ERK/MAPK signaling and the regulation of light-evoked entrainment of the circadian clock in the suprachiasmatic nucleus.

Yoon, Hyojung

January 2021

No description available.

Molecular Biology

Nanoscience

THE INFLUENCE OF MODIFICATION OF BMAL1 EXPRESSION IN SKELETAL MUSCLE ON WHOLE-BODY METABOLISM AND FUNCTION

Mesfin, Fikir

15 May 2012

No description available.

Biology

Circadian rhythm

SCN

CLOCK

BMAL1

skeletal muscle

THE EFFECTS OF ORAL COCAINE ON THE CIRCADIAN TIMING SYSTEM

Amicarelli, Mario Joseph

30 July 2014

No description available.

Biology

Neurobiology

Physiology

SCN

Cocaine

Circadian Rhythm

Light

Mouse

Deep Defects in Wide Bandgap Materials Investigated Using Deep Level Transient Spectroscopy

Perjeru, Florentine

11 October 2001

No description available.

Physics, Condensed Matter

DLTS

GaN

ScN

defects

electrical characterization

Impact de la rétinopathie diabétique sur le fonctionnement et l’entraînement par la lumière des horloges centrale et rétinienne / .

Lahouaoui, Hasna

17 December 2014

La rétinopathie diabétique est une cause majeure de cécité et de malvoyance qui affecte jusqu'à 90% des patients atteints de diabète. Le Maroc n’échappe pas à cette pathologie, qui est connue pour altérer le fonctionnement du système visuel et pourrait conduire également à des désordres chronobiologiques, aussi bien chez l’Homme que chez des modèles animaux. Ces altérations pourraient être liées aux dégénérescences neuronales des systèmes de photoréception classique (cône et bâtonnet) et des cellules ganglionnaires à mélanopsine, impliqués dans la régulation et l’entraînement par la lumière du système circadien. Cependant, à l’heure actuelle, peu d’études ont analysé précisément l’impact de la rétinopathie diabétique sur le système circadien. L’objectif de notre travail est d’analyser au cours de la rétinopathie diabétique (1) l’atteinte des cônes, des bâtonnets et des cellules ganglionnaires à mélanopsine, (2) le fonctionnement endogène moléculaire et la réponse à la lumière des horloges centrale et rétinienne et (3) la réponse comportementale du système circadien à la lumière. Notre stratégie est basée sur l’utilisation d’un modèle murin, chez lequel le diabète est induit expérimentalement par l’administration d’un agent chimique la streptozotocine (STZ), toxique pour les cellules β pancréatiques. Des approches morphométriques, moléculaires et comportementales ont été utilisées. Nos résultats montrent que le diabète induit des changements morphologiques des cellules ganglionnaires à mélanopsine tels que des gonflements des somas et des varicosités au niveau des dendrites avec une préservation du nombre total de ces cellules. Ceci est associé à une diminution de l’induction par la lumière du gène c-fos et des gènes de l’horloge Per1 et Per2 au niveau du SCN et à l’absence de cette induction au niveau rétinien au stade 12 semaines après l’induction du diabète. La machinerie moléculaire des horloges rétinienne et centrale évaluée par l’analyse de l’expression circadienne des gènes de l’horloge et des gènes contrôlés par les gènes de l’horloge montre que certains gènes de l’horloge clés pour chaque tissu sont altérés. A l’échelle comportementale, les souris STZ (souris diabétiques) montrent une réduction de l’amplitude du rythme de leur activité locomotrice totale et une diminution de la sensibilité à la lumière aux faibles intensités. Après une avance de phase du cycle 12L/12D, ces animaux présentent également une diminution de la vitesse de resynchronisation au nouveau cycle lumineux imposé par rapport aux animaux témoins. Ces nouvelles données montrent que le diabète de type 1 altère les réponses du système circadien à la lumière d’un point de vue moléculaire et comportemental et suggèrent que les patients diabétiques peuvent présenter des troubles circadiens particulièrement lorsqu’ils sont soumis aux challenges chronobiologiques / Diabetic retinopathy is a major cause of blindness and is commonly viewed as a vascular complication of type 1 diabetes. However, this kind of diabetes causes visual dysfunction before the onset of clinically visible microvascular changes, associated with diabetic retinopathy. Several histopathological studies in diabetic patients and in chemically-induced or genetic rodent models of diabetes indicate that photoreceptors and retinal ganglion cells (RGCs) are affected by diabetes with apoptotic degeneration. There is increasing evidence that melanopsin-expressing ganglion cells that are crucial for the regulation of a range of non-visual functions including the photic synchronization of circadian rhythms are altered in retinal pathologies. The link between diabetes and circadian rhythms has only been addressed in a relatively limited number of studies. Using a streptozotocin-induced (STZ) model of diabetes, we investigated the impact of diabetic retinopathy on non-visual functions by analyzing the morphology of melanopsin ganglion cells and light-induced c-fos and Period 1-2 clock genes in the central (SCN) and the retina clocks. The effect of this pathology on the endogenous circadian function of clock and controlled clock genes was assessed in the SCN and the retina at 12 weeks post-diabetes. Behaviorally, the ability of STZdiabetic mice to entrain to light was challenged by the exposure of animals to 1) successive light/dark (LD) cycle of decreasing or increasing light intensities during the light phase and 2) 6-hr advance of the LD cycle. Our results show that diabetes induces morphological changes of melanopsin-expressing ganglion cells including soma swelling and dendritic varicosities with no reduction in their total number, associated with decreased c-fos and clock genes induction by light in the SCN and also in the retina at 12 weeks post-onset of diabetes. In addition, the circadian expression of major clock genes was altered in the central and retinal clocks, suggesting that RD affects the endogenous molecular machinery and the light response of these two clocks. Moreover, STZ-diabetic mice exhibited a reduction of overall locomotor activity, a decrease of circadian sensitivity to light at low intensities, and a delay in the time to re-entrain after a phase advance of the LD cycle. These novel findings demonstrate that diabetes alters clock genes and behavioral responses of the circadian timing system to light and suggest that diabetic patients may show an increased propensity for circadian disturbances, in particular when they are exposed to chronobiological challenges

Rétinopathie diabétique

STZ

Système circadien

Horloge

Rétine

SCN

Photorécepteurs

Mélanopsine

Diabetic retinopathy

STZ

Melanopsin

SCN

Retina

Clock genes

Locomotor activity

Light intensity

570

Characterization of the electrical and physical properties of scandium nitride grown using hydride vapor phase epitaxy

Richards, Paul

January 1900

Master of Science / Department of Electrical and Computer Engineering / Andrew Rys / It is important in semiconductor manufacturing to understand the physical and electrical characteristics of new proposed semiconductors to determine their usefulness. Many tests are used in order to achieve this goal, such as x-ray diffraction, Hall effect measurements, and the scanning electron microscope. With these tests, the usefulness of the semiconductor can be determined, leading to more possibilities for growth in industry. The purpose of the present study was to look at the semiconductor scandium nitride (ScN), grown using the hydride vapor phase epitaxy (HVPE) method on various substrates, and determine the physical and electrical properties of the sample. This study also sought to answer the following questions: 1) Can any trends be found from the results?, and 2) What possible application could scandium nitride be used for in the future? A sample set of scandium nitride samples was selected. Each one of these samples was checked for contaminants from the growth procedure, such as chlorine, under the scanning electron microscope and checked for good conduction of current needed for the Hall effect measurements. The thickness of the scandium nitride layer was computed using the scanning electron microscope. Using the thickness of the scandium nitride, Hall effect measurement values were computed. The plane the samples lie on was checked using x-ray diffraction. The test results shed light on many trends in the scandium nitride. Many of the samples were determined to have an aluminum nitride (AlN) contamination. This contamination led to a much higher resistivity and a much lower mobility no matter what thickness the scandium nitride was. The data from the samples was then used to offer suggestions on how to improve the growth process.

Scandium

Nitride

HVPE

Epitaxy

characterization

ScN

Engineering, Chemical (0542)

Evolution of the Neuropeptide Y and Opioid Systems and their Genomic Regions

Sundström, Görel

January 2010

Two whole genome duplications (2R) occurred early in vertebrate evolution. By using combined information from phylogenetic analyses and chromosomal location of genes, this thesis delineates the evolutionary history of two receptor-ligand systems that expanded by these large scale events. A third whole genome duplication (3R) took place in the teleost fish lineage and has also contributed to the complexity of the gene families. New members of neuropeptide Y (NPY) peptide and receptor families were generated in 2R and 3R. Evolutionary comparisons show that the ancestral teleost fish had four peptides; subsequently, differential losses of the peptide genes occurred. In zebrafish the peptides and receptors display differences in tissue distribution and have  evolved binding preferences. In the frog Silurana tropicalis three peptides and six receptors werev identified, also displaying some differences in tissue distribution and receptor-ligand preferences. The findings in these experimental animals highlight both evolutionary conservation and lineage-specific features of the NPY system. The opioid system consists of four receptors and several peptides originating from four precursors. These results show that the receptor family was formed in 2R and 3R and that 2R together with one local duplication gave rise to the peptide family. The ancestral receptor and peptide genes were located on the same chromosome, suggesting coevolution. The Hox gene clusters, important in early development, provided the first strong evidence for 2R. Several neighboring gene families were analyzed and found to have expanded in 2R and 3R. In depth analyses of insulin-like growth factor binding protein (IGFBP) and voltage-gated sodium channel (SCN) gene families illustrates the importance of local duplications in combination with whole genome duplications in the formation of gene families. These findings provide additional strong evidence for two genome duplications in early vertebrate evolution and show that these events generated many new genes that could evolve new or more specialized functions.

neuropeptide Y

opioid

evolution

genome duplication

gene duplication

Hox

SCN

IGFBP

MEDICINE

MEDICIN

CIRCADIAN AND HOMEOSTATIC REGULATION OF SLEEP IN CAST/EiJ AND C57BL/6J MICE

Jiang, Peng

01 January 2011

Sleep is essential for mammals and possibly for all animals. Advancing our knowledge of sleep regulation is crucial for the development of interventions in sleep-related health and social problems. With this aim, this study utilizes laboratory mice to explore sleep regulatory mechanisms at behavioral, molecular, and genetic levels. Sleep is regulated by the interaction of circadian and homeostatic processes. The circadian clock facilitates sleep to occur at a favorable time of the day. Normal mice, such as the C57BL/6J (B6) strain, sleep mostly during the day and initiate activities at dark onset. Here, I show mice of the CAST/EiJ (CAST) strain initiate activity unusually early (hours before dark). The circadian gating of photic phase-shifting responses was phase-lagged in the CAST mice relative to their activity rhythms, implying an altered coupling between the clock and its output. Light failed to suppress activity in the CAST mice, allowing full expression of the early activity. A previously identified quantitative trait locus that contributes to the advanced circadian phase was also confirmed and refined to a smaller genomic region. The circadian oscillation and light-induction of clock-genes Per1 and Per2 expression was not different between B6 and CAST mice in the suprachiasmatic nucleus (SCN) of the brain, where the mammalian master circadian clock is located. However, in the cerebral cortex and paraventricular hypothalamic nucleus of CAST mice, Per mRNA oscillations were phase-advanced coordinately with their advanced behavioral rhythms. These data thus provide direct evidence that the cause of the early runner phenotype is located downstream of the master circadian clock. The rhythms of cortical Per expression may not be a result of direct SCN effector mechanisms, but rather driven by activity-rest and sleep-wake. I further show that prolonged waking induces cortical Per expression, and this induction persisted in SCN-lesioned animals. SCN Per expression in intact animals was not affected. Thus, a homeostatic drive, independent of the SCN clock, regulates cortical Per expression, although a possible circadian influence in the intact animals was also suggested by detailed analyses. These data may suggest a molecular mechanism bridging the circadian and homeostatic processes for sleep regulation and functions.

Era1

phase response curve

Per expression

SCN

cerebral cortex

Genetics

Molecular Biology

Neuroscience and Neurobiology

Alternate Substrates and Isotope Effects as a Probe of the Malic Enzyme Reaction

Gavva, Sandhya Reddy

08 1900

Dissociation constants for alternate dirmcleotide substrates and competitive inhibitors suggest that the dinucleotide binding site of the Ascaris suum NAD-malic enzyme is hydrophobic in the vicinity of the nicotinamide ring. Changes in the divalent metal ion activator from Mg^2+ to Mn^2+ or Cd^2+ results in a decrease in the dinucleotide affinity and an increase in the affinity for malate. Primary deuterium and 13-C isotope effects obtained with the different metal ions suggest either a change in the transition state structure for the hydride transfer or decarboxylation steps or both. Deuterium isotope effects are finite whether reactants are maintained at saturating or limiting concentrations with all the metal ions and dinucleotide substrates used. With Cd^2+ as the divalent metal ion, inactivation of the enzyme occurs whether enzyme alone is present or is turning over. Upon inactivation only Cd^2+ ions are bound to the enzyme which becomes denatured. Modification of the enzyme to give an SCN-enzyme decreases the ability of Cd^2+ to cause inactivation. The modified enzyme generally exhibits increases in K_NAD and K_i_metai and decreases in V_max as the metal size increases from Mg^2+ to Mn^2+ or Cd^2+, indicative of crowding in the site. In all cases, affinity for malate greatly decreases, suggesting that malate does not bind optimally to the modified enzyme. For the native enzyme, primary deuterium isotope effects increase with a concomitant decrease in the 13-C effects when NAD is replaced by an alternate dinucleotide substrate different in redox potential. This suggests that when the alternate dinucleotides are used, a switch in the rate limitation of the chemical steps occurs with hydride transfer more rate limiting than decarboxylation. Deuteration of malate decreases the 13-C effect with NAD for the native enzyme, but an increase in 13-C effect is obtained with alternate dinucleotides. These suggest the presence of a secondary 13-C effect in the hydride transfer step. This phenomenon is also applicable to the modified enzyme with NAD as the substrate.

dinucleotides

NAD-malic enzyme

isotope effects

SCN-enzyme

Enzymes.

Ascaris suum.

Isotopes.

時差環境下における視交叉上核分子神経シグナルに関する研究

鈴木, 暢

23 March 2015

京都大学 / 0048 / 新制・課程博士 / 博士(薬科学) / 甲第18925号 / 薬科博第39号 / 新制||薬||5(附属図書館) / 31876 / 京都大学大学院薬学研究科医薬創成情報科学専攻 / (主査)教授 岡村 均, 教授 中山 和久, 教授 竹島 浩 / 学位規則第4条第1項該当 / Doctor of Pharmaceutical Sciences / Kyoto University / DFAM

概日時計

時計遺伝子

SCN

jet-lag

AVP

499.3