Down-Regulation of the Na+,Cl- Coupled Creatine Transporter CreaT (SLC6A8) by Glycogen Synthase Kinase GSK3ß

Fezai, Myriam; Jemaà, Mohamed; Fakhri, Hajar; Chen, Hong; Elsir, Bhaeldin; Pelzl, Lisann; Lang, Florian

doi:10.1159/000453177

Abstract

Background: The Na⁺,Cl^- coupled creatine transporter CreaT (SLC6A8) is expressed in a variety of tissues including the brain. Genetic defects of CreaT lead to mental retardation with seizures. The present study explored the regulation of CreaT by the ubiquitously expressed glycogen synthase kinase GSK3ß, which contributes to the regulation of neuroexcitation. GSK3ß is phosphorylated and thus inhibited by PKB/Akt. Moreover, GSK3ß is inhibited by the antidepressant lithium. The present study thus further tested for the effects of PKB/Akt and of lithium. Methods: CreaT was expressed in Xenopus laevis oocytes with or without wild-type GSK3ß or inactive ^K85RGSK3ß. CreaT and GSK3ß were further expressed without and with additional expression of wild type PKB/Akt. Creatine transport in those oocytes was quantified utilizing dual electrode voltage clamp. Results: Electrogenic creatine transport was observed in CreaT expressing oocytes but not in water-injected oocytes. In CreaT expressing oocytes, co-expression of GSK3ß but not of ^K85RGSK3ß, resulted in a significant decrease of creatine induced current. Kinetic analysis revealed that GSK3ß significantly decreased the maximal creatine transport rate. Exposure of CreaT and GSK3ß expressing oocytes for 24 hours to Lithium was followed by a significant increase of the creatine induced current. The effect of GSK3ß on CreaT was abolished by co-expression of PKB/Akt. Conclusion: GSK3ß down-regulates the creatine transporter CreaT, an effect reversed by treatment with the antidepressant Lithium and by co-expression of PKB/Akt.

Introduction

The creatine transporter CreaT (SLC6A8), a member of the superfamily of sodium and chloride coupled transporters for neurotransmitters [1,2,3] and organic osmolytes [4,5], is expressed in a variety of tissues including brain, retina, skeletal muscle, heart, and several epithelia [6,7,8,9]. Defects of the CreaT (SLC6A8) gene lead to mental retardation with seizures [10,11,12,13,14,15,16,17,18,19,20,21,22,23,24,25,26,27].

Neuronal excitability [28] and cell volume [29] are regulated by the glycogen synthase kinase GSK3ß, a serine/threonine kinase inhibited by the antidepressant Lithium [30]. GSK3ß is phosphorylated and down-regulated by protein kinase B (PKB/Akt) [31].

The present study explored, whether CreaT activity is modified by GSK3ß. To this end, CreaT was expressed in Xenopus laevis oocytes without or with additional expression of wild type GSK3ß, inactive mutant ^K85RGSK3ß or wild-type GSK3ß together with wild type PKB/Akt. Creatine induced current determined by dual electrode voltage clamp was taken as measure of CreaT transport activity.

Materials and Methods

Ethical Statement

All experiments conform with the 'European Convention for the Protection of Vertebrate Animals used for Experimental and other Scientific Purposes' (Council of Europe No 123, Strasbourg 1985) and were conducted according to the German law for the welfare of animals and the surgical procedures on the adult Xenopus laevis frogs were reviewed and approved by the respective government authority of the state Baden-Württemberg (Regierungspräsidium) prior to the start of the study (Anzeige für Organentnahme nach §36).

Constructs

Constructs encoding bovine wild-type CreaT (SLC6A8) [3] (kindly provided by J Lingle), wild-type human GSK3ß [32], inactive mutant ^K85RGSK3ß [33], and wild-type PKB [34] were used for generation of cRNA as described previously [35,36,37,38].

Voltage clamp in Xenopus laevis oocytes

Xenopus laevis oocytes were prepared as previously described [37,38]. 15 ng cRNA encoding CreaT (SLC6A8) and 7.5 ng of cRNA encoding wild-type or inactive kinase were injected on the same day after preparation of the oocytes [36,39,40,41]. The oocytes were maintained at 17°C in ND96-A, a solution containing (in mM): 88.5 NaCl, 2 KCl, 1 MgCl₂, 1.8 CaCl₂, 2.5 NaOH, 5 HEPES, 5 Sodium pyruvate, Gentamycin (100 mg/l), Tetracycline (50 mg/l), Ciprofloxacin (1.6 mg/l), and Theophiline (90 mg/l). The pH was titrated to 7.4 by addition of NaOH [38,42]. Where indicated 1 mM Lithium chloride was added. The voltage clamp experiments were performed at room temperature 4 days after the first injection. Two-electrode voltage-clamp recordings were performed at a holding potential of -60 mV. The data were filtered at 10 Hz and recorded with a Digidata A/D-D/A converter (1322A Axon Instruments) [34,43]. The Clampex 9.2 software was used for data acquisition and analysis (Axon Instruments) [34,41,44]. The control superfusate (ND96-B) contained (in mM): 93.5 NaCl, 2 KCl, 1.8 CaCl₂, 1 MgCl₂, 2.5 NaOH and 5 HEPES, pH 7.4. The flow rate of the superfusion was approx. 20 ml/min, and a complete exchange of the bath solution was reached within about 10 s [45].

Statistical analysis

Data are provided as means ± SEM, n represents the number of oocytes investigated. As different batches of oocytes may yield different results, comparisons were always made within a given oocyte batch. All voltage clamp experiments were repeated with at least 3 batches of oocytes; in all repetitions qualitatively similar data were obtained. Data were tested for significance using ANOVA or t-test, as appropriate. Results with p < 0.05 were considered statistically significant.

Results

In order to test whether the glycogen synthase kinase GSK3ß modifies the function of the creatine transporter CreaT (SLC6A8), cRNA encoding CreaT was injected into Xenopus laevis oocytes with or without additional injection of cRNA encoding GSK3ß. Creatine-induced current was determined by dual electrode voltage clamp and taken as measure of transport. As shown in Fig. 1, addition of creatine to the superfusate did not elicit an appreciable current in water-injected oocytes. Accordingly, the oocytes did not express significant endogenous electrogenic creatine transport. In CreaT expressing oocytes, however, the addition of creatine to the superfusate was followed by appearance of an inward current. The additional co-expression of wild-type GSK3ß was followed by a significant decrease of creatine-induced current in CreaT expressing Xenopus laevis oocytes.

Fig. 1

View large Download slide

Effect of wild-type GSK3ß or inactive mutant ^K85RGSK3ß on electrogenic creatine transport in CreaT (SLC6A8) expressing Xenopus laevis oocytes. A: Representative original tracings showing I_creat in Xenopus laevis oocytes injected with water (a), expressing CreaT alone (b) or expressing CreaT with additional co-expression of wild-type GSK3ß (c), or inactive ^K85RGSK3ß (d). B: Arithmetic means ± SEM (n = 10-16) of I_creatXenopus laevis oocytes injected with water (dotted bar) or expressing CreaT without (white bar) or with wild-type GSK3ß (black bar), or inactive ^K85RGSK3ß (grey bar) *** (p<0.001) indicates statistically significant difference from oocytes expressing CreaT alone.

In contrast to wild-type GSK3ß, the inactive ^K85RGSK3ß mutant did not significantly modify the creatine-induced current in CreaT expressing Xenopus oocytes (Fig. 1).

In order to test whether GSK3ß co-expression modifies the maximal creatine-induced current or the affinity of the carrier, the current induced by creatine concentrations ranging from 3 µM to 3 mM was determined in Xenopus laevis oocytes expressing CreaT without or with additional expression of wild-type GSK3ß. As illustrated in Fig. 2, the creatine-induced current was a function of the extracellular creatine concentration. Kinetic analysis revealed that the maximal creatine-induced current was significantly (p<0.001) higher in Xenopus laevis oocytes expressing CreaT alone (17.66 ± 1.97 nA, n = 6) than in Xenopus laevis oocytes expressing CreaT together with wild-type GSK3ß (6.88 ± 0.45 nA, n = 6). The concentration required for half-maximal creatine-induced current tended to be higher in Xenopus oocytes expressing CreaT alone (185.06 ± 96.50 µM, n = 6) than in Xenopus oocytes expressing CreaT together with wild-type GSK3ß (21.16 ± 6.62 µM, n = 6). Due to the large scatter of the calculated values, however, the difference did not reach statistical significance.

Fig. 2

View large Download slide

Electrogenic creatine transport as a function of creatine concentration in CreaT (SLC6A8)-expressing Xenopus laevis oocytes without or with additional expression of GSK3ß. A: Representative original tracings showing the current induced by increasing concentrations of creatine (from 3 µM to 3 mM) in Xenopus laevis oocytes expressing CreaT without (upper panel) or with (lower panel) additional co-expression of wild-type GSK3ß. B: Arithmetic means ± SEM (n = 6) of I_creat as a function of creatine concentration in Xenopus laevis oocytes expressing CreaT without (white circles), or with (black circles) additional co-expression of wild-type GSK3ß.

As GSK3ß could be inhibited by Lithium, additional experiments were performed in Xenopus oocytes expressing both CreaT and wild-type GSK3ß with or without prior exposure to 1 mM Lithium. As illustrated in Fig. 3, Lithium-treatment significantly enhanced the creatine-induced current in Xenopus oocytes expressing both CreaT and wild-type GSK3ß.

Fig. 3

View large Download slide

Effect of Lithium on electrogenic creatine transport in CreaT (SLC6A8) and GSK3ß expressing Xenopus laevis oocytes. A: Representative original tracings showing I_creat in Xenopus oocytes injected with water (a), expressing CreaT alone (b), or expressing CreaT with additional co-expression of wild-type GSK3ß without (c) or with (d, e) prior exposure to Lithium [1 mM] for 24 hours. B: Arithmetic means ± SEM (n = 9-16) of I_creat in Xenopus oocytes injected with water (dotted bar) or expressing CreaT alone (white bars), or expressing CreaT together with wild-type GSK3ß (black bars) either without (left bars) or with (right bars) prior exposure to 1mM Lithium for 24 hours. ***(p< 0.001) indicates statistically significant difference from Xenopus oocytes expressing CreaT alone, ### (p< 0.001) indicates statistically significant difference from the absence of Lithium.

GSK3ß is phosphorylated and thus inactivated by protein kinase PKB/Akt. Additional experiments thus explored whether the effect of GSK3ß could be reversed by additional co-expression of PKB/Akt. As illustrated in Fig. 4, the co-expression of PKB/Akt significantly enhanced the creatine-induced current in Xenopus oocytes expressing both CreaT and wild-type GSK3ß.

Fig. 4

View large Download slide

Effect of additional co-expression of PKB on creatine transport in CreaT (SLC6A8) and GSK3ß expressing Xenopus laevis oocytes. A: Representative original tracings showing I_creat in Xenopus laevis oocytes injected with water (a), expressing CreaT alone (b) or with additional co-expression of wild-type GSK3ß (c), or wild-type GSK3ß and PKB/Akt (d). B: Arithmetic means ± SEM (n = 9-13) of I_creat in Xenopus laevis oocytes injected with water (dotted bar) or expressing CreaT without (white bar) or with wild-type GSK3ß (black bar), or GSK3ß +PKB/Akt (grey bar). ** (p<0.01) indicates statistically significant difference from oocytes expressing CreaT alone, ## (p<0.01) indicates statistically significant difference from oocytes expressing CreaT and GSK3ß.

Discussion

The present study discloses a novel regulator of the creatine transporter CreaT (SLC6A8), i.e. the glycogen synthase kinase GSK3ß. Co-expression of the wild-type GSK3ß but not of the inactive mutant ^K85RGSK3ß was followed by a significant decrease of creatine-induced inward current reflecting electrogenic creatine transport. GSK3ß thus contributes to the complex regulation of this widely expressed carrier.

The effect of GSK3ß was dissipated by the additional co-expression of protein kinase B which is known to phosphorylate and thus to negatively regulate GSK3ß [31]. Moreover, the effect of GSK3ß on CreaT was blunted by the antidepressant Lithium, a known inhibitor of GSK3ß [30].

The present observations did not address the molecular mechanisms involved in the down-regulation of CreaT activity by GSK3ß. In theory the kinase could be effective by directly phosphorylating the carrier-protein or by phosphorylating proteins involved in the regulation of trafficking or function of the carrier. CreaT has previously been shown to be regulated by JAK2 [46], JAK3 [45], AMPK [47,48], PKC [49], SPAK [39], OSR1 [39], PIKfyve [50], mTOR [51], SGK1 [52], SGK3 [52], klotho [38], and peroxisome proliferator-activated receptor-gamma co-activator-1alpha (PGC-1α) or beta (PGC-1β) [53].

Dual electrode voltage clamp in Xenopus oocytes is a powerful experimental approach to uncover interactions between signalling molecules and carriers. Observations made utilizing this experimental approach have frequently been confirmed by analysing gene targeted mice lacking or overexpressing the respective kinase or mutants [35,41,42,54,55,56,57,58,59]. Nevertheless, the present study does not allow safe predictions as to the functional significance of GSK3ß-sensitive CreaT activity. In the brain, CreaT accomplishes synaptic re-uptake of the neurotransmitter creatine and thus influences GABAergic and glutamatergic neurotransmission [47]. In theory, the observed effect of GSK3ß on CreaT could thus contribute to the known effect of the kinase on neuronal excitability [28] and on cell size [29]. Specifically, stimulation of GSK3ß phosphorylation and thus inhibition of GSK3ß has been shown to facilitate translocation of the Ca²⁺-sensitive and depolarization-induced transcription factor NFAT [28] and to increase of cell size [29].

In conclusion, GSK3ß down-regulates CreaT activity, an effect possibly influencing neuroexcitation and cell volume regulation.

Acknowledgements

The authors acknowledge the meticulous preparation of the manuscript by Lejla Subasic and technical support by Elfriede Faber. This study was supported by the Deutsche Forschungsgemeinschaft and Open Access Publishing Fund of Tuebingen University .

Disclosure Statement

The authors of this manuscript state that they do not have any conflict of interests and nothing to disclose.

References

1.

Christie DL: Functional insights into the creatine transporter. Subcell Biochem 2007;46:99-118.

2.

Dodd JR, Christie DL: Cysteine 144 in the third transmembrane domain of the creatine transporter is located close to a substrate-binding site. J Biol Chem 2001;276:46983-46988.

3.

Sora I, Richman J, Santoro G, Wei H, Wang Y, Vanderah T, Horvath R, Nguyen M, Waite S, Roeske WR, et al.: The cloning and expression of a human creatine transporter. Biochem Biophys Res Commun 1994;204:419-427.

4.

Takenaka M, Bagnasco SM, Preston AS, Uchida S, Yamauchi A, Kwon HM, Handler JS: The canine betaine gamma-amino-n-butyric acid transporter gene: diverse mRNA isoforms are regulated by hypertonicity and are expressed in a tissue-specific manner. Proc Natl Acad Sci U S A 1995;92:1072-1076.

5.

Uchida S, Kwon HM, Yamauchi A, Preston AS, Marumo F, Handler JS: Molecular cloning of the cDNA for an MDCK cell Na(+)- and Cl(-)-dependent taurine transporter that is regulated by hypertonicity. Proc Natl Acad Sci U S A 1992;89:8230-8234.

6.

Braissant O, Henry H: AGAT, GAMT and SLC6A8 distribution in the central nervous system, in relation to creatine deficiency syndromes: a review. J Inherit Metab Dis 2008;31:230-239.

7.

Guimbal C, Kilimann MW: A Na(+)-dependent creatine transporter in rabbit brain, muscle, heart, and kidney. cDNA cloning and functional expression. J Biol Chem 1993;268:8418-8421.

8.

Mak CS, Waldvogel HJ, Dodd JR, Gilbert RT, Lowe MT, Birch NP, Faull RL, Christie DL: Immunohistochemical localisation of the creatine transporter in the rat brain. Neuroscience 2009;163:571-585.

9.

Mellott TJ, Kowall NW, Lopez-Coviella I, Blusztajn JK: Prenatal choline deficiency increases choline transporter expression in the septum and hippocampus during postnatal development and in adulthood in rats. Brain Res 2007;1151:1-11.

10.

Alcaide P, Merinero B, Ruiz-Sala P, Richard E, Navarrete R, Arias A, Ribes A, Artuch R, Campistol J, Ugarte M, Rodriguez-Pombo P: Defining the pathogenicity of creatine deficiency syndrome. Hum Mutat 2011;32:282-291.

11.

Alcaide P, Rodriguez-Pombo P, Ruiz-Sala P, Ferrer I, Castro P, Ruiz Martin Y, Merinero B, Ugarte M: A new case of creatine transporter deficiency associated with mild clinical phenotype and a novel mutation in the SLC6A8 gene. Dev Med Child Neurol 2010;52:215-217.

12.

Ardon O, Amat di San Filippo C, Salomons GS, Longo N: Creatine transporter deficiency in two half-brothers. Am J Med Genet A 2010;152A:1979-1983.

13.

Battini R, Chilosi A, Mei D, Casarano M, Alessandri MG, Leuzzi V, Ferretti G, Tosetti M, Bianchi MC, Cioni G: Mental retardation and verbal dyspraxia in a new patient with de novo creatine transporter (SLC6A8) mutation. Am J Med Genet A 2007;143A:1771-1774.

14.

Battini R, Chilosi AM, Casarano M, Moro F, Comparini A, Alessandri MG, Leuzzi V, Tosetti M, Cioni G: Language disorder with mild intellectual disability in a child affected by a novel mutation of SLC6A8 gene. Mol Genet Metab 2011;102:153-156.

15.

Braissant O, Beard E, Torrent C, Henry H: Dissociation of AGAT, GAMT and SLC6A8 in CNS: relevance to creatine deficiency syndromes. Neurobiol Dis 2010;37:423-433.

16.

Braissant O, Henry H, Beard E, Uldry J: Creatine deficiency syndromes and the importance of creatine synthesis in the brain. Amino Acids 2011;40:1315-1324.

17.

Haan C, Rolvering C, Raulf F, Kapp M, Druckes P, Thoma G, Behrmann I, Zerwes HG: Jak1 has a dominant role over Jak3 in signal transduction through gammac-containing cytokine receptors. Chem Biol 2011;18:314-323.

18.

Jensen TE, Rose AJ, Hellsten Y, Wojtaszewski JF, Richter EA: Caffeine-induced Ca(2+) release increases AMPK-dependent glucose uptake in rodent soleus muscle. Am J Physiol Endocrinol Metab 2007;293:E286-E292.

19.

Longo N, Ardon O, Vanzo R, Schwartz E, Pasquali M: Disorders of creatine transport and metabolism. Am J Med Genet C Semin Med Genet 2011;157C:72-78.

20.

Mancardi MM, Caruso U, Schiaffino MC, Baglietto MG, Rossi A, Battaglia FM, Salomons GS, Jakobs C, Zara F, Veneselli E, Gaggero R: Severe epilepsy in X-linked creatine transporter defect (CRTR-D). Epilepsia 2007;48:1211-1213.

21.

Mercimek-Mahmutoglu S, Connolly MB, Poskitt KJ, Horvath GA, Lowry N, Salomons GS, Casey B, Sinclair G, Davis C, Jakobs C, Stockler-Ipsiroglu S: Treatment of intractable epilepsy in a female with SLC6A8 deficiency. Mol Genet Metab 2010;101:409-412.

22.

Puusepp H, Kall K, Salomons GS, Talvik I, Mannamaa M, Rein R, Jakobs C, Ounap K: The screening of SLC6A8 deficiency among Estonian families with X-linked mental retardation. J Inherit Metab Dis 2010;33 Suppl 3:S5-11.

23.

Rosenberg EH, Martinez Munoz C, Betsalel OT, van Dooren SJ, Fernandez M, Jakobs C, deGrauw TJ, Kleefstra T, Schwartz CE, Salomons GS: Functional characterization of missense variants in the creatine transporter gene (SLC6A8): improved diagnostic application. Hum Mutat 2007;28:890-896.

24.

Salomons GS, van Dooren SJ, Verhoeven NM, Marsden D, Schwartz C, Cecil KM, DeGrauw TJ, Jakobs C: X-linked creatine transporter defect: an overview. J Inherit Metab Dis 2003;26:309-318.

25.

Skelton MR, Schaefer TL, Graham DL, Degrauw TJ, Clark JF, Williams MT, Vorhees CV: Creatine transporter (CrT; Slc6a8) knockout mice as a model of human CrT deficiency. PLoS One 2011;6:e16187.

26.

Stockler S, Schutz PW, Salomons GS: Cerebral creatine deficiency syndromes: clinical aspects, treatment and pathophysiology. Subcell Biochem 2007;46:149-166.

27.

van de Kamp JM, Mancini GM, Pouwels PJ, Betsalel OT, van Dooren SJ, de Koning I, Steenweg ME, Jakobs C, van der Knaap MS, Salomons GS: Clinical features and X-inactivation in females heterozygous for creatine transporter defect. Clin Genet 2011;79:264-272.

28.

Kim MS, Shutov LP, Gnanasekaran A, Lin Z, Rysted JE, Ulrich JD, Usachev YM: Nerve growth factor (NGF) regulates activity of nuclear factor of activated T-cells (NFAT) in neurons via the phosphatidylinositol 3-kinase (PI3K)-Akt-glycogen synthase kinase 3beta (GSK3beta) pathway. J Biol Chem 2014;289:31349-31360.

29.

Gruson D, Ginion A, Decroly N, Lause P, Vanoverschelde JL, Ketelslegers JM, Bertrand L, Thissen JP: Urocortin-induced cardiomyocytes hypertrophy is associated with regulation of the GSK-3beta pathway. Heart Vessels 2012;27:202-207.

30.

O'Brien WT, Klein PS: Validating GSK3 as an in vivo target of lithium action. Biochem Soc Trans 2009;37:1133-1138.

31.

Valvezan AJ, Klein PS: GSK-3 and Wnt Signaling in Neurogenesis and Bipolar Disorder. Front Mol Neurosci 2012;5:1.

32.

Rexhepaj R, Dermaku-Sopjani M, Gehring EM, Sopjani M, Kempe DS, Foller M, Lang F: Stimulation of electrogenic glucose transport by glycogen synthase kinase 3. Cell Physiol Biochem 2010;26:641-646.

33.

Sun H, Jiang YJ, Yu QS, Luo CC, Zou JW: Effect of mutation K85R on GSK-3beta: Molecular dynamics simulation. Biochem Biophys Res Commun 2008;377:962-965.

34.

Munoz C, Almilaji A, Setiawan I, Foller M, Lang F: Up-regulation of the inwardly rectifying K(+) channel Kir2.1 (KCNJ2) by protein kinase B (PKB/Akt) and PIKfyve. J Membr Biol 2013;246:189-197.

35.

Ahmed M, Salker MS, Elvira B, Umbach AT, Fakhri H, Saeed AM, Shumilina E, Hosseinzadeh Z, Lang F: SPAK Sensitive Regulation of the Epithelial Na Channel ENaC. Kidney Blood Press Res 2015;40:335-343.

36.

Warsi J, Elvira B, Bissinger R, Shumilina E, Hosseinzadeh Z, Lang F: Downregulation of peptide transporters PEPT1 and PEPT2 by oxidative stress responsive kinase OSR1. Kidney Blood Press Res 2014;39:591-599.

37.

Fezai M, Ahmed M, Hosseinzadeh Z, Elvira B, Lang F: SPAK and OSR1 Sensitive Kir2.1 K+ Channels. Neurosignals 2015;23:20-33.

38.

Almilaji A, Sopjani M, Elvira B, Borras J, Dermaku-Sopjani M, Munoz C, Warsi J, Lang UE, Lang F: Upregulation of the creatine transporter Slc6A8 by Klotho. Kidney Blood Press Res 2014;39:516-525.

39.

Fezai M, Elvira B, Borras J, Ben-Attia M, Hoseinzadeh Z, Lang F: Negative regulation of the creatine transporter SLC6A8 by SPAK and OSR1. Kidney Blood Press Res 2014;39:546-554.

40.

Fezai M, Elvira B, Warsi J, Ben-Attia M, Hosseinzadeh Z, Lang F: Up-Regulation of Intestinal Phosphate Transporter NaPi-IIb (SLC34A2) by the Kinases SPAK and OSR1. Kidney Blood Press Res 2015;40:555-564.

41.

Warsi J, Dong L, Elvira B, Salker MS, Shumilina E, Hosseinzadeh Z, Lang F: SPAK dependent regulation of peptide transporters PEPT1 and PEPT2. Kidney Blood Press Res 2014;39:388-398.

42.

Warsi J, Singh Y, Elvira B, Hosseinzadeh Z, Lang F: Regulation of Large Conductance Voltage-and Ca2+-Activated K+ Channels by the Janus Kinase JAK3. Cell Physiol Biochem 2015;37:297-305.

43.

Alesutan I, Voelkl J, Stockigt F, Mia S, Feger M, Primessnig U, Sopjani M, Munoz C, Borst O, Gawaz M, Pieske B, Metzler B, Heinzel F, Schrickel JW, Lang F: AMP-activated protein kinase alpha1 regulates cardiac gap junction protein connexin 43 and electrical remodeling following pressure overload. Cell Physiol Biochem 2015;35:406-418.

44.

Hosseinzadeh Z, Sopjani M, Pakladok T, Bhavsar SK, Lang F: Downregulation of KCNQ4 by Janus kinase 2. J Membr Biol 2013;246:335-341.

45.

Fezai M, Warsi J, Lang F: Regulation of the Na+,Cl- coupled Creatine Transporter CreaT (SLC6A8) by the Janus Kinase JAK3. Neurosignals 2015;23:11-19.

46.

Shojaiefard M, Hosseinzadeh Z, Bhavsar SK, Lang F: Downregulation of the creatine transporter SLC6A8 by JAK2. J Membr Biol 2012;245:157-163.

47.

Joncquel-Chevalier Curt M, Voicu PM, Fontaine M, Dessein AF, Porchet N, Mention-Mulliez K, Dobbelaere D, Soto-Ares G, Cheillan D, Vamecq J: Creatine biosynthesis and transport in health and disease. Biochimie 2015;10.1016/j.biochi.2015.10.022

48.

Li H, Thali RF, Smolak C, Gong F, Alzamora R, Wallimann T, Scholz R, Pastor-Soler NM, Neumann D, Hallows KR: Regulation of the creatine transporter by AMP-activated protein kinase in kidney epithelial cells. Am J Physiol Renal Physiol 2010;299:F167-177.

49.

Black SA, Ribeiro FM, Ferguson SS, Rylett RJ: Rapid, transient effects of the protein kinase C activator phorbol 12-myristate 13-acetate on activity and trafficking of the rat high-affinity choline transporter. Neuroscience 2010;167:765-773.

50.

Strutz-Seebohm N, Shojaiefard M, Christie D, Tavare J, Seebohm G, Lang F: PIKfyve in the SGK1 mediated regulation of the creatine transporter SLC6A8. Cell Physiol Biochem 2007;20:729-734.

51.

Shojaiefard M, Christie DL, Lang F: Stimulation of the creatine transporter SLC6A8 by the protein kinase mTOR. Biochem Biophys Res Commun 2006;341:945-949.

52.

Shojaiefard M, Christie DL, Lang F: Stimulation of the creatine transporter SLC6A8 by the protein kinases SGK1 and SGK3. Biochem Biophys Res Commun 2005;334:742-746.

53.

Brown EL, Snow RJ, Wright CR, Cho Y, Wallace MA, Kralli A, Russell AP: PGC-1alpha and PGC-1beta increase CrT expression and creatine uptake in myotubes via ERRalpha. Biochim Biophys Acta 2014;1843:2937-2943.

54.

Borras J, Salker MS, Elvira B, Warsi J, Fezai M, Hoseinzadeh Z, Lang F: SPAK and OSR1 Sensitivity of Excitatory Amino Acid Transporter EAAT3. Nephron 2015;130:221-228.

55.

Elvira B, Blecua M, Luo D, Yang W, Shumilina E, Munoz C, Lang F: SPAK-sensitive regulation of glucose transporter SGLT1. J Membr Biol 2014;247:1191-1197.

56.

Hosseinzadeh Z, Honisch S, Schmid E, Jilani K, Szteyn K, Bhavsar S, Singh Y, Palmada M, Umbach AT, Shumilina E, Lang F: The Role of Janus Kinase 3 in the Regulation of Na(+)/K(+) ATPase under Energy Depletion. Cell Physiol Biochem 2015;36:727-740.

57.

Pathare G, Foller M, Daryadel A, Mutig K, Bogatikov E, Fajol A, Almilaji A, Michael D, Stange G, Voelkl J, Wagner CA, Bachmann S, Lang F: OSR1-sensitive renal tubular phosphate reabsorption. Kidney Blood Press Res 2012;36:149-161.

58.

Siraskar B, Huang DY, Pakladok T, Siraskar G, Sopjani M, Alesutan I, Kucherenko Y, Almilaji A, Devanathan V, Shumilina E, Foller M, Munoz C, Lang F: Downregulation of the renal outer medullary K(+) channel ROMK by the AMP-activated protein kinase. Pflugers Arch 2013;465:233-245.

59.

Warsi J, Luo D, Elvira B, Jilani K, Shumilina E, Hosseinzadeh Z, Lang F: Upregulation of excitatory amino acid transporters by coexpression of Janus kinase 3. J Membr Biol 2014;247:713-720.

2016

Open Access License / Drug Dosage / Disclaimer

This article is licensed under the Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License (CC BY-NC-ND). Usage and distribution for commercial purposes as well as any distribution of modified material requires written permission. Drug Dosage: The authors and the publisher have exerted every effort to ensure that drug selection and dosage set forth in this text are in accord with current recommendations and practice at the time of publication. However, in view of ongoing research, changes in government regulations, and the constant flow of information relating to drug therapy and drug reactions, the reader is urged to check the package insert for each drug for any changes in indications and dosage and for added warnings and precautions. This is particularly important when the recommended agent is a new and/or infrequently employed drug. Disclaimer: The statements, opinions and data contained in this publication are solely those of the individual authors and contributors and not of the publishers and the editor(s). The appearance of advertisements or/and product references in the publication is not a warranty, endorsement, or approval of the products or services advertised or of their effectiveness, quality or safety. The publisher and the editor(s) disclaim responsibility for any injury to persons or property resulting from any ideas, methods, instructions or products referred to in the content or advertisements.

Down-Regulation of the Na⁺,Cl^- Coupled Creatine Transporter CreaT (SLC6A8) by Glycogen Synthase Kinase GSK3ß

Abstract

Introduction