Function and regulation of the scaffold protein IB1/JIP-1 in the uro-genital tract.

RESUME Ce mémoire de thèse traite de l'étude de la « scaffold »protéine ou protéine «échafaud», « Islet-Brain1/ JNK Interacting Protein 1 » (IB1/JIP-1) dans la vessie et la prostate, deux organes importants de l'appareil uro-genital. Cette protéine, mise en évidence dans notre laboratoire à la fin des année 90, a été reconnue pour réguler la voie de signalisation des « Mitogen-Activated Protein Kinases » (MAPKs), et en particulier de la MAPK appelée c-Jun N-terminal Kinase (JNK). Le réseau de voie de signalisation permet aux cellules de percevoir les changements dans le milieu extracellulaire et de permettre une réponse appropriée à ces différents stimuli. La connaissance des voies de signalisation a permis de mettre en évidence leur rôle crucial tant dans l'homéostase des tissus sains que dans des processus pathologiques comme l'oncogenèse. Parmi une vingtaine de voie de signalisation, la voie de signalisation des «MAPKinases » est une des plus importantes et a été montrée pour participer à diverses fonctions cellulaires telles que la différentiation, la motilité, la division et la mort cellulaire. La voie de signalisation des « MAPKinases » est typiquement constituée d'un module de trois kinases qui s'activent séquentiellement par phosphorylation. On note la présence d'une MAPK, d'un activateur de MAPK et d'un activateur de l'activateur de MAPK. Une fois la MAPK activée, elle permettra la régulation de différentes cibles dont certain facteur de transcription. Chez les mammifères, il existe 3 grands groupes de MAPKs : the extracellular signal-regulated kinase 1 and 2 (ERK 1/2) cascade, qui régule préférentiellement la croissance et la différentiation cellulaire, ainsi que les cascades JNK et p38 qui régulent préférentiellement la réponse à différents stress cellulaires telle que l'inflammation ou l'apoptose. JNK est activé par différents stress cellulaire telle que les cytokines inflammatoires. JNK est également requis au cours du développement embryonnaire et contribue à la mort (apoptose) ou à la prolifération cellulaire. Plusieurs études ont mis en évidence le rôle de JNK durant le processus tumoral, sans que son rôle soit clairement identifié. JNK pourrait avoir des fonctions différentes durant l'initiation puis de la progression tumorale. Chez les mammifères, les voies de signalisation intracellulaires forment un réseau complexe et elles interagissent entre elles, ce qui permet aux cellules une réponse adéquate aux multitudes de stimuli existants dans les organismes pluricellulaires. Parmi plusieurs mécanismes de régulation, les protéines dites « scaffold » ou «échafaud » jouent un rôle crucial dans l'homéostase de la voie de signalisation des «MAPKinase ». L'introduction revoit brièvement ces différents aspects, de la voie de signalisation des «MAPKinase et des connaissance sur IB1/JIP-1. Les premières études effectuées sur IB1/JIP-1 ont montré une expression relativement spécifique de cette protéine dans certains types de neurones ainsi que dans la cellule beta-sécrétrice d'insuline. IB1/JIP-1 régule la voie de signalisation JNK par interaction avec les différents composants du module, modifiant ainsi le spectre de substrats activés par JNK. La fonction précise de IB1/JIP-1 n'était pas encore élucidée, mais plusieurs travaux mettaient en lumière un rôle dans la régulation, et la sous-location cellulaire des composants de la voie de signalisation JNK, ainsi que dans la survie cellulaire à certain stress. Cette expression relativement spécifique est intrigante car elle suggère que sa présence serait nécessaire à une régulation spécifique de la MAPKinase JNK ou à certaines autres fonctions cellulaires également spécifiques de certains tissus. Le premier but de ce travail a consisté à mettre en évidence l'expression de IB1/JIP-1 dans l'appareil uro-génital et plus particulièrement dans la vessie et la prostate. Nos résultats ont montré que IB1/JIP-1 est spécifiquement exprimé au niveau de l'urothélium vésical, mais pas dans le muscle lisse. Il en est de même au niveau de la prostate où IB1/JIP-1 est exprimé spécifiquement au niveau de l'épithélium sécrétoire et absent au niveau du stroma fibro-musculaire. La vessie et la prostate sont des organes ou l'activité JNK pourrait être crucial tant dans l' homeostase tissulaire que dans le développement de pathologies bénignes ou malignes. La vessie et la prostate sont le siège fréquent de tumeur. La base pour le développement du cancer est complexe et implique plusieurs anomalies génétiques. Ce processus complexe lié au développement tumoral est encore loin d`être complètement élucidé, raison pour laquelle il est crucial de poursuivre l'étude des différents gènes pouvant être impliqué dans ces processus ou pouvant être utilisé comme outil thérapeutique. Dans l'urothelium de la vessie, la fonction de la MAPK JNK n'a été que très peu étudiée. Il existe quelques études, in vitro, suggérant une implication possible de cette voie de signalisation dans des processus telle que le développement ou la progression tumorale. Le chapitre 1 décrit une étude in vivo dans la vessie un modèle de stress mécanique, connu pour activer les MAPKinase. La dilatation vésicale, due à une obstruction urétrale, a mis en évidence une diminution de l'expression de IB1/JIP-1 ainsi qu'une activation de la MAPKinase JNK. Dans ce modèle, la régulation de IB1/JIP-1, par l'intermédiaire d'un vecteur viral, a permis de démontrer que IB1/JIP-1 régulait l'activité de JNK dans ce tissu. Pour poursuivre l'étude de cette fonction d' IB1/JIP-1 dans l'urothélium, nous avons investigué l'activité JNK dans des souris génétiquement modifiées et porteuse d'une délétion de 1 des 2 allèles du gène codant pour IB1/JIP-1, avec un contenu en IB1/JIP-1 diminué de moitié. L'activation de JNK est également augmentée dans l'urothelium au repos de ces souris, ce qui confirme la fonction régulatrice de JNK par IB1/JIP-1. Ces résultats ont permis de mettre en évidence un rôle critique de celle-ci dans l'homéostase de I`urothelium et suggère une nouvelle cible pour réguler la voie de signalisation dans ce tissu. En outre, la modulation des niveaux d'expression d'IB1/JIP-1 dans la vessie, in vivo, par l'intermédiaire de vecteurs viraux s'est révélée réalisable et indique un moyen élégant pour développer une thérapie génique dans cet organe. Un autre élément de ce travail de thèse, révélée au chapitre 2, a été d'étudier la régulation dans la vessie de rat de la communication intercellulaire de type « GAP ». Les cellules adjacentes partagent des ions, messagers secondaires et des petits métabolites par l'intermédiaire de canaux intercellulaire qui forment les jonctions de type « GAP ». Ce type de communications intercellulaire permet une activité cellulaire coordonnée, une caractéristique importante pour l'homéostase des organismes multicellulaire. Ce type de communication intercellulaire est formé de 2 demi-canaux appelés connexons. Chaque connexon est formé de six protéines appelées connexins (Cx). Il existe environ vingt connexines différentes nommées par leur poids moléculaire respectif. Les jonctions de type canaux "GAP" permettent aux cellules de communiquer avec les cellules voisines au quelles elles sont mécaniquement ou électriquement couplées. La vessie peut être particulièrement dépendante de la communication intercellulaire par les canaux « Gap » qui permettrait de coordonner la réponse de la musculature ainsi que de l'urothélium à l'augmentation de la pression transmurale du à l'accumulation d'urine, situation fréquemment observée dans le cadre de l'hyperplasie bénigne de la prostate. Dans la vessie de rat, la connexine26 est exprimée uniquement dans l'urothelium. La Cx26, a été montrée pour être un possible « tumor suppressor gene » dans le cancer de vessie. Une augmentation de la Cx26 ainsi que du couplage des cellules urothéliales a été démontré dans notre modèle de stress mécanique sur la vessie de rat et est dépendante de 2 éléments de réponses connues pour interagir avec AP-1. La régulation de IB1/JIP-1 a permis de montrer que celle-ci régulait l'activité JNK, ainsi que l'activité du facteur de transcription AP-1, composé de c-Jun lui-même cible de JNK. Cette réduction de l'activité de AP-1 est associée à une diminution de l'expression du transcipt de la Cx26. En résumé, la Cx26 pourrait être régulée par le complexe AP-1 lui-même dépendant du contenu en IB1/JIP-1. Dans le chapitre 3, l'étude de IB1/J1P-1 s'est portée sur la prostate. Cet organe, siège fréquent de pathologie telle que le cancer ou l'hyperplasie bénigne de la prostate, exprime IB1/JIP-1 au niveau de son épithélium sécrétoire. Cette expression est maintenue dans une lignée cellulaire humaine largement étudiée est reconnue comme un modèle adéquat de cellules tumorales de type androgène-sensible. IB1/JIP-1 a été investigué dans un modèle in vitro d'apoptose en réponse à un agent appelé N-(4-hydroxyphenyl)retinamide (4-HPR) qui induit une activation de la MAPK JNK ainsi que également un diminution du contenu en IB1/JIP-1. La surexpression de IB1/JIP-1 en utilisant à nouveau des virus comme vecteur a démontré que IB1/JIP-1 était capable de réguler l'activité de JNK ainsi que les taux d'apoptose. Dans le cancer de la prostate, certains travaux ont montré que la différentiation neuroendocrine des cellules tumorales est associée à la progression tumorale et à la perte de sensibilité aux androgènes. Ce travail a permis de dévoiler l'augmentation d'expression de IB1/JIP-1 dans un modèle de neurodifferentiation des cellules d'une lignée prostatique humaine (LNCaP). Les mécanismes qui permettent une expression spécifique de IB1/JIP-1 ont été partiellement investiguée dans notre laboratoire. Son promoteur humain contient un « Neuron Restricive Silencer Element » (NRSE) connu pour se lier a répresseur transcriptionel appelé « RE-1 Silencer Transcription Factor » ou « Neuron Restrictive Silencer Factor » (REST/NRSF). NRSF/REST est capable de réprimer l'expression de gènes neuronaux en dehors du système neuronal. Il prend part à la différentiation terminale des gènes neuronaux. Dans le chapitre 3, on observe que l'activité de REST/NRSF est diminuée dans les cellules LNCaP qui se transdifferencient de manière neuroendocrine, et que REST/NRSF est capable de moduler l'expression de ces gènes cibles dans ce type cellulaire. Ces travaux laissent suggérer que NRSF/REST participe à l'acquisition du phénotype neuroendocrinien et pourrait être une cible pour réguler ce phénomène. En conclusion, ce travail de thèse présente l'expression de IB1/JIP-1 dans 2 organes de l'appareil uro-génital ; la vessie et la prostate. La fonction de IB1/JIP-1 a été étudiée in vivo dans la vessie de rat, ce qui a mis en évidence sa fonction régulatrice de l'activité de la MAPKinase JNK, et de l'activité du facteur de transcription AP-1 ; ainsi que sa possible implication régulatrice de gène cible tel que la Connexin 26 (Cx26). AP-1 et la Cx26 pourraient jouer un rôle dans le processus oncologique, tant dans le control de l'invasion cellulaire ou le control de la croissance cellulaire. Dans la prostate, IB1/JIP-1 régule également l'activité JNK; crucial dans la transmission de certains stimulis pro-apoptotiques. Dans un modèle de transdifférenciation neuroendocrinienne, phénotype possiblement lié au caractère agressif du cancer de la prostate, l'expression de IB1/JIP-1 est augmenté, suggérant soit un rôle possible dans le développement du phénotype neuronal ou une implication dans une fonction anti-apoptotique. Ce travail a donc permis d'élargir nos connaissances sur la régulation et le control de la voie de signalisation des MAPKinases par IB1/JIP-1, qui pourrait avoir encore d'autres fonctions dans ces tissus.

The scaffold protein IB1/JIP-1 is a critical mediator of cytokine-induced apoptosis in pancreatic beta cells.

In insulin-secreting cells, cytokines activate the c-Jun N-terminal kinase (JNK), which contributes to a cell signaling towards apoptosis. The JNK activation requires the presence of the murine scaffold protein JNK-interacting protein 1 (JIP-1) or human Islet-brain 1(IB1), which organizes MLK3, MKK7 and JNK for proper signaling specificity. Here, we used adenovirus-mediated gene transfer to modulate IB1/JIP-1 cellular content in order to investigate the contribution of IB1/JIP-1 to beta-cell survival. Exposure of the insulin-producing cell line INS-1 or isolated rat pancreatic islets to cytokines (interferon-gamma, tumor necrosis factor-alpha and interleukin-1beta) induced a marked reduction of IB1/JIP-1 content and a concomitant increase in JNK activity and apoptosis rate. This JNK-induced pro-apoptotic program was prevented in INS-1 cells by overproducing IB1/JIP-1 and this effect was associated with inhibition of caspase-3 cleavage. Conversely, reducing IB1/JIP-1 content in INS-1 cells and isolated pancreatic islets induced a robust increase in basal and cytokine-stimulated apoptosis. In heterozygous mice carrying a selective disruption of the IB1/JIP-1 gene, the reduction in IB1/JIP-1 content in happloinsufficient isolated pancreatic islets was associated with an increased JNK activity and basal apoptosis. These data demonstrate that modulation of the IB1-JIP-1 content in beta cells is a crucial regulator of JNK signaling pathway and of cytokine-induced apoptosis.

Immune cell impact of three differently coated lipid nanocapsules: pluronic, chitosan and polyethylene glycol.

Lipid nanocapsules (NCs) represent promising tools in clinical practice for diagnosis and therapy applications. However, the NC appropriate functionalization is essential to guarantee high biocompatibility and molecule loading ability. In any medical application, the immune system-impact of differently functionalized NCs still remains to be fully understood. A comprehensive study on the action exerted on human peripheral blood mononuclear cells (PBMCs) and major immune subpopulations by three different NC coatings: pluronic, chitosan and polyethylene glycol-polylactic acid (PEG) is reported. After a deep particle characterization, the uptake was assessed by flow-cytometry and confocal microscopy, focusing then on apoptosis, necrosis and proliferation impact in T cells and monocytes. Cell functionality by cell diameter variations, different activation marker analysis and cytokine assays were performed. We demonstrated that the NCs impact on the immune cell response is strongly correlated to their coating. Pluronic-NCs were able to induce immunomodulation of innate immunity inducing monocyte activations. Immunomodulation was observed in monocytes and T lymphocytes treated with Chitosan-NCs. Conversely, PEG-NCs were completely inert. These findings are of particular value towards a pre-selection of specific NC coatings depending on biomedical purposes for pre-clinical investigations; i.e. the immune-specific action of particular NC coating can be excellent for immunotherapy applications.

The scaffold protein IB1/JIP-1 controls the activation of JNK in rat stressed urothelium.

The c-Jun N-terminal kinase (JNK) is critical for cell survival, differentiation, apoptosis and tumorigenesis. This signalling pathway requires the presence of the scaffold protein Islet-Brain1/c-Jun N-terminal kinase interacting protein-1 (IB1/JIP-1). Immunolabeling and in situ hybridisation of bladder sections showed that IB1/JIP-1 is expressed in urothelial cells. The functional role of IB1/JIP-1 in the urothelium was therefore studied in vivo in a model of complete rat bladder outlet obstruction. This parietal stress, which is due to urine retention, reduced the content of IB1/JIP-1 in urothelial cells and consequently induced a drastic increase in JNK activity and AP-1 binding activity. Using a viral gene transfer approach, the stress-induced activation of JNK was prevented by overexpressing IB1/JIP-1. Conversely, the JNK activity was increased in urothelial cells where the IB1/JIP-1 content was experimentally reduced using an antisense RNA strategy. Furthermore, JNK activation was found to be increased in non-stressed urothelial cells of heterozygous mice carrying a selective disruption of the IB1/JIP-1 gene. These data established that mechanical stress in urothelial cells in vivo induces a robust JNK activation as a consequence of regulated expression of the scaffold protein IB1/JIP-1. This result highlights a critical role for that scaffold protein in the homeostasis of the urothelium and unravels a new potential target to regulate the JNK pathway in this tissue.

Chitosan-based nanogels for selective delivery of photosensitizers to macrophages and improved retention in and therapy of articular joints.

Macrophages play key roles in inflammatory disorders. Therefore, they are targets of treatments aiming at their local destruction in inflammation sites. However, injection of low molecular mass therapeutics, including photosensitizers, in inflamed joints results in their rapid efflux out of the joints, and poor therapeutic index. To improve selective uptake and increase retention of therapeutics in inflamed tissues, hydrophilic nanogels based on chitosan, of which surface was decorated with hyaluronate and which were loaded with one of three different anionic photosensitizers were developed. Optimal uptake of these functionalized nanogels by murine RAW 264.7 or human THP-1 macrophages as models was achieved after <4h incubation, whereas only negligible uptake by murine fibroblasts used as control cells was observed. The uptake by cells and the intracellular localization of the photosensitizers, of the fluorescein-tagged chitosan and of the rhodamine-tagged hyaluronate were confirmed by fluorescence microscopy. Photodynamic experiments revealed good cell photocytotoxicity of the photosensitizers entrapped in the nanogels. In a mouse model of rheumatoid arthritis, injection of free photosensitizers resulted in their rapid clearance from the joints, while nanogel-encapsulated photosensitizers were retained in the inflamed joints over a longer period of time. The photodynamic treatment of the inflamed joints resulted in a reduction of inflammation comparable to a standard corticoid treatment. Thus, hyaluronate-chitosan nanogels encapsulating therapeutic agents are promising materials for the targeted delivery to macrophages and long-term retention of therapeutics in leaky inflamed articular joints.

In vivo loading increases mechanical properties of scaffold by affecting bone formation and bone resorption rates.

A successful bone tissue engineering strategy entails producing bone-scaffold constructs with adequate mechanical properties. Apart from the mechanical properties of the scaffold itself, the forming bone inside the scaffold also adds to the strength of the construct. In this study, we investigated the role of in vivo cyclic loading on mechanical properties of a bone scaffold. We implanted PLA/β-TCP scaffolds in the distal femur of six rats, applied external cyclic loading on the right leg, and kept the left leg as a control. We monitored bone formation at 7 time points over 35 weeks using time-lapsed micro-computed tomography (CT) imaging. The images were then used to construct micro-finite element models of bone-scaffold constructs, with which we estimated the stiffness for each sample at all time points. We found that loading increased the stiffness by 60% at 35 weeks. The increase of stiffness was correlated to an increase in bone volume fraction of 18% in the loaded scaffold compared to control scaffold. These changes in volume fraction and related stiffness in the bone scaffold are regulated by two independent processes, bone formation and bone resorption. Using time-lapsed micro-CT imaging and a newly-developed longitudinal image registration technique, we observed that mechanical stimulation increases the bone formation rate during 4-10 weeks, and decreases the bone resorption rate during 9-18 weeks post-operatively. For the first time, we report that in vivo cyclic loading increases mechanical properties of the scaffold by increasing the bone formation rate and decreasing the bone resorption rate.

Controlled nerve growth factor release from multi-ply alginate/chitosan-based nerve conduits.

The delivery kinetics of growth factors has been suggested to play an important role in the regeneration of peripheral nerves following axotomy. In this context, we designed a nerve conduit (NC) with adjustable release kinetics of nerve growth factor (NGF). A multi-ply system was designed where NC consisting of a polyelectrolyte alginate/chitosan complex was coated with layers of poly(lactide-co-glycolide) (PLGA) to control the release of embedded NGF. Prior to assessing the in vitro NGF release from NC, various release test media, with and without stabilizers for NGF, were evaluated to ensure adequate quantification of NGF by ELISA. Citrate (pH 5.0) and acetate (pH 5.5) buffered saline solutions containing 0.05% Tween 20 yielded the most reliable results for ELISA active NGF. The in vitro release experiments revealed that the best results in terms of reproducibility and release control were achieved when the NGF was embedded between two PLGA layers and the ends of the NC tightly sealed by the PLGA coatings. The release kinetics could be efficiently adjusted by accommodating NGF at different radial locations within the NC. A sustained release of bioactive NGF in the low nanogram per day range was obtained for at least 15days. In conclusion, the developed multi-ply NGF loaded NC is considered a suitable candidate for future implantation studies to gain insight into the relationship between local growth factor availability and nerve regeneration.

Crystallization and preliminary crystallographic characterization of an SH3 domain from the IB1 scaffold protein.

IB1 is a mammalian scaffold protein that interacts with components of the c-Jun N-terminal kinase (JNK) signal-transduction pathway mainly via its protein-protein interaction domains. Crystallization of the key Src homology 3 (SH3) domain of IB1 has been achieved. Crystallization experiments with unmodified protein and deliberately oxidized protein have led to different crystal forms. X-ray data have been collected to 3.0 A resolution from a crystal form with rectangular prism morphology. These crystals are orthorhombic (P2(1)2(1)2(1)), with unit-cell parameters a = 45.9, b = 57.0, c = 145.5 A. These are the first crystallographic data on a scaffold molecule such as IB1 to be reported.

A collagen-poly(lactic acid-co-ɛ-caprolactone) hybrid scaffold for bladder tissue regeneration.

Scaffold materials should favor cell attachment and proliferation, and provide designable 3D structures with appropriate mechanical strength. Collagen matrices have proven to be beneficial scaffolds for tissue regeneration. However, apart from small intestinal submucosa, they offer a limited mechanical strength even if crosslinking can enhance their mechanical properties. A more cell-friendly way to increase material strength is to combine synthetic polymer meshes with plastic compressed collagen gels. This work describes the potential of plastic compressed collagen-poly(lactic acid-co-ɛ-caprolactone) (PLAC) hybrids as scaffolds for bladder tissue regeneration. Human bladder smooth muscle and urothelial cells were cultured on and inside collagen-PLAC hybrids in vitro. Scaffolds were analyzed by electron microscopy, histology, immunohistochemistry, and AlamarBlue assay. Both cell types proliferated in and on the hybrid, forming dense cell layers on top after two weeks. Furthermore, hybrids were implanted subcutaneously in the backs of nude mice. Host cell infiltration, scaffold degradation, and the presence of the seeded bladder cells were analyzed. Hybrids showed a lower inflammatory reaction in vivo than PLAC meshes alone, and first signs of polymer degradation were visible at six months. Collagen-PLAC hybrids have potential for bladder tissue regeneration, as they show efficient cell seeding, proliferation, and good mechanical properties.

Connexin26 is regulated in rat urothelium by the scaffold protein IB1/JIP-1.

Proper function of the wall of bladder requires gap junctional communication for coordinating the responses of smooth muscle (SMC) and urothelial cells exposed to urine pressure. In the rat bladder, Cx43 is expressed by SMC and urothelial cells, whereas Cx26 expression is restricted to the epithelium. We used a model of bladder outlet obstruction, in which a ligature is placed around the urethra to increase voiding pressure. Increased fluid pressure was associated with increased Cx43 and Cx26 mRNA expression and with the activation of a signaling cascade including the transcription factor c-Jun, which is a component of the AP-1 complex. The signaling pathway of the c-Jun NH2 terminal kinase (JNK) requires the presence of the scaffold protein Islet-Brain1/c-Jun amino-terminal kinase Interacting Protein-1 (IB1/JIP-1). Under stress conditions resulting from urine retention, we have found a reduced content of IB1/JIP-1 in urothelial cells, which in turn induced a drastic increase of JNK and AP-1 binding activities. The stress-induced activation of JNK was prevented by overexpressing IB1/JIP-1, using a viral gene transfer approach, a condition which also resulted in a decrease in Cx26 mRNA. The data show that: 1) mechanical stress of urothelial cells activates in vivo JNK, as a consequence of a regulated expression of IB1/JIP-1 and 2) that urothelial Cx26 may be directly regulated by the AP-1 complex.

Nuclear scaffold proteins are differently sensitive to stabilizing treatment by heat or Cu++.

The distribution of three nuclear scaffold proteins (of which one is a component of a particular class of nuclear bodies) has been studied in intact K562 human erythroleukemia cells, isolated nuclei, and nuclear scaffolds. Nuclear scaffolds were obtained by extraction with the ionic detergent lithium diidosalicylate (LIS), using nuclei prepared in the absence of divalent cations (metal-depleted nuclei) and stabilized either by a brief heat exposure (20 min at 37C or 42C) or by Cu++ ions at 0C. Proteins were visualized by in situ immunocytochemistry and confocal microscopy. Only a 160-kD nuclear scaffold protein was unaffected by all the stabilization procedures performed on isolated nuclei. However, LIS extraction and scaffold preparation procedures markedly modified the distribution of the polypeptide seen in intact cells, unless stabilization had been performed by Cu++. In isolated nuclei, only Cu++ treatment preserved the original distribution of the two other antigens (M(r), 125 and 126 kD), whereas in heat-stabilized nuclei we detected dramatic changes. In nuclear scaffolds reacted with antibodies to 125 and 126-kD proteins, the fluorescent pattern was always disarranged regardless of the stabilization procedure. These results, obtained with nuclei prepared in the absence of Mg+2 ions, indicate that heat treatment per se can induce changes in the distribution of nuclear proteins, at variance with previous suggestions. Nevertheless, each of the proteins we have studied behaves in a different way, possibly because of its specific association with the nuclear scaffold.

Cell Response to the Exposure to Chitosan-TPP//Alginate Nanogels.

Hydrophilic nanocarriers formed by electrostatic interaction of chitosan with oppositely charged macromolecules have a high potential as vectors in biomedical and pharmaceutical applications. However, comprehensive information about the fate of such nanomaterials in biological environment is lacking. We used chitosan from both animal and fungal sources to form well-characterized chitosan-pentasodium triphosphate (TPP)//alginate nanogels suitable for comparative studies. Upon exposure of human colon cancer cells (HT29 and CaCo2), breast cancer cells (MDA-MB-231 and MCF-7), glioblastoma cells (LN229), lung cancer cells (A549), and brain-derived endothelial cells (HCEC) to chitosan-(TPP)//alginate nanogels, cell type-, nanogel dosage-, and exposure time-dependent responses are observed. Comparing chitosan-TPP//alginate nanogels prepared from either animal or fungal source in terms of nanogel formation, cell uptake, reactive oxygen species production, and metabolic cell activity, no significant differences become obvious. The results identify fungal chitosan as an alternative to animal chitosan in particular if biomedical/pharmaceutical applications are intended.

Microtubule-associated protein 1B, a growth-associated and phosphorylated scaffold protein.

Microtubule-associated protein 1B, MAP1B, is one of the major growth associated and cytoskeletal proteins in neuronal and glial cells. It is present as a full length protein or may be fragmented into a heavy chain and a light chain. It is essential to stabilize microtubules during the elongation of dendrites and neurites and is involved in the dynamics of morphological structures such as microtubules, microfilaments and growth cones. MAP1B function is modulated by phosphorylation and influences microtubule stability, microfilaments and growth cone motility. Considering its large size, several interactions with a variety of other proteins have been reported and there is increasing evidence that MAP1B plays a crucial role in the stability of the cytoskeleton and may have other cellular functions. Here we review molecular and functional aspects of this protein, evoke its role as a scaffold protein and have a look at several pathologies where the protein may be involved.

Augmentation of bone defect healing using a new biocomposite scaffold: an in vivo study in sheep.

Previous studies support resorbable biocomposites made of poly(L-lactic acid) (PLA) and beta-tricalcium phosphate (TCP) produced by supercritical gas foaming as a suitable scaffold for tissue engineering. The present study was undertaken to demonstrate the biocompatibility and osteoconductive properties of such a scaffold in a large animal cancellous bone model. The biocomposite (PLA/TCP) was compared with a currently used beta-TCP bone substitute (ChronOS, Dr. Robert Mathys Foundation), representing a positive control, and empty defects, representing a negative control. Ten defects were created in sheep cancellous bone, three in the distal femur and two in the proximal tibia of each hind limb, with diameters of 5 mm and depths of 15 mm. New bone in-growth (osteoconductivity) and biocompatibility were evaluated using microcomputed tomography and histology at 2, 4 and 12 months after surgery. The in vivo study was validated by the positive control (good bone formation with ChronOS) and the negative control (no healing with the empty defect). A major finding of this study was incorporation of the biocomposite in bone after 12 months. Bone in-growth was observed in the biocomposite scaffold, including its central part. Despite initial fibrous tissue formation observed at 2 and 4 months, but not at 12 months, this initial fibrous tissue does not preclude long-term application of the biocomposite, as demonstrated by its osteointegration after 12 months, as well as the absence of chronic or long-term inflammation at this time point.