Rôle du CD40 dans la mort cellulaire

Jundi, Malek

January 2008

Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal

CD40

CD40

Mort cellulaire

Celle death

Lymphocyte B

B cells

Cathepsine B

Cathepsin B

Lysosome

Functional analysis of the MERS-coronavirus spike protein

Gierer, Stefanie

26 June 2014

Zehn Jahre nach dem Ausbruch des Severe Acute Respiratory Syndrome Coronavirus, SARS-CoV, ist ein neues Betacoronavirus, das Middle East Respiratory Syndrome Coronavirus, MERS-CoV, auf der arabischen Halbinsel entdeckt worden. Seine anhaltende Ausbreitung stellt eine Bedrohung für die öffentliche Gesundheit dar. Das Spike (S) Protein der Coronaviren vermittelt den viralen Eintritt in Wirtszellen und bestimmt wesentlich den viralen Tropismus und die virale Pathogenese. Das Verständnis der Determinanten des MERS-CoV Spike (MERS-S)-vermittelnden Eintritts in Zellen könnte daher wichtige Einblicke in die MERS-CoV-Biologie liefern und war somit das erste Ziel dieser Arbeit. Um den Eintritt in die Zelle zu ermöglichen, muss das Coronavirus S-Protein durch Wirtszellproteasen aktiviert werden, welche potentielle Ziele für die therapeutischen Intervention darstellen. Daher sollten im zweiten Ziel dieser Arbeit Proteasen identifiziert werden, die MERS-S aktivieren. Das S-Protein ist das Hauptangriffsziel neutralisierender Antikörper und experimentelle Systeme zur S-Analyse können für die Diagnostik eingesetzt werden. Das letzte Ziel dieser Arbeit war es daher, die MERS-CoV Seroprävalenz in Saudi Arabien zu ermitteln. Es wurde ein lentivirales Vektorensystem etabliert, welches die Analyse des MERS-S-getriebenen Zelleintritts ermöglicht. Mit Hilfe dieses Systems konnte gezeigt werden, dass MERS-S den Eintritt in ein breites Spektrum humaner Zelllinien, wie Lungen-, Nieren- und Darmzellen vermittelt, was mit der klinischen Manifestation von MERS einhergeht. Der Wirtszelleintritt war unabhängig von bereits beschriebenen Coronavirus Eintrittsrezeptoren, wurde jedoch durch die endosomale Cysteinprotease Cathepsin L und die Transmembranserinprotease TMPRSS2 gefördert. Im Gegensatz dazu war die Aktivität von Proprotein Konvertasen für den S-Protein-vermittelnden Eintritt entbehrlich. Schließlich zeigten Neutralisationstests, dass Seren von Patienten aus der östlichen Provinz Saudi Arabiens, die zwischen 2010-2011 und 2012 entnommen wurden, keine MERS-S-neutralisierenden Antikörper enthielten. Dies deutet darauf hin, dass MERS-CoV-Infektionen vor dem Ausbruch 2012 nur selten vorkamen. Die gewonnen Ergebnisse tragen wesentlich zum Verständnis des MERS-CoV-Eintritts in Zellen bei und liefern wichtige Informationen zur MERS-CoV-Epidemiologie. Weiterhin könnte die Beobachtung, dass der Protease-Inhibitor Camostat, der für den Einsatz im Menschen zugelassen ist (in Japan), TMPRSS2 blockiert und damit den MERS-CoV Eintritt inhibiert, helfen, Behandlungsstrategien für MERS-Patienten zu etablieren.

570

Biologie (PPN619462639)

Cathepsin S as a Biomarker of Low-grade Inflammation, Insulin Resistance, and Cardiometabolic Disease Risk

Jobs, Elisabeth

January 2014

Cathepsin S is a protease important in major histocompatibility complex (MHC) class II antigen presentation and also in degrading the extracellular matrix. Studies, most of them experimental, have shown that cathepsin S is involved in different pathological conditions such as obesity, inflammation, atherosclerosis, diabetes, and cancer. The overall hypothesis of this report is that high levels of circulating cathepsin S, is a biomarker that reflects pathology induced by inflammation and obesity. The overall aim of this report was to investigate possible associations between circulating cathepsin S, inflammation, glucometabolic disturbance, and its associated diseases in the community. As cathepsin S appears to be a novel risk marker for several pathological conditions, we also wanted to examine the effect of dietary intervention on circulating cathepsin S concentrations. This thesis is based on data from three community-based cohorts, the Uppsala longitudinal study of adult men (ULSAM), the prospective investigation of the vasculature in Uppsala seniors (PIVUS), and a post-hoc study from the randomized controlled NORDIET trial. In the first study, we identified a cross-sectional positive association between serum cathepsin S and two markers of cytokine-mediated inflammation, CRP and IL-6. These associations were similar in non-obese individuals. In longitudinal analyses, higher cathepsin S at baseline was associated with higher CRP and IL-6 levels after six years of follow-up. In the second study, we identified a cross-sectional association between increased serum levels of cathepsin S and reduced insulin sensitivity. These associations were similar in non-obese individuals. No significant association was observed between cathepsin S and insulin secretion. In longitudinal analysis, higher cathepsin S levels were associated with an increased risk of developing diabetes during the six-year follow-up. In the third study, we found that higher serum levels of cathepsin S were associated with increased mortality risk. Moreover, in the ULSAM cohort, serum cathepsin S was independently associated with cause-specific mortality from cardiovascular disease and cancer. In the fourth study, we identified that adherence to an ad libitum healthy Nordic diet for 6 weeks slightly decreased the levels of plasma cathepsin S in normal or marginally overweight individuals, relative to the control group. Changes in circulating cathepsin S concentrations were correlated with changes in body weight, LDL-C, and total cholesterol. Conclusion: This thesis shows that circulating cathepsin S is a biomarker that independently reflects inflammation, insulin resistance, the risk of developing diabetes, and mortality risk. Furthermore, a Nordic diet moderately reduced cathepsin S levels in normal-weight and overweight men and women. This effect may be partially mediated by diet-induced weight loss and possibly by reduced LDL-C concentrations.

epidemiology

cathepsin S

inflammation

insulin resistance

diabetes

mortality

cardiovascular mortality

cancer mortality

healthy Nordic diet.

Characterization of cathepsin b mrna and protein expression, enzymatic activity and cellular localization following contusion spinal cord injury in rats

Ellis, Rebecca Catherine,

January 2004

Thesis (Ph.D.)--University of Florida, 2004. / Typescript. Title from title page of source document. Document formatted into pages; contains 97 pages. Includes Vita. Includes bibliographical references.

Papel das proteases na erosão dentinária / The role of proteases on dental erosion

Bruno Lara Zarella

22 February 2017

Na dentina, a matriz orgânica desmineralizada tem um papel protetor contra desafios erosivos subsequentes. Porém, essa camada pode ser degradada por proteases, como as metaloproteinases da matriz (MMPs) e cisteína catepsinas (CCs). Recentemente, o uso de inibidores de proteases da matriz surgiu como uma importante ferramenta preventiva contra a erosão dentinária. Entretanto, o(s) mecanismo(s) exato(s) pelo(s) qual(is) os inibidores de proteases podem prevenir a erosão dentinária, bem como os tipos de proteases mais envolvidas neste processo ainda não são completamente conhecidos. O projeto foi desenvolvido em 2 subprojetos, com os seguintes objetivos: A)Subprojeto 1:Avaliar o papel das proteases na progressão da erosão dentária; B)subprojeto 2: Testar o potencial inibitório do NaF em CCs dentinárias. Para cumprir esses objetivos, foram utilizadas dentina de terceiros molares humanos para a preparação dos espécimes. A)Subprojeto1:Blocos de dentina (4 X 4 x 2 mm) (n=119) foram obtidos de raízes. Os espécimes foram divididos em 7 grupos de acordo com o seu tratamento (E-64, inibidor especifico II de catepsinas B, clorexidina, galardina NaF, placebo) ou sem tratamento, géis foram aplicados uma única vez sobre a superfície e feito o desafio erosivo (90s, 4x por dia por 5 dias) e feita analise perfilométrica. Os espécimes foram incubadas em solução contendo colagenase de Clostridium histolyticum tipo VII por 96hrs e então feita uma segunda analise perfilometrica para se determinar a espessura da MOD. Dois espécimes foram separados para análise de microscopia eletrônica de varredura. B)Subprojeto 2: Palitos de dentina (6 mm X 2 mm X 1 mm) (n=60) foram cortados da porção médio coronária dos dentes e completamente desmineralizados por imersão em EDTA 0,5 M (pH7,4) por 30 dias e lavados em água deionizada sob constante agitação a 4ºC por 72 h. Os espécimes foram divididos em 6 grupos (E-64, NaF e controle negativo, pH 5,5 ou 7,2) e incubados em saliva artificial contendo seus respectivos inibidores por 24 h 7 dias e 21 dias; ao termino de cada período, os espécimes eram pesados para avaliar a perda de massa e analisada a presença de CTX. A)Subprojeto 1: a perda de tecido desmineralizado (m, média± SD) foi: CHX 8,4±1,7b, Gala 8,6±1,9b, IECB 9,6±1,4a, E64 9,9±1,3a, NaF 9,9±1,7a, P 10,9±2,2a, ST 11,0±1,5a. A perda de tecido mineralizado foi: CHX 15,4±2,2b, Gala 16,0±1,8b, IECB 17,6±2,4a, E64 17,6±2,0a, NaF 17,3±2,8a, P 19,1±2,1a, ST 18,9±2,4a. Os inibidores de MMP reduziu significativamente a perda de matriz orgânica e tecido mineralizado em comparação com os outros grupos (p<0,05). Não foi achada diferença significante entre a espessura da matriz orgânica desmineralizada remanescente (p=0,845). B)Subprojeto 2: Na perda de massa houve diferença significante em relação ao inibidor (F=20,047, p<0,0001) e tempo de incubação (F=222,462, p<0,0001) com significante interação entre esses critérios, nos período de menor tempo de incubação, a perda foi similar para todos os grupos testados, no período de maior tempo de incubação, o grupo contendo NaF demostrou os melhores resultados. Na analise de CTX, houve diferença significante em relação aos inibidores (F46,543, p<0,0001), pH (F=14,836, p<0,0004) e tempo de incubação (F=161,438, p<0,0001) com significante interação entre esses critérios, como ocorrido na perda de massa, não houve diferença estatística nos períodos de menor incubação. No período de maior tempo de incubação, mais uma vez o grupo NaF mostrou os melhores resultados. No valor acumulado de CTX, os grupos E64 e controle negativo tiveram os maiores valores de CTX acumulado, o grupo NaF, independente do pH mostrou redução significante em relação aos demais grupos. Após analise dos resultados dos dois subprojetos, podemos indicar que as MMPs são as proteases de maior importância na progressão da erosão dentinária, assim, sua inibição é de maior importância para a redução desta patologia. Mesmo as CCs não exercendo papel direto para a progressão da erosão, elas são efetivas na cascata da ativação de outras proteases, como as próprias MMPs. Com isso, sua inibição também pode ser importante para a redução indireta da progressão da erosão. Neste presente estudo, pudemos comprovar que o NaF tem potencial inibitório sobre as CCs dentinárias, assim, sugerindo um novo inbidor de CCs. Com os resultados deste estudo, podemos afirmar que as MMPs são as principais proteases na progressão da erosão dentinária e que o NaF tem potencial inibitório nas CCs dentinárias. / In the dentine, the demineralized organic matrix has a protector part against the following erosive challenges. Nevertheless, this layer can be degraded by proteases, like the matrix metalloproteinases (MMPS) and cystein cathepsins (CCs). Recently, the use of proteases of the matrix´s inhibitors, emerged as an important preventive tool against the dentinária erosion. However, the exact mechanisms from which the inhibitors of the proteases may prevent the dentin erosion, as much as the kinds of proteases more involved in this process are not completely known yet. Therefore, the general objective of this project was to investigate the part of the two main proteases of the matrix (MMPs and CCs) in the dental erosion. The project was developed in 2 subprojects, with the following objectives: A)Subproject 1: Evaluate the part of the proteases in the progression of the dental erosion; B)subproject 2: To test the NaF inhibitory potencial in the dentin CCs. To accomplish these objectives, human third molar dentin were used for the preparation of the specimens, obtained in the surgery and urgency clinics of FOB-USP (subproject 1) or granted by the University of Oulu (subproject 2). A) Subproject 1: Dentine blocks 4 X 4 X 2 mm) (n=119) were obtained from the roots of the obtained teeth. The specimens were divided in 7 groups according with their treatment. Gels containing inhibitors (E-64, specific cathepsin B inhibitor II, chlorhexidine, galardin NaF, placebo), or without treatment, were produced, applied only one time over the surface and made the erosive challenge (90s, 4x a day for 5 days) and made profilometric analysis. The specimens were incubated in a solution containing collagenase of Clostridium histolyticum type VII for 96 hours and then a second profilometric analysis was made to determine the thickness of the MOD. Two specimens were separated for the electronic microscopy scan analysis. B) Subproject 2: Dentine sticks (6 mm X 2 mm X 1 mm) (n=60) were cut from the medium coronary portion of the teeth and completely demineralized by immersion in EDTA 0,5 M (pH7,4) ifor 30 days and washed in deionized water under constant agitation in 4º C for 72 hours. The specimens were divided in 6 groups (divided by inhibitors: E-64, NaF and negative control, pH 5,5 or 7,2) and incubated in artificial saliva containing their respective inhibitors for 24 hours, 7 days and 21 days; by the end of each period, the specimens were weighted to evaluate the loss of mass and analised the presence of CTX. A)Subproject 1: the loss of demineralized tissue (m, média± SD) was : CHX 8,4±1,7b, Gala 8,6±1,9b, IECB 9,6±1,4a, E64 9,9±1,3a, NaF 9,9±1,7a, P 10,9±2,2a, ST 11,0±1,5a. The loss of demineralized tissue was: CHX 15,4±2,2b, Gala 16,0±1,8b, IECB 17,6±2,4a, E64 17,6±2,0a, NaF 17,3±2,8a, P 19,1±2,1a, ST 18,9±2,4a. The MMP inhibitors reduced significantly the loss of organic matrix and demineralized tissue in comparison with other groups (p<0,05). There was no significant difference found between the thickness of the remaining demineralized organic matrix.(p=0,845). B)Subproject: In the loss of mass, there was a significant difference in relation to the inhibitor (F=20,047, p<0,0001) and incubation time (F=222,462, p<0,0001) with significant interaction between these criteria, in the periods of lesser time of incubation, the loss was similar for all the tested groups, in the period of higher time of incubation, the group containing NaF demonstrated the best results. In the analysis of CTX, there was significant difference in relation the inhibitors (F46,543, p<0,0001), pH (F=14,836, p<0,0004) and time of incubation (F=161,438, p<0,0001)with significant interaction between these criteria, as occurred in the mass loss, there was no statistic difference in the period of lesser incubation. In the period of higher time of incubation, once again, the NaF group demonstrated the best results. The CTX accumulated value, the E64 groups and negative control had the greater accumulated values of CTX, the NaF group, regardlessof the pH, demonstrated significant reduction in relation to the other groups. After the analysisof the results of both subprojects, we can indicate that the MMPs are the proteases of greater importance in the progression of the dentin erosion, thus, its inhibition is of graeter importance for the reduction of this pathology. Even the CCs don´t playing the part directly for the progression of erosion, they are effective in the cascade of the activation of other proteases, like the MMPs themselves. In this manner, its inhibition can also be important for the indirect reduction of the progression of the erosion. In this present study, we can prove that the NaF has inhibiting potential over the dentin CCs, thus, suggesting a new inhibitor of CCs. With the results of this study, we can affirm that the MMPs are the main proteases in the progression of the dentin erosion and that the NaF has inhibiting potential in the dentin CCs.

Cisteíno catepsinas

Dentina

Erosão dentária

Metaloproteinases da matriz

Cystein cathepsin

Dental erosion

Dentin

Matrix metalloproteinases

Inibição seletiva da catepsina S atenua ateroscleroses em camundongos deficientes na apolipoproteína e com doença renal crônica

FIGUEIREDO, Jose Luiz de

24 August 2015

Submitted by Irene Nascimento (irene.kessia@ufpe.br) on 2016-06-27T19:16:23Z No. of bitstreams: 2 license_rdf: 1232 bytes, checksum: 66e71c371cc565284e70f40736c94386 (MD5) José Luiz de Figueiredo_TESE DE DOUTORADO_SA.pdf: 20285168 bytes, checksum: 2ae5d11950e2cb6dc18e886511b1c189 (MD5) / Made available in DSpace on 2016-06-27T19:16:23Z (GMT). No. of bitstreams: 2 license_rdf: 1232 bytes, checksum: 66e71c371cc565284e70f40736c94386 (MD5) José Luiz de Figueiredo_TESE DE DOUTORADO_SA.pdf: 20285168 bytes, checksum: 2ae5d11950e2cb6dc18e886511b1c189 (MD5) Previous issue date: 2015-08-24 / Doença renal crônica acelera o desenvolvimento de ateroscleroses. A catepsina S é uma potente protease que quebra as fibras de elastina na parede das artérias e gera peptídeos bioativos de elastina, promovendo inflamação e calcificação vascular. Objetivo: Verificar os efeitos da inibição seletiva da catepsina S nas ateroscleroses de camundongos deficientes em apolipoproteína E (ApoE-/-) com doença renal crônica. Método: A doença renal crônica foi induzida por nefrectomia subtotal (5/6) em camundongos ApoE-/-, alimentados com uma dieta com alto teor de gorduras e colesterol. Os camundongos hipercolesterolêmicos, com doença renal crônica receberam essa dieta misturada com 6,6 ou 60 mg / kg do inibidor seletivo da catepsina S - RO5444101 ou a mesma dieta sem o inibidor seletivo da catepsina S (controle). Resultados: Camundongos com doença renal crônica tinham níveis plasmáticos significativamente mais elevados de osteopontina, osteocalcina e osteoprotegerina (204%, 148%, e 55%, respectivamente; p<0,05), que foram inibidos pelo RO5444101 (60%, 40%, e 36%, respectivamente; P<0,05). Imagens moleculares fluorescentes revelaram uma redução significativa na atividade da catepsina em camundongos tratados. O RO5444101 diminuiu também a atividade osteogênica. Avaliação histológica na placa aterosclerótica demonstrou que o RO5444101 reduziu a imunorreatividade da catepsina S (P<0,05), a degradação da elastina (P=0.01), o tamanho da placa (P=0.01), a acumulação de macrófagos (P<0,01), o fator de diferenciação do crescimento-15 (P=0.0001), a calcificação (atividade da fosfatase alcalina), P<0,01; e a osteocalcina, P<0,05). Além disso, o inibidor da catepsina S ou o siRNA significativamente diminuiu a expressão do fator de diferenciação do crescimento-15 e a proteína quimiotáctica de monócitos-1 numa linha de células de macrófagos de camundongos e macrófagos primários humanos. Conclusão: A inibição seletiva da catepsina S atenua a progressão de lesões ateroscleróticas em camundongos deficientes em apolipoproteína E com doença renal crônica. / Chronic kidney disease accelerates the development of atherosclerosis. Cathepsin S is a potent protease that cleaves elastin in the arteries wall and generates bioactive elastin peptides, promoting vascular inflammation and calcification. Objective: To verify the effects of selective inhibition of cathepsin S in atherosclerosis in apolipoprotein E deficient (ApoE-/-) mice with chronic kidney disease. Methods: chronic kidney disease was induced by a subtotal (5/6) nephrectomy in a high-fat high-cholesterol fed ApoE-/- mice. Hypercholesterolemic mice with CRD received a diet admixed with 6.6 or 60 mg/kg of the selective cathepsin S inhibitor RO5444101 or a diet without the selective inibidor of the catepsina S (control). Results: chronic kidney disease mice had significantly higher plasma levels of osteopontin, osteocalcin, and osteoprotegerin (204%, 148%, and 55%, respectively; P<0.05), which were inhibited by RO5444101 (60%, 40%, and 36%, respectively; P<0.05). Near-infrared fluorescence molecular imaging revealed a significant reduction in cathepsin activity in treated mice. RO5444101 decreased osteogenic activity. Histologic assessment in atherosclerotic plaque demonstrated that RO5444101 reduced immunoreactive cathepsin S (P<0.05), elastin degradation (P<0.01), plaque size (P<0.01), macrophage accumulation (P<0.01), growth differentiation factor-15 (P<0.0001), and calcification, alkaline phosphatase activity, (P<0.01); osteocalcin, (P<0.05). Furthermore, cathepsin S inhibitor or siRNA significantly decreased expression of growth differentiation factor-15 and monocyte chemotactic protein-1 in a murine macrophage cell line and human primary macrophages. Conclusion: The selective inhibition of cathepsin S attenuates the progression of atherosclerotic lesions in apolipoprotein E deficient mice with chronic kidney disease

Decreased expression of angiotensinogen and dipeptidyl peptidase 1 may be associated with the development of proliferative verrucous leukoplakia = Diminuição da expressão de angiotensinogênio e dipeptidil peptidase 1 pode estar associada ao desenvolvimento de leucoplasia verrucosa proliferativa / Diminuição da expressão de angiotensinogênio e dipeptidil peptidase 1 pode estar associada ao desenvolvimento de leucoplasia verrucosa proliferativa

Flores, Isadora Luana, 1984-

24 August 2018

Orientador: Marcio Ajudarte Lopes / Tese (doutorado) - Universidade Estadual de Campinas, Faculdade de Odontologia de Piracicaba / Made available in DSpace on 2018-08-24T18:31:33Z (GMT). No. of bitstreams: 1 Flores_IsadoraLuana_D.pdf: 2280685 bytes, checksum: 4c70e1fe2979897700a7a4161710b445 (MD5) Previous issue date: 2014 / Resumo: OBJETIVO: A leucoplasia verrucosa proliferativa (LVP) é uma variante rara e ainda pouco compreendida de leucoplasia oral com um comportamento de progressão persistente para malignidade apresentando uma taxa de malignização entre 40-100%. Além disso, a detecção precoce da LVP às vezes é um desafio para os clínicos, porém desempenha um papel crucial para estabelecer um contínuo e rigoroso acompanhamento. Aspectos moleculares subjacentes são relevantes e nenhum estudo anterior investigou a saliva de pacientes com LVP. O aumento do interesse no estudo do proteoma salivar ocorre porque as proteínas são consideradas as moléculas mais importantes do fluido salivar com potencial para atuar como biomarcador para o diagnóstico de várias doenças sistêmicas e locais. Com base nestes aspectos, o presente estudo teve como objetivo traçar o perfil do proteoma salivar de pacientes com LVP, a fim de identificar potenciais biomarcadores para a melhor compreensão desta entidade visando o possível uso clínico. MATERIAIS E MÉTODOS: A saliva total não estimulada foi coletada de 30 voluntários (15 pacientes com LVP e 15 controles). Uma abordagem proteômica baseada na associação de cromatografia líquida acoplada à espectrometria de massa foi realizada para análise de 20 µg de proteínas das amostras. Os testes de qui-quadrado, análise de variância e regressão logística foram utilizados na análise estatística. RESULTADOS: Um total de duzentas e oitenta e três proteínas foram identificadas. Entre estas, 31 proteínas apresentaram diferença estatisticamente significativa em relação à abundância, sendo 25 proteínas com maior abundância no grupo controle e 6 proteínas com maior abundância no grupo LVP. A combinação das proteínas angiotensinogênio e dipeptidil peptidase 1 criaram um modelo de diferenciação de grupo com um índice de concordância de 94,2% revelando ambas as proteínas como potenciais biomarcadores para o diagnóstico de LPV. CONCLUSÕES: Apesar deste estudo ser o primeiro a avaliar o proteoma salivar em pacientes com LVP, os resultados mostraram que a triagem da saliva pode ser um teste útil no diagnóstico de indivíduos com risco para o desenvolvimento de LPV / Abstract: OBJECTIVE: Proliferative verrucous leukoplakia (PVL) is a rare variant and still poorly understood of oral leukoplakia with a behavior of persistent progression to malignancy showing a rate of malignancy between 40-100%. Moreover, the early detection of PVL is sometimes challenging for clinicians, but plays a crucial role to establish a continuous and rigorous follow-up. Underlying molecular aspects are relevants and no previous study investigated the saliva of PVL patients. The increased interest in the salivary proteome study is because proteins are considered the most important molecules in the salivary fluid with potential to act as biomarker for diagnosis of various systemic and local diseases. Based on these aspects, the present study aimed to draw the salivary proteome profile of patients with PVL in order to identify potential biomarkers to better understanding of this entity targeting the possible clinical use. MATERIALS AND METHODS: Unstimulated whole-mouth saliva was collected of 30 voluntaries (15 PVL patients and 15 controls). Proteomic approach based to liquid chromatography coupled to tandem mass spectrometry was performed to 20 µg of proteins of the samples. Chi-Square, analysis of variance and logistic regression test were used in the statistical analysis. RESULTS: A total of two hundred eighty-three proteins were identified. Among of them, 31 proteins showed statistical significance difference in relation to abundance, being 25 proteins with higher abundance in control group and 6 proteins with higher abundance in PVL group. The combination of angiotensinogen and dipeptidyl peptidase 1 created a model for group differentiation with a concordance index of 94.2% revealing both proteins as potential biomarkers for diagnosis of PVL. CONCLUSIONS: Although this study is the first to evaluate the salivary proteome in PVL patients, the results showed that saliva screening may be helpful test to diagnosis of individuals with risk to PVL development / Doutorado / Patologia / Doutora em Estomatopatologia

Saliva

Angiotensinogênio

Catepsina C

Marcadores biológicos

Leucoplasia bucal

Saliva

Angiotensinogen

Cathepsin C

Biomarkers

Leukoplakia, oral

Regulation of UV induced apoptosis in human melanocytes

Bivik, Cecilia

January 2007

Malignant melanoma arises from the pigment producing melanocytes in epidermis and is the most aggressive type of skin cancer. The incidence of malignant melanoma is increasing faster than any other type of cancer in white population worldwide, with a doubling rate every 10-20 years. So far, the only identified external risk factor for malignant melanoma is UV exposure. Elimination of photodamaged cells by apoptosis (programmed cell death) is essential to prevent tumor formation. Melanocytes are considered relatively resistant to apoptosis, however, the regulation of apoptosis in melanocytes is still unknown. The aim of this thesis was to investigate the apoptotic process following ultraviolet (UV) irradiation in primary cultures of human melanocytes. Focus was on regulation of mitochondrial stability by Bcl-2 family proteins and the possible participation of lysosomal proteases, cathepsins. UV irradiation activated the mitochondrial pathway of apoptosis, leading to cytochrome c release, caspase activation, and nuclear fragmentation. No change in protein expression of Bax and Bcl-2 was observed in response to UV. Instead, translocation of the Bcl-2 family proteins from cytosol to mitochondia was important in the regulation of survival and death of melanocytes. The findings further demonstrated permeabilization of the lysosomal membrane to occur early in the apoptotic process, resulting in cathepsin release into the cytosol. The cathepsins were potent pro-apoptotic mediators and triggered apoptosis upstream of Bax translocation and mitochondrial membrane permeabilization. In response to both heat and UV irradiation, there was a marked increase in expression of stress-induced heat shock protein 70 (Hsp70), which inhibited apoptosis by binding lysosomal and mitochondrial membranes and counteracting the release of cathepsins and cytochrome c. Furthermore, UV irradiation activated c-jun N-terminal kinase (JNK), which triggered apoptosis upstream of cathepsins release from the lysosomes. In addition, JNK mediated apoptosis through phosphorylation of pro-apoptotic Bim, which was released from anti-apoptotic Mcl-1, by UV induced Mcl-1 depletion. This thesis illustrates that permeabilization of mitochondria and lysosomes and release of their constituents to the cytosol participates in UV induced apoptosis signaling in human melanocytes in vitro. The process is regulated by a complex network of pro- and anti-apoptotic proteins, exerting their effects through intracellular translocation and alteration of protein expression.

apoptosis

UV

melanocyte

lysosome

cathepsin

Bcl-2

Bax

Hsp70

JNK

Dermatology and Venereal Diseases

Dermatologi och venereologi

Enzymatic cleavage of HMGB1

Rensing, Merlin

January 2017

Alarmins and damage associated molecular pattern (DAMP) are endogenous proteins with distinct and various intracellular roles that when released extracellularly act as startingsignals for inflammatory immune responses. The endogenous protein High mobility group box 1 (HMGB1) acts as a DAMP and has been shown to drive progression of multiple inflammatory and autoimmune diseases. During homeostasis HMGB1 is localized in the nucleus of almost any cell, where its main function is organization of the DNA and regulation of transcription. Upon cell death or immune cell activation HMGB1 can be translocated into the cytoplasm for subsequent release into the extracellular space. Extracellular HMGB1 can act as a DAMP by activating several receptors of the immune system. Recent studies focus on HMGB1 release and functional regulation due to prost-translational modifications (PTMs) on cysteine residues. However, little is known about enzymatic regulation of HMGB1. The aim of this thesis was to investigate the possibility of proteolytic processing of HMGB1 by enzymes, which play a crucial role in inflammatory diseases and their progression. We utilized an in vitro model that mimics natural conditions of the autoimmune disease arthritis. Enzymatic digestion of HMGB1 was performed in kinetics studies using the neutrophilic enzymes cathepsin G, neutrophil Elastase as well as matrix metalloproteinase-3, which is released from tissues at the site of inflammation. We defined that HMGB1 is a novel substrate of all of the tested enzymes. All enzymes induced different cleavage pattern. In conclusion, my findings open up the possibility for future studies involving the observed fragments of HMGB1 and their functional features. It also demonstrated that HMGB1 is affected by protease modifications in a disease relevant environment.

HMGB1

enzymatic cleavage

neutrophil Elastase

cathepsin G

matrix metalloproteinase-3

arthritis

Biological Sciences

Biologiska vetenskaper

Diagnóstico, caracterização molecular e epidemiologia de Trypanosamas de ungulados. / Diagnosis, molecular characterization and epidemiology of Trypanosame of ungulates.

Herakles Antonio Garcia Perez

18 May 2012

Trypanosamas de diversas espécies podem infectar mamíferos de interesse econômico em todo o mundo. Trypanosoma vivax, T. evansi, T. equiperdum, T. congolense, T. b. brucei e T. simiae geram importantes doenças em ungulados na África, Ásia e Américas Central e do Sul; enquanto T. theileri e espécies relacionadas são pouco patogênicas. Compreender a epidemiologia e as interações parasita-vector-hospedeiro requer estudos de estrutura populacional, filogeográficos e de diversidade e relações filogenéticas entre isolados. Sequências de microssatelites e dos genes SSUrRNA, gGAPDH, CatL, ITS, SL, 5S, Cytb e ESAG6 mostraram ampla diversidade biológica e diferenciaram genótipos com associação geográfica e restrição de hospedeiros em T. theileri e espécies relacionadas. T. evansi mostrou importante heterogeneidade de sequências no gene ESAG6, enquanto populações de T. vivax muito divergentes foram observadas em regiões preservadas e com transmissão cíclica quando comparadas com a microheterogeneidade biológica de áreas de transmissão mecânica. / Trypanosames can infect diverse species of mammals of economic interest worldwide. Trypanosoma vivax, T. evansi, T. equiperdum, T. congolense, T. brucei brucei and T. simiae cause important diseases in ungulates in Africa, Asia and Central and South America, while T. theileri and related species are of low pathogenicity. Understanding the epidemiology and host-parasite-vector interactions requires studies of population structure, phylogeography and diversity and phylogenetic relationships among isolates. Microsatellite loci and sequences from genes SSUrRNA, gGAPDH, CatL, ITS, SL, 5S, Cytb and ESAG6 revealed high biological diversity and allowed differentiation of genotypes with geographic structure and host-restriction event in T. theileri and related species. T. evansi showed significant heterogeneity in ESAG6 sequences, while populations of T. vivax widely divergent were observed in pristine regions and cyclical transmission compared to the microheterogeneity showed by isolates from mechanical transmission areas.

Trypanosamas

Catepsina

Diagnóstico

Filogenia

Genótipos

Marcador molecular

Ungulata

Trypanosame

Cathepsin

Diagnostics

Genotypes

Molecular marker

Phylogeny

Ungulata