Kinetic Study of Neuropeptide Y (NPY) Proteolysis in Blood and Identification of NPY3–35

Abid, Karim; Rochat, Bertrand; Lassahn, Paul-Gerhard; Stöcklin, Reto; Michalet, Sophie; Brakch, Noureddine; Aubert, Jean‐François; Vatansever, Bilgin; Tella, Patricia; Meester, Ingrid De; Grouzmann, Eric

doi:10.1074/jbc.m109.035253

Cited by 61 publications

(64 citation statements)

References 47 publications

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“…Previous studies have shown that in vitro incubations of NPY in human plasma resulted in cleavage of the COOHterminal amino acid and dipeptide (1,22). We have demonstrated that PYY is significantly degraded to PYY in the pig and also shown that the liver is involved in the COOHterminal truncation (35).…”

Section: Discussionmentioning

confidence: 61%

“…A method for exact measurements of active PYY 3-36 levels (e.g., sandwich ELISA or LC-MS) would therefore be very valuable in the interpretation of the physiological effects of PYY. In vitro degradation of NPY in human plasma has indicated that NPY is COOH terminally cleaved to primarily NPY , and only trace amounts of NPY have been identified (1). As in pig blood and plasma, PYY was COOH terminally degraded in human blood and plasma in vitro.…”

Section: Discussionmentioning

confidence: 99%

“…PYY and NPY are COOH terminally amidated and therefore considered relatively protected from COOH-terminal degradation. However, COOH-terminal degradation of NPY, rendering the peptide inactive on the Y1-and Y2-receptors, has been demonstrated in vitro (1,9,22,24). As the sequences of NPY and PYY are 70% homologous, we speculated that PYY might also be prone to COOH-terminal degradation.…”

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confidence: 99%

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In vivo and in vitro degradation of peptide YY_3–36 to inactive peptide YY_3–34 in humans

Toräng

Bojsen‐Møller

Svane

et al. 2016

American Journal of Physiology-Regulatory, Integrative and Comp

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-Peptide YY (PYY) is a 36-amino-acid peptide released from enteroendocrine cells upon food intake. The NH 2 terminally truncated metabolite, PYY3-36, exerts anorexic effects and has received considerable attention as a possible antiobesity drug target. The kinetics and degradation products of PYY metabolism are not well described. A related peptide, neuropeptide Y, may be degraded from the COOH terminus, and in vivo studies in pigs revealed significant COOH-terminal degradation of PYY. We therefore investigated PYY metabolism in vitro after incubation in human blood and plasma and in vivo after infusion of PYY 1-36 and PYY3-36 in eight young, healthy men. A metabolite, corresponding to PYY 3-34, was formed after incubation in plasma and blood and during the infusion of PYY. PYY 3-34 exhibited no agonistic or antagonistic effects on the Y2 receptor. PYY 1-36 infused with and without coadministration of sitagliptin was eliminated with half-lives of 10.1 Ϯ 0.5 and 9.4 Ϯ 0.8 min (means Ϯ SE) and metabolic clearance rates of 15.7 Ϯ 1.5 and 14.1 Ϯ 1.1 ml·kg Ϫ1 ·min Ϫ1 after infusion, whereas PYY 3-36 was eliminated with a significantly longer half-life of 14.9 Ϯ 1.3 min and a metabolic clearance rate of 9.4 Ϯ 0.6 ml·kg Ϫ1 ·min Ϫ1 . We conclude that, upon intravenous infusion in healthy men, PYY is inactivated by cleavage of the two COOHterminal amino acids. In healthy men, PYY 3-36 has a longer half-life than PYY 1-36. peptide YY; kinetics; degradation PEPTIDE YY (PYY) is a gastrointestinal peptide hormone, released into the circulation in response to food intake (3,4,8,18), belonging to the pancreatic polypeptide family together with neuropeptide Y (NPY) and pancreatic polypeptide. These are all 36-amino-acid peptides characterized by a high content of tyrosine, proline, and arginine and a hairpin structure, the so-called " 21).PYY is synthesized and released from endocrine L-cells in the intestinal mucosa, often together with proglugacon-derived peptides, namely glucagon-like peptide-1 (GLP-1), GLP-2, oxyntomodulin, and glicentin. PYY immunoreactive cells are found primarily in ileum and colon with increasing density distally (4).PYY is present in plasma in two major molecular forms, the 36-amino-acid form, PYY 1-36 , and the 34-amino-acid NH 2 -terminally truncated form, PYY 3-36 , which is formed by cleavage of the two NH 2 -terminal amino acids by the enzyme dipeptidyl peptidase-4 (DPP-4) (28). DPP-4 is present in both a soluble form and as a transmembrane protein in endothelial, epithelial, and lymphoid tissue. DPP-4 cleaves and inactivates, e.g., glucose-dependent insulinotropic polypeptide and GLP-1 with short plasma half-lives of 5 and 1-2 min, respectively (15,23,36).Anorexigenic effects of PYY 3-36 have been demonstrated in several studies with intravenous administration of PYY 3-36 (6, 16, 32, 34), whereas infusions of PYY 1-36 have no effect on food intake (34), suggesting that the cleavage of PYY 1-36 to PYY 3-36 is not as complete and rapid as for GLP-1 (34). The half-life of PYY 1-36 has been deter...

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Section: Discussionmentioning

confidence: 61%

Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 99%

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In vivo and in vitro degradation of peptide YY_3–36 to inactive peptide YY_3–34 in humans

Toräng

Bojsen‐Møller

Svane

et al. 2016

American Journal of Physiology-Regulatory, Integrative and Comp

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“…Moreover mass spectrometry has been used to examine peptides without previously understood biological activities (Habermann et al, 2006;Albrethsen et al, 2006b;Aivado et al, 2007). If enzymes are released into, or activated in, the blood and specifically fragment or modify target proteins in a time and dose dependant fashion then these enzyme activities might be assayed using mass spectrometry and pharmacological inhibition (Marshall et al, 2003;Abid et al, 2009;He et al, 2009;Schebb et al, 2009). Biological activities that process blood proteins to release peptides associated with protein regulation might be directly detected by mass spectrometry and independently confirmed by SDS-PAGE and Western blot (Mansfield, 1995;Marshall et al, 2003).…”

Section: F Biological Activitymentioning

confidence: 99%

Mass spectrometry of peptides and proteins from human blood

Zhu

Bowden

Zhang

et al. 2010

Mass Spectrometry Reviews

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It is difficult to convey the accelerating rate and growing importance of mass spectrometry applications to human blood proteins and peptides. Mass spectrometry can rapidly detect and identify the ionizable peptides from the proteins in a simple mixture and reveal many of their post-translational modifications. However, blood is a complex mixture that may contain many proteins first expressed in cells and tissues. The complete analysis of blood proteins is a daunting task that will rely on a wide range of disciplines from physics, chemistry, biochemistry, genetics, electromagnetic instrumentation, mathematics and computation. Therefore the comprehensive discovery and analysis of blood proteins will rank among the great technical challenges and require the cumulative sum of many of mankind's scientific achievements together. A variety of methods have been used to fractionate, analyze and identify proteins from blood, each yielding a small piece of the whole and throwing the great size of the task into sharp relief. The approaches attempted to date clearly indicate that enumerating the proteins and peptides of blood can be accomplished. There is no doubt that the mass spectrometry of blood will be crucial to the discovery and analysis of proteins, enzyme activities, and post-translational processes that underlay the mechanisms of disease. At present both discovery and quantification of proteins from blood are commonly reaching sensitivities of ∼1 ng/mL.

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“…In addition, PK can function as a plasminogen activator, which could contribute to plasminmediated fibrinolysis, activation of metalloproteinases, and adipocyte differentiation [16,17]. Recently, PK has been shown to cleave neuropeptide Y to generate an inactive fragment [18]. Thus, in addition to PK's well-characterized effects in the intrinsic coagulation pathway and the kallikrein kinin system, these recent findings suggest that PK could have a broader array of substrates that could mediate its effects on vascular physiology and metabolism.…”

Section: Introductionmentioning

confidence: 98%

Proteomic Identification of Novel Plasma Kallikrein Substrates in the Astrocyte Secretome

Liu

Gao

Feener

2010

Transl. Stroke Res.

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Plasma kallikrein (PK) is activated during hemorrhage and has been implicated in cerebral vascular permeability and edema. To further characterize the potential effects of PK on the brain that may follow cerebral vascular injury, we have utilized a proteomics approach to search for novel PK substrates in the astrocyte secretome. Extracellular proteins released by astrocytes are critical mediators of cerebral homeostasis, including roles in synapse function and vascular integrity. We identified 1,108 proteins in astrocyte condition medium and 295 of these were annotated as secreted proteins. The total abundance of nine proteins was changed after treatment with PK. Characterization of the secreted proteins revealed low molecular weight fragments for 59 proteins in conditioned media exposed to PK that were not observed in untreated controls. The most striking finding from this study was the appearance of fragmentation of 26 extracellular matrix-associated proteins including collagen isoforms 1-6 and11, nidogen-1 and -2, lysyl oxidase-like protein 1, and matrix metalloproteinase 19 in the presence of PK. We also demonstrated that PK induced the fragmentation of non-matrix proteins, including apolipoprotein E. This report further characterizes the astrocyte secretome and identifies novel potential targets of PK-induced proteolysis that may contribute to its effects on the brain following vascular injury.

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Kinetic Study of Neuropeptide Y (NPY) Proteolysis in Blood and Identification of NPY3–35

Cited by 61 publications

References 47 publications

In vivo and in vitro degradation of peptide YY_3–36 to inactive peptide YY_3–34 in humans

In vivo and in vitro degradation of peptide YY_3–36 to inactive peptide YY_3–34 in humans

Mass spectrometry of peptides and proteins from human blood

Proteomic Identification of Novel Plasma Kallikrein Substrates in the Astrocyte Secretome

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Kinetic Study of Neuropeptide Y (NPY) Proteolysis in Blood and Identification of NPY3–35

Cited by 61 publications

References 47 publications

In vivo and in vitro degradation of peptide YY3–36 to inactive peptide YY3–34 in humans

In vivo and in vitro degradation of peptide YY3–36 to inactive peptide YY3–34 in humans

Mass spectrometry of peptides and proteins from human blood

Proteomic Identification of Novel Plasma Kallikrein Substrates in the Astrocyte Secretome

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In vivo and in vitro degradation of peptide YY_3–36 to inactive peptide YY_3–34 in humans

In vivo and in vitro degradation of peptide YY_3–36 to inactive peptide YY_3–34 in humans