Effet stimulateur du neuropeptide Y sur la sécrétion du facteur de relâche de la corticostimuline (CRF) par les cellules trophoblastiques du placenta humain

Robidoux, Jacques

12 1900

Thèse numérisée par la Direction des bibliothèques de l'Université de Montréal. / L'accouchement, l'aboutissement ultime de la grossesse, est un processus bien orchestré mettant en œuvre une pléiade de peptides produits par le placenta. Récemment, la mise en évidence d'une relation entre la durée de la grossesse et la concentration plasmatique du facteur de relâche de la corticostimuline (CRF) a permis de proposer un lien entre ce peptide et l'horloge placentaire déterminant la durée de la grossesse. Or, le neuropeptide Y (NPY), un peptide produit abondamment par le placenta tout au long de la grossesse, stimule in vitro la relâche du CRF par le syncytiotrophoblaste. Puisque ce syncytiotrophoblaste est connu pour être, du moins durant le troisième trimestre de la grossesse, la principale origine du CRF circulant, le but de cette thèse est d'étudier les modalités de cet effet du NPY. Les hypothèses principales ayant balisé cette étude ont été: 1) le syncytiotrophoblaste arbore des récepteurs pour le NPY; 2) un mode de relâche du CRF dépendant du calcium est présent dans le syncytiotrophoblaste et 3) la stimulation de la relâche du CRF par le NPY dans les cellules trophoblastiques implique des voies de signalisation en amont et en aval d'une hausse de la concentration du calcium intracellulaire. En premier lieu, étant donné la nature polaire du syncytiotrophoblaste, les études de liaison ont été effectuées en parallèle sur des membranes d'origine apicale (BBM) et basale (BPM) afin de déterminer s'il y a une ségrégation des sites de liaisons pour le NPY. Les résultats obtenus suggèrent l'existence d'une population mixte de sites de liaison du NPY (Y1 et Y3) se retrouvant exclusivement sur les BBM. Par la suite, les voies de signalisation associées aux récepteurs du NPY ont été explorées sur des préparations de BBM ou sur des cellules trophoblastiques en culture primaire. Les résultats obtenus montrent que dans les BBM, l'interaction du NPY avec le récepteur de sous-type Y1 est couplée à l'activation des phospholipases C-P (PLC-P), ces dernières étant responsables, en partie, d'une activation des protéines kinases C (PKCs). L'autre portion de l'activation de ces PKCs étant attribuable à l'activation des kinases de la position D3 des phosphoinositides (PI3-K). Les résultats obtenus à l'aide des cellules trophoblastiques montrent que le NPY entraîne l'activation de la kinase dépendante du calcium et de la calmoduline de type II (CaMK.11) et des MAP kinases de type ERKv2 (ERKv2). En troisième lieu, afin de vérifier lesquelles de ces voies de signalisation sont impliquées dans le contrôle de la relâche du CRF par le NPY, nous avons, dans un premier temps, caractérisé l'habileté des cellules trophoblastiques à sécréter le CRF. Cette étape importante montre que les cytotrophoblastes issus de placentas à terme, acquièrent, en parallèle avec leur différenciation vers le phénotype apparenté au syncytiotrophoblaste, l'habileté de sécréter le CRF. En dernier lieu, nous avons démontré que le NPY, en interagissant avec des récepteurs de type Y1, induit la synthèse et la relâche du CRF par les cellules trophoblastiques. L'augmentation de la synthèse est, en grande partie, attribuable à l'activation des PLC-P, la relâche subséquente du calcium des réserves intracellulaires et à l'activation de la CaMKII. L'augmentation de la relâche est subséquente à l'activation de PKCs indépendantes du calcium, à l'activation de l'axe initié par les PLC-P et à un influx calcique ne passant pas par les L-VOCC. Intéressement, l'activation directe des L­VOCC avec le Bay K8644, bien qu'entraînant l'activation des CaMKII, favorise la relâche du CRF sans influencer la synthèse du peptide. Pris dans leur globalité, ces résultats illustrent bien la pluralité de la signalisation des récepteurs de sous-type Y 1 et la complexité du contrôle de la relâche du CRF par le NPY. De plus, ces résultats sont une étape importante dans la compréhension des mécanismes qui permettent aux peptides interagissant avec un récepteur couplé aux protéines liant les nucléotides guanyliques (protéines G), sensibles à la toxine pertussique (PTX), de réguler la relâche du CRF.

Accouchement

Grossesse

Syncytiotrophoblaste

Neuropeptide Y (NPY)

Medicine / Médecine (UMI : 0564)

Métrologie de la douleur animale sur modèles expérimentaux : développement et validation de biomarqueurs neuroprotéomiques.

Otis, Colombe

08 1900

No description available.

biomarqueur

neuroprotéomique

sensibilisation centrale

douleur

modèle animal

neuropeptide

métrologie de la douleur

validation

biomarker

neuroproteomic

central sensitization

pain

animal model

neuropeptide

pain metrology

validation

Regulation of human endocardial endothelial cells' secretion of endothelin-1 by neuropeptide Y

Abdel-Samad, Dima

January 2008

Endocardial endothelial cells (EECs) can exert a significant influence on cardiac function by releasing various factors such as nitric oxide (NO), prostanoids, endothelin-1 (ET-1) and angiotensin II (Ang II). Recently, results obtained in our laboratory demonstrated the presence of NPY and its receptors, Y[subscript 1] and Y[subscript 2], as well as ET-1 and its receptors, ET[subscript A] and ET[subscript B], at the level of endocardial endothelial cells (EECs). We have also shown that NPY induces a sustained rise in the intracellular calcium level of these cells, and that only right ventricular EECs have the capacity of secreting NPY. Moreover, the evidence in the literature has become plentiful about complex interactions existing between ET-1 and other cardioactive mediators, such as NO and Ang II. Based on the above-mentioned data, the objective of this study was to investigate if a dialogue equally exists between the systems of NPY and ET-1 at the level of human right (hREECs) and left (hLEECs) ventricular EECs. Using the technique of indirect immunofluorescence coupled to 3-D confocal microscopy, as well as ELISA, our results show that increasing concentrations of NPY (10[superscript -15], 10[superscript -10] and 10[superscript -5]M) induce the release of ET-1 from REECs and LEECs in a time- and dose-dependent fashion. However, right ventricular EECs seem to have a higher ET-1 secretory capacity as compared to their left counterparts. Upon the use of selective antagonists for the NPY receptors, Y[subscript 1], Y[subscript 2] and Y[subscript 5], and the ET-1 receptors, ET[subscript A] and ET[subscript B], our results demonstrated that in REECs the NPY-induced release of ET-1 seems to be primarily due to Y[subscript 2] receptor activation, with the subsequent activation of the ET[subscript A] and ET[subscript B] receptors by the released ET-1. On the other hand, in LEECs, the NPY-evoked secretion of ET-1 seems to be mainly the result of Y[subscript 5] receptor activation by NPY. Unlike REECs, the ET-1 released by NPY in this type of cells does not seem to be contributing further to its own release by activation of its ET[subscript A] and ET[subscript B] receptors. Therefore, our results suggest that NPY is a regulator of ET-I secretion at the level of human EECs, and that this secretory process of ET-1 is different between the right and left ventricular cells. Moreover, these results serve to highlight and endorse the important sensory and tuning roles that right and left ventricular EECs possess, respectively. The ability of EECs to contribute to the local as well as systemic release of factors, such as NPY and ET-1, can affect not only the excitation-secretion coupling of EECs and the excitation-contraction coupling of cardiomyocytes, but also the physiological and pathophysiological state of the underlying, heart muscle.

NPY-induced ET-1 secretion

Human endocardial endothelial cells

Endothelin-1

Neuropeptide Y

Migration on extracellular matrix surface and infiltration into matrix - two distinguishable activities of human T cells

Ivanoff, Jyrki

January 2003

<p>Migration of T-lymphocytes on a surface coated with extracellular matrix (ECM) components (two-dimensional (2-D) migration) and migration (infiltration) into a matrix (Three-dimesional (3-D) migration) are complex events and the underlying mechanisms are not yet fully understood. Here 2-D and 3-D migration were studied by use of seven leukemic T-cell lines representing discrete differentiation stages, a non-leukemic T-cell clone, and normal peripheral blood T cells. peripheral blood lymphocytes and the T-cell clone produced nanogram quantities of various chemokines, as compared to a production of ≤ 0.05 ng/ml by the T leukemia cell lines. In a Boyden chamber system, the leukemic T-cell lines showed haptotactic migration on fibronectin. The migration was augmented bu exposure to chemokines, including RANTES, MIP-1α, MIP-1β, and IL-8. The T-cell lines showed a peak response at a chemokine concentration of 10-50 ng/ml, whereas the T-cell clone responded optimally at 100 ng/ml. In contrast to a general capability of T-cells to migrate on 2-D ECM, only some of the T-cell lines were capable of 3-D migration into Matrigel or a collagen matrix. The infiltrative capacity was unrelated to the capacity to migrate on or adhere to the substrata. T-cell lines with a capacity to infiltrate produced matrix metalloproteinase-9 (MMP-9) and tissue inhibitor of matrix metalloproteinases-1 (TIMP-1), whereas non-infiltrating cell lines did not produce MMP-9. T-cell lines capable of infiltrating Matrigel or collagen responded to chemokines exposure with increased infiltration, but the chemokines did not render non-infiltrative cell lines infiltrative. Stimulation of infiltration of T-cell lines into collagen by the chemokine SDF-1α was inhibited by somatostatin, a neuropeptide with immunosuppressive properties. In conclusion, the ability to migrate on 2-D substrata and to infiltrate into 3.D substrata was found to be distinguishable properties of T cells. failure of some T-cell lines to infiltrate correlated with the lack of expression of MMP-9. Chemokines stimulated infiltration of infiltrative T-cell lines into collagen and Matrigel but did not render non-infiltrative T-cell lines infiltrative. Finally, a possible physiological mechanism for modulation of the chemokine-stimulated 3-D migration was demonstrated.</p>

Immunology

extracellular matrix

fibronectin

collagen type IV

laminin

neuropeptide

chemokine

TIMP-1

MMP-9

T cells

Migration

Immunologi

Immunology

Immunologi

Substance P Endopeptidase : Purification and Characterizataion of Enzyme Activity and Evaluation of its Function during Stressful Condition

Karlsson, Krister

January 2004

<p>The purification and biochemical characterization of the substance P (SP) hydrolyzing enzyme, substance P endopeptidase (SPE), have been carried out; with subsequent orientation in neurobiological fundamental processes involved in opioid dependence, withdrawal, and heat-stress.</p><p>SPE was purified from rat spinal cord, human spinal cord and cerebrospinal fluid (CSF), rat ventral tegemental area (VTA), and rat hippocampus. The enzyme activity was found to release the biologically active fragments SP(1-7) and SP(1-8) as major products. The purified enzymes were characterized with regard to their biochemical and kinetic properties. The typical SPE is neither inhibited by phosphoramidon nor captopril nor phenylmethanesulfonylflourid (PMSF). In comparison to other known proteases SPE differed in characteristics regarding substrate specificity, inhibition-profile, cleavage pattern, and other kinetic parameters. The technically very delicate approach of micro purification of SPE from the rat ventral tegemental area (VTA) (this is a very small tissue), turned out to be possible with the ÄKTA™-purifier system. Studies revealed a crucial role of SPE in a series of clinically important neuropathological conditions, such as opioid tolerance, and withdrawal (SPE, increased); and heat-stress (SPE, increased). These findings emerged from assessment of enzyme activity in hypothalamus, nucleus accumbens (NAc) periaqueductal gray (PAG), pituitary, striatum, substantia nigra (SN), VTA, spinal cord. Viewing the role of SPE in morphine tolerance, it was possible to note regional differences with a decrease in PAG, and striatum, whereas an increase was seen in SN, and VTA. After heat-stress treatment, SPE was raised in several regions (cerebral cortex, hippocampus, diencephalon, cerebellum, spinal cord), and the most precise observation of this was located to the hippocampus structure.</p>

Pharmacology

Substance P Endopeptidase

Neuropeptide

Central Nervous System

Purification

Drug Dependence

Heat Stress

Farmakologi

Pharmacological research

Farmakologisk forskning

Functional Studies of the Neuropeptide Y System : Receptor-Ligand Interaction and Regulation of Food Intake

Åkerberg, Helena

January 2009

The members of the mammalian neuropeptide Y family, i.e. the peptides neuropeptide Y (NPY), peptide YY (PYY) and pancreatic polypeptide (PP), are all involved in regulation of food intake. In human and most other mammals they act via receptors Y1, Y2, Y4 and Y5. NPY is released in the hypothalamus and is one of the strongest appetite-stimulating neurotransmitters whereas PP and PYY are secreted from gut endocrine cells after meals and function as appetite-reducing hormones. This thesis describes studies of the NPY system at both the molecular and the physiological level. The first part describes two investigations of receptor-ligand interactions with the human Y1 and Y2 receptors. The results clarify the importance of several amino-acid residues of the human Y1 receptor. Three amino acids previously suggested by others to form a binding pocket for the carboxy-terminus of the peptide were confirmed to be crucial for interaction with peptide ligands. However, they were found to be too distantly located from each other to be able to form a binding pocket. Further investigation of the three corresponding positions in the human Y2 receptor showed that only one of the positions was important for interaction with full-length peptides. The results indicate overlapping but, surprisingly, non-identical binding of the different peptides to human Y1 and Y2 receptors, despite the fact that the two receptors share a common ancestor. The second part of the thesis describes an investigation of the effect of PP on food intake in six beagle dogs and a test for personality characteristics in dogs (TFPC). Treatment with physiological doses of PP decreased both the appetitive and the consummatory drive but had no effect on the amount food consumed. The TFPC protocol was used to map individual behavioral differences in a population of sixteen beagle dogs. The test, which included several situations that may appear in an experimental study, revealed considerable inter-individual differences in behavioral responses despite the fact that the dogs were born and housed in the same animal facility in constant controlled conditions. These results demonstrate that PP can influence food intake in distantly related mammals and emphasize the importance of considering differences in personality in experimental animals.

neuropeptide Y

G-protein coupled receptor (GPCR)

site-directed mutagenesis

pancreatic polypeptide

food intake

dog

Pharmacology

Farmakologi

Migration on extracellular matrix surface and infiltration into matrix - two distinguishable activities of human T cells

Ivanoff, Jyrki

January 2003

Migration of T-lymphocytes on a surface coated with extracellular matrix (ECM) components (two-dimensional (2-D) migration) and migration (infiltration) into a matrix (Three-dimesional (3-D) migration) are complex events and the underlying mechanisms are not yet fully understood. Here 2-D and 3-D migration were studied by use of seven leukemic T-cell lines representing discrete differentiation stages, a non-leukemic T-cell clone, and normal peripheral blood T cells. peripheral blood lymphocytes and the T-cell clone produced nanogram quantities of various chemokines, as compared to a production of ≤ 0.05 ng/ml by the T leukemia cell lines. In a Boyden chamber system, the leukemic T-cell lines showed haptotactic migration on fibronectin. The migration was augmented bu exposure to chemokines, including RANTES, MIP-1α, MIP-1β, and IL-8. The T-cell lines showed a peak response at a chemokine concentration of 10-50 ng/ml, whereas the T-cell clone responded optimally at 100 ng/ml. In contrast to a general capability of T-cells to migrate on 2-D ECM, only some of the T-cell lines were capable of 3-D migration into Matrigel or a collagen matrix. The infiltrative capacity was unrelated to the capacity to migrate on or adhere to the substrata. T-cell lines with a capacity to infiltrate produced matrix metalloproteinase-9 (MMP-9) and tissue inhibitor of matrix metalloproteinases-1 (TIMP-1), whereas non-infiltrating cell lines did not produce MMP-9. T-cell lines capable of infiltrating Matrigel or collagen responded to chemokines exposure with increased infiltration, but the chemokines did not render non-infiltrative cell lines infiltrative. Stimulation of infiltration of T-cell lines into collagen by the chemokine SDF-1α was inhibited by somatostatin, a neuropeptide with immunosuppressive properties. In conclusion, the ability to migrate on 2-D substrata and to infiltrate into 3.D substrata was found to be distinguishable properties of T cells. failure of some T-cell lines to infiltrate correlated with the lack of expression of MMP-9. Chemokines stimulated infiltration of infiltrative T-cell lines into collagen and Matrigel but did not render non-infiltrative T-cell lines infiltrative. Finally, a possible physiological mechanism for modulation of the chemokine-stimulated 3-D migration was demonstrated.

Immunology

extracellular matrix

fibronectin

collagen type IV

laminin

neuropeptide

chemokine

TIMP-1

MMP-9

T cells

Migration

Immunologi

Immunology

Immunologi

Substance P Endopeptidase : Purification and Characterizataion of Enzyme Activity and Evaluation of its Function during Stressful Condition

Karlsson, Krister

January 2004

The purification and biochemical characterization of the substance P (SP) hydrolyzing enzyme, substance P endopeptidase (SPE), have been carried out; with subsequent orientation in neurobiological fundamental processes involved in opioid dependence, withdrawal, and heat-stress. SPE was purified from rat spinal cord, human spinal cord and cerebrospinal fluid (CSF), rat ventral tegemental area (VTA), and rat hippocampus. The enzyme activity was found to release the biologically active fragments SP(1-7) and SP(1-8) as major products. The purified enzymes were characterized with regard to their biochemical and kinetic properties. The typical SPE is neither inhibited by phosphoramidon nor captopril nor phenylmethanesulfonylflourid (PMSF). In comparison to other known proteases SPE differed in characteristics regarding substrate specificity, inhibition-profile, cleavage pattern, and other kinetic parameters. The technically very delicate approach of micro purification of SPE from the rat ventral tegemental area (VTA) (this is a very small tissue), turned out to be possible with the ÄKTA™-purifier system. Studies revealed a crucial role of SPE in a series of clinically important neuropathological conditions, such as opioid tolerance, and withdrawal (SPE, increased); and heat-stress (SPE, increased). These findings emerged from assessment of enzyme activity in hypothalamus, nucleus accumbens (NAc) periaqueductal gray (PAG), pituitary, striatum, substantia nigra (SN), VTA, spinal cord. Viewing the role of SPE in morphine tolerance, it was possible to note regional differences with a decrease in PAG, and striatum, whereas an increase was seen in SN, and VTA. After heat-stress treatment, SPE was raised in several regions (cerebral cortex, hippocampus, diencephalon, cerebellum, spinal cord), and the most precise observation of this was located to the hippocampus structure.

Pharmacology

Substance P Endopeptidase

Neuropeptide

Central Nervous System

Purification

Drug Dependence

Heat Stress

Farmakologi

Pharmacological research

Farmakologisk forskning

Anti-diuresis in the Blood-gorging Bug, Rhodnius prolixus: The Role of CAPA Peptides

Paluzzi, Jean-Paul

17 February 2011

CAPA-related peptides belong to a family of neuropeptides localized to the central nervous system that can function in diverse roles in the regulation of water and salt homeostasis in insects. These peptides are known to stimulate fluid secretion by Malpighian tubules (MTs) in Dipteran species, thus serving a diuretic function. In contrast, this thesis demonstrates that members of this family of peptides in Rhodnius prolixus serve an anti-diuretic role and have multiple tissue targets, whereby they oppose the activity of diuretic hormones such as serotonin (5-Hydroxytryptamine hydrochloride; 5-HT). I have identified two genes each encoding three peptides in R. prolixus, suggesting this insect is capable of producing a greater number of CAPA-peptides compared to other insects that contain only a single CAPA gene. Interestingly, while the second peptide encoded in each R. prolixus gene (RhoprCAPA-α2/-β2) inhibits the stimulatory effects of serotonin on tissues such as the anterior midgut and Malpighian tubules, it appears the other CAPA-related and pyrokinin-related peptides do not play a major role in inhibiting the effects of serotonin on these tissues. More specifically, serotonin-stimulated fluid secretion by MTs and fluid absorption by the anterior midgut are reduced by the anti-diuretic peptide, RhoprCAPA-α2. In addition, I have also identified a G protein-coupled receptor which likely mediates the anti-diuretic effect associated with RhoprCAPA-α2 and have functionally characterized this receptor in Chinese hamster ovary cells. Spatial transcript expression analysis in fifth-instars reveals a wide distribution of the receptor in tissues associated with the rapid post-gorging diuresis. Thus, my findings suggest that numerous tissues are regulated by the CAPA peptides in R. prolixus. Gene structure and phylogenetic analyses demonstrate that this receptor is the orthologue of the D. melanogaster capa receptor (CG14575) with homologs in other insects. Taken together, my thesis demonstrates that the RhoprCAPA peptides play an integral role in the coordination and maintenance of anti-diuresis in R. prolixus. This mechanism is necessary following the rapid diuresis associated with blood-feeding by this medically-important insect.

anti-diuresis

Rhodnius prolixus

Chagas' disease

CAPA

neuropeptide

neurohormone

diuresis

G protein coupled receptor

0433

0317

0307

0719

0472

The Physiological Roles of Rhopr-kinins and the Molecular Characterization of their Gene in the Blood-gorging Insect, Rhodnius prolixus

Bhatt, Garima

20 November 2012

The dramatic feeding-related activities of the Chagas' disease vector, Rhodnius prolixus are under neurohormonal regulation of serotonin and various neuropeptides. One such family of neuropeptides, the insect kinins, possesses diuretic, digestive and myotropic activities in many insects. In R. prolixus, they co-localize with the corticotropin-releasing factor (CRF)-like diuretic hormone (DH) in neurosecretory cell bodies and their abdominal neurohaemal sites. Additionally, kinins are present in endocrine cells of the midgut and are known to stimulate hindgut and midgut contractions. Through the experimentation presented in this dissertation, the cloning and spatial expression of the R. prolixus kinin (Rhopr-kinin) transcript is described. Physiological bioassays demonstrate the myostimulatory effects of selected Rhopr-kinin peptides and also illustrate the augmented responses of hindgut contractions to co-application of Rhopr-kinin and Rhopr-CRF/DH. The irreversible effects of two synthetic kinin analogs on the hindgut relative to the native kinins also exhibit the prospective biotechnological significance of this study.

neurohormone

insect

Rhodnius prolixus

kinin

neuropeptide

CRF

cloning

Rhopr-kinin

analog

diuresis

serotonin

receptor

hindgut

myotropic

Insect Neuroendocrinology

Insect Neurophysiology