La subérine chez Arabidopsis thaliana : Mécanisme d'export et contribution des alcools gras / Export mecanisms and fatty alcohols importance in Arabidopsis thaliana suberin

Delude, Camille

15 December 2015

Chez les plantes, la subérine est un biopolymère constitué de composés aliphatiques etaromatiques déposés au niveau de la paroi des cellules de plusieurs tissus comme l’endodermeet le périderme des racines ou encore le manteau des graines. La subérine forme une barrièrehydrophobe permettant entre autres de contrôler les flux d’eau et de solutés, et de protéger laplante de stress environnementaux comme la sécheresse ou les pathogènes. Grâce à desanalyses en LC-MS/MS et en GC-MS, nous avons pu montrer que la majorité des alcools grasprésents dans la fraction soluble de racines d’Arabidopsis thaliana est sous forme d’alkylcaféates et d’alkyl coumarates. De plus, nous avons montré que ces cires associées aupolymère de subérine sont présentes dès les premiers stades du développement de la racine.Une étude de la distribution des chaînes acyles des racines nous a permis de mettre enévidence la contribution majeure des alcools gras dans la composition de la subérine ainsi quel’importance de la subérine dans le métabolisme lipidique des racines. Afin d’identifier desacteurs impliqués dans l’export des précurseurs de la subérine vers l’espace extracellulaire,nous avons mené une approche de génétique inverse en utilisant des lignées mutées pour desgènes codant notamment pour des ABCG transporteurs co-exprimés avec des gènes connuspour participer à la biosynthèse de la subérine. Les résultats de ces analyses ont confirmé quele processus d’export fait intervenir plusieurs protéines pouvant avoir des fonctionsredondantes et ont suggéré l’implication d’un nouveau transporteur dans l’export desprécurseurs de subérine. / In plants, suberin is a complex biopolymer made of aliphatic and aromatic compounds.It is deposited in the cell wall of tissues such as the endoderm and the periderm of roots or thecoat of the seeds. Suberin forms a hydrophobic barrier controlling the flow of water andsolutes, and protecting the plant from environmental stresses such as drought or pathogens.Through LC-MS/MS and GC-MS analyses, we have shown that the majority of the fattyalcohols present in the soluble fraction of Arabidopsis roots is in the form of alkyl caffeatesand alkyl coumarates. Such waxes, most probably associated with the suberin polymer, arealready detected at early stages of root development. A study of the distribution of all acylchains present in roots allowed us to highlight the major contribution of fatty alcohols in thecomposition of suberin and the importance of suberin in the global lipid metabolism of theroots. To identify proteins involved in the export of suberin precursors to the extracellularspace, we conducted a reverse genetic approach using lines mutated in genes coding forseveral ABCG transporters which were co-expressed with genes known to participate in thebiosynthesis of suberin. The results of these analyses confirmed that the export processinvolves several proteins that can have redundant functions, and supported the involvement ofa new transporter in the export of the suberin precursors.

Subérine

Arabidopsis

Racine

Alcools gras

Alkyl hydroxycinnamates

Cires

Transport

ABCG transporteurs

Suberin

Arabidopsis

Root

Fatty alcohols

Alkyl hydroxycinnamates

Wax

Transport

ABCG transporters

Etude structure/fonction du demi-transporteur ABCD2 dans le contexte de l'Adrénoleucodystrophie liée à l'X / Structure/function study of the ABCD2 half-transporter in the context of X-linked Adrenoleukodystrophy

Geillon, Flore

30 August 2013

L’Adrénoleucodystrophie liée à l’X est une maladie neurodégénérative rare due à des mutations dans le gène ABCD1. Ce gène code un demi-transporteur ABC peroxysomal, impliqué dans l’importation d’acides gras à très longue chaîne. Deux autres demi-transporteurs sont localisés dans la membrane peroxysomale : ABCD2 et ABCD3. La surexpression d’ABCD2 permet de compenser la déficience en ABCD1, ouvrant ainsi des perspectives thérapeutiques. Dans cette optique, l’objectif principal de ma thèse était d’étudier la fonction et la structure d’ABCD2, et plus largement des transporteurs ABC peroxysomaux.Les demi-transporteurs doivent au minimum se dimériser pour constituer un transporteur fonctionnel. Leur dimérisation alternative pourrait moduler leur spécificité de substrat. Afin de tester cette hypothèse, nous avons réalisé des constructions plasmidiques codant différents dimères chimériques, dont la fonctionnalité a été vérifiée par transfection transitoire dans deux modèles cellulaires (fibroblastes humains et levures). D’après nos résultats, ABCD1 et ABCD2 seraient fonctionnels quel que soit leur agencement dimérique. De plus, comme d’autres transporteurs ABC, les transporteurs ABC peroxysomaux pourraient s’oligomériser. En utilisant différentes techniques biochimiques (co-immunoprécipitation, sédimentation sur gradient de sucrose et électrophorèse en conditions natives), sur un modèle cellulaire surexprimant ABCD2-EGFP, nous démontrons qu’ABCD2-EGFP interagit avec ABCD1 et ABCD3, et que les transporteurs ABC peroxysomaux sont capables de s’oligomériser. Il reste désormais à déterminer les facteurs qui contrôlent cette oligomérisation et comprendre la valeur fonctionnelle de ces interactions. / X-linked Adrenoleukodystrophy (X-ALD) is a rare neurodegenerative disease caused by deficiency of the peroxisomal half-transporter ABCD1, implicated in very long chain fatty acids import. Two additional half-transporters are located in the peroxisomal membrane: ABCD2 and ABCD3. Over-expression of ABCD2 is known to compensate for ABCD1 deficiency, making ABCD2 a therapeutic target for X-ALD treatment. In this context, the main objective of my thesis was to investigate the function and the structure of ABCD2, and more broadly, of peroxisomal ABC transporters.Half-transporters must at least dimerize to form a functional transporter. Alternative dimerization could modulate substrate specificity. In order to test this hypothesis, we engineered plasmidic constructs encoding chimeric ABCD dimers, whose functionality has been evaluated by transient transfection in two cell models (human fibroblasts and yeasts). Our results show that, ABCD1 and ABCD2 are functional whatever their dimeric organization. Besides, like other ABC transporters, peroxisomal ABC transporters could oligomerize. By using a multi-technical approach (co-immunoprecipitation, velocity sucrose gradient and native polyacrylamide gel electrophoresis experiments) on stably transfected hepatoma cells expressing ABCD2-EGFP, we demonstrate that ABCD2-EGFP interacts with ABCD1 and ABCD3, and that peroxisomal ABC transporters oligomerize. The perspectives will consist in determining which factors control the oligomerization process and understanding the functional value of these interactions.

X-ALD

Transporteurs ABC

Peroxysome

Oligomérisation

Redondance fonctionnelle

Dimères ABC chimériques

X-ALD

ABC transporters

Peroxisome

Oligomerization

Functional redundancy

Chimeric ABC dimers

571.6

571.8

Analyse écophysiologique et génétique de l’absorption d’azote post-floraison chez le blé tendre (Triticum aestivum L.) en relation avec la concentration en protéines des grains / Ecophysiological and genetic analysis of post-flowering nitrogen uptake in bread wheat (Triticum aestivum L.) in relation with grain protein concentration

Taulemesse, François

16 June 2015

La concentration en protéines des grains est un critère qualitatif majeur qui conditionne la valeur économique et technologique du blé tendre (Triticum aestivum L.). Cependant, la forte relation négative existant entre concentration en protéines et rendement en grains implique que l’amélioration de la concentration en protéines par une approche génétique soit complexe à atteindre sans impacter négativement le rendement. Pour contourner cette difficulté, il a été proposé qu’une sélection variétale basée sur l’écart à cette relation négative (nommé Grain Protein Deviation ; GPD) permette d’améliorer la concentration en protéines indépendamment du rendement. Au niveau physiologique, le GPD est fortement corrélé à la capacité des génotypes à absorber de l’azote après floraison indépendamment de la quantité d’azote déjà absorbée à floraison, suggérant que la satiété en azote soit à la base de son établissement. Envisager une sélection sur la base du GPD nécessite cependant d’acquérir des connaissances approfondies des mécanismes impliqués dans la régulation de l’absorption d’azote par la satiété en azote, qui permettraient de cibler précisément des traits simples à quantifier et robustement associés à cette capacité accrue d’accumulation de protéines dans les grains.Cette étude se base sur deux expérimentations conduites en conditions contrôlées et une expérimentation au champ. Dans chacune de ces expérimentations, différents niveaux de fertilisation ont été appliqués en pré-floraison afin d’obtenir des statuts azotés contrastés à floraison. L’effet du statut azoté à floraison sur l’absorption post-floraison a ensuite été observé dans différentes conditions de disponibilités d’azote après floraison. Des mesures physiologiques et moléculaires ont été réalisées en parallèle des mesures d’absorption d’azote.Nous avons mis en évidence que l’absorption d’azote post-floraison présente une dynamique élaborée qui suppose qu’elle est soumise à des régulations complexes. Parmi celles-ci, le statut azoté des plantes à floraison conditionne en grande part la quantité d’azote absorbée dans les jours qui suivent la floraison (PANUprécoce , de floraison à floraison + 250 degrés-jour). La quantité de PANUprécoce se présente comme un déterminant fort de la concentration en protéines des grains du fait de la forte corrélation positive observée entre ces deux traits en conditions contrôlées et au champ, et ce indépendamment du niveau de rendement. L’étude de deux génotypes robustement contrastés pour le GPD a montré qu’à statuts azotés équivalents, la quantité de PANUprécoce est sujette à des effets génétiques qui tendent à confirmer l’impact de la variabilité génétique de satiété en azote sur l’établissement du GPD.Ces travaux ont permis de proposer des marqueurs du GPD potentiellement valorisables en sélection. Au niveau physiologique, la croissance des tiges après floraison se présente comme un marqueur prometteur du GPD car ce trait est fortement corrélé à la PANUprécoce. Au niveau moléculaire, la concentration en nitrates des racines, également soumise à des effets génétiques, est proposée comme marqueur potentiel du fait de son rôle probable dans la régulation expressionnelle des gènes impliqués dans l’absorption et l’assimilation d’azote. / Grain protein concentration is one of the major qualitative criteria of bread wheat (Triticum aestivum L.) economic and technological value. However, the negative relationship existing between protein concentration and grain yield implies that grain protein concentration improvement is complex to achieve without detrimental effect on grain yield. Breeding programs based on the deviation to this negative relationship (Grain protein deviation of GPD) have been proposed to be a suitable strategy to improve grain nitrogen concentration without detrimental effects on yield. At a physiological level, GPD is strongly correlated with genotypes aptitude to uptake nitrogen after flowering independently of the nitrogen amount already taken up before this stage, suggesting that satiety for nitrogen could be involved in its establishment. Breeding for GPD implies however a more detailed knowledge of the processes implied in nitrogen uptake regulation by nitrogen plant satiety. This would allow targeting traits both simple to measure and robustly associated with this increased capacity to accumulate proteins in grains.The present study is based on two experiments carried on under controlled conditions and a third led under field conditions. In all experiments, various levels of pre-flowering fertilization were applied in order to obtain contrasted plant nitrogen status at flowering. Nitrogen status effect on post-flowering nitrogen uptake was observed under various post-flowering N availability conditions. Physiological and molecular measurements were carried out in parallel with uptake measurements.We highlighted that post-flowering nitrogen uptake has an elaborate dynamic, suggesting the involvement of complex regulations. Among these, plant nitrogen status at flowering determines to a great extent the amount of nitrogen taken up during the days following flowering (early PANU, from flowering to flowering +250 °C.days-1). Early PANU appears to be a strong determinant of grain protein concentration, as strong positive correlations were observed between these two traits both under controlled conditions and field conditions, independently of grain yield level. The study of two genotypes strongly contrasted for GPD highlighted that, despite comparable N status, early PANU is subjected to strong genetic variations which tend to identify N satiety as a determinant of GPD.The present study identified robust markers of GPD of potential use in plant breeding. At a physiological level, post flowering stem elongation appears to be a promising marker of GPD since this trait is strongly correlated with early PANU. At a molecular level, root nitrate concentration, a trait submitted to genetic variations, is also proposed as a marker of GPD because of its role in the expression regulation of the genes governing nitrogen uptake and assimilation.

Absorption d’azote

Concentration en protéines

Nitrate

Satiété

Transporteurs racinaires

Triticum aestivum L.

Grain protein concentration

Nitrate

Nitrogen uptake

Satiety

Root transporters

Triticum aestivum L.

Self-organization of Saccharomyces cerevisiae colonies / Auto-organisation des colonies de Saccharomyces cerevisiae

Marinkovic, Zoran

30 November 2017

L’environnement naturel des levures est constitué d’une communauté de cellules. Les chercheurs, cependant, préfèrent étudier les levures dans des environnements plus simples et homogènes, comme des cultures en cellule unique ou en population, s’affranchissant ainsi de la complexité de la croissance spatiotemporelle, la différentiation, l’auto-organisation, ainsi que la façon dont ces caractéristiques sont formées et s’entrelacent à travers l’évolution et l’écologie. Nous avons mis en place un dispositif microfluidique multicouches permettant la croissance de colonie de levures dans des environnements dynamiques, spatialement structurés, contrôlés, partant d’une monocouche de levures à une colonie multicouches. La croissance des colonies, dans son ensemble comme à des positions spécifiques, est le résultat de la formation d’un gradient de nutriment au sein de celles-ci - gradient qui trouve son origine dans le différent taux de diffusion des nutriments, des taux d’absorption de ceux-ci par les cellules, ainsi que de leurs concentrations initiales. Lorsqu’un nutriment en quantité limitante (par exemple le glucose ou un acide aminé) est épuisé, à une distance spécifique de la source de nutriments, les cellules au sein de la colonie cessent de croitre. Nous avons été en mesure de moduler cette distance spécifique en variant la concentration initiale de nutriments ainsi que le taux d’absorption des cellules. Les motifs d’expression de gènes de la colonie nous ont donné des informations sur la formation de micro environnements spécifiques ainsi que sur le développement subséquent, la différentiation et l’auto-organisation. Nous avons quantifié les motifs d’expression de sept gènes de transport du glucose (HXT1-7), chacun exprimé spécifiquement suivant la concentration de glucose, ce qui nous a permis de reconstituer la formation de gradients de glucose au sein d’une colonie. En étudiant des gènes spécifiques de la fermentation et de la respiration, nous avons pu observer la différentiation en deux sous-populations. Nous avons de plus cartographié l’expression de gènes impliqués dans différentes parties du métabolisme des glucides, suivi et quantifié la dynamique spatio-temporelle de croissance et d’expression génétique et finalement modélisé la croissance de la colonie ainsi que la formation du gradient de nutriment. Pour la première fois, nous avons observé la croissance, la différentiation et l’auto-organisation des colonies de S. cerevisiae avec une résolution spatio-temporelle jusqu’à maintenant inégalée / The natural environment of yeast is often a community of cells but researchers prefer to study them in simpler homogeneous environments like single cell or bulk liquid cultures, losing insight into complex spatiotemporal growth, differentiation and self-organization and how those features are intertwined and shaped through evolution and ecology. I developed a multi-layered microfluidic device that allows us to grow yeast colonies in spatially controlled dynamically structured changing environments from a monolayer of single yeast cells to a multi-layered colony. Colony growth, as a whole and at specific locations, is a result of the nutrient gradient formation within a colony through interplay of nutrient diffusion rates, nutrient uptake rates by the cells and starting nutrient concentrations. Once a limiting nutrient (e.g. glucose or amino acids) is depleted at a specific distance from the nutrients source the cells within a colony stop to grow. I was able to modulate this specific distance by changing the starting nutrient concentrations and uptake rates of cells. Colony gene expression patterns gave us information on specific micro environments formation and consequential development, differentiation and self-organization. I quantified the patterns of expression of seven glucose transporter genes (HXT1-7), each of them specifically expressed depending on the glucose concentration. This enabled us to reconstruct glucose gradients formation in a colony. I further followed the expression of fermentation and respiration specific genes and observed differentiation between two subpopulations. We also mapped other genes specific for different parts of carbohydrate metabolism, followed and quantified the spatiotemporal dynamics of growth and gene expression, and finally modelled the colony growth and nutrient gradient formation. For the first time, we were able to observe growth, differentiation and self-organization of S. cerevisiae colony with such an unprecedented spatiotemporal resolution

Auto-organisation

Levure Saccharomyces cerevisiae

Différenciation

Croissance

Microfluidique

Biophysique

Transporteurs d'hexose

Écologie

Émergence

Métabolisme

Self-organisation

Yeast Saccharomyces cerevisiae

Differentiation

Growth

Microfluidics

Biophysics

Hexose transporters

Ecology

Emergence

Metabolism

Surface diffusion of the astrocytic glutamate transporter glt-1 shapes synaptic transmission / Traffic membranaire des transporteurs du glutamate astrocytaires GLT-1

Murphy-Royal, Ciaran

06 June 2014

Le glutamate est le principal neurotransmetteur excitateur du système nerveux central des vertébrés, et le codage de l’information cérébrale repose en partie sur des modulations de l’amplitude et de la fréquence des transmissions synaptiques glutamatergiques. De ce fait, la résolution spatiale et temporelle de ces transmissions nécessite un contrôle fin de la présence de glutamate dans la fente synaptique. Cette durée de vie du glutamate dans les synapses dépend directement de l’action de transporteurs spécifiques exprimés à la surface des astrocytes, en particulier les transporteurs de type GLT-1, qui retirent le neurotransmetteur et permettent ainsi de « nettoyer » la fente synaptique avant la survenue d’un nouvel épisode de neurotransmission. / A classic understanding of neurotransmitter clearance at glutamatergic synapses is that, in order to ensure sufficient glutamate uptake on a fast timescale, it is necessary to have high numbers of glutamate transporters in the vicinity of release sites to compensate for their slow transport kinetics. Using a combination of single molecule imaging and electrophysiological approaches, we now challenge this view by first demonstrating that GLT-1 transporters are not static but highly mobile at the surface of astrocytes, and that their surface diffusion is dependent upon both neuronal and glial cell activities. In the vicinity of glutamate synapses, GLT-1 dynamics are strongly reduced favoring their retention within this strategic location. Remarkably, glutamate uncaging at synaptic sites instantaneously increases GLT-1 diffusion, displacing the glutamate-bound transporter away from this compartment. Functionally, impairment of the transporter lateral diffusion through an antibody-based surface cross linking, both in vitro and in vivo, significantly slows the kinetics of excitatory postsynaptic currents. Taken together, these data reveal the unexpected and major role of the astrocytic surface GLT-1 fast dynamics in shaping glutamatergic synaptic transmission.Keywords:

Transporteurs du glutamate

Recapture du glutamate

Diffusion de surface

Imagerie de nanoparticules unique

Synapse tripartite

Interactions neurone-glie

Glutamate transporters

Glutamate uptake

Lateral diffusion

Single nanoparticle imaging

Tripartite synapse

Neuron-glia interactions

Mechanismy rezistence a metabolismus železa u nádorových kmenových buněk / Mechanisms of resistance and iron metabolism in cancer stem cells

Lettlová, Sandra

January 2019

(EN) Analogously to normal stem cells within the tissues, cancer stem cells (CSCs) have been proposed to be responsible for maintenance and growth of tumours. CSCs represent a small fraction of cells within the tumour, which is characterised by self-renewal capacity and ability to give rise to a tumour when grafted into immunocompromised mice. Cells with increased stemness properties are believed to be responsible for tumour resistance, metastases formation and relapse after tumour treatment. The first part of this work concentrates on resistance of the tumours, which is often associated with increased expression of ATP-binding cassete (ABC) transporters pumping chemotherapeutics out of the cells. For the purposes of this study, we utilized an in vitro model of CSCs, based on cultivation of cells as 3D "spheres". Expression profiling demonstrates that our model of CSCs derived from breast and prostate cancer cell lines express higher mRNA level of ABC transporters, particularly ABCA1, ABCA3, ABCA5, ABCA12, ABCA13, ABCB7, ABCB9, ABCB10, ABCC1, ABCC2, ABCC3, ABCC5, ABCC8, ABCC10, ABCC11 and ABCG2 among the cell lines tested. The protein level of ABC transporters tested in breast CSCs showed higher expression of ABCB8, ABCC1, ABCC2, ABCC10 and ABCG2 but downregulation of ABCB10 and ABCF2 proteins....

Astrocytic regulation of seizure-like behavior

Cho, Sukhee

14 December 2017

Astrocytes are emerging as important regulators of neural circuit function and behavior in the healthy and diseased nervous system. In a screen for astrocyte molecules that modulate neuronal hyperexcitability we identified multiple components of focal adhesion complexes (FAs) as potent suppressors of genetically- or pharmacologically-induced seizure-like activity. Depletion of astrocytic Tensin, b-integrin, Talin, Focal adhesion kinase (FAK), or matrix metalloproteinase 1 (Mmp1), which degrades extracellular matrix to activate b-integrin receptors, resulted in enhanced recovery from, or resistance to seizure activity. Reciprocally, promoting FA signaling by overexpression of Mmp1 in astrocytes led to enhanced-seizure severity. Blockade of FA signaling in astrocytes led to reduced-astrocytic coverage of the synaptic neuropil and reduced expression of the excitatory amino acid transporter EAAT1. However, upon seizure induction, depletion of FA signaling components resulted in enhanced astrocyte coverage of the synaptic neuropil and a ~2-fold increase in EAAT1 levels compared to controls. Our data indicate that FAs promote astrocyte coverage in neuropil and EAAT1 expression under normal physiological conditions, but in the context of hyperexcitability, FAs negatively regulate the extent of astrocytic processes within neuropil and EAAT1 expression, thereby inhibiting a more rapid recovery from conditions of excessive neuronal activity.

astrocyte

morphology

electron microscopy

Drosophila

genetics

seizure

focal adhesions

tensin

integrin

glutamate transporters

Life Sciences

Medicine and Health Sciences

Molecular and Cellular Neuroscience

Growth Hormone Receptor in Melanoma: A Unique Approach to Therapy

Basu, Reetobrata

21 September 2016

No description available.

Molecular Biology

Endocrinology

Oncology

Biology

Biochemistry

melanoma

growth hormone

growth hormone receptor

drug resistance

GH

GHR

cancer

drug resistance

melanogenesis

MITF

EMT

ABC transporters

RNAi

chemotherapy

Studium regulace genové exprese nukleosidových transportérů v buněčné linii BeWo / Study of gene regulation of nucleoside transporters in BeWo cell line

Strachoňová, Šárka

January 2019

Charles University in Prague Faculty of Pharmacy in Hradec Králové Department of Pharmacology & Toxicology Student: Šárka Strachoňová Supervisor: PharmDr. Lukáš Červený, Ph.D. Title of diploma thesis: Studium of gene regulation of nucleoside transporters in BeWo cell line Nucleoside transporters (NTs) localized in syncytiotrophoblast control placental uptake of nucleosides. Dysregulation of NTs can disrupt nucleoside homeostasis with a negative consequences on placental and fetal development and can lead to a change in placental pharmacokinetics of nucleoside-derived drugs. Therefore, understanding the expression and function of NTs is necessary for effective and safe pharmacotherapy during pregnancy. The aim of this diploma thesis was to study the adenylate cyclase (AC) activated regulatory pathways of gene expression of concentrative nukleoside transporter 2 (CNT2). For this purpose, qRT-PCR and in vitro accumulation assays using the model substrate [3 H]-adenosine were employed. The human placental choriocarcinoma-derived BeWo cell line has been exposed to an AC activator, forskolin (50 µM), and/or inhibitors of AC/cAMP/PKA, AC/cAMP/MAPK (MEK1/2, p38 MAPK) signaling pathways, PKA inhibitor, KT 5720 (5 μM), an inhibitor of MEK1/2, U0126 (10 μM) and an inhibitor of p38 MAPK, SB202190 (10 μM). The...

JAK/STAT signalling in the induction of the L-arginine-nitric oxide pathway in macrophages and vascular smooth muscle cells

Garr, Edmund Dzigbordi

January 2014

The production of Nitric Oxide (NO) under physiological conditions has beneficial roles in acting as a key signaling component of many biological processes as well as having an anti-microbial effect. However its effects following excess production by the inducible NO pathway is potentially detrimental in the pathogenesis of chronic inflammation including sepsis and several other inflammatory diseases. Understanding the mechanisms that regulate the expression of the inducible nitric oxide synthase (iNOS) responsible for producing the excessive amounts of NO in disease states is therefore critical. In this regards, experiments were carried out to identify the signaling pathways that may mediate this process, focusing specifically on the JAK/STAT cascade. The reason for selecting the latter is because our research group, amongst others, has carried out extensive work investigating other signaling pathways, including the mitogen activated kinases (MAPK). Moreover, studies have also been carried out in an attempt to identify the critical role of JAK/STAT signaling for iNOS induction. These studies however failed to conclusively demonstrate whether, as with the MAPKs, the JAK/STATs may also play an essential role. Furthermore there is indeed controversy in the literature with researchers unable to agree whether expression of iNOS does require JAK/STAT activation. Thus, the aim of the project described in this thesis was to establish unequivocally whether activation of the JAK/STATs preceeds induction of iNOS. The studies were extended to L-arginine transport as well because the latter is widely reported to be induced in parallel with iNOS and substrate supply to iNOS may be critical for sustained NO production. Changes in transporter activity as well as their expression profiles were assessed. All experiments were carried out in either rat aortic smooth muscle cells (RASMCs) or in the J774 macrophage cell line. These cell types were selected because RASMCs are one of the prime targets for induced NO production in vascular inflammation and the macrophages are involved in host defence, acting in part through NO production. To establish the role of JAK/STATs, pharmacological and molecular approaches were used. Pharmacologically, two inhibitors were used and these were AG490 and JAK inhibitor I. The former is reported to be a selective JAK2 inhibitor and the other blocks all known JAK proteins. The potential of the GTPases to regulate the induction of iNOS was also examined using selective inhibitor known to regulate these proteins. In addition to these drugs, siRNA targeting JAK2 was also exploited and western blotting was extensively used to detect expression of various proteins including iNOS, native and phosphorylated JAK2 and TYK2. Changes in iNOS activity was monitored by determining nitrite production using the Griess assay and L-arginine transport was monitored using tritiated arginine (L-[3H]arginine). RASMCs were treated with a combination of LPS (100 µg/ml) and IFN- (100 U/ml) and the macrophages with LPS (1 µg/ml) to induce iNOS and transporter activity. Consistent with previous reports, the above treatment of both cell types resulted in the expression of iNOS, production of NO and enhanced transport of L-arginine. These effects were not affected by AG490 but blocked by JAK inhibitor I. Furthermore, although both cell types expressed the key JAKs (JAK2 and TYK2), neither of these proteins were phosphorylated under conditions of induced NO production. Moreover, siRNA experiments showed that JAK2 expression could be abolished without any significant change in NO production, confirming that at least JAK2 may not be required for this process. Whether TYK2 is involved still remains to be resolved as the phosphor-protein could not be detected. However the conclusive siRNA knockdown studies could not be carried out due to time and cost constraints. Apart from iNOS and NO production, changes in induced L-arginine transport were also not significantly affected under the experimental conditions described above suggesting that like with iNOS, induction of L-arginine transport is independent of at least JAK2. Interestingly however, STAT-1 was phosphorylated and this was blocked by JAK inhibitor I but not AG490. Thus, STAT-1 activation may be essential but its activation may be independent of the JAKs. One possible alternate upstream activator of STAT-1 may be the GTPases. Indeed these proteins have been indicated to phosphorylate STAT-1 independent of the JAKs. However, in this project, inhibition of the GTPase pathway enhanced NO production and L-arginine transport suggesting that the GTPases downregulate these processes. In conclusion, the studies carried out in this thesis have shown that induction of iNOS, NO production and L-arginine transport in both RASMCs and J774 macrophages are independent of JAK2 but require STAT-1 activation which may be phosphorylated independently of the JAKs. The role of other JAKs such as TYK2 although unlikely, will need to be resolved using a more specific approach such as siRNA.

616.07