Systematic ultrastructural analyses of meningeal and parenchymal vessels of the central nervous system

Dyrna, Felix

26 March 2019

The direct endothelial contact with adjacent astrocytic end-feet is believed to establish blood-brain barrier (BBB) typical characteristics in endothelial cells of the central nervous system (CNS). However, this contact is only present in capillary vessels of the brain parenchyma and absent in larger veins, arteries and vessels within the meninges. To investigate a potential impact of direct endothelial interactions with adjacent astrocytic end-feet on the molecular tight junction (TJ) composition and ultrastructure, we performed a systematic analysis of endothelial cell contacts within the vascular tree of parenchymal and leptomeningeal vessels. Immunofluorescence labeling for claudin-3, claudin-5, zonula occludens-1 and occludin was used to compare the molecular composition, without showing significant differences in their distribution along the vascular tree of parenchymal and leptomeningeal vessels. Furthermore, electron microscopy in combination with quantitative analyses was performed to investigate the endothelial ultrastructure revealing significant differences within the length of endothelial overlaps between the different vessel types. Here, parenchymal arteries exhibit noticeably longer cell contacts compared to capillaries, which could not be observed in leptomeningeal vessels. It was also observed that arterial vessels regularly contain a higher density of endothelial vesicles throughout the parenchyma and meninges as a sign for transendothelial traffic. Hence, endothelial expression of blood-brain barrier typical TJs is not limited to capillary vessels with an intimate contact to surrounding astrocytes, but is also observed in arteries and veins of the brain parenchyma as well as the meninges, the latter of which are lacking a direct astrocyte-endothelial interaction. These vessel-specific characteristics can now be used to address and compare alterations of the BBB in different settings of CNS pathologies.:Table of Content 1. INTRODUCTION 4 1.1 THE BLOOD-BRAIN BARRIER 4 1.2 HISTORY 5 1.3 STRUCTURE AND COMPOSITION 6 1.4 THE ROLE OF THE MICROENVIRONMENT 8 1.4.1 ASTROCYTES 8 1.4.2 PERICYTES 9 1.5 BLOOD BRAIN BARRIER FUNCTION 10 1.5.1 PHYSIOLOGIC CONDITIONS 10 1. 5.2 PATHOLOGIC CONDITIONS 11 2. OPEN QUESTIONS AND SCIENTIFIC APPROACH 12 3. PUBLICATIONS 13 3.1 DIFFERENT SEGMENTS OF THE CEREBRAL VASCULATURE REVEAL SPECIFIC ENDOTHELIAL SPECIFICATIONS, WHILE TIGHT JUNCTION PROTEINS APPEAR EQUALLY DISTRIBUTED 13 3.2 THE BLOOD-BRAIN BARRIER 28 4. SUMMARY 40 5. REFERENCES 43 6. PROOF OF SIGNIFICANT CONTRIBUTION 48 7. DECLARATION OF ACADEMIC HONESTY 49 8. ACKNOWLEDGMENT 50 9. CURRICULUM VITAE 51

info:eu-repo/classification/ddc/610

ddc:610

Exploring causes of pericyte expansion in postnatal brain of Rbpj-mediated mouse model of arteriovenous malformation

Kandalai, Shruthi M.

18 May 2021

No description available.

Biology

Neurobiology

Neurosciences

Developmental Biology

AVM

arteriovenous malformation

pericyte

neurovascular unit

blood-brain barrier

brain

retina

Model mozkové fokální korové ischémie a jeho parametrizace / Model of cerebral focal cortical ischemia and its parametrization

Svoboda, Jan

January 2015

Title of work: Model of cerebral focal cortical ischemia and its parametrization Work objectives: The aim of this diploma thesis was to apply modified model of focal cortical brain ischemia induced by phototrombosis and subsequently determinate its parameters. Methods: Intravenous application of photosensitive Rose Bengal dye was followed by continual illumination of green laser beam over the left sensorimotocortex for 10 minutes. Following illumination, the dye is activated and produces singlet oxygen that damages components of endothelial cell membranes, with subsequent platelet aggregation and thrombin formation, which eventually determines the interruption of local blood flow. This approach, initially proposed by Rosenblum and El-Sabban in 1977, was later improved by Watson in 1985 in rat brain. For histological evaluation of ischemic brain damage, animals were overdosed with urethane and transcardially perfused. Results: Histological examination of brains showed significant ischemic damage in all experimental animals. Lesion was located in left hemisphere and penetrated thought the grey matter in various extents. Size of lesion, its localization and depth has shown only a small variability in the individual groups. Noticeable differences were found right after comparing experimental groups....

THE EFFECTS OF EXERCISE PRECONDITIONING ON FOCAL ISCHEMIC STROKE

Grohs, Gillian

01 January 2017

Cleaved fragments of the extracellular matrix protein perlecan have been shown to promote neuroprotection and repair after ischemic stroke. The cysteine proteases cathepsin B and L as well as the metalloprotease bone morphogenic protein 1 (BMP-1) are capable of releasing the biologically active C-terminal laminin-like globular domain (LG3) of perlecan. Exercise, a known method of reducing stroke risk and severity, has been shown to increase the expression of some proteases associated with perlecan processing. Using a transient distal middle cerebral artery occlusion (MCAo) model for focal ischemic stroke we show that while 7 days of running only slightly decreased infarct volume, BMP1 and perlecan (HSPG2) RNA expression in skeletal muscle was significantly increased in 3-month-old male wild type C57/BL6 mice. Moreover, elevated levels of BMP1 RNA were still detectable after 3 days of detraining, suggesting a prolonged effect of exercise on BMP1 expression. Levels of LG3 in the blood were below the limit of detection in the current study, however it is likely that a more sensitive method would enable analysis of serum. These preliminary findings suggest that LG3 could be a molecular mediator of neuroprotection afforded by exercise though further studies are required.

Ischemic Stroke

Exercise Preconditioning

Neurovascular Unit

Perlecan Laminin-like Globular Domain 3

Skeletal Muscle

Neurosciences

Physiological Processes

Analyzing consequences to astrocytes in a mouse model of brain arteriovenous malformation

Ward, Brittney M.

18 May 2021

No description available.

Neurosciences

Neurobiology

Biology

Biomedical Research

Developmental Biology

Regionally Altered Immunosignals of Surfactant Protein-G, Vascular and Non-Vascular Elements of the Neurovascular Unit after Experimental Focal Cerebral Ischemia in Mice, Rats, and Sheep

Michalski, Dominik, Reimann, Willi, Spielvogel, Emma, Mages, Bianca, Biedermann, Bernd, Barthel, Henryk, Nitzsche, Björn, Schob, Stefan, Härtig, Wolfgang

20 January 2024

The surfactant protein-G (SP-G) has recently been discovered in the brain and linked to fluid balance regulations. Stroke is characterized by impaired vessel integrity, promoting water influx and edema formation. The neurovascular unit concept (NVU) has been generated to cover not only ischemic affections of neurons or vessels but also other regionally associated cells. This study provides the first spatio-temporal characterization of SP-G and NVU elements after experimental stroke. Immunofluorescence labeling was applied to explore SP-G, vascular and cellular markers in mice (4, 24, and 72 h of ischemia), rats (24 h of ischemia), and sheep (two weeks of ischemia). Extravasated albumin indicated vascular damage within ischemic areas. Quantifications revealed decreasing SP-G signals in the ischemia-affected neocortex and subcortex. Inverse immunosignals of SP-G and vascular elements existed throughout all models. Despite local associations between SP-G and the vasculature, a definite co-localization was not seen. Along with a decreased SP- G-immunoreactivity in ischemic areas, signals originating from neurons, glial elements, and the extracellular matrix exhibited morphological alterations or changed intensities. Collectively, this study revealed regional alterations of SP-G, vascular, and non-vascular NVU elements after ischemia, and may thus stimulate the discussion about the role of SP-G during stroke.

info:eu-repo/classification/ddc/610

ddc:610

Caractérisation neuro-immunitaire d'un modèle d'encéphalomyélite auto-immune expérimentale spontanée

Saint-Laurent, Olivia

08 1900

La sclérose en plaques est une maladie neuroinflammatoire idiopathique caractérisée par la formation de lésions focales de démyélinisation, qui apparaissent suite à l’infiltration périvasculaire de cellules immunitaires et à l’augmentation de la perméabilité de la barrière hémato-encéphalique. L’encéphalomyélite auto-immune expérimentale (EAE) est le modèle animal de cette maladie. Cependant, ce modèle présente des différences importantes avec la sclérose en plaques. L’objectif de ce projet de maîtrise était d’approfondir la caractérisation d’un nouveau modèle transgénique d’encéphalomyélite auto-immune expérimentale spontanée, le modèle TCR1640, afin de valider celui-ci pour l’étude des phénomènes physiopathologiques qui surviennent à différents stades de la sclérose en plaques, ainsi que pour le développement de nouveaux traitements de la maladie. La souris TCR1640 porte un récepteur des cellules T (TCR) transgénique autoréactif, qui reconnaît un peptide de la myéline et déclenche une réaction auto-immune contre la myéline endogène au sein du système nerveux central (SNC). Des observations faites in situ et in vitro ont permis d’identifier des changements qui surviennent de façon très précoce dans l’unité neurovasculaire chez les animaux TCR1640 présymptomatiques, et qui sont liés à la présence d’un profil immunitaire périphérique proinflammatoire. Lors des phases actives de l’EAE spontanée, les animaux TCR1640 au stade chronique présentent une inflammation accrue du système nerveux central associée à une infiltration leucocytaire massive, par rapport aux animaux au stade aigu de la maladie. Une étude in vivo a également permis de moduler la maladie développée par des animaux ayant subi une immunisation passive avec des cellules T auxiliaires en provenance de souris TCR1640. Enfin, l’implication de nouvelles molécules d’adhésion cellulaire dans le développement et le maintien de l’EAE spontanée a été suggérée par des observations in vitro. L’ensemble de ces résultats suggère que le modèle TCR1640 présente plusieurs avantages pour l’étude de la physiopathologie de maladies neuroinflammatoires telles que la sclérose en plaques, et servira d’outil afin de valider de nouvelles stratégies thérapeutiques. / Multiple sclerosis is an idiopathic inflammatory disease of the central nervous system. It is characterized by the formation of focal perivascular lesions and demyelination of the surrounding area, which appear concomitantly to a massive immune cell infiltration and disruption of the blood brain barrier. Experimental autoimmune encephalomyelitis is the animal model most extensively used for the study of multiple sclerosis. Unfortunately, this model does not mimic many aspects of the human disease. The goal of this project is to further the characterization of a new transgenic model of spontaneous experimental autoimmune encephalomyelitis, the TCR1640 model, and to validate it as a relevant tool for the study of multiple sclerosis physiopathology and treatment. The TCR1640 mouse possesses a transgenic T cell receptor which recognizes a myelin peptide and triggers an autoimmune response against endogenous myelin in the central nervous system. In situ and in vitro observations have led to the identification of early changes which appear at the neurovascular unit in presymptomatic TCR1640 animals. This early disruption of blood brain barrier homeostasis is linked to the establishment of a proinflammatory immune profile in the periphery. Animals at the chronic stage show sustained inflammation of the central nervous system parenchyma and massive leukocyte infiltration, compared to animals in acute phase of disease. An in vivo experiment has allowed modulating the disease by treatment with a multiple sclerosis-approved therapy, in wild type mice which had received reactivated CD4+ T cells from TCR1640 animals. Finally, the implication of new cell adhesion molecules in the development and maintenance of spontaneous experimental autoimmune encephalomyelitis has been suggested by in vitro study of melanoma cell adhesion molecule (CD146) and activated leucocyte cell adhesion molecule (CD166). The results obtained in this study suggest that the TCR1640 model is a valuable asset in the study of neuroimmune diseases such as multiple sclerosis. It could also be used to validate new therapeutic strategies for the treatment of this disease.

Barrière hémato-encéphalique

Système nerveux central

Neuroinflammation

Unité neurovasculaire

Sclérose en plaques

Molécules d’adhésion cellulaire

Blood-brain barrier

Central nervous system

Neuroinflammation

Neurovascular unit

Multiple sclerosis

Cell adhesion molecules

Caractérisation neuro-immunitaire d'un modèle d'encéphalomyélite auto-immune expérimentale spontanée

Saint-Laurent, Olivia

08 1900

La sclérose en plaques est une maladie neuroinflammatoire idiopathique caractérisée par la formation de lésions focales de démyélinisation, qui apparaissent suite à l’infiltration périvasculaire de cellules immunitaires et à l’augmentation de la perméabilité de la barrière hémato-encéphalique. L’encéphalomyélite auto-immune expérimentale (EAE) est le modèle animal de cette maladie. Cependant, ce modèle présente des différences importantes avec la sclérose en plaques. L’objectif de ce projet de maîtrise était d’approfondir la caractérisation d’un nouveau modèle transgénique d’encéphalomyélite auto-immune expérimentale spontanée, le modèle TCR1640, afin de valider celui-ci pour l’étude des phénomènes physiopathologiques qui surviennent à différents stades de la sclérose en plaques, ainsi que pour le développement de nouveaux traitements de la maladie. La souris TCR1640 porte un récepteur des cellules T (TCR) transgénique autoréactif, qui reconnaît un peptide de la myéline et déclenche une réaction auto-immune contre la myéline endogène au sein du système nerveux central (SNC). Des observations faites in situ et in vitro ont permis d’identifier des changements qui surviennent de façon très précoce dans l’unité neurovasculaire chez les animaux TCR1640 présymptomatiques, et qui sont liés à la présence d’un profil immunitaire périphérique proinflammatoire. Lors des phases actives de l’EAE spontanée, les animaux TCR1640 au stade chronique présentent une inflammation accrue du système nerveux central associée à une infiltration leucocytaire massive, par rapport aux animaux au stade aigu de la maladie. Une étude in vivo a également permis de moduler la maladie développée par des animaux ayant subi une immunisation passive avec des cellules T auxiliaires en provenance de souris TCR1640. Enfin, l’implication de nouvelles molécules d’adhésion cellulaire dans le développement et le maintien de l’EAE spontanée a été suggérée par des observations in vitro. L’ensemble de ces résultats suggère que le modèle TCR1640 présente plusieurs avantages pour l’étude de la physiopathologie de maladies neuroinflammatoires telles que la sclérose en plaques, et servira d’outil afin de valider de nouvelles stratégies thérapeutiques. / Multiple sclerosis is an idiopathic inflammatory disease of the central nervous system. It is characterized by the formation of focal perivascular lesions and demyelination of the surrounding area, which appear concomitantly to a massive immune cell infiltration and disruption of the blood brain barrier. Experimental autoimmune encephalomyelitis is the animal model most extensively used for the study of multiple sclerosis. Unfortunately, this model does not mimic many aspects of the human disease. The goal of this project is to further the characterization of a new transgenic model of spontaneous experimental autoimmune encephalomyelitis, the TCR1640 model, and to validate it as a relevant tool for the study of multiple sclerosis physiopathology and treatment. The TCR1640 mouse possesses a transgenic T cell receptor which recognizes a myelin peptide and triggers an autoimmune response against endogenous myelin in the central nervous system. In situ and in vitro observations have led to the identification of early changes which appear at the neurovascular unit in presymptomatic TCR1640 animals. This early disruption of blood brain barrier homeostasis is linked to the establishment of a proinflammatory immune profile in the periphery. Animals at the chronic stage show sustained inflammation of the central nervous system parenchyma and massive leukocyte infiltration, compared to animals in acute phase of disease. An in vivo experiment has allowed modulating the disease by treatment with a multiple sclerosis-approved therapy, in wild type mice which had received reactivated CD4+ T cells from TCR1640 animals. Finally, the implication of new cell adhesion molecules in the development and maintenance of spontaneous experimental autoimmune encephalomyelitis has been suggested by in vitro study of melanoma cell adhesion molecule (CD146) and activated leucocyte cell adhesion molecule (CD166). The results obtained in this study suggest that the TCR1640 model is a valuable asset in the study of neuroimmune diseases such as multiple sclerosis. It could also be used to validate new therapeutic strategies for the treatment of this disease.

Barrière hémato-encéphalique

Système nerveux central

Neuroinflammation

Unité neurovasculaire

Sclérose en plaques

Molécules d’adhésion cellulaire

Blood-brain barrier

Central nervous system

Neuroinflammation

Neurovascular unit

Multiple sclerosis

Cell adhesion molecules

Exploration of the Cerebral Dysfunctions Induced by Arterial Rigidity and/or the Overexpression of TGFβ in a Mouse Model

Bloch, Sherri

06 1900

No description available.

TGF beta

behavioral testing

Morris Water Maze

Neurovascular coupling

Alzheimer's disease

Vascular dementia

Dementia

Neurovascular unit

Mouse model

Oxidative stress

Gliosis

Novel object recognition

Cerebral dysfunction

Calcification

Arterial rigidity

TGFβ

Rigidité artérielle

Démence

Alzheimer

Démence vasculaire

Piscine de Morris

Dysfunction cérébrale

Unité neurovasculaire