Enteral delivery of proteins stimulates protein synthesis in human duodenal mucosa in the fed state through a mammalian target of rapamycin–independent pathway

Coëffier, Moı̈se; Claeyssens, Sophie; Bôle‐Feysot, Christine; Guérin, Charlène; Lecleire, Stéphane; Lavoinne, Alain; Donnadieu, N.; Cailleux, Anne-Françoise; Déchelotte, Pierre

doi:10.3945/ajcn.112.046946

Cited by 17 publications

(16 citation statements)

References 47 publications

(61 reference statements)

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“…In contrast, in healthy subjects in the fed state, enteral proteins, but not glutamine, increased protein synthesis via an mTOR-independent pathway in humans. 66 Nakajo et al 38 have proposed a new concept for the biological role of phosphorylation of mTOR and intestinal cell growth: the signal induced by glutamine may stimulate cellular proliferation and increase cell number, whereas leucine or arginine induces the signal for cell growth (increase in cell size) in rat intestinal epithelial cells.…”

Section: Glutamine Signaling In the Intestinementioning

confidence: 99%

Glutamine metabolism in advanced age

Meynial-Denis

2016

Nutr Rev

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Glutamine, reviewed extensively in the last century, is a key substrate for the splanchnic bed in the whole body and is a nutrient of particular interest in gastrointestinal research. A marked decrease in the plasma glutamine concentration has recently been observed in neonates and adults during acute illness and stress. Although some studies in newborns have shown parenteral and enteral supplementation with glutamine to be of benefit (by decreasing proteolysis and activating the immune system), clinical trials have not demonstrated prolonged advantages such as reductions in mortality or risk of infections in adults. In addition, glutamine is not able to combat the muscle wasting associated with disease or age-related sarcopenia. Oral glutamine supplementation initiated before advanced age in rats increases gut mass and improves the villus height of mucosa, thereby preventing the gut atrophy encountered in advanced age. Enterocytes from very old rats continuously metabolize glutamine into citrulline, which allowed, for the first time, the use of citrulline as a noninvasive marker of intestinal atrophy induced by advanced age.

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Section: Glutamine Signaling In the Intestinementioning

confidence: 99%

Glutamine metabolism in advanced age

Meynial-Denis

2016

Nutr Rev

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“…Overall, the data reported by Coëffier et al (11) are interpreted to support a model in which amino acids act to stimulate protein synthesis in the duodenal mucosa through a mechanism distinct from the established one involving activation of mTORC1. Future studies should aim to confirm the initial conclusion and to identify the mTORC1-independent pathway involved in regulating protein synthesis in the duodenal mucosa.…”

Section: Scot R Kimballmentioning

confidence: 54%

“…It is important that Western blot analysis, rather than dot-blot analysis, be used to assess potential changes in p70S6K1 and mTOR phosphorylation, and changes in protein phosphorylation should be expressed relative to the respective target protein, rather than GAPDH, to account for potential changes in expression. Finally, possible mTORC1-independent pathways, such as those involving eIF2 and eIF2B, which were not assessed in the Coëffier et al study (11), should be evaluated in future studies. It is possible that such measurements were performed and not reported in the present study or are planned for a future report.…”

Section: Scot R Kimballmentioning

confidence: 99%

“…It is therefore imperative that future studies not only confirm the results of the present one but also test possible alternative pathways that might be involved in the effect. For example, in the Coëffier et al study (11), measurements were taken at a single time point, 5 h after the start of enteral delivery of the protein mixture and intravenous infusion of [ ]phenylalanine into protein may have occurred transiently at a time when mTORC1 signaling was activated, and that both may have returned to basal values by the time biopsies were taken, a time course analysis would be necessary. Moreover, a study that uses rapamycin to inhibit mTOR signaling could be performed, as has been used by others to assess the role of mTORC1 in the amino acid-and exerciseinduced stimulation of protein synthesis in humans (8,12).…”

Section: Scot R Kimballmentioning

confidence: 99%

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Does enteral protein administration stimulate duodenal mucosa protein synthesis through an mTORC1-independent signaling pathway?

Kimball¹

2013

The American Journal of Clinical Nutrition

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More than 40 y ago, Morgan et al (1,2) reported that in the isolated perfused rat heart, elevating amino acid concentrations in the perfusate to 5 times the concentrations observed in the plasma of a fasted animal stimulated protein synthesis rates by enhancing the initiation phase of mRNA translation. Since that time, a plethora of studies have focused on delineating the mechanism or mechanisms through which amino acids act to upregulate translation initiation. The results of those studies have identified 2 steps in initiation as targets of amino acid signaling: the binding of initiator methionyl-tRNA (met-tRNA i ) 4 to the 40S ribosomal subunit to form the 43S preinitiation complex and the binding of mRNA to the 43S preinitiation complex. The binding of met-tRNA i to the 40S ribosomal subunit is mediated by eukaryotic initiation factor (eIF) 2 and regulated by the guanine nucleotide exchange factor (GEF) eIF2B. Both proteins are phosphorylated in cells in culture on specific subunits (eIF2 on its a-subunit and eIF2B on its e-subunit) in response to changes in amino acid concentrations. Specifically, the deprivation of essential amino acids leads to activation of the protein kinase general control non-derepressing 2, which phosphorylates eIF2a, converting it from a substrate into a competitive inhibitor of eIF2B (3). Amino acid deprivation also leads to increased phosphorylation of eIF2B on its catalytic e-subunit, resulting in inhibition of its GEF activity toward eIF2 (4). Together, phosphorylation of eIF2a and eIF2Be leads to repressed rates of translation initiation by perturbing the assembly of the eIF2ÁGTPÁmet-tRNA i complex that mediates transfer of mettRNA i to the 40S ribosomal subunit.The deprivation of essential amino acids also results in development of an impairment in the binding of mRNA to the 43S preinitiation complex, an event mediated by the eIF4F complex composed of eIF4A, eIF4E, and eIF4G (5). For most mRNAs, binding to the 43S preinitiation complex occurs through the interaction of eIF4E with the m 7 GTP cap at the 5#-end of the message and the subsequent binding of eIF4G to eIF3 that is part of the 43S preinitiation complex. The deprivation of essential amino acids leads to the disassembly of the eIF4F complex by promoting the interaction of eIF4E with eIF4E binding proteins (eg, 4E-BP1) and the interaction of eIF4A with programmed cell death 4 (PDCD4), thereby preventing their interaction with eIF4G.

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“…Immunoblots were performed as previously described; briefly, total proteins (25 μg proteins/lane) were separated on a 4%‐20% gradient polyacrylamide gel (Biorad, Marnes‐la‐Coquette, France). After transfer, nitrocellulose membrane were overnight incubated at 4°C with specific primary antibodies: goat polyclonal antibodies [anti‐HSPD1, #sc‐1052, SantaCruz Biotechnology; anti‐GAPDH, #SAB2500451, Sigma‐Aldrich], rabbit monoclonal antibody [anti‐HSPA8, #8444, Cell Signaling Technology], rabbit polyclonal antibody [anti VCL, #4650, Cell Signaling Technology], and mouse monoclonal antibody [anti‐ACTA2, #A5228, Sigma‐Aldrich].…”

Section: Methodsmentioning

confidence: 99%