Use of functionalized hydrogels for rapid re-epithelialization of hybrid implants in tissue engineering / Utilisation d’hydrogels fonctionnalisés pour une ré-épithélialisation rapide des implants hybrides en ingénierie tissulaire

Ciftci, Saït

20 September 2019

Dans le cadre du développement d’un larynx artificiel, les expérimentations sur l’animal et les essais cliniques ont mis en évidence un défaut de ré-épithélialisation de la face endoluminale de la prothèse. Cet épithélium respiratoire est absolument nécessaire pour obtenir un dispositif implantable totalement intégré dans le corps mais également pour la fonctionnalité d’un tel implant. Dans ce travail nous avons développé de nouveaux films d’hydrogels de collagène et d’acide hyaluronique interpénétrés et réticulés pour assurer une repousse épithéliale rapide. Ces films d’hydrogels optimisés ont une résistance suffisante à l’hydrolyse pour limiter leur dégradation précoce une fois implantés. Ils ont été fonctionnalisés par des facteurs de croissance et de différenciation cellulaire libérés de façon progressive avec un résultat objectivé sur la prolifération cellulaire. L’encapsulation de cellules immunitaire et l’utilisation de cytokines dans ces gels permettent également de moduler la réponse inflammatoire vers un processus de cicatrisation plutôt que de rejet. / As part of the development of an artificial larynx, in vivo experiments and clinical trials have revealed a defect in re-epithelialization of the endoluminal side of the prosthesis. This respiratory epithelium is absolutely necessary to obtain an implantable device fully integrated into the body but also for the functionality of such an implant. In this work we have developed patches of interpenetrated and reticulated hydrogels based on collagen and hyaluronic acid to ensure rapid epithelial regrowth. These optimized hydrogel patches have sufficient resistance to hydrolysis to limit their early degradation once implanted. They have been functionalized by growth and cell differentiation factors that are released gradually with an objectified result on cell proliferation. Encapsulation of immune cells and the use of cytokines in these gels also modulate the inflammatory response towards a healing process rather than rejection.

Larynx

Epithélium respiratoire

Hydrogels

Intégration

Ingénierie tissulaire

Implants

Larynx

Epithelium

Respiratory

Hydrogels

Integration

Implants

Tissue engineering

616.22

541.345

571.5

Fenotypická charakterizace zdravé lidské rohovky a její změny při zadní polymorfní dystrofií rohovky / Phenotypical characterization of the healthy human cornea and the alterations caused by posterior polymorphous corneal dystrophy

Reinštein Merjavá, Stanislava

January 2011

Purpose: The aim of this work was to characterize the healthy human cornea and the cornea of patients suffering from posterior polymorphous corneal dystrophy (PPCD) using different antibodies. Despite the fact that PPCD is a very rare disorder, one of the largest groups of PPCD patients in the world comes from the Czech Republic. This offers us the opportunity to investigate the changes on the clinical, cellular and molecular levels. Material and Methods: A collection of 25 control corneas as well as 16 pathological corneas from PPCD patients were used. Epithelial (cytokeratins) and mesothelial markers (mesothelin, calbindin 2, HBME-1 protein) were detected in all layers of the healthy corneas using immunocyto- and immunohistochemistry. The expression of all markers was confirmed using molecular methods as well (RT-PCR and Western blot). Changes in the expression of cytokeratins and changes in the extracellular matrix structure (collagen IV and VIII) were studied in the PPCD corneas. Combined fluorescent immunohistochemistry with fluorescence in situ hybridization were used in order to characterize the origin of abnormal cells on the posterior graft surface, which cause the recurrence of the PPCD after penetrating keratoplasty surgery. Results: Changes in the cytokeratin expression (strong...

P/Q Type Calcium Channel Cav2.1 Defines a Unique Subset of Glomeruli in the Mouse Olfactory Bulb

Pyrski, Martina, Tusty, Mahbuba, Eckstein, Eugenia, Oboti, Livio, Rodriguez-Gil, Diego J., Greer, Charles A., Zufall, Frank

04 September 2018

Voltage-gated calcium (Cav) channels are a prerequisite for signal transmission at the first olfactory sensory neuron (OSN) synapse within the glomeruli of the main olfactory bulb (MOB). We showed previously that the N-type Cav channel subunit Cav2.2 is present in the vast majority of glomeruli and plays a central role in presynaptic transmitter release. Here, we identify a distinct subset of glomeruli in the MOB of adult mice that is characterized by expression of the P/Q-type channel subunit Cav2.1. Immunolocalization shows that Cav2.1+ glomeruli reside predominantly in the medial and dorsal MOB, and in the vicinity of the necklace glomerular region close to the accessory olfactory bulb. Few glomeruli are detected on the ventral and lateral MOB. Cav2.1 labeling in glomeruli colocalizes with the presynaptic marker vGlut2 in the axon terminals of OSNs. Electron microscopy shows that Cav2.1+ presynaptic boutons establish characteristic asymmetrical synapses with the dendrites of second-order neurons in the glomerular neuropil. Cav2.1+ glomeruli receive axonal input from OSNs that express molecules of canonical OSNs: olfactory marker protein, the ion channel Cnga2, and the phosphodiesterase Pde4a. In the main olfactory epithelium, Cav2.1 labels a distinct subpopulation of OSNs whose distribution mirrors the topography of the MOB glomeruli, that shows the same molecular signature, and is already present at birth. Together, these experiments identify a unique Cav2.1+ multiglomerular domain in the MOB that may form a previously unrecognized olfactory subsystem distinct from other groups of necklace glomeruli that rely on cGMP signaling mechanisms.

Cacna1a

Cav2.1α-1a subunit

olfactory bulb

olfactory epithelium

olfactory glomerulus

olfactory subsystem

synaptic localization

voltage-gated calcium channel

Biomedical Sciences

Analyse protéomique et propriétés de ré-épithélialisation des membranes amniotiques humaines en vue d'une greffe de la surface oculaire / Proteomic analysis and re-epithelialization properties of human amniotic membranes after lyophilization for ocular surface grafting

Nazari Hashemi, Parvin Sadat

11 December 2019

La greffe de Membrane Amniotique Humaine (MAH) permet la cicatrisation des ulcères pré-perforants de la cornée et de sauver un nombre significatif d'yeux victimes de brûlures chimiques. La MAH est un matériel biologique, son utilisation pour le traitement des maladies de la surface oculaire donne de bons résultats en raison de sa capacité à réduire l'inflammation et promouvoir une épithélialisation rapide. Pour son utilisation en clinique, la MAH doit bien évidemment être stérile, mais aussi facile à transporter du centre préleveur au centre greffeur, et stockable longtemps et facilement. Actuellement en routine à la banque de tissus de Rouen, la membrane amniotique est séparée de l’amnios puis dénudée de leur couche spongieuse. Par la suite cette membrane est conservée par cryopréservation (congélation à –80°C) ce qui complique potentiellement l’acheminement des membranes. Par conséquent, dans le cadre de cette étude avec la Banque Normande de Cornées du CHU de Rouen nous avons développé la lyophilisation des MAH pour faciliter son utilisation et sa distribution. L’étude du mapping de la MAH permettra également de déterminer si le taux de facteurs de croissance est homogène dans la MAH ou s’il dépend sa distance par rapport au cordon ombilical. L’étude de la biocompatibilité in vivo d’un deuxième matériau composé de collagène nous permet également d’envisager une alternative pour une implantation du stroma. Nos analyses protéiques (ELISA et Label-free) des MAH la lyophilisées ne montrent pas de différence significative en terme de quantité et de qualité protéique. L’approche protéomique est complétée par l’analyse de la capacité des cellules épithéliales de cornée humaines (CEC) à se multiplier sur la membrane amniotique lyophilisée in vitro. Nous n’avons pas observé de différence entre la croissance des cellules épithéliales sur la MAH lyophilisée ou congelée. L’analyse du total de protéines extraites montre également que la lyophilisation ne dégrade pas les MAH au niveau protéique.Au niveau structurel les résultats de la microscopie électronique ont montré que la structure du stroma de la MAH est impactée par la lyophilisation. La greffe des MAH a été réalisée sur les ulcères cornéens chez le lapin. Au cours de l’expérimentation les lapins n’ont pas montré de signe d’inflammation, les analyses histologiques ont mis en évidence l’épithélialisation de la surface oculaire. Ce projet est en collaboration avec l‘association ophtalmo sans frontière pour qu’à terme le développement de l’utilisation clinique des MAHL répondant notamment à des besoins humanitaires (Cameroun). Notre étude de la cartographie de la MAH a également montré qu’une variabilité en termes de quantité de protéine existe entre les différents donneurs. Dans cette étude nous avons également montré que la couche spongieuse est une source de facteurs de croissance importante dans le processus de cicatrisation des ulcères cornéens. / The Human Amniotic Membrane (HAM) graft allows the healing of corneal ulcers and rescues a significant number of eyes with chemical burn. HAM is a biological material, its use for the treatment of ocular surface diseases gives good results because of its ability to reduce inflammation and promote rapid epithelialization. For its clinical use, the HAM must of course be sterile, but also easy to transport from the sampling center to the transplant center, and easily storable and for a long time. Currently on routine in the tissue bank of Rouen, the amniotic membrane is separated from the amnion and denuded of its spongy layer. Subsequently this membrane is stored by cryopreservation (freezing at -80 ° C) which potentially complicates the delivery of membranes. Consequently, as part of this study with the Banque Normande de Cornées of Rouen University Hospital, we have developed freeze-drying of HAM to facilitate its use and distribution. The HAM mapping study will also determine whether the level of growth factors is homogeneous in the HAM or whether it depends on its distance from the umbilical cord. The study of the in vivo biocompatibility of a second material composed of collagen also allows us to consider an alternative for implantation at the level of the stroma. Our protein analyzes (ELISA and Label-free) of freeze-dried HAM do not show any significant difference in terms of quantity and protein quality. The proteomic approach is complemented by the analysis of the ability of human corneal epithelial cells (CECs) to multiply on the freeze-dried amniotic membrane in vitro. We did not observe any difference between the epithelial cells growths on freeze-dried or frozen HAM. The analysis of the extracted protein total also shows that freeze-drying does not degrade the HAM at the protein level. At the structural level the electron microscopy results showed that the structure of the MAH stroma is impacted by freeze-drying. The MAH transplant performed on corneal ulcers in rabbits was performed. During the experiment the rabbits did not show any sign of inflammation, the histological analyzes highlighted the epithelialization of the ocular surface.This project is in collaboration with OSF association for the development of the clinical use of MAHL responding in particular to humanitarian needs (Cameroon). Our study of HAM mapping also showed that variability in terms of amount of protein exists between different donors. We have also shown that the spongy layer is an important source of important growth factor in the healing process of corneal ulcers.

Ulcère

Membrane amniotique

Protéomique

Matrice de collagène

Corneal epithelium renewal

Ulcer

Amniotic membrane

Proteomics

Collagen matrix

617.7

CLINICAL AND GENETIC CHARACTERISTICS OF JAPANESE PATIENTS WITH AGE-RELATED MACULAR DEGENERATION AND PSEUDODRUSEN / 日本人における加齢黄斑変性とシュードドルーゼンの臨床的および遺伝学的特徴

Sufian, Elfandi

26 March 2018

京都大学 / 0048 / 新制・課程博士 / 博士(医学) / 甲第21002号 / 医博第4348号 / 新制||医||1027(附属図書館) / 京都大学大学院医学研究科医学専攻 / (主査)教授 大森 孝一, 教授 山田 亮, 教授 Shohab YOUSSEFIAN / 学位規則第4条第1項該当 / Doctor of Medical Science / Kyoto University / DFAM

age-related macular degeneration

choroidal neovascularization

polypoidal choroidal vasculopathy

pseudodrusen

retinal angiomatous proliferation

geographic atrophy

retinal pigment epithelium

490

The cytoprotective role of Ras signaling in glomerular epithelial cell injury /

Huynh, Carl.

January 2007

No description available.

Complement Membrane Attack Complex.

Kidney Glomerulus -- metabolism.

ras Proteins -- metabolism.

Epithelium -- metabolism.

Cytoprotection -- physiology.

THE ROLE OF HYALURONAN IN INNATE INTESTINAL DEFENSE

Hill, David Richard

16 August 2013

No description available.

Biochemistry

Biomedical Research

Biology

Immunology

Microbiology

Molecular Biology

Pharmaceuticals

hyaluronan

defensin

epithelium

innate barrier defense

glycosaminoglycan

milk

molecular medicine

Biochemical Investigations of Macular Degeneration: The Significance of Protein Oxidation including Novel Methods for Its Study

Warburton, Sarah

06 November 2006

The retinal pigment epithelium (RPE) is a monolayer of cells located directly behind the photoreceptor cells in the retina. These cells are involved in a variety of functions that support the visual process in the eye, namely 1) they form a blood-retina barrier which separates the neural retina from the choroid's blood supply, 2) the apical processes of RPE cells diurnally phagocytose the outer segments of photoreceptor cells, and 3) they participate in the renewal of the photopigment 11-cis retinal. Age-related macular degneration (AMD) is the leading cause of blindness in people over the age of 50 years in North America and other developed countries. AMD involves the death of retinal pigment epithelial (RPE) cells in the macula early in the progress of the disease. Like some other postmitotic cells, the RPE accumulates autofluorescent lysosomal storage bodies (lipofuscin) during senescence. Lipofuscin is reported to begin accumulating in the human RPE around age 20 and continues to accumulate throughout an individual's life. This progressive accumulation of lipofuscin can eventually occupy a substantial fraction of the RPE cytoplasmic volume and may lead to impairment of normal RPE functions, resulting in retinal degeneration and loss of visual function as in AMD. Another autofluorescent granule that accumulates in RPE cells and may contribute to the etiology of AMD is a complex granule exhibiting properties of both melanosomes and lipofuscin granules called melanolipofuscin (MLF). In contrast with the accumulation of LF in the RPE, MLF accumulation has been reported by Feeney-Burns to more closely reflect the onset of AMD. Although there have been significant advances in our understanding of AMD, knowledge of the mechanisms responsible for its progression remain unclear. This dissertation details experiments that were designed to better understand the factors that may play a causal role in AMD as well as the development of methods to assist in AMD research. Specifically, the protein composition of retinal LF was assessed to elucidate its origin. These findings are reported in chapter 2. The accumulation, composition and phototoxicity of MLF were analyzed to assess MLF's origin and possible contribution to AMD. These results are reported in chapter 3. Because protein oxidation is possibly a common posttranslational modification to proteins which accumulate in lipofuscin and melanolipofuscin granules, a method for the detection and analysis of oxidized proteins was developed and is reported in chapter 4. Chapter 5 details the proteomic differences between ARPE-19 cells - the only human RPE cell line available for research - in their differentiated and undifferentiated states and compares these to the proteome of human RPE cells. These results are also compared to the phenotypic difference of these cells as observed by transmission electron microscopy.

age-related macular degeneration

amd

retinal pigment epithelium

rpe

proteomics

oxidation

lipofuscin

melanolipofuscin

mass spectrometry

protein

biochemistry

Biochemistry

Chemistry

Pyridinium Bis-retinoids: Extraction, Synthesis, and Folate Coupling

Alvarez, Mary Allison

08 March 2007

This thesis is divided into two parts.Part I describes the organic extraction, separation, and liquid chromatographic-mass spectrometric analysis of chromophores from human and bovine retinal pigment epithelium. Flurorophores in the retinal pigment epithelium have been implicated in age related macular degeneration. In addition, the synthesis and characterization of a number of bis-retinoid type compounds that may potentially be found in such extracts, or that may be used for insight into pyridinium bis-retinoid reactivity, was accomplished.Part II describes a study of pyridinium bis-retinoid-folic acid coupling with respect to linker type, linker length, and nature of the linkage. Folic acid has been used as a targeting compound for a variety of cancer types. Development of HPLC and UV-Vis conditions suitable for the analysis of this new type of macromolecule was performed.

retinal pigment epithelium

RPE

extraction

pyridinium bis-retinoid

A2E

folic acid coupling

photodynamic therapy

targeted drug delivery

Chemistry

The Fast Lane of Hypoxic Adaptation: Glucose Transport Is Modulated via A HIF-Hydroxylase-AMPK-Axis in Jejunum Epithelium

Dengler, Franziska, Gäbel, Gotthold

10 January 2024

The intestinal epithelium is able to adapt to varying blood flow and, thus, oxygen availability. Still, the adaptation fails under pathologic situations. A better understanding of the mechanisms underlying the epithelial adaptation to hypoxia could help to improve the therapeutic approach. We hypothesized that the short-term adaptation to hypoxia is mediated via AMP-activated protein kinase (AMPK) and that it is coupled to the long-term adaptation by a common regulation mechanism, the HIF-hydroxylase enzymes. Further, we hypothesized the transepithelial transport of glucose to be part of this short-term adaptation. We conducted Ussing chamber studies using isolated lagomorph jejunum epithelium and cell culture experiments with CaCo-2 cells. The epithelia and cells were incubated under 100% and 21% O2, respectively, with the panhydroxylase inhibitor dimethyloxalylglycine (DMOG) or under 1% O2. We showed an activation of AMPK under hypoxia and after incubation with DMOG by Western blot. This could be related to functional effects like an impairment of Na+-coupled glucose transport. Inhibitor studies revealed a recruitment of glucose transporter 1 under hypoxia, but not after incubation with DMOG. Summing up, we showed an influence of hydroxylase enzymes on AMPK activity and similarities between hypoxia and the effects of hydroxylase inhibition on functional changes.

info:eu-repo/classification/ddc/570

ddc:570