using immunofluorescence and confocal microscopy assay in human salivary gland cells. In resting conditions, STIM1 shows a diffused cytosolic localization while TRPC1 is located in the PM colocalizing with Orai1, although it is also expressed in the cytosolic region. After Ca2+ store depletion, STIM1 co-localized in the PM with both proteins, TRPC1 and Orai1, without modifying the TRPC1 and Orai1 colocalization [59]. Different studies have demonstrated that a functional Orai1 plays an essential role in the STIM1-Orai1-TRPC1 complex formation using different approaches. In human platelets, the STIM1-Orai1-TRPC1 ternary complex formation, including Orai1-STIM1 binding, was demonstrated using immunoprecipitation assays and the electrotransjection with an anti-Orai1 C-terminal antibody impairs the interaction between STIM1 and TRPC1, as well as SOCE activation after intracellular Ca2+ store depletion [58]. In Orai1 knockdown HEK-293 by siRNA-mediated gene silencing, cell transfection with the dominant negative mutants Orai1 E106Q or Orai1R91W, but not with a functional Orai1 construct, failed to restore SOCE [22,60][7][60]. Concerning Orai1 splicing variants, an elegant study demonstrated that both variants of Orai1, Orai1α and Orai1β, are equally involved in the generation of ISOC currents in HEK-293 transfected with STIM1, TRPC1 and either Orai1α or Orai1β [43]. This finding suggests that the STIM1-Orai1-TRPC1 complex might include both Orai1α or Orai1β proteins. A model proposed by Cheng and coworkers, in human salivary gland cells, suggests that depletion of intracellular stores promotes Ca2+ influx via Orai1-STIM1 complex, providing a local increase in free Ca2+ concentration that induces the translocation of TRPC1 to the vicinity of the STIM1-Orai1 complex (Figure 2). Beyond the activation of TRPC1 by STIM1, this transition also leads to the association of TRPC1 and Orai1 in the same complex. Interestingly, this model could explain the essential role of Orai1 and the lack of strong evidence supporting the direct association between Orai1 and TRPC1 in the assembly of the STIM1-Orai1-TRPC1 complex [69]. Besides different biophysical properties, the Orai1-STIM1 complex to mediate the ICRAC current and the STIM1-Orai1-TRPC1 ternary complex to mediate the ISOC current also display specific temporal and spatial Ca2+ oscillatory patterns involved in the activation of different physiological functions and in the pathogenesis of a number of diseases (revised in [70]). For instance, Orai1-STIM1-mediated Ca2+ entry promotes the activation and nuclear translocation of the NFAT (nuclear factor of activated T-cells) transcription factor, while a TRPC1-dependent Ca2+ entry is responsible for NF-κB transcription factor activation in human submandibular gland cells [71]. STIM1-Orai1-TRPC1-mediated Ca2+ entry is also required for platelet aggregation [72], insulin release [73], adipocyte differentiation and adiponectin secretion [74], among other functions. Moreover, STIM1-Orai1-TRPC1-dependent Ca2+ currents have been associated to the Ca2+ mobilization responsible for the development of distinct cancer hallmarks in different cancer cell types, including prostate cancer cells [75] and colon cancer cells [76[76][77],77], while STIM1-Orai1-TRPC1-TRPC4-mediated Ca2+ currents are involved in the Ca2+ remodelling involved in hypertrophic cardiomyopathy in rat ventricular myocytes [78]. A more recent study has reported that in anterior pituitary (AP) cells from Orai1-lacking mice TG-induced SOCE as well as Ca2+ entry evoked by TRH and LHRH were impaired, by contrast, SOCE was unaffected in AP cells from mice lacking expression of all seven TRPC channels, although spontaneous intracellular Ca2+-oscillations associated to electrical activity as well as Ca2+ responses to TRH and GHRH were significantly reduced in the absence of TRPC channels, thus suggesting that SOCE might function independently of TRPC channels and that Orai1 and TRPC channels, such as TRPC1, might play different functional roles [79].
Figure 2. Cartoon depicting the activation of TRPC1 channels upon Ca2+ store depletion. (a) In the resting state, TRPC1 shows both plasma membrane and cytosolic localization. (b) Upon Ca2+ store depletion, Ca2+ influx via Orai1 has been reported to induce the translocation of intracellularly-located TRPC1 to the plasma membrane where it might be activated by STIM1. The model shows two alternatives for functional (mediating Ca2+ entry for the translocation of TRPC1 to the plasma membrane; left panel) or direct participation of Orai1 in the activation of TRPC1 (forming a STIM1–Orai1–TRPC1 ternary complex; right panel).
Despite the findings that proposed the STIM1-Orai1-TRPC1 ternary complex as the SOC channel, different observations suggest that ORAI1-STIM1 and TRPC1-STIM1 complexes can also drive ISOC currents depending on the cell type and the components of its Ca2+ signalling toolkit. Hence in cells with a robust ICRAC, such as Jurkat cells, the Orai1-STIM1 complex is involved in both ICRAC and ISOC currents [22][7]. Furthermore, different studies have shown that TRPC1 interacts with STIM1 forming a complex without the involvement of Orai1 to mediate SOCE in vascular smooth muscle cells with a contractile phenotype [80]. In human myotubes, where Orai1 has been reported to be essential for SOCE and differentiation [81[81][82],82], the TRPC1-TRPC4-STIM1L complex has been reported to form a SOC channel whose Ca2+ inward current is required for human myogenesis and to maintain fast repetitive Ca2+ release in human myotubes [83]. Interestingly, the integration of Orai1 in this complex promotes an enhanced ICRAC-like current involved in the development of the hypertrophic cardiomyopathy in rat ventricular myocytes, as described above [78].

3. Modulation of Orai1 Function by TRPC Channels

As mentioned previously, TRPC channels, especially TRPC1 [22,58,70,77][7][58][70][77] but also other members of the TRPC subfamily, such as TRPC4 [84,85][84][85] and TRPC6 [86,87[86][87][88][89],88,89], have been reported to conduct Ca2+ entry upon Ca2+ store depletion. However, there is a growing body of evidence indicating that TRPC channels play a more complex role shaping Ca2+ signals through Orai1 channels. TRPC5 and TRPC6 show the greatest selectivity for Ca2+ relative to Na+ of the TRPC subfamily with Ca2+/Na+ permeability ratios around 9 and 5, respectively, while TRPC4 and TRPC1 are approximately equally permeable to Ca2+ and Na+ [90]. The latter means that TRPC channel gating leads to Ca2+ and Na+ influx in favor of an electrochemical gradient, which, in turn, might attenuate the inward flux of Ca2+ through Orai1 channels in two different manners: (1) inducing Ca2+-dependent inactivation of the Orai1 channels and (2) attenuating the driving force for Ca2+ entry as a result of membrane depolarization (Figure 3a,b). Concerning the first issue, fast Ca2+-dependent Orai1 inactivation has been suggested to be evoked by the interaction of Ca2+ entering through the channel itself to cytosolic inactivating sites in close proximity to the channel pore [91,92][91][92]; however, slow inactivation of Orai1 channels is associated to global increases in cytosolic Ca2+ concentration [93] that might be influenced by opening of TRPC channels in the vicinity of Orai1. In tumor cells with a gain of function of TRPC channels, in addition to Ca2+ entry, Na+ influx has been associated to Ca2+ efflux from the mitochondria due to exchange for Na+, thus resulting in further Ca2+-dependent inactivation of Orai1 channels (revised in [94]). Furthermore, the opening of TRPC channels might increase the amount of Ca2+ available to SERCA (sarco/endoplasmic reticulum Ca2+-ATPase) pumps and, therefore, store refilling, thus accelerating the deactivation of Orai1 channels. On the other hand, it has long been reported that TRP channel opening results in membrane depolarization. A well-known depolarizing TRP channel is TRPM4, which has been found to depolarize T lymphocytes [95]. Membrane depolarization induced by TRPC channel gating has been associated to a functional activation of voltage-dependent Ca2+ channels in electrically excitable cells [96,97][96][97]. In addition, depolarization evoked by Ca2+ and Na+ influx through TRPC channels leads to subsequent attenuation of the driving force for Ca2+ entry via Orai1 channels.
Figure 3. Overview of the modulation of Orai1 by TRPC channels. Orai1 channel function might be positively or negatively regulated by TRPC channels in the vicinity. (a) Ca2+ and Na+ entry through TRPC channels might lead to membrane depolarization and thus attenuation of the electrical gradient that favors Ca2+ influx via Orai1. (b) Ca2+ entry via TRPC channels participates in global rises in [Ca2+]c, thus leading to Ca2+-dependent inactivation of Orai1 channels. (c) Some TRPC channels are required for Orai1 recycling at the plasma membrane.
TRPC channels have also been reported to modulate the localization of other Ca2+-permeable channels in the plasma membrane. Schindl and coworkers have reported that co-expression of TRPC1 with TRPV6 down-regulates the plasma membrane expression of the latter [98]. TRPC channels has been found to be involved in the modulation of cytoskeletal rearrangements [99]. We have recently reported that TRPC6 modulates the plasma membrane expression of Orai1 and Orai3 channels in triple negative and luminal, respectively, breast cancer cells. Thus, attenuation of the expression of TRPC6, either by using interference RNA or by cell treatment with the phenolic compound oleocanthal, results in a significant decrease in SOCE in these cells [100,101][100][101]. TRPC6-dependent plasma membrane recycling of Orai1 is entirely dependent on Ca2+ and Na+ influx through TRPC6 channels as it is abolished by expression of the pore-dead dominant-negative TRPC6 mutant [100] (Figure 3c). Whether this mechanism is mediated by cytoskeletal remodeling remains to be determined.

References

  1. Ringer, S. A further Contribution regarding the influence of the different Constituents of the Blood on the Contraction of the Heart. J. Physiol. 1883, 4, 29–42.
  2. Putney, J.W., Jr. A model for receptor-regulated calcium entry. Cell Calcium 1986, 7, 1–12.
  3. Hoth, M.; Penner, R. Depletion of intracellular calcium stores activates a calcium current in mast cells. Nature 1992, 355, 353–356.
  4. Parekh, A.B.; Putney, J.W., Jr. Store-operated calcium channels. Physiol. Rev. 2005, 85, 757–810.
  5. Feske, S.; Gwack, Y.; Prakriya, M.; Srikanth, S.; Puppel, S.H.; Tanasa, B.; Hogan, P.G.; Lewis, R.S.; Daly, M.; Rao, A. A mutation in Orai1 causes immune deficiency by abrogating CRAC channel function. Nature 2006, 441, 179–185.
  6. Penner, R.; Matthews, G.; Neher, E. Regulation of calcium influx by second messengers in rat mast cells. Nature 1988, 334, 499–504.
  7. Kim, M.S.; Zeng, W.; Yuan, J.P.; Shin, D.M.; Worley, P.F.; Muallem, S. Native Store-operated Ca2+ Influx Requires the Channel Function of Orai1 and TRPC1. J. Biol. Chem. 2009, 284, 9733–9741.
  8. Parekh, A.B.; Penner, R. Store depletion and calcium influx. Physiol. Rev. 1997, 77, 901–930.
  9. Yuan, J.P.; Zeng, W.; Dorwart, M.R.; Choi, Y.J.; Worley, P.F.; Muallem, S. SOAR and the polybasic STIM1 domains gate and regulate Orai channels. Nat. Cell Biol. 2009, 11, 337–343.
  10. Zeng, W.; Yuan, J.P.; Kim, M.S.; Choi, Y.J.; Huang, G.N.; Worley, P.F.; Muallem, S. STIM1 gates TRPC channels, but not Orai1, by electrostatic interaction. Mol. Cell 2008, 32, 439–448.
  11. Zhang, X.; Gueguinou, M.; Trebak, M. Store-Independent Orai Channels Regulated by STIM. In Calcium Entry Channels in Non-Excitable Cells; Kozak, J.A., Putney, J.W., Jr., Eds.; Taylor and Francis Group: Boca Raton, FL, USA, 2018; pp. 197–214.
  12. Derler, I.; Fahrner, M.; Muik, M.; Lackner, B.; Schindl, R.; Groschner, K.; Romanin, C. A Ca2+release-activated Ca2+ (CRAC) modulatory domain (CMD) within STIM1 mediates fast Ca2+-dependent inactivation of ORAI1 channels. J. Biol. Chem. 2009, 284, 24933–24938.
  13. Lis, A.; Peinelt, C.; Beck, A.; Parvez, S.; Monteilh-Zoller, M.; Fleig, A.; Penner, R. CRACM1, CRACM2, and CRACM3 are store-operated Ca2+ channels with distinct functional properties. Curr. Biol. 2007, 17, 794–800.
  14. Albarran, L.; Lopez, J.J.; Gomez, L.J.; Salido, G.M.; Rosado, J.A. SARAF modulates TRPC1, but not TRPC6, channel function in a STIM1-independent manner. Biochem. J. 2016, 473, 3581–3595.
  15. Jha, A.; Ahuja, M.; Maleth, J.; Moreno, C.M.; Yuan, J.P.; Kim, M.S.; Muallem, S. The STIM1 CTID domain determines access of SARAF to SOAR to regulate Orai1 channel function. J. Cell Biol. 2013, 202, 71–79.
  16. Palty, R.; Raveh, A.; Kaminsky, I.; Meller, R.; Reuveny, E. SARAF inactivates the store operated calcium entry machinery to prevent excess calcium refilling. Cell 2012, 149, 425–438.
  17. Iwasaki, H.; Mori, Y.; Hara, Y.; Uchida, K.; Zhou, H.; Mikoshiba, K. 2-Aminoethoxydiphenyl borate (2-APB) inhibits capacitative calcium entry independently of the function of inositol 1,4,5-trisphosphate receptors. Recept. Channels 2001, 7, 429–439.
  18. Schindl, R.; Bergsmann, J.; Frischauf, I.; Derler, I.; Fahrner, M.; Muik, M.; Fritsch, R.; Groschner, K.; Romanin, C. 2-aminoethoxydiphenyl borate alters selectivity of Orai3 channels by increasing their pore size. J. Biol. Chem. 2008, 283, 20261–20267.
  19. Beech, D.J. Orai1 calcium channels in the vasculature. Pflug. Arch. 2012, 463, 635–647.
  20. Scrimgeour, N.; Litjens, T.; Ma, L.; Barritt, G.J.; Rychkov, G.Y. Properties of Orai1 mediated store-operated current depend on the expression levels of STIM1 and Orai1 proteins. J. Physiol. 2009, 587, 2903–2918.
  21. Derler, I.; Schindl, R.; Fritsch, R.; Heftberger, P.; Riedl, M.C.; Begg, M.; House, D.; Romanin, C. The action of selective CRAC channel blockers is affected by the Orai pore geometry. Cell Calcium 2013, 53, 139–151.
  22. Sadaghiani, A.M.; Lee, S.M.; Odegaard, J.I.; Leveson-Gower, D.B.; McPherson, O.M.; Novick, P.; Kim, M.R.; Koehler, A.N.; Negrin, R.; Dolmetsch, R.E.; et al. Identification of Orai1 channel inhibitors by using minimal functional domains to screen small molecule microarrays. Chem. Biol. 2014, 21, 1278–1292.
  23. Cosens, D.J.; Manning, A. Abnormal electroretinogram from a Drosophila mutant. Nature 1969, 224, 285–287.
  24. Minke, B.; Wu, C.; Pak, W.L. Induction of photoreceptor voltage noise in the dark in Drosophila mutant. Nature 1975, 258, 84–87.
  25. Hardie, R.C. Projection and connectivity of sex-specific photoreceptors in the compound eye of the male housefly (Musca domestica). Cell Tissue Res. 1983, 233, 1–21.
  26. Wes, P.D.; Chevesich, J.; Jeromin, A.; Rosenberg, C.; Stetten, G.; Montell, C. TRPC1, a human homolog of a Drosophila store-operated channel. Proc. Natl. Acad. Sci. USA 1995, 92, 9652–9656.
  27. Zhu, X.; Chu, P.B.; Peyton, M.; Birnbaumer, L. Molecular cloning of a widely expressed human homologue for the Drosophila trp gene. FEBS Lett. 1995, 373, 193–198.
  28. Venkatachalam, K.; Montell, C. TRP channels. Annu. Rev. Biochem. 2007, 76, 387–417.
  29. Montell, C. The TRP superfamily of cation channels. Sci. Singal. 2005, 2005, re3.
  30. Hellmich, U.A.; Gaudet, R. Structural biology of TRP channels. Handb. Exp. Pharmacol. 2014, 223, 963–990.
  31. Schaefer, M. Homo-and heteromeric assembly of TRP channel subunits. Pflug. Arch. 2005, 451, 35–42.
  32. Gregorio-Teruel, L.; Valente, P.; Gonzalez-Ros, J.M.; Fernandez-Ballester, G.; Ferrer-Montiel, A. Mutation of I696 and W697 in the TRP box of vanilloid receptor subtype I modulates allosteric channel activation. J. Gen. Physiol. 2014, 143, 361–375.
  33. Baez-Nieto, D.; Castillo, J.P.; Dragicevic, C.; Alvarez, O.; Latorre, R. Thermo-TRP channels: Biophysics of polymodal receptors. Adv. Exp. Med. Biol. 2011, 704, 469–490.
  34. Lee, K.P.; Choi, S.; Hong, J.H.; Ahuja, M.; Graham, S.; Ma, R.; So, I.; Shin, D.M.; Muallem, S.; Yuan, J.P. Molecular determinants mediating gating of Transient Receptor Potential Canonical (TRPC) channels by stromal interaction molecule 1 (STIM1). J. Biol. Chem. 2014, 289, 6372–6382.
  35. Wedel, B.J.; Vazquez, G.; McKay, R.R.; St, J.B.G.; Putney, J.W., Jr. A calmodulin/inositol 1,4,5-trisphosphate (IP3) receptor-binding region targets TRPC3 to the plasma membrane in a calmodulin/IP3 receptor-independent process. J. Biol. Chem. 2003, 278, 25758–25765.
  36. Dionisio, N.; Albarran, L.; Berna-Erro, A.; Hernandez-Cruz, J.M.; Salido, G.M.; Rosado, J.A. Functional role of the calmodulin-and inositol 1,4,5-trisphosphate receptor-binding (CIRB) site of TRPC6 in human platelet activation. Cell. Signal. 2011, 23, 1850–1856.
  37. Talavera, K.; Nilius, B. Electrophysiological Methods for the Study of TRP Channels. In TRP Channels; Zhu, M.X., Ed.; Taylor and Francis Group: Boca Raton, FL, USA, 2011.
  38. Yeromin, A.V.; Zhang, S.L.; Jiang, W.; Yu, Y.; Safrina, O.; Cahalan, M.D. Molecular identification of the CRAC channel by altered ion selectivity in a mutant of Orai. Nature 2006, 443, 226–229.
  39. Luik, R.M.; Wu, M.M.; Buchanan, J.; Lewis, R.S. The elementary unit of store-operated Ca2+ entry: Local activation of CRAC channels by STIM1 at ER-plasma membrane junctions. J. Cell Biol. 2006, 174, 815–825.
  40. Vig, M.; Beck, A.; Billingsley, J.M.; Lis, A.; Parvez, S.; Peinelt, C.; Koomoa, D.L.; Soboloff, J.; Gill, D.L.; Fleig, A.; et al. CRACM1 multimers form the ion-selective pore of the CRAC channel. Curr. Biol. 2006, 16, 2073–2079.
  41. Prakriya, M.; Feske, S.; Gwack, Y.; Srikanth, S.; Rao, A.; Hogan, P.G. Orai1 is an essential pore subunit of the CRAC channel. Nature 2006, 443, 230–233.
  42. Darbellay, B.; Arnaudeau, S.; Bader, C.R.; Konig, S.; Bernheim, L. STIM1L is a new actin-binding splice variant involved in fast repetitive Ca2+ release. J. Cell Biol. 2011, 194, 335–346.
  43. Desai, P.N.; Zhang, X.; Wu, S.; Janoshazi, A.; Bolimuntha, S.; Putney, J.W.; Trebak, M. Multiple types of calcium channels arising from alternative translation initiation of the Orai1 message. Sci. Signal. 2015, 8, ra74.
  44. Fukushima, M.; Tomita, T.; Janoshazi, A.; Putney, J.W. Alternative translation initiation gives rise to two isoforms of Orai1 with distinct plasma membrane mobilities. J. Cell Sci. 2012, 125, 4354–4361.
  45. Stathopulos, P.B.; Zheng, L.; Ikura, M. Stromal interaction molecule (STIM) 1 and STIM2 calcium sensing regions exhibit distinct unfolding and oligomerization kinetics. J. Biol. Chem. 2009, 284, 728–732.
  46. Miederer, A.M.; Alansary, D.; Schwar, G.; Lee, P.H.; Jung, M.; Helms, V.; Niemeyer, B.A. A STIM2 splice variant negatively regulates store-operated calcium entry. Nat. Commun. 2015, 6, 6899.
  47. Rana, A.; Yen, M.; Sadaghiani, A.M.; Malmersjo, S.; Park, C.Y.; Dolmetsch, R.E.; Lewis, R.S. Alternative splicing converts STIM2 from an activator to an inhibitor of store-operated calcium channels. J. Cell Biol. 2015, 209, 653–669.
  48. Vaeth, M.; Yang, J.; Yamashita, M.; Zee, I.; Eckstein, M.; Knosp, C.; Kaufmann, U.; Karoly Jani, P.; Lacruz, R.S.; Flockerzi, V.; et al. ORAI2 modulates store-operated calcium entry and T cell-mediated immunity. Nat. Commun. 2017, 8, 14714.
  49. Wang, J.; Xu, C.; Zheng, Q.; Yang, K.; Lai, N.; Wang, T.; Tang, H.; Lu, W. Orai1, 2, 3 and STIM1 promote store-operated calcium entry in pulmonary arterial smooth muscle cells. Cell Death Discov. 2017, 3, 17074.
  50. Wei, D.; Mei, Y.; Xia, J.; Hu, H. Orai1 and Orai3 Mediate Store-Operated Calcium Entry Contributing to Neuronal Excitability in Dorsal Root Ganglion Neurons. Front. Cell. Neurosci. 2017, 11, 400.
  51. Zitt, C.; Zobel, A.; Obukhov, A.G.; Harteneck, C.; Kalkbrenner, F.; Luckhoff, A.; Schultz, G. Cloning and functional expression of a human Ca2+-permeable cation channel activated by calcium store depletion. Neuron 1996, 16, 1189–1196.
  52. Zhu, X.; Jiang, M.; Peyton, M.; Boulay, G.; Hurst, R.; Stefani, E.; Birnbaumer, L. Trp, a novel mammalian gene family essential for agonist-activated capacitative Ca2+ entry. Cell 1996, 85, 661–671.
  53. Liu, X.; Wang, W.; Singh, B.B.; Lockwich, T.; Jadlowiec, J.; O’Connell, B.; Wellner, R.; Zhu, M.X.; Ambudkar, I.S. Trp1, a candidate protein for the store-operated Ca2+ influx mechanism in salivary gland cells. J. Biol. Chem. 2000, 275, 3403–3411.
  54. Brough, G.H.; Wu, S.; Cioffi, D.; Moore, T.M.; Li, M.; Dean, N.; Stevens, T. Contribution of endogenously expressed Trp1 to a Ca2+-selective, store-operated Ca2+ entry pathway. FASEB J. 2001, 15, 1727–1738.
  55. Rosado, J.A.; Brownlow, S.L.; Sage, S.O. Endogenously expressed Trp1 is involved in store-mediated Ca2+ entry by conformational coupling in human platelets. J. Biol. Chem. 2002, 277, 42157–42163.
  56. Zitt, C.; Obukhov, A.G.; Strubing, C.; Zobel, A.; Kalkbrenner, F.; Luckhoff, A.; Schultz, G. Expression of TRPC3 in Chinese hamster ovary cells results in calcium-activated cation currents not related to store depletion. J. Cell Biol. 1997, 138, 1333–1341.
  57. Trebak, M.; St, J.B.G.; McKay, R.R.; Birnbaumer, L.; Putney, J.W., Jr. Signaling mechanism for receptor-activated canonical transient receptor potential 3 (TRPC3) channels. J. Biol. Chem. 2003, 278, 16244–16252.
  58. Jardin, I.; Lopez, J.J.; Salido, G.M.; Rosado, J.A. Orai1 mediates the interaction between STIM1 and hTRPC1 and regulates the mode of activation of hTRPC1-forming Ca2+ channels. J. Biol. Chem. 2008, 283, 25296–25304.
  59. Ong, H.L.; Cheng, K.T.; Liu, X.; Bandyopadhyay, B.C.; Paria, B.C.; Soboloff, J.; Pani, B.; Gwack, Y.; Srikanth, S.; Singh, B.B.; et al. Dynamic assembly of TRPC1-STIM1-Orai1 ternary complex is involved in store-operated calcium influx. Evidence for similarities in store-operated and calcium release-activated calcium channel components. J. Biol. Chem. 2007, 282, 9105–9116.
  60. Cheng, K.T.; Liu, X.; Ong, H.L.; Ambudkar, I.S. Functional requirement for Orai1 in store-operated TRPC1-STIM1 channels. J. Biol. Chem. 2008, 283, 12935–12940.
  61. Lopez, J.J.; Salido, G.M.; Pariente, J.A.; Rosado, J.A. Interaction of STIM1 with endogenously expressed human canonical TRP1 upon depletion of intracellular Ca2+ stores. J. Biol. Chem. 2006, 281, 28254–28264.
  62. Yuan, J.P.; Zeng, W.; Huang, G.N.; Worley, P.F.; Muallem, S. STIM1 heteromultimerizes TRPC channels to determine their function as store-operated channels. Nat. Cell Biol. 2007, 9, 636–645.
  63. Jardin, I.; Salido, G.M.; Rosado, J.A. Role of lipid rafts in the interaction between hTRPC1, Orai1 and STIM1. Channels 2008, 2, 401–403.
  64. Liao, Y.; Plummer, N.W.; George, M.D.; Abramowitz, J.; Zhu, M.X.; Birnbaumer, L. A role for Orai in TRPC-mediated Ca2+ entry suggests that a TRPC:Orai complex may mediate store and receptor operated Ca2+ entry. Proc. Natl. Acad. Sci. USA 2009, 106, 3202–3206.
  65. Derler, I.; Plenk, P.; Fahrner, M.; Muik, M.; Jardin, I.; Schindl, R.; Gruber, H.J.; Groschner, K.; Romanin, C. The extended transmembrane Orai1 N-terminal (ETON) region combines binding interface and gate for Orai1 activation by STIM1. J. Biol. Chem. 2013, 288, 29025–29034.
  66. Stathopulos, P.B.; Schindl, R.; Fahrner, M.; Zheng, L.; Gasmi-Seabrook, G.M.; Muik, M.; Romanin, C.; Ikura, M. STIM1/Orai1 coiled-coil interplay in the regulation of store-operated calcium entry. Nat. Commun. 2013, 4, 2963.
  67. Fahrner, M.; Muik, M.; Schindl, R.; Butorac, C.; Stathopulos, P.; Zheng, L.; Jardin, I.; Ikura, M.; Romanin, C. A coiled-coil clamp controls both conformation and clustering of stromal interaction molecule 1 (STIM1). J. Biol. Chem. 2014, 289, 33231–33244.
  68. Jia, S.; Rodriguez, M.; Williams, A.G.; Yuan, J.P. Homer binds to Orai1 and TRPC channels in the neointima and regulates vascular smooth muscle cell migration and proliferation. Sci. Rep. 2017, 7, 5075.
  69. Cheng, K.T.; Liu, X.; Ong, H.L.; Swaim, W.; Ambudkar, I.S. Local Ca2+ entry via Orai1 regulates plasma membrane recruitment of TRPC1 and controls cytosolic Ca2+ signals required for specific cell functions. PLoS Biol. 2011, 9, e1001025.
  70. Ambudkar, I.S.; de Souza, L.B.; Ong, H.L. TRPC1, Orai1, and STIM1 in SOCE: Friends in tight spaces. Cell Calcium 2017, 63, 33–39.
  71. Ong, H.L.; Jang, S.I.; Ambudkar, I.S. Distinct contributions of Orai1 and TRPC1 to agonist-induced [Ca2+](i) signals determine specificity of Ca2+-dependent gene expression. PLoS ONE 2012, 7, e47146.
  72. Galan, C.; Zbidi, H.; Bartegi, A.; Salido, G.M.; Rosado, J.A. STIM1, Orai1 and hTRPC1 are important for thrombin- and ADP-induced aggregation in human platelets. Arch. Biochem. Biophys. 2009, 490, 137–144.
  73. Sabourin, J.; Le Gal, L.; Saurwein, L.; Haefliger, J.A.; Raddatz, E.; Allagnat, F. Store-operated Ca2+ Entry Mediated by Orai1 and TRPC1 Participates to Insulin Secretion in Rat beta-Cells. J. Biol. Chem. 2015, 290, 30530–30539.
  74. Schaar, A.; Sun, Y.; Sukumaran, P.; Rosenberger, T.A.; Krout, D.; Roemmich, J.N.; Brinbaumer, L.; Claycombe-Larson, K.; Singh, B.B. Ca2+ entry via TRPC1 is essential for cellular differentiation and modulates secretion via the SNARE complex. J. Cell Sci. 2019, 132.
  75. Perrouin-Verbe, M.A.; Schoentgen, N.; Talagas, M.; Garlantezec, R.; Uguen, A.; Doucet, L.; Rosec, S.; Marcorelles, P.; Potier-Cartereau, M.; Vandier, C.; et al. Overexpression of certain transient receptor potential and Orai channels in prostate cancer is associated with decreased risk of systemic recurrence after radical prostatectomy. Prostate 2019, 79, 1793–1804.
  76. Gutierrez, L.G.; Hernandez-Morales, M.; Nunez, L.; Villalobos, C. Inhibition of Polyamine Biosynthesis Reverses Ca2+ Channel Remodeling in Colon Cancer Cells. Cancers 2019, 11, 83.
  77. Gueguinou, M.; Harnois, T.; Crottes, D.; Uguen, A.; Deliot, N.; Gambade, A.; Chantome, A.; Haelters, J.P.; Jaffres, P.A.; Jourdan, M.L.; et al. SK3/TRPC1/Orai1 complex regulates SOCE-dependent colon cancer cell migration: A novel opportunity to modulate anti-EGFR mAb action by the alkyl-lipid Ohmline. Oncotarget 2016, 7, 36168–36184.
  78. Sabourin, J.; Boet, A.; Rucker-Martin, C.; Lambert, M.; Gomez, A.M.; Benitah, J.P.; Perros, F.; Humbert, M.; Antigny, F. Ca2+ handling remodeling and STIM1L/Orai1/TRPC1/TRPC4 upregulation in monocrotaline-induced right ventricular hypertrophy. J. Mol. Cell. Cardiol. 2018, 118, 208–224.
  79. Nunez, L.; Bird, G.S.; Hernando-Perez, E.; Perez-Riesgo, E.; Putney, J.W., Jr.; Villalobos, C. Store-operated Ca2+ entry and Ca2+ responses to hypothalamic releasing hormones in anterior pituitary cells from Orai1-/-and heptaTRPC knockout mice. Biochim. Biophys. Acta Mol. Cell Res. 2019, 1866, 1124–1136.
  80. Shi, J.; Miralles, F.; Kinet, J.P.; Birnbaumer, L.; Large, W.A.; Albert, A.P. Evidence that Orai1 does not contribute to store-operated TRPC1 channels in vascular smooth muscle cells. Channels 2017, 11, 329–339.
  81. Darbellay, B.; Arnaudeau, S.; Konig, S.; Jousset, H.; Bader, C.; Demaurex, N.; Bernheim, L. STIM1- and Orai1-dependent store-operated calcium entry regulates human myoblast differentiation. J. Biol. Chem. 2009, 284, 5370–5380.
  82. Antigny, F.; Koenig, S.; Bernheim, L.; Frieden, M. During post-natal human myogenesis, normal myotube size requires TRPC1-and TRPC4-mediated Ca2+ entry. J. Cell Sci. 2013, 126, 2525–2533.
  83. Antigny, F.; Sabourin, J.; Sauc, S.; Bernheim, L.; Koenig, S.; Frieden, M. TRPC1 and TRPC4 channels functionally interact with STIM1L to promote myogenesis and maintain fast repetitive Ca2+ release in human myotubes. Biochim. Biophys. Acta Mol. Cell Res. 2017, 1864, 806–813.
  84. Fatherazi, S.; Presland, R.B.; Belton, C.M.; Goodwin, P.; Al-Qutub, M.; Trbic, Z.; Macdonald, G.; Schubert, M.M.; Izutsu, K.T. Evidence that TRPC4 supports the calcium selective I(CRAC)-like current in human gingival keratinocytes. Pflug. Arch. 2007, 453, 879–889.
  85. Sundivakkam, P.C.; Freichel, M.; Singh, V.; Yuan, J.P.; Vogel, S.M.; Flockerzi, V.; Malik, A.B.; Tiruppathi, C. The Ca2+ sensor stromal interaction molecule 1 (STIM1) is necessary and sufficient for the store-operated Ca2+ entry function of transient receptor potential canonical (TRPC) 1 and 4 channels in endothelial cells. Mol. Pharmacol. 2012, 81, 510–526.
  86. Brechard, S.; Melchior, C.; Plancon, S.; Schenten, V.; Tschirhart, E.J. Store-operated Ca2+ channels formed by TRPC1, TRPC6 and Orai1 and non-store-operated channels formed by TRPC3 are involved in the regulation of NADPH oxidase in HL-60 granulocytes. Cell Calcium 2008, 44, 492–506.
  87. Jardin, I.; Redondo, P.C.; Salido, G.M.; Rosado, J.A. Phosphatidylinositol 4,5-bisphosphate enhances store-operated calcium entry through hTRPC6 channel in human platelets. Biochim. Biophys. Acta 2008, 1783, 84–97.
  88. Selli, C.; Erac, Y.; Kosova, B.; Tosun, M. Post-transcriptional silencing of TRPC1 ion channel gene by RNA interference upregulates TRPC6 expression and store-operated Ca2+ entry in A7r5 vascular smooth muscle cells. Vasc. Pharmacol. 2009, 51, 96–100.
  89. Jardin, I.; Gomez, L.J.; Salido, G.M.; Rosado, J.A. Dynamic interaction of hTRPC6 with the Orai1/STIM1 complex or hTRPC3 mediates its role in capacitative or non-capacitative Ca2+ entry pathways. Biochem. J. 2009, 420, 267–276.
  90. Gees, M.; Colsoul, B.; Nilius, B. The role of transient receptor potential cation channels in Ca2+ signaling. Cold Spring Harb. Perspect. Biol. 2010, 2, a003962.
  91. Zweifach, A.; Lewis, R.S. Rapid inactivation of depletion-activated calcium current (ICRAC) due to local calcium feedback. J. Gen. Physiol. 1995, 105, 209–226.
  92. Fierro, L.; Parekh, A.B. Fast calcium-dependent inactivation of calcium release-activated calcium current (CRAC) in RBL-1 cells. J. Membr. Biol. 1999, 168, 9–17.
  93. Zweifach, A.; Lewis, R.S. Slow calcium-dependent inactivation of depletion-activated calcium current. Store-dependent and -independent mechanisms. J. Biol. Chem. 1995, 270, 14445–14451.
  94. Villalobos, C.; Gutierrez, L.G.; Hernandez-Morales, M.; Del Bosque, D.; Nunez, L. Mitochondrial control of store-operated Ca2+ channels in cancer: Pharmacological implications. Pharmacol. Res. 2018, 135, 136–143.
  95. Launay, P.; Cheng, H.; Srivatsan, S.; Penner, R.; Fleig, A.; Kinet, J.P. TRPM4 regulates calcium oscillations after T cell activation. Science 2004, 306, 1374–1377.
  96. Avila-Medina, J.; Calderon-Sanchez, E.; Gonzalez-Rodriguez, P.; Monje-Quiroga, F.; Rosado, J.A.; Castellano, A.; Ordonez, A.; Smani, T. Orai1 and TRPC1 Proteins Co-localize with CaV1.2 Channels to Form a Signal Complex in Vascular Smooth Muscle Cells. J. Biol. Chem. 2016, 291, 21148–21159.
  97. Beck, A.; Gotz, V.; Qiao, S.; Weissgerber, P.; Flockerzi, V.; Freichel, M.; Boehm, U. Functional Characterization of Transient Receptor Potential (TRP) Channel C5 in Female Murine Gonadotropes. Endocrinology 2017, 158, 887–902.
  98. Schindl, R.; Fritsch, R.; Jardin, I.; Frischauf, I.; Kahr, H.; Muik, M.; Riedl, M.C.; Groschner, K.; Romanin, C. Canonical transient receptor potential (TRPC) 1 acts as a negative regulator for vanilloid TRPV6-mediated Ca2+ influx. J. Biol. Chem. 2012, 287, 35612–35620.
  99. Moore, T.M.; Brough, G.H.; Babal, P.; Kelly, J.J.; Li, M.; Stevens, T. Store-operated calcium entry promotes shape change in pulmonary endothelial cells expressing Trp1. Am. J. Physiol. 1998, 275, L574–L582.
  100. Jardin, I.; Diez-Bello, R.; Lopez, J.J.; Redondo, P.C.; Salido, G.M.; Smani, T.; Rosado, J.A. TRPC6 Channels Are Required for Proliferation, Migration and Invasion of Breast Cancer Cell Lines by Modulation of Orai1 and Orai3 Surface Exposure. Cancers 2018, 10, 331.
  101. Diez-Bello, R.; Jardin, I.; Lopez, J.J.; El Haouari, M.; Ortega-Vidal, J.; Altarejos, J.; Salido, G.M.; Salido, S.; Rosado, J.A. (-)Oleocanthal inhibits proliferation and migration by modulating Ca2+ entry through TRPC6 in breast cancer cells. Biochim. Biophys. Acta Mol. Cell Res. 2019, 1866, 474–485.
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