A common trafficking route for GLUT4 in cardiomyocytes in response to insulin, contraction and energy-status signalling

Fazakerley, Daniel J.; Lawrence, Scott P.; Lizunov, Vladimir A.; Cushman, Samuel W.; Holman, Geoffrey D.

doi:10.1242/jcs.041178

Cited by 49 publications

(41 citation statements)

References 45 publications

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“…Myotubes have been fixed at specific time points and labeled with a surface membrane impermeant anti-myc antibody in order to measure GLUT4-myc (with or without GFP) inserted into the plasma membrane by detecting the exofacial loop containing the myc eptitope (44). The tags have been combined, including GLUT4-myc-GFP, which allows simultaneously the detection of the GLUT4-GFP and the fraction of GLUT4-myc actually inserted into the membranes (15,44).…”

Section: Cell Systems Used To Study Glut4 Translocation With High Spamentioning

confidence: 99%

“…3). Another approach has been to isolate mature muscle fibers or cardiomyocytes from transgenic mice overexpressing tagged (myc, HA, and/or GFP) versions of GLUT4 and subsequently perform analysis in vitro (15,54). Alternatively, the use of various generations of membrane impermeable affinity photolabels that bind to endogenous glucose transporters have also provided important information about GLUT4 traffic in mature muscle (26) (Fig.…”

Section: Investigating Glut4 Translocation In Mature Musclementioning

confidence: 99%

“…This means that GLUT4-GFP actually inserted in the plasma membranes cannot be separated from GLUT4-GFP in close vicinity of the membrane (within 200 nm). Despite this lack in resolution, recent studies using GLUT4-GFP with different exofacial tags have demonstrated that the fold increase in GFP fluorescence staining of the sarcolemma and T-tubules correlates well with the fold increase in the GLUT4 actually inserted into the membrane (assayed by antibody staining for the exofacial tags myc or HA) (15,54). Furthermore, compared with in vitro preparations of muscle, the extracellular environment that the muscle fiber is exposed to cannot be rapidly changed due to dependence on internal clearance of injected drugs by organs such as the liver and kidneys.…”

Section: In Situ Detection Of Tagged Glut4mentioning

confidence: 99%

“…Muscle-specific transgenic overexpression of GLUT4-GFP with an HA tag in the exofacial membrane loop has been achieved recently, although potential effects on whole body glucose homeostasis were not reported (15). Also, musclespecific expression of GLUT4-myc in transgenic mice resulted in a threefold increase in GLUT4 levels in muscle and was in turn associated with increased glucose tolerance (54).…”

Section: Transgenic Expression Of Tagged Glut4mentioning

confidence: 99%

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Measuring GLUT4 translocation in mature muscle fibers

Lauritzen

Schertzer

2010

American Journal of Physiology-Endocrinology and Metabolism

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Skeletal muscle is the major tissue for postprandial glucose disposal. Facilitated glucose uptake into muscle fibers is mediated by increases in surface membrane levels of the glucose transporter GLUT4 via insulin- and/or muscle contraction-mediated GLUT4 translocation. However, the regulatory mechanisms controlling GLUT4 translocation in skeletal muscle have been difficult to characterize at the cell biology level due to muscle tissue complexity. Muscle cell culture models have improved our understanding of GLUT4 translocation and glucose transport regulation, but in vitro muscle models lack many of the characteristics of mature muscle fibers. Thus, the molecular and cellular details of GLUT4 translocation in mature skeletal muscle are deficient. The objective of this review is to highlight how advances in recent experimental approaches translate into an enhanced understanding of the regulation of GLUT4 translocation and glucose transport in mature skeletal muscle.

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Section: Cell Systems Used To Study Glut4 Translocation With High Spamentioning

confidence: 99%

Section: Investigating Glut4 Translocation In Mature Musclementioning

confidence: 99%

Section: In Situ Detection Of Tagged Glut4mentioning

confidence: 99%

Section: Transgenic Expression Of Tagged Glut4mentioning

confidence: 99%

See 2 more Smart Citations

Measuring GLUT4 translocation in mature muscle fibers

Lauritzen

Schertzer

2010

American Journal of Physiology-Endocrinology and Metabolism

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“…The extent of label remaining on the surface, or alternatively that internalized, is then quantified. Suitable labels for these types of experiments are nonpermeating affinity photolabels (Fazakerley et al 2009;Karlsson et al 2009) or antibodies to exofacially exposed epitopes (Antonescu et al 2008a;Kao et al 2000). Methodological details for the latter can be found in Antonescu et al 2008b andIshikura et al 2009.…”

Section: How Is This Documented?mentioning

confidence: 99%

The many ways to regulate glucose transporter 4This paper is one of a selection of papers published in this Special Issue, entitled 14th International Biochemistry of Exercise Conference – Muscles as Molecular and Metabolic Machines, and has undergone the Journal’s usual peer review process.

Klip

2009

Appl. Physiol. Nutr. Metab.

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Glucose uptake into skeletal muscle is primarily mediated by glucose transporter 4 (GLUT4). The number of GLUT4 polypeptides at the surface of muscle cells rises rapidly in response to insulin, contraction, depolarization, or energy deprivation. However, distinct mechanisms underlie the gain in surface GLUT4 in each case. Insulin promotes its exocytosis to the membrane, regulating vesicle movement, tethering, docking, and fusion. In contrast, muscle contraction, depolarization, and energy demand reduce GLUT4 endocytosis. The signals involved in each case also differ. Insulin utilizes Akt, Rabs, and selective actin remodelling, whereas depolarization and energy deprivation engage AMP-activated protein kinase and Ca2+-dependent signals. GLUT4 internalizes via 2 major routes that involve dynamin, but only one requires clathrin. The clathrin-independent route is slowed down by energy deprivation, and is regulated by AMP-activated protein kinase. In addition to regulation of the exocytic and endocytic movement of GLUT4, glucose uptake is also modulated through changes in the transporter's intrinsic activity. The glycolytic enzymes glyceraldehyde-3-dehydrogenase and hexokinase II contribute to such regulation, through differential binding to GLUT4.

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Modified UCN2 peptide treatment improves skeletal muscle mass and function in mouse models of obesity‐induced insulin resistance

Borg

Massart

Barbosa

et al. 2021

J cachexia sarcopenia muscle

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Background Type 2 diabetes and obesity are often seen concurrently with skeletal muscle wasting, leading to further derangements in function and metabolism. Muscle wasting remains an unmet need for metabolic disease, and new approaches are warranted. The neuropeptide urocortin 2 (UCN2) and its receptor corticotropin releasing factor receptor 2 (CRHR2) are highly expressed in skeletal muscle and play a role in regulating energy balance, glucose metabolism, and muscle mass. The aim of this study was to investigate the effects of modified UCN2 peptides as a pharmaceutical therapy to counteract the loss of skeletal muscle mass associated with obesity and casting immobilization. Methods High-fat-fed mice (C57Bl/6J; 26 weeks old) and ob/ob mice (11 weeks old) were injected daily with a PEGylated (Compound A) and non-PEGylated (Compound B) modified human UCN2 at 0.3 mg/kg subcutaneously for 14 days. A separate group of chow-fed C57Bl/6J mice (12 weeks old) was subjected to hindlimb cast immobilization and, after 1 week, received daily injections with Compound A. In vivo functional tests were performed to measure protein synthesis rates and skeletal muscle function. Ex vivo functional and molecular tests were performed to measure contractile force and signal transduction of catabolic and anabolic pathways in skeletal muscle. Results Skeletal muscles (extensor digitorum longus, soleus, and tibialis anterior) from high-fat-fed mice treated with Compound A were ~14% heavier than muscles from vehicle-treated mice. Chronic treatment with modified UCN2 peptides altered the expression of structural genes and transcription factors in skeletal muscle in high-fat diet-induced obesity including down-regulation of Trim63 and up-regulation of Nr4a2 and Igf1 (P < 0.05 vs. vehicle). Signal transduction via both catabolic and anabolic pathways was increased in tibialis anterior muscle, with increased phosphorylation of ribosomal protein S6 at Ser 235/236 , FOXO1 at Ser 256 , and ULK1 at Ser 317 , suggesting that UCN2 treatment modulates protein synthesis and degradation pathways (P < 0.05 vs. vehicle). Acutely, a single injection of Compound A in drug-naïve mice had no effect on the rate of protein synthesis in skeletal muscle, as measured via the surface sensing of translation method, while the expression of Nr4a3 and Ppargc1a4 was increased (P < 0.05 vs. vehicle). Compound A treatment prevented the loss of force production from disuse due to casting. Compound B treatment increased time to fatigue during ex vivo contractions of fast-twitch extensor digitorum longus muscle. Compound A and B treatment increased lean mass and rates of skeletal muscle protein synthesis in ob/ob mice. Conclusions Modified human UCN2 is a pharmacological candidate for the prevention of the loss of skeletal muscle mass associated with obesity and immobilization.

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A common trafficking route for GLUT4 in cardiomyocytes in response to insulin, contraction and energy-status signalling

Cited by 49 publications

References 45 publications

Measuring GLUT4 translocation in mature muscle fibers

Measuring GLUT4 translocation in mature muscle fibers

The many ways to regulate glucose transporter 4This paper is one of a selection of papers published in this Special Issue, entitled 14th International Biochemistry of Exercise Conference – Muscles as Molecular and Metabolic Machines, and has undergone the Journal’s usual peer review process.

Modified UCN2 peptide treatment improves skeletal muscle mass and function in mouse models of obesity‐induced insulin resistance

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