Monday, April 1, 2019
Ataxia Telangiectasia Mutated in Glucose Transport
Ataxia Telangiectasia Mutated in Glucose TransportA agency for motor ataxia telangiectasia mutated in insulin-independent excitant of glucose conveyanceAbstr dissembleLiterature reports suggest that ataxia telangiectasia mutated ( atmospheric state) can activate the AMP-activated protein kinase (AMPK), a protein that can give birth glucose shift in careworn vigor-builder. We hypothesized that 5-aminoimidazole-4-carboxamide ribonucleotide (AICAR), an AMPK activator, would increase glucose dribble in computer cower extensor digitorum longus (EDL) ponderousnesss in an asynchronous transfer mode-dependent manner. AICAR- stimulated glucose ravish was prevented by the cash machine mortifyor KU-55933 and in ambience- unequal ( standard pressure-/-) muscle despite form stimulation of AMPK phosphorylation. S231 of TBC1D1 matches the sequence subject of ATM substrates, and phosphorylation of this site is known to inhibit TBC1D1 and lead to increased glucose transport. Accord ingly, we assessed TBC1D1 phosphorylation and found that AICAR-stimulated phosphorylation of TBC1D1 at S231did non occurin ATM-/- muscle. However, activating of ATM without energizing of AMPK was insufficient to increase TBC1D1 phosphorylation.The information suggest that ATM plays a mathematical function in AICAR stimulated glucose transport downstream of AMPK.Keywords AMP-activated protein kinase ataxia telangiectasia mutated TBC1D1 AICAR glucose transport purposeless muscleIntroductionThe serine-threonine kinase ataxia telangiectasia mutated (ATM) appears to play a portion in glucose homeostasis. For example, recent genome-wide connection studies have found that genetic variations approach the ATM gene are related to glycemic responses to metformin 1, 2, a commonly-prescribed dose for blood glucose control. While the mechanism for metformins effect on blood glucose levels is under debate 3-6, it is known that metformin acutely stimulates glucose transport into skeletal m uscle tender with activating of the AMP-activated protein kinase (AMPK) 7.Activation of AMPK is sufficient to stimulate insulin-independent glucose transport into skeletal muscle 8, 9. Intriguingly, ATM dependence has been reported for activation of AMPK in response to DNA damage or insulin- same growth component 1 in HeLa cells and fibroblasts, exposure of lung genus Cancer cells to ionizing radiation,exposure of lymphoblaststo H2O2, or treatment of HeLa cells and mouse embryonic fibroblasts with the adenosine analog AICAR 10-14. Despite these suggestive data on the intention of ATM upriver of AMPK, the potential portion of ATM in AMPK-dependent stimulation of glucose transport has not previously been investigated in skeletal muscle, the predominant whole-body transshipment center depot for glucose.Accordingly, the purpose of this study was to test the hypothesis that glucose use stimulated by the AMPK activator AICAR would be dependent on ATM in skeletal muscle.MethodsMate rialsAntibodies against TBC1D1, AMPK, phosphorylated AMPK T172 (P-AMPK), and phosphorylated ATM S1981 (P-ATM) were purchased from Cell Signaling Technology (Beverly, MA, USA). Antibodies against phosphorylated TBC1D1 (P-TBC1D1) S237 (S231 in mouse) were purchased from EMD Millipore Corporation (Billerica, MA, USA). Antibodies against tubulin and ATM were obtained from Sigma-Aldrich Corporation (St. Louis, MO, USA). Horseradish peroxidase-conjugated secondary antibodies were obtained from Pierce Biotechnology (Rockford, IL, USA). The ATM inhibitor KU-55933 was a generous gift from Dr. Graeme Smith (KuDOSPhramaceuticals, Cambridge, UK). The AMPK inhibitor Compound C was provided by Merck Co., Inc. (Rahway, NJ, USA). Doxorubicin was purchased from Sigma-Aldrich Corporation. Radiolabeled 2-deoxyglucose and mannitol were purchased from American Radiolabeled Chemicals, Inc. (St. Louis, MO, USA).Collection and Processing of Animal MuscleAll procedures victimization live animals were appro ved by the Saint Louis University Institutional Animal allot and Use Committee. Transgenic mice expressing a t trialcation mutation of ATM 15 were obtained from The Jackson testing ground (Bar Harbor, ME, USA). Mice that were heterozygous for the transgene were used to breed wild type (ATM+/+) and ATM deficient (ATM-/) mice. After weaning, each mouse was anesthetized with ketamine/xylazine (55 mg ketamine and 5.5 mg xylazine per kg), and a tail sample was obtained for genotyping as previously exposit 15, 16.Mice were anesthetized with sodium pentobarbital (50 mg/kg) and extensor digitorum longus (EDL) muscles were removed and incubated in vitro as described previously 16, 17. The incubation media for the muscle consisted of Krebs Henseleit bicarbonate buffer (KHB) containing 8 mM glucose and 32 mM mannitol. Vials containing EDL muscles were gassed with 95% O2 5% CO2 and kept gently shaking at 35C.Muscles were incubated for one hour to allow retrieval from dissection. Muscles we re whence transferred into KHB containing 32 mM mannitol and 8 mM glucose in the movement of 0.1% dimethyl sulfoxide vehicle (DMSO) or 1 M KU-55933, a closeness sufficient to inhibit ATM 18, 19 but low enough to turn away proscription of phosphatidylinositol 3-kinase 19. After 30 minutes, muscles were incubated in KHB with 8 mM glucose and the absence seizure or presence of 2 mM AICAR for one hour with the proceed presence of DMSO or KU and 32 mM or 30 mM mannitol to keep osmolarity constant across media. At this point, some muscles were blotted and clamp-frozen with aluminium tongs cooled in liquid nitrogen and stored at -80 C for later on western blot analysis. Other muscles were subjected to 2-deoxyglucose (2DG) uptake assays as described below.In parallel procedures, EDL muscles from wild-type or ATM-deficient animals were allowed to recover in vitro for one hour, incubated in KHB containing mannitol as described above and in the absence or presence of 2 mM AICAR for one hour and then either clamp-frozen or subjected to 2DG uptake assays as previously reported 16, 17 and briefly described below.2DG uptakeMuscles were washed at 30 C in glucose-free KHB containing 40 mM mannitol in the absence or presence of KU-55933 (DMSO vehicle) or, for procedures with the ATM-/- mice, in spiritualist containing neither KU nor DMSO. Muscles were then incubated in KHB containing 4 mM 2DG, 2 Ci/ml 3H-2DG, 36 mM mannitol, 0.3 Ci/ml 14C-mannitol, and 0.1% DMSO or 1 M KU-55933 if they had been present in earlier incubations. Muscles were clamp-frozen and stored at -80 C. Muscles were then homogenised in Kontes ground glass tubes in ice-cold buffer containing protease and phosphatase inhibitors (50 mM HEPES, pH 7.4, 2 mM Na3VO4, 150 mM NaF,10 g/ml leupeptin, 10 g/ml aprotinin, 0.5 g/mL pepstatin and 1 mM phenymethylsulfonylflouride). Homogenates were centrifuged at 4 C for 10 minutes at 14,000g, and supernatant protein concentration was examine by the bicinchoninic ac id (BCA) method (Pierce Protein Technologies, Rockland, IL, USA). supernatant aliquots and aliquots of the incubation media were mixed with Ultima Gold XR flicker fluid (Perkin Elmer, Boston, MA, USA), and samples were assessed by scintillation counting (TriCarb 3110TR, Perkin Elmer, Boston, MA, USA). The disintegrations per minute (DPM) of 14C-mannitol were used to measure the extracellular volume, and intracellular 2DG was deliberate from 3H DPM after accounting for 3H DPM in the extracellular space. 2DG transport was expressed as nmol 2DG/mg protein/10 minutes.Western BlottingSamples were homogenized, centrifuged, assayed for protein content as described above, thin out in Laemmli sample buffer containing dithiothreitol, and boiled for 5 minutes. Samples were then analyzed development SDS-PAGE as described previously 20. Samples were run on 4-20% Tris-HEPES gels (Pierce) and then transferred onto nitrocellulose membranes. After transfer, membranes were blocked with 5% non-fat dry milk in Tris-buffered saline containing 0.1% Tween. Proteins on the nitrocellulose membranes were probed with primary and secondary antibodies described in the Materials section and then visualized using enhanced chemiluminescence (Western Lightning PerkinElmer, Waltham, MA, USA). Western blots were quantified using TotalLab software purchased from TotalLab Nonlinear Dynamics (Newcastle on Tyre, UK). For probing ATM and P-ATM, samples were run on 3-8% Tris-Acetate gels (Invitrogen, Carlsbad, CA, USA) alongside HiMark (Invitrogen) molecular weight markers.StatisticsData were analyzed by ANOVA with post hoc LSD comparisons. A level of PResultsAICAR-stimulated glucose transportATMs role in AICAR stimulated glucose transport was assessed in isolated EDL muscle by using either ATM deficient mice or by using the specific ATM inhibitor, KU-55933. As shown in figure 1A, ATM protein was present in only background levels in EDL from ATM-/- mice. As shown in figure 1B, AICAR increased glu cose transport in muscle from wild type mice(PAICAR-stimulated phosphorylation of AMPKIt has previously been reported that ATM plays a role in AICAR-stimulated AMPK phosphorylation in HeLa cells and mouse embryonic fibroblasts 12. Thus, we assessed phosphorylation of AMPK to determine whether ATMs role in AICAR-stimulated glucose transport was by means of an influence on AMPK phosphorylation. As shown in figure 2A, AICAR-stimulated AMPK phosphorylation was normal in muscle from ATM-/- mice. Likewise, AICAR-stimulated AMPK phosphorylation was unaffected by the ATM inhibitor KU-55933 (figure 2B).Phosphorylation of TBC1D1The RabGTPase activating protein (GAP) TBC1D1 is required for stimulation of glucose transport by AICAR 21. Furthermore, phosphorylation of mouse TBC1D1 at S231 (corresponding to S237 of human TBC1D1) in response to AICAR occurs concomitant with an increase in glucosetransport 22-24, and S231 phosphorylation appears to be necessary to convey insulin-responsiveness to TBC1D1 25. Intriguingly, S231 and the surrounding amino acids (F-S-Q) match the consensushydrophobic-serine/threonine-glutamine (-S/T-Q) motif of ATM targets 26, 27. While phosphorylation of this site is increased by the AMPK activators phenformin and AICAR 28, and the site is an in vitro target of AMPK 28, this does not rule out the possibility that another kinase could act on the site. Thus, we hypothesized that S231 phosphorylation in response to AICAR would be dependent on ATM. As shown in figure3, AICAR increased phosphorylation of TBC1D1 S231 in EDL from wild type mice (PDiscussionThe sensitive information provided by this study is that AICAR-stimulated glucose uptake in skeletal muscle is dependent on ATM. Additionally, this role for ATM in AICAR-stimulated glucose uptake does not involve an effect at the level of AMPK phosphorylation but instead is associated with neutered phosphorylation of TBC1D1, downstream of AMPK.Based on data that the ATM inhibitor KU-55933 blunted a ctivation of AMPK by metformin in a hepatoma cell line, cabbage et al proposed that ATM acts upstream of AMPK 2. However, two independent groups have shown that KU-55933 prevents AMPK activation by metformin through forbiddance of the cation transporter responsible for metformin uptake rather than through inhibition of ATM 3, 4. In hepatocytes, ultraviolet illumination light irradiation stimulated phosphorylation of the ATM target H2AX, but had no effect on AMPK action 4. Additionally, caffeine, which inhibits ATM,suppressed phosphorylation of H2AX but not activation of AMPK by metformin 4 . Finally, while hydrogen peroxide activated both AMPK and ATM in HEK293 cells, KU-55933 prevented ATM autophosphorylation but did not interfere with AMPK activity 4. Together, these data 4 suggest that ATM does not act upstream of AMPK, at to the lowest degree in hepatocytes or HEK293 cells.While it has been reported that ATM acts upstream of AMPK inHeLa cells, lung cancer cells, fibroblasts, lymphoblasts, and embryonic fibroblasts 10-14, it seems unlikely that tissues corresponding to these cell lines would play a substantive role in glucose homeostasis. Intriguingly, however, the increase in insulin sensitivity and a concomitant increase in autophosphorylated ATM in L6 myotubes in response to blood serum starvation was found to be dependent on AMPK, while inhibition of ATM prevented increased insulin action but not an increase in AMPK phosphorylation in serum starved myotubes 18. Together, the data from serum-starved myotubes 18suggest that ATM could act downstream of AMPK in regulation of glucose transport. The current data showing blunted glucose transport despite normal phosphorylation of AMPK in response to AICAR in ATM-deficient skeletal muscle or muscle exposed to KU-55933 are consistent with the idea of ATM acting downstream of AMPK.AMPK is a heterotrimerof , , and subunits, each with multiple isoforms 30. The two primary(prenominal) activating upstream kin ases for AMPK are liver kinase B1 (LKB1) and calcium/calmodulin-dependent kinase kinase 31, though there are some reports that ATM-dependent phosphorylation of AMPK does not require LKB1 11, 32 and could indeed be through direct phosphorylation of AMPK by ATM 11. Intriguingly, LKB1 is an in vitro substrate for ATM 33, suggesting a potential mechanism for the ATM-dependent phosphorylation of AMPK 14. However, phosphorylation of LKB1 by ATM does not affect LKB1 activity in vitro or LKB1 localization in vivo 33, so the precise role of LKB1 phosphorylation in activation of AMPK remains uncertain. Clearly, there are cell-type differences in the role of ATM upstream of AMPK, and perhaps these are influenced by factors including the expression compose of AMPK subunit isoforms or the subcellular localizations of ATM, AMPK, and LKB1.The current study, as the first to demonstrate a role of ATM in insulin-independent glucose transport, adds to the growing body of literature suggesting a rol e for ATM in glucoregulation. For example, young mice that lack functional ATM are hyperglycemic compared to wild-type animals during oral glucose tolerance tests 34. Likewise, for mice with an ApoE-/- background, animals that have only one allelomorph ofATMthat codes for functional protein are hyperglycemic during intraperitoneal glucose tolerance tests and insulin tolerance tests compared to mice with two wild-type ATM alleles 35. Finally, inhibition of ATM decreases insulin-stimulated glucose uptake in muscle-derived cell lines 16, 32, and insulin-stimulated glucose uptake is blunted in L6 cells expressing kinase-dead ATM and in mouse skeletal muscle from animals deficient in ATM 16, 32. Quite interestingly, while ATM plays a role upstream of Akt in response to insulin in some cell lines and in glycolytic skeletal muscle 16, 20, 36, the point of influence of ATM in insulin signaling take to glucose transport in oxidative muscle is downstream of Akt at theRabGAP AS160/TBC1D4 16, 20which, like TBC1D1, acts on Rabs 2A, 8A, 8B, 10, and 14 37. Thus, ATM influences both insulin-stimulated phosphorylation of AS160 16, 20 and AICAR-stimulated phosphorylation of TBC1D1 in skeletal muscle.In summary, this study provides the first evidence for a role of ATM in AICAR-stimulated glucose uptake by skeletal muscle. Thus, ATM plays key roles in both insulin-dependent 16and insulin-independent stimulation of glucose uptake in skeletal muscle, suggesting a basis for the association of ATM variants with glycemic profiles recently reported 2, 7.
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