Relationships between Mechanical Stress and Markers of Inflammation in Diseased Human Coronary Arteries

Hallow, Karen Melissa

05 July 2007

Rupture of atherosclerotic plaque is one of the primary causes of death due to cardiovascular disease. The factors directing plaque progression to instability are poorly understood. It is well-known that arteries respond to changes in mechanical stress by remodeling, and that remodeling is mediated by the inflammatory response. Studies have shown that both mechanical stress and markers of inflammation are increased in the fibrous cap and shoulder regions of plaque, where rupture most often occurs. In this study we hypothesized that there are spatial relationships between the local mechanical environment and expression of markers of inflammation in atherosclerosis, and that these relationships are plaque-progression dependent. To test these hypotheses, we analyzed cross-sections at intervals along the length of human coronary atherosclerotic arteries. For each cross-section, a heterogeneous finite element model was developed to determine the spatial distribution of stress. In addition, novel techniques for quantifying inflammatory markers at high spatial resolution were used to determine the distributions of inflammatory markers. The distributions of stress and five markers of inflammation activated NF-kB, macrophages, MMP-1, nitrotyrosine, and microvessels - were then compared to determine whether spatial relationships exists. We demonstrated that the probability of activated NF-kB expression increases monotonically with increasing stress in all stages of plaque progression. This indicates that the relationship between mechanical stress and NF-kB activation is a player throughout the disease process. We found that the relationship between mechanical stress and macrophages is highly dependent on the state of plaque progression. In intermediate stages of progression macrophages increase with moderate stress but drop off again at very high stresses, while in the advanced stage macrophages continue to increase monotonically with stress. We found that MMP1 increases with stress in stages of progression where active remodeling is occurring, but decreases with stress in mature stable plaque. We found no relationship between mechanical stress and nitrotyrosine expression or microvessels. Taken together, these results support the role of mechanical stress in instigating and maintaining the inflammatory response, and help explain how mechanical input is able to direct the complex biological changes involved in remodeling.

Atherosclerosis

Plaque rupture

Inflammation

Nuclear factor - kappa B

Matrix metalloproteinase

Macrophages

Reactive oxygen species

Nitrotyrosine

Microvessels

Heterogeneous finite element model

Strains and stresses

Atherosclerotic plaque

Coronary heart disease

Inflammation

Le locus 1q32 : susceptibilité aux maladies inflammatoires de l’intestin et rôles biologiques de C1orf106 et KIF21B

David, Geneviève

04 1900

La maladie de Crohn (MC) et la colite ulcéreuse (CU) sont des maladies inflammatoires de l’intestin (MII) caractérisées par une inflammation chronique du tube digestif. Ces maladies à traits complexes sont le résultat d’un dérèglement du système immunitaire. Les études d’association pangénomique ont identifié au total 99 loci de susceptibilité aux MII. La région 1q32 du chromosome 1 a été identifiée comme locus de susceptibilité à la MC, la CU et la sclérose en plaque. La région autour du marqueur génétique (rs11584383) contient quatre gènes : Chromosome 1 open reading frame 106 (C1orf106), Kinesin family member 21B (KIF21B), Calcium channel, voltage-dependant, L type, alpha 1S subunit (CACNA1S) et Chromosome 1 open reading frame 81 (C1orf81). L’objectif de l’étude est de mettre ces quatres gènes dans un contexte biologique et de déterminer leur rôle potentiel dans les MII. Par réaction de polymérisation en chaîne quantitatif (qPCR), nous avons déterminé le profil d’expression de ces gènes dans des tissus murins et des lignées cellulaires humaines. KIF21B et C1orf106 sont exprimés dans les tissus gastrointestinal et immunitaire. Par la suite, nous avons testé l’implication de KIF21B et C1orf106 dans les voies biologiques connues pour leur rôle dans les MII comme l’activité NF-kB et le stress du réticulum endoplasmique (RE). Nos résultats montrent que la surexpression de KIF21B dans les cellules HEK293T diminue l’activité de NF-kB et la surexpression de C1orf106 augmente le stress du RE et l’activité de la voie Wnt. Globalement, ces résultats suggèrent que KIF21B et C1orf106, dans la région 1q32, sont des gènes candidats prometteurs puisqu’ils interviennent dans des voies biologiques connues des maladies inflammatoire de l’intestin. / Crohn’s disease (CD) and ulcerative colitis (UC) are inflammatory bowel diseases (IBD) characterized by chronic inflammation along the gastrointestinal tract. These complex diseases appear to be the result of an immune system dysregulation. Genome-wide association studies have identified 99 loci that contribute to IBD susceptibility. Region 1q32 of chromosome 1 has been identified as a CD, UC and multiple sclerosis susceptibility locus and the region around this marker (rs11584383) contains four genes: Chromosome 1 open reading frame 106 (C1orf106), Kinesin family member 21B (KIF21B), Calcium channel, voltage-dependant, L type, alpha 1S subunit (CACNA1S) and Chromosome 1 open reading frame 81 (C1orf81). The goal of the present study is to place these genes in a biological context and to determine their possible involvement in IBD. By using quantitative PCR (qPCR), we determined the expression profile of these genes in murine tissues and human cell lines and we observed that KIF21B and C1orf106 were expressed in immune as well as gastrointestinal tissues. Next, we tested the involvement of KIF21B and C1orf106 in biological pathways previously implicated in IBD, more specifically NF-kB activity and endoplasmic reticulum (ER) stress. We found that overexpression of KIF21B in HEK293T cells decreased the activity of NF-kB whereas C1orf106 overexpression increased ER stress and Wnt activity. Taken together, these results suggest that KIF21B and C1orf106 are good candidate causal genes in the 1q32 region.

Maladies inflammatoires

Maladie de Crohn

Colite ulcéreuse

Génétique

1q32

Inflammation

Stress du réticulum endoplasmique

Nuclear factor kappa B

KIF21B

C1orf106

Le rôle des cellules gliales de Müller dans la mort des cellules ganglionnaires de la rétine par des mécanismes cellulaires non-autonomes

Lebrun-Julien, Frédéric

11 1900

Les cellules gliales sont essentielles au fonctionnement du système nerveux. Dans la rétine, les cellules gliales de Müller assurent à la fois l’homéostasie du tissu et la protection des neurones, notamment celle des cellules ganglionnaires de la rétine (CGRs). L’hypothèse principale de la thèse est que les cellules de Müller joueraient un rôle primordial dans la survie neuronale tant au plan de la signalisation des neurotrophines/proneurotrophines par suite d’une blessure que lors des mécanismes d’excitotoxicité. Contrairement au brain-derived neurotrophic factor (BDNF), le nerve growth factor (NGF) n’est pas en mesure d’induire la survie des CGRs après une section du nerf optique. Le premier objectif de la thèse a donc été de localiser les récepteurs p75NTR et TrkA du NGF dans la rétine adulte et d’établir leur fonction respective en utilisant des ligands peptidomimétiques agonistes ou antagonistes spécifiques pour chacun des récepteurs. Nos résultats ont démontré que TrkA est surexprimé par les CGRs après l’axotomie, tandis que p75NTR est spécifiquement exprimé par les cellules de Müller. Alors que NGF n’est pas en mesure d’induire la survie des CGRs, l’activation spécifique de TrkA par des ligands peptidomimétique est nettement neuroprotectrice. De façon surprenante, le blocage sélectif de p75NTR ou l’absence de celui-ci protège les CGRs de la mort induite par l’axotomie. De plus, la combinaison de NGF avec l’antagoniste de p75NTR agit de façon synergique sur la survie des CGRS. Ces résultats révèlent un nouveau mécanisme par lequel le récepteur p75NTR exprimé par les cellules gliales de Müller peut grandement influencer la survie neuronale. Ensuite, nous avons voulu déterminer l’effet des proneurotrophines dans la rétine adulte. Nous avons démontré que l’injection de proNGF induit la mort des CGRs chez le rat et la souris par un mécanisme dépendant de p75NTR. L’expression de p75NTR étant exclusive aux cellules de Müller, nous avons testé l’hypothèse que le proNGF active une signalisation cellulaire non-autonome qui aboutit à la mort des CGRs. En suivant cette idée, nous avons montré que le proNGF induit une forte expression du tumor necrosis factor α (TNFα) dans les cellules de Müller et que l’inhibition du TNF bloque la mort neuronale induite par le proNGF. L’utilisation de souris knock-out pour la protéine p75NTR, son co-récepteur sortiline, ou la protéine adaptatrice NRAGE a permis de montrer que la production de TNF par les cellules gliales était dépendante de ces protéines. Le proNGF semble activer une signalisation cellulaire non-autonome qui cause la mort des neurones de façon dépendante du TNF in vivo. L’hypothèse centrale de l’excitotoxicité est que la stimulation excessive des récepteurs du glutamate sensibles au N-Methyl-D-Aspartate (NMDA) est dommageable pour les neurones et contribue à plusieurs maladies neurodégénératives. Les cellules gliales sont soupçonnées de contribuer à la mort neuronale par excitotoxicité, mais leur rôle précis est encore méconnu. Le dernier objectif de ma thèse était d’établir le rôle des cellules de Müller dans cette mort neuronale. Nos résultats ont démontré que l’injection de NMDA induit une activation du nuclear factor κB (NF-κB) dans les cellules de Müller, mais pas dans les CGRs, et que l’utilisation d’inhibiteurs du NF-κB empêche la mort des CGRs. De plus, nous avons montré que les cellules de Müller en réaction à l’activation du NF-κB produisent la protéine TNFα laquelle semble être directement impliquée dans la mort des CGRs par excitotoxicité. Cette mort cellulaire se produit principalement par l’augmentation à la surface des neurones des récepteurs AMPA perméables au Ca2+, un phénomène dépendant du TNFα. Ces donnés révèlent un nouveau mécanisme cellululaire non-autonome par lequel les cellules gliales peuvent exacerber la mort neuronale lors de la mise en jeu de mécanismes excitotoxiques. / Glial cells are essential for the functioning of the nervous system. In the retina, the Müller glial cells ensure the homeostasis of this tissue as well as the protection of neurons including the retinal ganglion cells (RGCs). The main hypothesis of this thesis is that Müller cells play a predominant role in neuronal survival both at the levels of neurotrophin/proneurotrophin signaling following injury and excitotoxic mechanisms. Unlike the brain-derived neurotrophic factor (BDNF), the nerve growth factor (NGF) is unable to induce RGCs survival following optic nerve transection. The first objective of the thesis was therefore to describe the expression of the two receptors of NGF, p75NTR and TrkA, in the adult retina and to address their functional role by using peptidomimetic agonistic or antagonistic ligands specific for each receptor. Our results showed that TrkA is overexpressed by RGCs following axotomy, whereas p75NTR is specifically expressed by Müller cells. While NGF by itself does not promote RGC survival, selective activation of TrkA receptors using peptidomimetic ligands is markedly neuroprotective. Surprisingly, selective blockers of p75NTR, or the absence of p75NTR, protect RGCs from axotomy-induced death. Moreover, combination of NGF or TrkA agonists with p75NTR antagonists functions synergistically to enhance RGC survival. These results reveal a new mechanism by which p75NTR expression by Müller glia may profoundly influence neuronal survival. Next, we wanted to address the effect of proneurotrophins in the adult retina. We showed that injection of proNGF induces the death of RGCs in rats and mice by a p75NTR-dependent signaling mechanism. Expression of p75NTR in the adult retina being confined to Müller glial cells, we tested the hypothesis that proNGF activates a non-cell autonomous signaling pathway to induce RGC death. Consistent with this notion, we showed that proNGF induced a robust expression of tumor necrosis factor α (TNFα) in Müller cells, and that genetic or biochemical ablation of TNFα blocked proNGF-induced death of retinal neurons. Mice rendered null for p75NTR, its co-receptor sortilin, or the adaptor protein NRAGE were defective in proNGF-induced glial TNFα production and did not undergo proNGF-induced retinal ganglion cell death. We concluded that proNGF activates a non-cell autonomous signaling pathway that causes TNFα-dependent death of retinal neurons in vivo. The central hypothesis of excitotoxicity is that excessive stimulation of neuronal N-Methyl-D-Aspartate (NMDA)-sensitive glutamate receptors is harmful to neurons and contributes to a variety of neurological disorders. Glial cells have been proposed to participate in excitotoxic neuronal loss, but their precise role is poorly defined. In this in vivo study, we showed that NMDA induces a strong NF-κB activation in Müller glia, but not in retinal neurons. Intriguingly, NMDA-induced death of retinal neurons was effectively blocked by inhibitors of NF-κB activity. We demonstrated that TNFα protein produced in Müller glial cells via an NMDA-induced NF-κB dependent pathway plays a crucial role in the excitotoxic loss of retinal neurons. This cell loss occurs mainly through a TNFα-dependent increase in Ca2+-permeable AMPA receptors on susceptible neurons. Thus, our data reveal a novel non-cell-autonomous mechanism by which glial cells can profoundly exacerbate neuronal death following excitotoxic injury.

Cellules ganglionnaires de la rétine

cellules de Müller

Survie neuronale

Nerve growth factor

pro-NGF

p75NTR

Excitotoxicité

Facteur nécrosant des tumeurs

Nuclear Factor K B

INVESTIGATIONS INTO MODULATION OF BRAIN OXIDATIVE STRESS BY VARIOUS INTERVENTIONS

Harris, Jessica Lynn

01 January 2012

In this thesis study we examined glycogen synthase kinase-3β (GSK-3β) and its effects over Nrf2 and Pin 1 as it relates to Alzheimer’s disease (AD). AD is a neurodegenerative disease characterized by a prolonged high oxidative environment. Transcription factor Nrf2 is vital in the brain’s defense against oxidative insults through its up-regulation of over 100 antioxidants. Depletion of the brain’s antioxidant defense system results in intolerance to an oxidative environment, contributing to the progression of AD. The regulatory Pin 1 protein promotes cellular homeostasis, and when down-regulated results in increased deposits of neurofibrillary tangles (NFTs) and amyloid-β (Aβ) plaques, the two pathological hallmarks of AD. Using aged SAMP8 mice treated with antisense oligonucleotide (AO) directed at GSK-3β and random AO, the data presented here demonstrate decreased oxidative stress and increased Nrf2 transcriptional activity and Pin 1 levels as a result of the down-regulation of GSK-3β. Collectively, these results implicate GSK-3β activity in the increased oxidative stress of AD and support its inhibition as a possible therapeutic treatment for the disease. Further, we elucidate a possible mechanism connecting GSK-3β to the loss of tolerance to an oxidative environment and increased deposits of NFTs and Aβ plaques observed in AD.

Alzheimer’s disease

AD

oxidative stress

glycogen synthase kinase-3β

GSK-3β

nuclear factor-E2-related factor 2

Nrf2

Pin 1

Biochemistry

Chemistry

Neuroscience and Neurobiology

Hiperamonemia ativa HIF-1α pela via NF-kB : um possível mecanismo de sarcopenia em cirrose / Hyperammonemia activates HIF-1α via a NF-kB pathway : a possible mechanism for sarcopenia in cirrhosis

Silva, Rafaella Nascimento e

15 September 2016

Submitted by Ronildo Prado (ronisp@ufscar.br) on 2017-08-22T17:21:37Z No. of bitstreams: 1 TeseRNS.pdf: 3515617 bytes, checksum: 251005e22df508ed87d98457bd4a5d3d (MD5) / Approved for entry into archive by Ronildo Prado (ronisp@ufscar.br) on 2017-08-22T17:21:47Z (GMT) No. of bitstreams: 1 TeseRNS.pdf: 3515617 bytes, checksum: 251005e22df508ed87d98457bd4a5d3d (MD5) / Approved for entry into archive by Ronildo Prado (ronisp@ufscar.br) on 2017-08-22T17:21:54Z (GMT) No. of bitstreams: 1 TeseRNS.pdf: 3515617 bytes, checksum: 251005e22df508ed87d98457bd4a5d3d (MD5) / Made available in DSpace on 2017-08-22T17:22:00Z (GMT). No. of bitstreams: 1 TeseRNS.pdf: 3515617 bytes, checksum: 251005e22df508ed87d98457bd4a5d3d (MD5) Previous issue date: 2016-09-15 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) / Hyperammonemia impairs skeletal muscle protein synthesis and induces autophagy by upregulating myostatin via nuclear factor-kappaB (NF-kB). Skeletal muscle ammonia metabolism occurs via synthesis of glutamate and glutamine via critical TCA intermediate α-KG, that regulates increase expression of hypoxia inducible factor 1α (HIF-1α). Furthermore, there is a interaction between HIF-1α and NF-kB. Objective: This study evaluated the effects of hyperammonemia in NF-kB and HIF-1α cross-talking. Methods: To examine the effects of ammonium acetate intervention under HIF-1α signaling through NF-kB pathway it has generated a stable knockdown cell line for NFkB and the subunits α and β of the I kappa B kinase (IKK) complex (IKKα and IKKβ) evaluating the HIF-1α and myostatin activities. Results: The protein expression of HIF- 1α was significantly higher in C2C12 murine myotubes under ammonium acetate intervention compared to control. Once the deletion of NF-kB, IKKα and IKKβ occurs, the HIF-1α is not expressed, suggesting a cross-talking between them. The protein expression of myostatin was significantly higher in C2C12 IKKα deletion under ammonium acetate intervention compared to C2C12 random suggesting that myostatin is not IKKα dependent. Conclusion: We conclude that hyperammonemia is a normoxemic activator of HIF-1α through NF-kB pathway that results in sarcopenia via up-regulation of myostatin expression. / Um dos grandes mediadores de sarcopenia em cirrose é a hiperamonemia. Esta anormalidade metabólica é frequente em doenças hepáticas promovendo conversão danificada de amônia em uréia prejudicando a síntese protéica e induzindo autofagia do músculo esquelético pela up-regulação de miostatina via fator nuclear kappa B (NFkB). O metabolismo de amônia no músculo esquelético ocorre via síntese de glutamato e glutamina através do intermediário metabólico α-cetoglutarato do ciclo de Krebs, que regula o Fator Induzido por Hipóxia (HIF-1α). Além disso, existe um interação entre os dois fatores de transcrição HIF-1α and NF-kB. Objetivo: Este estudo avalia os efeitos da hiperamonemia no cross-talking entre NF-kB and HIF-1α. Métodos: Para examinar os efeitos do aumento da concentração de amônia na expressão de HIF-1α através da via NF-kB foi realizado um knockdown estável de NF-kB, e as subunidades IKKα e IKKβ do complexo I kappa B quinase (IKK) em células C2C12 avaliando as atividades de HIF- 1α e miostatina. Resultados: A expressão protéica de HIF-1α foi significativamente alta em células C2C12 sob tratamento com acetato de amônia comparado com controle. Uma vez que ocorre o silenciamento de NF-kB, IKKα and IKKβ em células C2C12, não é observada a expressão protéica de HIF-1α, sugerindo um cross-talking entre eles. A expressão protéica de miostatina foi significativamente alta em células C2C12 silenciadas para IKKα sob tratamento com acetato de amônia comparado com células C2C12 random (controle), sugerindo que miostatina não é dependente da quinase IKKα. Conclusão: Foi concluído que hiperamonemia é um ativador normóxico de HIF-1α através da via de sinalização NF-kB resultando em sarcopenia via up-regulação de miostatina.

Hiperamonemia

Fator induzido por hipóxia 1α

Miostatina

Músculo esquelético

Factor nuclear kappa B

Hyperammonemia

Hypoxia inducible factor 1α

Nuclear factor-kappaB

Myostatin

Skeletal muscle

CIENCIAS BIOLOGICAS::FISIOLOGIA

A melatonina atenua o estresse oxidativo, ativa o estresse de retículo endoplasmático e a apoptose na hepatocarcinogênese experimental

Moreira, Andréa Cristiane Janz

January 2015

O carcinoma hepatocelular (CHC) é a quarta causa mais frequente de morte por câncer em todo o mundo. Este estudo teve dois grandes objetivos, o primeiro foi estabelecer o carcinoma hpatocelular experimental por indução química e o segundo estudar os efeitos da melatonina sobre o estresse oxidativo, estresse de retículo endoplasmático e apoptose durante a hepatocarcinogênese. Foram realizados dois experimentos, ambos utilizaram dietilnitrosamina (DEN) mais acetilaminofluoreno (2-AAF) em ratos Wistar machos pesando 145-150 g. O primeiro estudo testou 3 protocolos de indução do câncer hepático. Os animais foram divididos em três grupos testes: DEN50: que recebeu DEN 50 mg duas vezes por semana até a 6ª semana e uma vez por semana nas semanas 11 a 13. DEN75: recebeu DEN 75mg uma vez por semana nas semanas até a 6ª semana e um reforço nas semanas de 11 a 13. DEN100: recebeu 5 doses de DEN 100mg uma a cada seis semanas por 28 semanas. Todos receberam 2- AAF dose única de 100 mg na 4ª semana. Após a indução foi comprovado por testes bioquímicos, macroscópico e histológico que o protocolo DEN50 desenvolve CHC avançado em 19 semanas, apresentou a fase inflamatória na 5ª semana e cirrose na 12ª semana. O protocolo DEN100 exibe padrão de lesões pré-cancerosas com cirrose em 28 semanas. O protocolo DEN75 foi o mais heterogêneo dos três, pois desenvolveu lesões pré-cancerosas, cancer inicial e CHC avançado. O segundo estudo, repetiu o protocolo DEN50 e administrou melatonina 20mg/L. Os tratamentos começaram nas semanas 5 e 12. Ao final de 19 semanas foi observado que animais do grupo que só recebeu DEN+2-AAF (DEN-CHC) desenvolveram carcinoma avançado, exibiram mais expressão de proteinas pró-inflamatórias (iNOS, COX-2 e NFkB). E animais tratados com Melatonina (DEN+MEL5 e DEN+MEL 12) apresentaram padrão histológico de cirrose e reduzida expressão destas proteinas. Quanto ao comportamento oxidativo foi observado que grupo DEN-CHC apresentou menor lipoperoxidação (LPO) por redução de ácidos graxos poliinsaturados, maior oxidação proteica, menor atividade da SOD e maior índice de danos ao DNA. O tratamento com melatonina ao longo da hepatocarcinogênese se mostrou efetivo para proteger a membrana lipidica, reduziu a oxidação proteica, aumentou a atividade da SOD e atenuou o dano ao DNA. Por fim, referente ao estresse de retículo endoplasmático e apoptose, animais com DEN-CHC não apresentaram ativação das proteinas de estresse de retículo (BiP, ATF6 e CHOP) nem acionaram as rotas apoptóticas. Entretanto, animais tratados com Melatonina tiveram aumento significativo na expressão de proteinas como BiP, ATF6 e CHOP, assim como proteinas pró-apoptóticas. Nossos resultados apontam que a melatonin, durante o processo de hepatocarcinogênese experimental, atuou como anti-inflamatório, antioxidante e pró-apoptótico. E estas ações contribuiram para evitar a progressão do carcinoma hepatocelular. / Hepatocellular carcinoma (HCC) is the fourth most frequent cause of cancer death worldwide. This study had two main objectives, the first was to establish the experimental hpatocelular carcinoma by chemical induction and the second study the effects of melatonin on oxidative stress, endoplasmic reticulum stress and apoptosis during hepatocarcinogenesis. Two experiments were conducted, both used Diethylnitrosamine (DEN) + acetylaminofluorene (2-AAF) in male Wistar rats weighing 145-150 g. The first study tested three induction protocols of liver cancer. The animals were divided into three test groups: DEN50: DEN that received 50 mg twice a week until 6 weeks and once a week during the weeks 11 and 13. DEN75: DEN received 75mg once a week during the weeks to 6 weeks and another reinforcement in weeks 11 to 13 DEN100: DEN received 5 doses of 100mg one every six weeks for 28 weeks. All received 2 AAF single dose of 100 mg at week 4. After induction was confirmed by biochemical, macroscopic and histological tests that DEN50 protocol develops advanced HCC in 19 weeks, presents inflammatory phase in the 5th week and cirrhosis at 12 weeks. The default display protocol DEN100 of precancerous lesions and cirrhosis in 28 weeks. DEN75 The protocol was the most heterogeneous of the three, as developed precancerous lesions, early cancer and advanced HCC. The second study, repeated the DEN50 protocol and administered melatonin 20mg / L. The treatments began on week 5 and 12. At the end of 19 weeks was observed that animals in the group that received only DEN (DEN-CHC) developed advanced carcinoma exhibited over expression of proinflammatory proteins (iNOS, COX-2 and NFkB). And animals treated with melatonin (DEN+ MEL5W and DEN+MEL 12W) showed histological pattern of cirrhosis and reduced expression of these proteins. As for the oxidative behavior was observed that DEN-HCC group had lower lipid peroxidation (LPO) by reducing polyunsaturated fatty acids, higher protein oxidation, lower activity of SOD and higher rate of DNA damage. Treatment with melatonin throughout hepatocarcinogenesis was effective to protect the lipid membrane, protein oxidation decreased, increased SOD activity and attenuated DNA damage. Finally, referring to the endoplasmic reticulum stress and apoptosis, animal DEN-CHC did not show activation of reticulum stress protein (BiP, ATF6 and CHOP) or triggered apoptotic routes. However, melatonin treated animals had a significant increase in the expression of proteins and BiP, CHOP and ATF6, as well as pro-apoptotic proteins. Our results indicate that melatonin, during the process of experimental hepatocarcinogenesis, acted as anti-inflammatory, antioxidant and pro-apoptotic. And these actions contributed to prevent progression of hepatocellular carcinoma.

Melatonina

Estresse oxidativo

Estresse do retículo endoplasmático

Apoptose

Hepatocarcinoma

Diethylnitrosamine

Oxidative stress

Nitric oxide synthase;

Heat shock protein

A melatonina atenua o estresse oxidativo, ativa o estresse de retículo endoplasmático e a apoptose na hepatocarcinogênese experimental

Moreira, Andréa Cristiane Janz

January 2015

O carcinoma hepatocelular (CHC) é a quarta causa mais frequente de morte por câncer em todo o mundo. Este estudo teve dois grandes objetivos, o primeiro foi estabelecer o carcinoma hpatocelular experimental por indução química e o segundo estudar os efeitos da melatonina sobre o estresse oxidativo, estresse de retículo endoplasmático e apoptose durante a hepatocarcinogênese. Foram realizados dois experimentos, ambos utilizaram dietilnitrosamina (DEN) mais acetilaminofluoreno (2-AAF) em ratos Wistar machos pesando 145-150 g. O primeiro estudo testou 3 protocolos de indução do câncer hepático. Os animais foram divididos em três grupos testes: DEN50: que recebeu DEN 50 mg duas vezes por semana até a 6ª semana e uma vez por semana nas semanas 11 a 13. DEN75: recebeu DEN 75mg uma vez por semana nas semanas até a 6ª semana e um reforço nas semanas de 11 a 13. DEN100: recebeu 5 doses de DEN 100mg uma a cada seis semanas por 28 semanas. Todos receberam 2- AAF dose única de 100 mg na 4ª semana. Após a indução foi comprovado por testes bioquímicos, macroscópico e histológico que o protocolo DEN50 desenvolve CHC avançado em 19 semanas, apresentou a fase inflamatória na 5ª semana e cirrose na 12ª semana. O protocolo DEN100 exibe padrão de lesões pré-cancerosas com cirrose em 28 semanas. O protocolo DEN75 foi o mais heterogêneo dos três, pois desenvolveu lesões pré-cancerosas, cancer inicial e CHC avançado. O segundo estudo, repetiu o protocolo DEN50 e administrou melatonina 20mg/L. Os tratamentos começaram nas semanas 5 e 12. Ao final de 19 semanas foi observado que animais do grupo que só recebeu DEN+2-AAF (DEN-CHC) desenvolveram carcinoma avançado, exibiram mais expressão de proteinas pró-inflamatórias (iNOS, COX-2 e NFkB). E animais tratados com Melatonina (DEN+MEL5 e DEN+MEL 12) apresentaram padrão histológico de cirrose e reduzida expressão destas proteinas. Quanto ao comportamento oxidativo foi observado que grupo DEN-CHC apresentou menor lipoperoxidação (LPO) por redução de ácidos graxos poliinsaturados, maior oxidação proteica, menor atividade da SOD e maior índice de danos ao DNA. O tratamento com melatonina ao longo da hepatocarcinogênese se mostrou efetivo para proteger a membrana lipidica, reduziu a oxidação proteica, aumentou a atividade da SOD e atenuou o dano ao DNA. Por fim, referente ao estresse de retículo endoplasmático e apoptose, animais com DEN-CHC não apresentaram ativação das proteinas de estresse de retículo (BiP, ATF6 e CHOP) nem acionaram as rotas apoptóticas. Entretanto, animais tratados com Melatonina tiveram aumento significativo na expressão de proteinas como BiP, ATF6 e CHOP, assim como proteinas pró-apoptóticas. Nossos resultados apontam que a melatonin, durante o processo de hepatocarcinogênese experimental, atuou como anti-inflamatório, antioxidante e pró-apoptótico. E estas ações contribuiram para evitar a progressão do carcinoma hepatocelular. / Hepatocellular carcinoma (HCC) is the fourth most frequent cause of cancer death worldwide. This study had two main objectives, the first was to establish the experimental hpatocelular carcinoma by chemical induction and the second study the effects of melatonin on oxidative stress, endoplasmic reticulum stress and apoptosis during hepatocarcinogenesis. Two experiments were conducted, both used Diethylnitrosamine (DEN) + acetylaminofluorene (2-AAF) in male Wistar rats weighing 145-150 g. The first study tested three induction protocols of liver cancer. The animals were divided into three test groups: DEN50: DEN that received 50 mg twice a week until 6 weeks and once a week during the weeks 11 and 13. DEN75: DEN received 75mg once a week during the weeks to 6 weeks and another reinforcement in weeks 11 to 13 DEN100: DEN received 5 doses of 100mg one every six weeks for 28 weeks. All received 2 AAF single dose of 100 mg at week 4. After induction was confirmed by biochemical, macroscopic and histological tests that DEN50 protocol develops advanced HCC in 19 weeks, presents inflammatory phase in the 5th week and cirrhosis at 12 weeks. The default display protocol DEN100 of precancerous lesions and cirrhosis in 28 weeks. DEN75 The protocol was the most heterogeneous of the three, as developed precancerous lesions, early cancer and advanced HCC. The second study, repeated the DEN50 protocol and administered melatonin 20mg / L. The treatments began on week 5 and 12. At the end of 19 weeks was observed that animals in the group that received only DEN (DEN-CHC) developed advanced carcinoma exhibited over expression of proinflammatory proteins (iNOS, COX-2 and NFkB). And animals treated with melatonin (DEN+ MEL5W and DEN+MEL 12W) showed histological pattern of cirrhosis and reduced expression of these proteins. As for the oxidative behavior was observed that DEN-HCC group had lower lipid peroxidation (LPO) by reducing polyunsaturated fatty acids, higher protein oxidation, lower activity of SOD and higher rate of DNA damage. Treatment with melatonin throughout hepatocarcinogenesis was effective to protect the lipid membrane, protein oxidation decreased, increased SOD activity and attenuated DNA damage. Finally, referring to the endoplasmic reticulum stress and apoptosis, animal DEN-CHC did not show activation of reticulum stress protein (BiP, ATF6 and CHOP) or triggered apoptotic routes. However, melatonin treated animals had a significant increase in the expression of proteins and BiP, CHOP and ATF6, as well as pro-apoptotic proteins. Our results indicate that melatonin, during the process of experimental hepatocarcinogenesis, acted as anti-inflammatory, antioxidant and pro-apoptotic. And these actions contributed to prevent progression of hepatocellular carcinoma.

Melatonina

Estresse oxidativo

Estresse do retículo endoplasmático

Apoptose

Hepatocarcinoma

Diethylnitrosamine

Oxidative stress

Nitric oxide synthase;

Heat shock protein

Receptor do tipo Toll 4 dentre os TLRs de membrana plasmática possui um papel na malignidade de astrocitomas / Toll-like receptor 4 among the plasmatic membrane Toll like receptors plays a role in astrocytoma malignancy

Isabele Fattori Moretti

03 September 2018

Os receptores do tipo Toll (TLRs) são as primeiras proteínas do sistema imune a identificarem distúrbios, reconhecem patógenos como bactérias, fungos e vírus. Como o processo inflamatório possui um importante papel em diversas doenças, os TLRs foram considerados potenciais alvos em estratégias terapêuticas, incluindo o tratamento de câncer. No entanto, o papel dos TLRs permanece ambíguo. Esse estudo teve como objetivos analisar os níveis de expressão dos TLRs presentes em membrana plasmática, TLRs (TLR1, TLR2, TLR4, TLR5, TLR6) em astrocitomas de diferentes graus de malignidade (grau II-IV), tumor mais prevalente do Sistema Nervoso Central (SNC). Nós demonstramos que a expressão dos TLRs foi mais alta em amostras de astrocitomas comparadas com tecido cerebral não-neoplásico, por qRT-PCR. A expressão gênica e proteica foi observada em células de linhagem de glioblastoma (GBM) U87MG e A172, mostrando sua presença em células tumorais. Foi observada expressão associada entre os heterodímeros TLR1- TLR2. Em GBMs, o subtipo mesenquimal mostrou maior nível de expressão dos TLRs comparados aos subtipos clássico e proneural. Com o objetivo de identificar o papel dos TLRs nas células tumorais, foi selecionado dentre os TLRs o que apresentou maior nível de expressão, o TLR4, e realizamos ensaios funcionais estimulando a U87MG com LPS, um agonista natural para TLR4. A taxa de proliferação da célula tratada com LPS foi similar a não tratada. No entanto, foi observado a ativação do NF-kB após 12hrs do estímulo com LPS. Quando a sinalização do receptor foi inibida por um composto químico (VGX-1027), o nível de proliferação da U87MG decaiu. Adicionalmente, análise in silico revelou uma forte associação dos TLRs hiperexpressos com aumento da expressão de genes relacionados à sinalização do ciclo celular, inflamassoma e ripoptossoma. O que sugere serem os TLRs alvos para complementação do tratamento do câncer / Toll-like receptors (TLRs) are the first to identify disturbances in the immune system, recognizing pathogens such as bacteria, fungi, and viruses. Since the inflammation process plays an important role in several diseases, TLRs have been considered potential therapeutic targets, including treatment for cancer. However, TLRs\' role in cancer remains ambiguous. This study aims to analyze the expression levels of plasmatic cell membrane TLRs (TLR1, TLR2, TLR4, TLR5, and TLR6) in different grades (II-IV) of human astrocytoma, the most prevalent tumor of CNS. We demonstrated that TLR expressions were higher in astrocytoma samples compared to non-neoplastic brain tissue, by qRT-PCR. The genes and proteins expressions were observed in U87MG and A172 GBM cell lines, proving their presence in the tumor cells. Associated expressions between the known heterodimers TLR1-TLR2 were found in diffusely infiltrative astrocytoma. In GBM, the mesenchymal subtype showed higher levels of TLR expressions in relation to classical and proneural subtypes. Aiming to indentify the role of TLRs in tumor cells, we chose the highest TLR expressed in GBM cells, the TLR4, and performed functional assays stimulating U87MG-GBM cell line with LPS, a natural agonist for TLR4. The proliferation rate was similar in treated and non-treated cell with LPS. However, NF-kB activation was detected after 12hrs of LPS stimulation. When TLR4 signaling pathway was inhibited by a chemical compound (VGX-1027) a decrease in the proliferation rate was observed. Additionally, in silico analysis revealed a strong association of TLRs upregulation with increased expression level of genes related to cell cycle, inflammasome and ripoptosome pathways, further highlighting TLRs as interesting targets for cancer complementary treatment

Astrocitoma

Fator nuclear - kappa B

Glioblastoma

Inflamação

Lipopolissacarídeos

Proliferação celular

Receptores Toll-like

Astrocytoma

Cell proliferation, Inflammation

Glioblastoma

Lipopolysaccharides

Nuclear factor - kappa B

Toll like receptors

Differential effects of arachidonic acid and docosahexaenoic acid on cell biology and osteoprotegerin synthesis in osteoblast-like cells

Coetzee, Magdalena

09 March 2006

The purpose of the study was to elucidate the mechanisms by which polyunsaturated fatty acids (PUFAs) prevent bone loss. MG-63 human osteoblasts and MC3T3-E1 murine osteoblasts were exposed to the n-6 PUFA arachidonic acid (AA) and the n-3 PUFA docosahexaenoic acid (DHA) as well as oestrogen (E2) and parathyroid hormone (PTH) and the effects thereof tested on a variety of biological parameters characteristic of osteoblasts. These parameters included prostaglandin E2 (PGE2) synthesis, proliferation, differentiation to mature mineralising osteoblasts as well as osteoprotegerin (OPG) and receptor activator of nuclear factor êB ligand (RANKL) secretion. Results showed that AA stimulates PGE2 production significantly in both cell lines. Stimulated PGE2 production by MC3T3-E1 cells however, was significantly higher, which might be attributed to auto-amplification by PGE2 itself in this cell line. Pre-incubation of the MG-63 cells with cyclo-oxygenase (COX)-blockers inhibited PGE2 production significantly, suggesting that both COX enzymes were involved in PGE2 synthesis. The number of functional osteoblasts is important for bone formation therefore in vitro osteoblastic cell proliferation was investigated. In contrast to the hormones E2 and PTH, both AA and DHA inhibited proliferation significantly. The AA-mediated anti-proliferative effect is possibly independent of PGE2 production, as PGE2 per se had little effect on proliferation. DHA inhibited proliferation of MG-63 cells more severely, which might be attributed to the osteosarcoma nature of the MG-63 cells. The anti-proliferative effect of these PUFAs might be attributed to modulation of cell cycle progression or anti-mitotic effects of PUFA peroxidation products. Morphological studies showed apoptotic cells after DHA exposure in MG-63 cells. There is a reciprocal relationship between reduced proliferation and the subsequent induction of cell differentiation in vitro. High basal levels of alkaline phosphatase (ALP) activity, a marker of the mature mineralising osteoblastic phenotype, were detected in MC3T3-E1 cells. Long-term exposure to AA inhibited ALP activity in these cells. This process might be PGE2-mediated. Exposure to PUFAs, however, did not compromise the ability of the MC3T3-E1 cells to differentiate to mature mineralising osteoblasts. In contrast with MC3T3-E1 cells, MG-63 cells demonstrated low basal ALP activity and were unable to differentiate to mature mineralising osteoblasts. In the absence of osteogenic-inducing supplements, PUFAs induced adipocyte-like features that might be due to the expression of high levels of PPARã in this cell line. Lipid-filled vacuoles were absent in the MC3T3-E1 cells suggesting that the MC3T3-E1 cell line may not express PPARã mRNA. The study furthermore demonstrated that PUFAs are able to modulate OPG and RANKL secretion in osteoblasts. AA inhibited OPG secretion dose-dependently in both cell lines, this could be PGE2-mediated. AA dose-dependently stimulated soluble RANKL (sRANKL) secretion in MC3T3-E1 cells thereby affecting the OPG/RANKL ratio in a negative way, supporting various reports that AA and PGE2 do cause bone resorption. No sRANKL could be detected after exposing the MC3T3-E1 cells to DHA suggesting that DHA could be protective to bone. In conclusion, contrary to in vivo evidence, this in vitro study could not indisputably demonstrate protective effects of PUFAs on the osteoblastic cell lines tested. / Thesis (PhD (Physiology))--University of Pretoria, 2006. / Physiology / unrestricted

Osteoblasts

Docosahexaenoic acid

Arachidonic acid

Prostaglandin e2

Differentiation

Osteoprotegerin (opg)

Alkaline phosphatase activity

Proliferation

Transdifferentiation

Polyunsaturated fatty acids

Mineralisation

UCTD

The Phenomenon Of Blastocyst Hatching : Role Of COX-2 And NF-kB

Roy, Shubhendu Sen

06 1900

The zona-pellucida (zona, ZP) is an adhesion-refractory, acellular coat enclosing the rapidly growing, free-living mammalian preimplantation embryo which undergoes successive cleavage divisions to form the blastocyst, composed of ICM-cells surrounded by outer TE-cells. For further development, the blastocyst must ‘hatch’ or ‘escape’ out of the zona before it can implant into the endometrium for further development (Fig. 5.1A). Hence, the event of hatching or ‘zona escape’ assumes critical importance for the establishment of a successful pregnancy. The golden-hamster blastocyst offers a very unique paradigm to understand hatching, whereby upon attainment of a fully-expanded state, the blastocyst undergoes a dramatic (and molecularly unexplained) deflation event, followed by appearance of TE-derived dynamic cellular projections called TE-projections, whose appearance in an embryonic-stage and -time dependant manner suggest an intimate association with the hatching phenomenon (Fig. 5.1B). Thirdly, embryo-derived zonalytic proteases have been shown to bring about a focal-lysis of the ZP followed by global zona dissolution. Earlier work in the laboratory had demonstrated the intimate involvement of signaling molecules like LIF, HB-EGF, TGF-β and (ER)-α with hatching (Seshagiri et al., 2002, 2009). Investigations also revealed the involvement of cysteine-proteases of the cathepsin (cts) family, especially cts-L, -B and-P to be involved in zona lysis (Sireesha et al., 2008). In order to achieve a better understanding of mammalian preimplantation development, especially hatching, it was important to investigate the role and impact of other critical regulators of developmental and reproductive physiology. COX-2 is one such key signaling moiety and it was decided to investigate the role, if any, of COX-2 and its derived PGs in hamster peri-implantation events. COX-2 transcripts and immunoreactive COX-2 protein were detected in the different preimplantation stages, from 8-cell onwards. COX-2 protein was abundant in both the ICM and TE, but was especially enriched in the TE-cells of the late blastocyst. In order to investigate the function of this enzyme in preimplantation development and hatching, two very-specific inhibitors of COX-2 catalytic action, NS-398 and CAY-10404, were tested in identical concentrations of 25, 50 and 75 μM on in vitro cultured hamster blastocysts. In order to assess the impact of COX-2 inhibition on an embryo-stage and time-dependant manner, inhibitors were tested on freshly recovered 8-cell embryos or early blastocysts, continuously for 72 h or 48 h, respectively. COX-2-selective inhibitors inhibited hamster blastocyst hatching in a dose-dependant manner with maximum inhibition observed in the 75 μM dose. Surprisingly, there was a profound dose-dependent failure of deflation of late-blastocysts upon inhibitor treatment and embryos which hatched, did so in an inflated state and retained intact zonae in cultures. Moreover, embryos subjected to NS-398 treatment phenocopied those subjected to CAY-10404 treatment. Results demonstrate that the effect of inhibitors, and hence the need for COX-2 mediated signaling events is more pronounced in 8¬cell embryos than with early-blastocysts, indicating that COX-2 dependant molecular and cellular processes required for blastocyst morphogenesis and ZP-lysis may have been initiated prior to compaction and cavitation. The reversal of effects of COX-2 inhibition on hatching with exogenous addition of PGE2 and Iloprost (a stable PGI2 analogue) to inhibitor cultures, show that COX-2-derived eicosanoids could, in effect bring about hamster hatching, which is in agreement with previous reports (Davis et al., 1999) and augment peri-implantation development including hatching (Huang et al., 2003). Additionally, it has been successfully demonstrated that PGE2 was superior to PGI2 in augmenting blastocyst hatching in inhibitor-cultures. In this study, the modulation of critical cts-L, -B, -P proteases in COX-2 mediated hamster zona hatching has been verified by quantifying cts in transcripts in control and inhibitor-subjected embryonic samples which was further substantiated by the decreased intra-embryonal protein levels of cts-L and -P. These results demonstrate that COX-2 mediated signaling components directly and effectively modulate hamster preimplantation development, especially zona-hatching phenomenon by transcriptional-regulation of the critical zonalytic proteases. Another potential hatching-associated molecule i.e., NF-κB which is known to exert a great deal of influence on overall reproductive and developmental biology, was investigated in this study. Its specific effects on mammalian preimplantation development, especially hatching, remain totally uninvestigated. This formed the rationale to investigate the reach and impact of NF-κB signaling network in the modulation of peri-hatching events. Transcripts and immunoreactive NF-κB protein of crucial pathway-components like IKK, IκB-β and RelA were detected from 8-cell embryo to the zona-free blastocyst. In order to ascertain the impact of NF-κB signaling on peri-hatching events, two very-specific inhibitors of the NF-κB pathway, BAY-11-7082 and JSH-23 were employed which acted at two strategic signaling points. In order to assess the impact of NF-κB inhibition on an embryo-stage and time-dependant manner, inhibitors were tested on freshly recovered 8-cell embryos or early blastocysts, continuously for 72 h or 48 h, respectively. NF-κB-selective inhibitors inhibited blastocyst hatching in a dose-dependent manner. Interestingly, a profound dose-dependent failure of deflation of late-blastocysts upon inhibitor treatment was observed and embryos which hatched did so in an inflated state and also retained intact zonae in cultures. Moreover, embryos subjected to BAY-11-7082 treatment phenocopied those subjected to JSH-23 treatment, indicating specificity of inhibitor action. Time-course experiments demonstrated that the need for efficient NF-κB mediated signaling is distinctively more for 8-cell embryos than early-blastocysts, indicating that NF-κB dependant molecular and cellular processes required for blastocyst morphogenesis and ZP-lysis may have been initiated prior to compaction and cavitation. Moreover, modulation of zonalysins cts-L, -B and -P by NF-κB-signaling, during the event of zona lysis, both by real-time quantitation of its transcripts and intracellular protein levels has been demonstrated. These results demonstrate that NF¬κB mediated signaling components directly and effectively modulate hamster preimplantation development, especially zona-hatching phenomenon by transcriptional-regulation of the critical zonalytic proteases. The profound inhibition of hatching and effects on blastocyst morphogenesis observed by inhibition of COX-2 and NF-κB signaling systems demonstrate a fundamental need of the growing embryo for these critical signaling moieties. Moreover, the underlying similarity of consequences obtained upon inhibition of both signaling networks i.e., NF-κB and COX-2, perhaps indicate a linear mode of signaling between these principles. It remains to be tested, though, if it really is the case. A striking observation made in this study was the detection of immunoreactive signals for critical signaling moieties like ER-α, COX-2 and RelA onto TEPs of the deflated hamster blastocyst, in addition to earlier TEP-localisation of cathepsins. A B C (Figure) ENDOMETRIUM ENDOMETRIUM ENDOMETRIUM Fig 5.1. Schematic representation of the role of molecular and cellular factors in the regulation of concordant phenomena of mammalian blastocyst hatching and endometrial implantation. (A) Depicts a zona-intact well-formed blastocyst. Preimplantation embryo development and blastocyst formation involves close cooperation between several molecular principles (discussed in sections 1.3.1 to 1.3.3), (B) as the embryo prepares to hatch, prior to implantation, it initiates egression from the non-adhesive ZP coat by cathepsin (cts) protease-mediated lysis of zona (pink circles); there is concomitant appearance of cellular principles such as TEPs (undulating projections shown in green). Of interest is the intimate association of hatching-promoting molecules such as COX-2, NF-κB, ER-α, Cts etc. with the TEPs. (C) depicts a zona-free, TEP-rich blastocyst initiating implantation into the maternal endometrium. It is possible, that the embryonic TEPs with the associated hatching-regulatory molecules are also critical for implantation phenomena during the embryo-maternal recognition and implantation during the establishment of early pregnancy. Preliminary results indicate that TEPs could be the site of membrane lipid-rafts, focal points of membrane-based signaling. The definitive role of TEPs in peri-hatching events is yet to be confirmed, but it is presumed that these actin-based undulating structures, harboring several key molecules involved in peri-implantation events in the embryo as well as the maternal uterus could be instrumental in successfully bringing about the concomitant processes of hatching and implantation. Interestingly, during rodent implantation (hamster, guinea-pig, mouse and rat), the blastocyst orients in such a way that the ICM is oriented away from the endometrium and, at least in the hamster, the TEP-carrying abembryonic (mural) pole remains closest to the luminal epithelium (LE) (Gonzales et al., 1996b; Seshagiri et al., 2009; Fig. 5.1C). In contrast, in humans and other primates, the embryonic pole is closest to LE before implantation (Kirby, 1971; Lee and DeMayo, 2004). Although direct evidence is lacking, but these observations gives rise to a possibility that both hatching and implantation could be intimately related to the polar appearance of TEPs in the embryo. Several key signaling molecules like ER-α, LIF, HB-EGF and TGF-β have been already demonstrated to play crucial roles in mammalian hatching. In this thesis, we have exemplified the need for COX-2 mediated prostanoid signaling and the pleotropic NF-κB signaling system in bringing about mammalian blastocyst hatching. How exactly do these molecular entities communicate among themselves and with cellular principles like TEPs thereby effectively enabling peri-implantation development, remain to be understood. Taken together, these results demonstrate, for the first time, the involvement of embryo-derived signaling molecules, like COX-2 and NF-κB in an embryo stage-and time-dependant manner in mammalian peri-implantation events, especially blastocyst hatching. The association of TEPs with key molecules common to embryonic and maternal preparation for hatching and implantation, respectively, indicates towards a molecular and cellular continuity between the concomitant events. These fundamental findings on hamster blastocyst biology have profound clinical implications in the management of human infertility. (For figures pl see the abstract file).

Golden Hamster Blastocyst

Blastocyst Hatching

Cox-2 Inhibitor

NF-kB Inhibitor

Cyclooxygenase-2

Nuclear Factor-Kappa B

Embryo Hatching

Zona Escape

Golden Hamster

Mammalian Embryogenesis

Hamster Blastocyst

Embryology