Papel da BjcuL, uma lectina isolada do veneno da serpente Bothrops jararacussu, na resposta imunológica mediada por linfócitos T

Pires, Weverson Luciano, 69-99917-3886

05 December 2017

Submitted by Divisão de Documentação/BC Biblioteca Central (ddbc@ufam.edu.br) on 2018-04-11T12:55:56Z No. of bitstreams: 2 license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) Reprodução Não Autorizada.pdf: 47716 bytes, checksum: 0353d988c60b584cfc9978721c498a11 (MD5) / Approved for entry into archive by Divisão de Documentação/BC Biblioteca Central (ddbc@ufam.edu.br) on 2018-04-11T12:56:11Z (GMT) No. of bitstreams: 2 license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) Reprodução Não Autorizada.pdf: 47716 bytes, checksum: 0353d988c60b584cfc9978721c498a11 (MD5) / Made available in DSpace on 2018-04-11T12:56:11Z (GMT). No. of bitstreams: 2 license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) Reprodução Não Autorizada.pdf: 47716 bytes, checksum: 0353d988c60b584cfc9978721c498a11 (MD5) Previous issue date: 2017-12-05 / FAPERO - Fundação Rondônia de Amparo ao Desenvolvimento das Ações Científicas e Tecnológicas e à Pesquisa do Estado de Rondônia / BjcuL is a type C lectin that depends on calcium ions to develop its biological activities. This protein is composed of two identical subunits that constitute the homodimer molecular structure. BjcuL has specificity for carbohydrate binding through its CDR region and exhibits hemagglutinating activity, inhibits proliferation of tumor cells, as well as the formation of bacterial biofilms. The purpose of this study was to investigate the effect of BjcuL under the human T lymphocyte mediated immune response and its different subpopulations. Results showed that BjcuL is not toxic to PBMCs and also does not exert mitogenic activity on these cells at concentrations of 5 and 10 μg/mL which can be regulated by the reactive oxygen species (ROS). The data evidenced that T lymphocytes are the cells responsible for ROS production induced by BjcuL, which contributes to the non-mitogenic activity for this lectin. BjcuL-FITC interacted with monocytes, B lymphocytes, Natural Killer cells and with subpopulations of T lymphocytes. The result of this interaction was the cellular activation that induced the production of pro-inflammatory cytokines such as IL-6 and TNF-α, and antiinflammatory cytokine such as IL-10. In addition, the data showed that the cells responsible for TNF-α production are mainly Natural Killer cells and monocytes, whereas IL-10 is produced by CD4+ T cells and Treg lymphocytes when stimulated by BjcuL. The cytokine profile produced by the cells when stimulated by this lectin allows us to confirm that BjcuL develops immunomodulatory activity. The results obtained may serve as a basis for the development of new drugs of clinical interest and as tools for biotechnological prospecting. / A BjcuL é uma lectina do tipo C que depende de íons cálcio para desenvolver suas atividades biológicas. Essa proteína é composta por duas subunidades idênticas que constituem a estrutura molecular de homodímero. A BjcuL tem especificidade para ligação a carboidratos por meio de sua região CDR, apresenta atividade hemaglutinante, inibe a proliferação de células tumorais, e a formação de biofilmes bacterianos. O objetivo deste estudo foi investigar os efeitos da BjcuL sob a resposta imunológica mediada por linfócitos T humanos e suas diferentes subpopulações. Os resultados mostraram que a BjcuL não é tóxica para os PBMCs e também não exerce atividade mitogênica sobre essas células, nas concentrações de 5 e 10 μg/mL, os quais podem ser regulados pela produção de espécies reativas do oxigênio (EROS). Os dados evidenciaram que os linfócitos T são as células responsáveis pela produção de EROS induzidas por BjcuL, contribuindo para a atividade não mitogênica dessa lectina. A BjcuL acoplada ao FITC interagiu com monócitos, linfócitos B, células Natural Killer e também com subpopulações de linfócitos T. O resultado dessa interação foi a ativação celular que induziu a produção de citocinas pró-inflamatórias como IL-6 e TNF-α, e antiinflamatórias como IL-10. Além disso, os dados mostraram que as células responsáveis pela produção de TNF-α são as células Natural Killer e os monócitos. A IL-10 é produzida pelas células T CD4+ e pelos linfócitos Treg, quando estimuladas pela BjcuL. O perfil de citocinas produzidas pelas células quando estimuladas por essa lectina permite afirmar que a BjcuL desenvolve atividade imunomoduladora. Os resultados obtidos poderão servir de base para o desenvolvimento de novos farmacos com interesse clínico e como ferramentas de prospecção biotecnológica.

Lectina

BjcuL

PBMCs

Proliferação

Linfócitos

Imunoregulação

CIENCIAS BIOLOGICAS

Expressão gênica de FOXP3, indoleamina 2,3 dioxigenase, IL10 e CSF1 em útero de vacas que receberam infusão intrauterina de antígenos maternos e paternos no período peri-ovulatório

Junqueira, Talita Vieta

05 October 2015

In cattles, most of pregnancy losses occurs at the beginning of gestation, notably from the 7th to the 16th day of the cycle, a period in which, the embryo depends entirely on the uterine environment to survive and to start their preimplantation growth. During this period, the embryonic death after embryo transfers performed in vitro (TE-IVP) or in vivo (TE-OM) is on average nearly twice as high as that produced by natural mating or artificial insemination (AI). The recipient sensitization against the paternal and maternal MHC molecules of allogeneic embryo might be one of the causes of high rates of pregnancy loss observed after TE. Studies in humans and in various species have pointed that the sensitization with conceptus antigens may affect the reproductive performance facilitating the recognition and the maternal acceptance of allogeneic embryo through induction of cytokyne and immunoregulatory cells in the the uterine microenvironment. The purpose of this study is to determine whether simultaneous or separate administration of paternal and maternal antigens in the uterus of the cows embryo recipientes, during the estrus, increases the expression of genes which can facilitate recognition and development of allogeneic embryos during early pregnancy. Forty-five crossbed cows were evaluated. The animals were divided in four treatments: T0: control; T1: Semen; T2: PBMCs and T3: PBMCs+Semen. The cows were estrus synchronized and received antigens in the uterine body on the estrus day. Uterine biopsies were collected in vivo on D0 for control, and after seven (D7) and fourteen (D14) days after the estrus and administration of antigens in order to evaluate the treatment effect on the uterine environment of the receiving at the moment of the anovoluation procedure would occur in TE-IVP, and during the period in which the bovine embryo would have their preimplantation growth, respectively. The gene expression was evaluated in real time PCR, and then transcribed from FOXP3, IDO, IL-10 and CSF-1 were detected in all RNA samples extracted from uterine biopsies. Semiquantitative analyses of relative gene expression among the control and the treat groups demonstrated that none of the treatments significantly incresed those gene expressions. Furthermore, at D14 all the treatments leaded to a decline in amount CSF-1 transcripts and, further, treatment with both antigens also to a drop in the abundance of IL-10 transcripts. In conclusion, the isolated or simultaneous antigens admnistration in the in the uterus of IVP embryo recipient cows seems not to increase the maternal tolerance to alloantigens embryo nor benefit conditions for their growth and preimplantation development, at least with regard to the effect mediated by FOXP3, IDO, IL- 10 and CSF-1 on D7 and D14 in the estrous cycle. / A maioria das perdas gestacionais em bovinos acontece no início da gestação, particularmente entre os dias 7 e 16, período no qual o embrião é totalmente dependente do ambiente uterino para sobreviver e iniciar seu crescimento pré-implantação. Durante esse período, a mortalidade embrionária após transferência de embriões produzidos in vitro (TEPIV) ou in vivo (TE-OM) é em média quase duas vezes mais elevada do que aquela derivada de embriões originados de monta natural ou inseminação artificial (IA). A sensibilização da receptora contra as moléculas MHC paternas e maternas do embrião alogênico pode ser uma das causas das altas taxas de perdas gestacionais observadas após TE. Estudos realizados em humanos e em várias espécies têm demonstrado que a sensibilização com antígenos do concepto pode ser uma maneira útil de afetar o desempenho reprodutivo facilitando o reconhecimento e a aceitação materna do embrião alogênico através da indução de citocinas e células imunorregulatórias no microambiente uterino. Nesse sentido, o presente estudo teve como foco principal determinar se a administração simultânea ou isolada de antígenos paterno e materno no útero de fêmeas bovinas receptoras de embrião PIV, no dia do estro, aumenta a expressão de genes que podem facilitar o reconhecimento e desenvolvimento do embrião alogênico durante o início da gestação. Para isto, foram utilizadas 45 vacas cruzadas divididas em 4 tratamentos: T0: controle; T1: Sêmen; T2: PBMCs e T3: PBMCs+Sêmen. As fêmeas bovinas foram sincronizadas ao estro e receberam os antígenos no corpo uterino no dia do cio (D0). Biópsias uterinas foram coletadas in vivo no D0, para controle, e 7 (D7) e 14 (D14) dias após o cio e a administração dos antígenos, para avaliar o efeito do tratamento no ambiente uterino da receptora no momento em que ocorreria o procedimento de anovulação em TE-PIV e durante o período no qual o embrião bovino já teria iniciado seu crescimento préimplantação, respectivamente. A expressão gênica foi avaliada por PCR em tempo real e transcritos de FOXP3, IDO, IL-10 e CSF-1 foram detectados em todas as amostras de RNA extraídas das biópsias uterinas. A análise semiquantitativa da expressão gênica relativa entre os grupos controle e tratado mostrou que nenhum dos tratamentos promoveu aumento significativo na expressão desses genes. Além disso, no D14 todos os tratamentos promoveram uma queda na quantidade de transcritos de CSF-1 e, ainda, o tratamento com ambos os antígenos também promoveu uma queda na abundância de transcritos de IL-10. Em conclusão, a administração isolada ou simultânea de ambos os antígenos no útero de vacas receptoras de embrião PIV parece não propiciar aumento da tolerância materna aos aloantígenos do embrião nem condições favoráveis a seu crescimento e desenvolvimento préimplantação, pelo menos no que se refere ao efeito mediado por FOXP3, IDO, IL-10 e CSF-1 no D7 e D14 do ciclo estral. / Mestre em Biologia Celular e Estrutural Aplicadas

Indução imunológica

PBMCs

Sêmen

Citologia

Bovino - Imunologia

Immunologic Induction

PBMCs

Semen

Macrophage Migration Inhibitory Factor Polymorphisms and Invasive Streptoccus Pneumoniae Infections

Doernberg, Sarah Beth

03 November 2006

Streptococcus pneumoniae[italicized everytime] (S. pneumoniae) causes a spectrum of disease severity, and human host factors likely play a role in this variation. One candidate factor is macrophage migration inhibitory factor (MIF), a pro-inflammatory cytokine and upstream regulator of innate immunity. The MIF[italicized when not in parenthesis] promoter contains two functional polymorphisms, a tetranucleotide (CATT) repeat such that MIF expression increases with repeat number from 5-8 and a single nucleotide polymorphism (SNP) leading to a G-to-C transition, which results in increased MIF expression in cell line reporter assays. Emerging data suggest an association between high-expression MIF alleles and inflammatory disease. This study comprised two parts. For the in vitro portion, we hypothesized that peripheral blood monocytic cells (pBMCs) cultured from healthy individuals with low-expressing MIF genotypes (5-CATT alleles or SNP-GG) would have lower MIF content and release than those from individuals with high-expressing MIF genotypes (7-CATT or SNP-C alleles). For the in vivo study, we hypothesized that individuals with low-expressing MIF genotypes would have less severe systemic inflammatory responses than individuals with high-expressing MIF genotypes in response to S. pneumoniae infection. Blood samples and chart findings were collected prospectively at three Connecticut hospitals from 30 inpatients with documented invasive S. pneumoniae infections. Genomic DNA was isolated from host blood, amplified, and genotyped using fragment analysis (CATT repeat) and allelic discrimination (SNP) methods. Fishers exact tests were used to compare genotypes and disease severity. For the in vitro experiments, there were no differences observed in serum MIF levels or MIF content or release from pBMCs based on MIF genotype. In the cohort of patients infected with S. pneumoniae, serum MIF levels among enrolled subjects were significantly higher than the reported normal values, but levels did not vary with genotype or disease severity. The SNP genotype was not correlated with disease severity or occurrence of meningitis. The CATT genotype did not correlate significantly with disease severity or occurrence of meningitis, although there was a trend suggesting an association between the 7-CATT allele and meningitis (p = 0.1188, 8% without meningitis had a 7-CATT allele vs. 40% with meningitis). More patient samples will need to be analyzed in order to definitively elucidate the role of MIF genetics in infection with S. pneumoniae

S. pneumoniae

streptococcus pneumoniae

macrophage migration-inhibitory factor

MIF

peripheral blood monocytic cells

pBMCs

A functional genomic model for predicting prognosis in idiopathic pulmonary fibrosis

Huang, Yong, Ma, Shwu-Fan, Vij, Rekha, Oldham, Justin M., Herazo-Maya, Jose, Broderick, Steven M., Strek, Mary E., White, Steven R., Hogarth, D. Kyle, Sandbo, Nathan K., Lussier, Yves A., Gibson, Kevin F., Kaminski, Naftali, Garcia, Joe G.N., Noth, Imre

January 2015

BACKGROUND: The course of disease for patients with idiopathic pulmonary fibrosis (IPF) is highly heterogeneous. Prognostic models rely on demographic and clinical characteristics and are not reproducible. Integrating data from genomic analyses may identify novel prognostic models and provide mechanistic insights into IPF. METHODS: Total RNA of peripheral blood mononuclear cells was subjected to microarray profiling in a training (45 IPF individuals) and two independent validation cohorts (21 IPF/10 controls, and 75 IPF individuals, respectively). To identify a gene set predictive of IPF prognosis, we incorporated genomic, clinical, and outcome data from the training cohort. Predictor genes were selected if all the following criteria were met: 1) Present in a gene co-expression module from Weighted Gene Co-expression Network Analysis (WGCNA) that correlated with pulmonary function (p < 0.05); 2) Differentially expressed between observed "good" vs. "poor" prognosis with fold change (FC) >1.5 and false discovery rate (FDR) < 2 %; and 3) Predictive of mortality (p < 0.05) in univariate Cox regression analysis. "Survival risk group prediction" was adopted to construct a functional genomic model that used the IPF prognostic predictor gene set to derive a prognostic index (PI) for each patient into either high or low risk for survival outcomes. Prediction accuracy was assessed with a repeated 10-fold cross-validation algorithm and independently assessed in two validation cohorts through multivariate Cox regression survival analysis. RESULTS: A set of 118 IPF prognostic predictor genes was used to derive the functional genomic model and PI. In the training cohort, high-risk IPF patients predicted by PI had significantly shorter survival compared to those labeled as low-risk patients (log rank p < 0.001). The prediction accuracy was further validated in two independent cohorts (log rank p < 0.001 and 0.002). Functional pathway analysis revealed that the canonical pathways enriched with the IPF prognostic predictor gene set were involved in T-cell biology, including iCOS, T-cell receptor, and CD28 signaling. CONCLUSIONS: Using supervised and unsupervised analyses, we identified a set of IPF prognostic predictor genes and derived a functional genomic model that predicted high and low-risk IPF patients with high accuracy. This genomic model may complement current prognostic tools to deliver more personalized care for IPF patients.

Idiopathic pulmonary fibrosis (IPF)

Gene expression profiling

Functional genomic model

Prognosis prediction

Efeito da atorvastatina sobre a atividade funcional e expressão de transportadores de membrana do tipo ABC e SLC / Effect of atorvastatin on the activity and expression of ABC and SLC membrane transporters.

Rodrigues, Alice Cristina

12 September 2008

Os transportadores de membrana do tipo ATP Binding Cassette (ABC) e solute carriers (SLC) regulam a homeostase intracelular de fármacos, modificando a biodisponibilidade e possivelmente a eficácia terapêutica. A variabilidade na resposta a hipolipemiantes, como as vastatinas, tem sido associada a vários fatores genéticos e ambientais. Com a finalidade de avaliarmos os mecanismos de regulação da expressão dos transportadores pela atorvastatina, a expressão de RNAm de transportadores ABC (ABCB1, ABCG2 e ABCC2) e SLC (SLCO1B1, SLCO2B1 e SLC22A1) foi avaliada por RT-PCRq em células mononucleares do sangue periférico (CMSP) de 18 indivíduos normolipidêmicos (NL) e 22 pacientes hipercolesterolêmicos (HC) tratados com atorvastatina (10mg/dia/4 semanas). A possível associação entre o polimorfismo ABCB1 C3435T e a expressão de RNAm também foi avaliada. Os estudos in vitro foram realizados com as células das linhagens HepG2 e Caco-2. Foram avaliados os efeitos da atorvastatina na ativação de fatores de transcrição (NF-kappaB, NF-Y, c-jun, SP-1 e PXR) por ensaio de mobilidade eletroforética retardada em gel de poliacrilamida (EMSA) e na meia-vida do RNAm do gene ABCB1 por RT-PCRq, e a expressão e atividade funcional da proteína ABCB1 por Western blot, imunohistoquimica e citometria de fluxo. A proteina ABCB1 foi localizada por imunohistoquimica na membrana apical do canalículo biliar das celulas HepG2 e na membrana apical das Caco-2. O tratamento das células HepG2 com atorvastatina causou redução da expressão de RNAm do gene ABCB1 e aumento na expressão dos genes ABCG2 e ABCC2. Esses efeitos foram dose e tempo dependentes. O tratamento com atorvastatina das células Caco-2 não modificou a expressão dos transportadores de efluxo após 30 a 120 min. Nas células HepG2, as concentrações de 10 e 20 M de atorvastatina causaram diminuição da expressão de ABCB1 (0 &#181;M: 1,00 ± 0,06; 10 &#181;M: 0,69 ± 0,25, p< 0,05; 20 &#181;M: 0,69 ± 0,06, p< 0,05). A atividade da ABCB1, avaliada pelo efluxo de Rh123, mostrou-se estar reduzida em 41% nas células HepG2, após tratamento com atorvastatina 20 &#181;M. Embora a diminuição da expressão do ABCB1 não tenha sido decorrente de uma menor ativação transcricional, avaliada indiretamente por EMSA, estudos de mecanismos de regulação pós-transcricionais, revelaram que a atorvastatina diminui a estabilidade de RNAm do gene ABCB1. Esse resultado parece estar de acordo com o ocorrido nas CMSP, já que o tratamento com atorvastatina diminuiu a expressão de RNAm do gene ABCB1 nos indivíduos HC. Essa modulação, no entanto não está associada à presença do polimorfismo ABCB1 C3435T. Em relação aos transportadores de captação, a expressão do SLC22A1 nas células Caco-2 diminui após tratamento com atorvastatina por 30 min e não foi modificada nas células HepG2. Já o gene SLCO2B1 encontrou-se muito aumentado após 24 h de tratamento nas células HepG2. Estudos in vivo nas CMSP, mostrou que a expressão de mRNA basal dos transportadores nos HC foi 10 vezes maior que nos NL e diminuiu após tratamento com atorvastatina nos HC. Com os resultados obtidos podemos sugerir que diferenças no efeito da atorvastatina nos tipos celulares podem ser em decorrência da expressão tecido-específica de fatores de transcrição. No modelo de hepatócito, HepG2, a atorvastatina é um inibidor do transporte mediado pela ABCB1 e é capaz de diminuir a síntese e a função da ABCB1, via aumento da degradação de RNAm do gene ABCB1. Em conseqüência ocorre uma redução do efluxo pelo sistema biliar, causando aumento da concentração intracelular. Ainda, podemos concluir que em CMSP o colesterol pode ser o responsável pela modulação dos genes dos transportadores de membrana e que isso pode implicar em diferenças na eficácia da atorvastatina. / Specific membrane transporters have a significant impact on drug absorption and disposition. Most of them belong to two super-families, ABC (ATP-binding cassette) and SLC (solute-linked carrier). Statins are important therapeutic agents in the management of hypercholesterolemia, and considerable inter-individual variation exists in response to its therapy. The effects of atorvastatin expression of efflux (ABCG2 and ABCC2) and uptake (SLCO1B1, SLCO2B1 and SLC22A1) drug transporters were investigated by qPCR in Caco-2 and HepG2 cell lines and in peripheral blood mononuclear cells (PBMCs) of eighteen normolipidemic (NL) and twenty two hypercholesterolemic (HC) individuals treated with atorvastatin (10mg/day/4 weeks). The possible involvement of ABCB1 C3435T polymorphism in ABCB1 mRNA expression was also evaluated. In vitro studies with the cell lines HepG2 and Caco-2 were also performed. The effect of atorvastatin on the activation of the promoter of ABCB1 by transcription factors (NF-kappaB, NF-Y, c-jun, SP-1, and PXR) was evaluated by electrophoretic mobility shift assay (EMSA), and ABCB1 mRNA half-life were measured by PCRq. The expression and functional activity of ABCB1 were investigated by Western blot, imunohistochemistry and flow cytometry. Immunohystochemical analysis revealed that ABCB1 is located at the apical membrane of the bile canaliculi in HepG2, and in apical membrane of Caco-2 cells. Atorvastatin treatment of HepG2 cells caused a decreased in ABCB1 and an increase in ABCC2 and ABCG2 transcript levels. These effects were time and dose-dependent. Treatment of Caco-2 cells did not present any differences in efflux transporters mRNA levels. Treatment of HepG2 cells with 10 and 20 M atorvastatin caused a reduction on ABCB1 expression (0 &#181;M: 1,00 ± 0,06; 10 &#181;M: 0,69 ± 0,25, p< 0,05; 20 &#181;M: 0,69 ± 0,06, p< 0,05), and a 41% decrease in ABCB1-mediated efflux of Rhodamine123 (p < 0.01). Although reduced ABCB1 mRNA expression was not due to any repressor protein suppressing ABCB1 promoter activation, mRNA stability studies revealed that mRNA stability of ABCB1 was markedly decreased by atorvastatin treatment (2h versus 7h for control). In agrrement with these results, in PBMCs of HC individuals, atorvastatin treatment also reduced ABCB1 mRNA expression. However, the down-regulation was not associated with the presence of 3435T allele. For the uptake transporters, atorvastatin decreased SLC22A1 transcript levels after 30min-treatment and it was not regulated in HepG2. On the other hand, SLCO2B1 was up-regulated after 24h-treatment of HepG2 cells. In vivo studies with PBMCs revealed that during hypercholesterolemia all the drug transporters analyzed were increased almost 10-fold (p< 0.05), and after atorvastatin therapy the efflux and uptake transporters transcript levels were all down-regulated. These findings suggest that atorvastatin exhibits differential effects on mRNA expression of drug transporters depending on the cell type, which may be related to tissue-specific expression of transcription factors. Atorvastatin leads to decreased ABCB1 function and synthesis in HepG2 cells by increasing degradation of ABCB1 mRNA. Therefore, inhibition of ABCB1 may reduce atorvastatin elimination via bile, increasing its cellular concentrations. We also may suggest that in PBMCs cholesterol modulates mRNA expression of drug transporters, and this may contribute to the variability of response to atorvastatin.

ABC transporters

Atorvastatin

Atorvastatina

Caco-2

Caco-2

CMSP

HepG2

HepG2

Hipercolesterolemia

Hypercholesterolemia

Lipídeos

Lipids

PBMCs

SLC transporters

Transportadores ABC

Transportadores SLC

Efeito da atorvastatina sobre a atividade funcional e expressão de transportadores de membrana do tipo ABC e SLC / Effect of atorvastatin on the activity and expression of ABC and SLC membrane transporters.

Alice Cristina Rodrigues

12 September 2008

Os transportadores de membrana do tipo ATP Binding Cassette (ABC) e solute carriers (SLC) regulam a homeostase intracelular de fármacos, modificando a biodisponibilidade e possivelmente a eficácia terapêutica. A variabilidade na resposta a hipolipemiantes, como as vastatinas, tem sido associada a vários fatores genéticos e ambientais. Com a finalidade de avaliarmos os mecanismos de regulação da expressão dos transportadores pela atorvastatina, a expressão de RNAm de transportadores ABC (ABCB1, ABCG2 e ABCC2) e SLC (SLCO1B1, SLCO2B1 e SLC22A1) foi avaliada por RT-PCRq em células mononucleares do sangue periférico (CMSP) de 18 indivíduos normolipidêmicos (NL) e 22 pacientes hipercolesterolêmicos (HC) tratados com atorvastatina (10mg/dia/4 semanas). A possível associação entre o polimorfismo ABCB1 C3435T e a expressão de RNAm também foi avaliada. Os estudos in vitro foram realizados com as células das linhagens HepG2 e Caco-2. Foram avaliados os efeitos da atorvastatina na ativação de fatores de transcrição (NF-kappaB, NF-Y, c-jun, SP-1 e PXR) por ensaio de mobilidade eletroforética retardada em gel de poliacrilamida (EMSA) e na meia-vida do RNAm do gene ABCB1 por RT-PCRq, e a expressão e atividade funcional da proteína ABCB1 por Western blot, imunohistoquimica e citometria de fluxo. A proteina ABCB1 foi localizada por imunohistoquimica na membrana apical do canalículo biliar das celulas HepG2 e na membrana apical das Caco-2. O tratamento das células HepG2 com atorvastatina causou redução da expressão de RNAm do gene ABCB1 e aumento na expressão dos genes ABCG2 e ABCC2. Esses efeitos foram dose e tempo dependentes. O tratamento com atorvastatina das células Caco-2 não modificou a expressão dos transportadores de efluxo após 30 a 120 min. Nas células HepG2, as concentrações de 10 e 20 M de atorvastatina causaram diminuição da expressão de ABCB1 (0 &#181;M: 1,00 ± 0,06; 10 &#181;M: 0,69 ± 0,25, p< 0,05; 20 &#181;M: 0,69 ± 0,06, p< 0,05). A atividade da ABCB1, avaliada pelo efluxo de Rh123, mostrou-se estar reduzida em 41% nas células HepG2, após tratamento com atorvastatina 20 &#181;M. Embora a diminuição da expressão do ABCB1 não tenha sido decorrente de uma menor ativação transcricional, avaliada indiretamente por EMSA, estudos de mecanismos de regulação pós-transcricionais, revelaram que a atorvastatina diminui a estabilidade de RNAm do gene ABCB1. Esse resultado parece estar de acordo com o ocorrido nas CMSP, já que o tratamento com atorvastatina diminuiu a expressão de RNAm do gene ABCB1 nos indivíduos HC. Essa modulação, no entanto não está associada à presença do polimorfismo ABCB1 C3435T. Em relação aos transportadores de captação, a expressão do SLC22A1 nas células Caco-2 diminui após tratamento com atorvastatina por 30 min e não foi modificada nas células HepG2. Já o gene SLCO2B1 encontrou-se muito aumentado após 24 h de tratamento nas células HepG2. Estudos in vivo nas CMSP, mostrou que a expressão de mRNA basal dos transportadores nos HC foi 10 vezes maior que nos NL e diminuiu após tratamento com atorvastatina nos HC. Com os resultados obtidos podemos sugerir que diferenças no efeito da atorvastatina nos tipos celulares podem ser em decorrência da expressão tecido-específica de fatores de transcrição. No modelo de hepatócito, HepG2, a atorvastatina é um inibidor do transporte mediado pela ABCB1 e é capaz de diminuir a síntese e a função da ABCB1, via aumento da degradação de RNAm do gene ABCB1. Em conseqüência ocorre uma redução do efluxo pelo sistema biliar, causando aumento da concentração intracelular. Ainda, podemos concluir que em CMSP o colesterol pode ser o responsável pela modulação dos genes dos transportadores de membrana e que isso pode implicar em diferenças na eficácia da atorvastatina. / Specific membrane transporters have a significant impact on drug absorption and disposition. Most of them belong to two super-families, ABC (ATP-binding cassette) and SLC (solute-linked carrier). Statins are important therapeutic agents in the management of hypercholesterolemia, and considerable inter-individual variation exists in response to its therapy. The effects of atorvastatin expression of efflux (ABCG2 and ABCC2) and uptake (SLCO1B1, SLCO2B1 and SLC22A1) drug transporters were investigated by qPCR in Caco-2 and HepG2 cell lines and in peripheral blood mononuclear cells (PBMCs) of eighteen normolipidemic (NL) and twenty two hypercholesterolemic (HC) individuals treated with atorvastatin (10mg/day/4 weeks). The possible involvement of ABCB1 C3435T polymorphism in ABCB1 mRNA expression was also evaluated. In vitro studies with the cell lines HepG2 and Caco-2 were also performed. The effect of atorvastatin on the activation of the promoter of ABCB1 by transcription factors (NF-kappaB, NF-Y, c-jun, SP-1, and PXR) was evaluated by electrophoretic mobility shift assay (EMSA), and ABCB1 mRNA half-life were measured by PCRq. The expression and functional activity of ABCB1 were investigated by Western blot, imunohistochemistry and flow cytometry. Immunohystochemical analysis revealed that ABCB1 is located at the apical membrane of the bile canaliculi in HepG2, and in apical membrane of Caco-2 cells. Atorvastatin treatment of HepG2 cells caused a decreased in ABCB1 and an increase in ABCC2 and ABCG2 transcript levels. These effects were time and dose-dependent. Treatment of Caco-2 cells did not present any differences in efflux transporters mRNA levels. Treatment of HepG2 cells with 10 and 20 M atorvastatin caused a reduction on ABCB1 expression (0 &#181;M: 1,00 ± 0,06; 10 &#181;M: 0,69 ± 0,25, p< 0,05; 20 &#181;M: 0,69 ± 0,06, p< 0,05), and a 41% decrease in ABCB1-mediated efflux of Rhodamine123 (p < 0.01). Although reduced ABCB1 mRNA expression was not due to any repressor protein suppressing ABCB1 promoter activation, mRNA stability studies revealed that mRNA stability of ABCB1 was markedly decreased by atorvastatin treatment (2h versus 7h for control). In agrrement with these results, in PBMCs of HC individuals, atorvastatin treatment also reduced ABCB1 mRNA expression. However, the down-regulation was not associated with the presence of 3435T allele. For the uptake transporters, atorvastatin decreased SLC22A1 transcript levels after 30min-treatment and it was not regulated in HepG2. On the other hand, SLCO2B1 was up-regulated after 24h-treatment of HepG2 cells. In vivo studies with PBMCs revealed that during hypercholesterolemia all the drug transporters analyzed were increased almost 10-fold (p< 0.05), and after atorvastatin therapy the efflux and uptake transporters transcript levels were all down-regulated. These findings suggest that atorvastatin exhibits differential effects on mRNA expression of drug transporters depending on the cell type, which may be related to tissue-specific expression of transcription factors. Atorvastatin leads to decreased ABCB1 function and synthesis in HepG2 cells by increasing degradation of ABCB1 mRNA. Therefore, inhibition of ABCB1 may reduce atorvastatin elimination via bile, increasing its cellular concentrations. We also may suggest that in PBMCs cholesterol modulates mRNA expression of drug transporters, and this may contribute to the variability of response to atorvastatin.

Atorvastatina

Caco-2

CMSP

HepG2

Hipercolesterolemia

Lipídeos

Transportadores ABC

Transportadores SLC

ABC transporters

Atorvastatin

Caco-2

HepG2

Hypercholesterolemia

Lipids

PBMCs

SLC transporters

Assessment of the Active Kinome Profile in Peripheral Blood Mononuclear Cells in Renal Transplant Patients

Shedroff, Elizabeth Sarah

28 July 2022

No description available.

Bioinformatics

Biomedical Research

Immunology

Medicine

Molecular Biology

Statistics

kinome

kinomics

transcriptomics

RNAseq

pathway analysis

bioinformatics

PLS-DA

machine learning

PBMCs

renal transplant

immunosuppression

Η συσχέτιση των τελικών προϊόντων προχωρημένης γλυκοζυλίωσης (AGEs), του υποδοχέα τους (RAGE) και του διαλυτού τμήματός του (sRAGE) σε παιδιά, εφήβους και νεαρούς ενήλικες με σακχαρώδη διαβήτη τύπου 1 (ΣΔ1) / Association between advanced glycation endproducts (AGEs), their receptor (RAGE) and its soluble isoform (sRAGE) in children, adolescents and young adults with diabetes mellitus type 1

Δεττοράκη, Αθηνά

30 May 2012

Τα τελικά προϊόντα προχωρημένης γλυκοζυλίωσης (AGEs: Advanced Glycation Endproducts) παίζουν σημαντικό ρόλο στην παθογένεια των διαβητικών αγγειακών επιπλοκών. Το καλύτερα χαρακτηριζόμενο είναι η N-καρβοξυμεθυλ-λυσίνη (CML). Τα AGEs προκαλούν σημαντικές επιδράσεις στα αγγεία με την πρόσδεσή τους σε ειδικούς υποδοχείς της κυτταρικής επιφάνειας, όπως τον RAGE (Receptor for Advanced Glycation Endproducts). Διαλυτές μορφές του RAGE (sRAGE) εμφανίζονται στο ανθρώπινο αίμα και δρουν ως παγίδα αιχμαλωτίζοντας τους φλεγμονώδεις προσδέτες του RAGE εξωκυττάρια, προστατεύοντας με αυτό τον τρόπο τα κύτταρα από τη βλάβη που προάγεται από τα AGEs. Σκοπός αυτής της εργασίας ήταν να μελετηθούν τα επίπεδα του sRAGE, η πρωτεϊνική έκφραση του RAGE, καθώς και τα επίπεδα CML σε σχέση με διάφορες κλινικές και βιοχημικές παραμέτρους σε παιδιά, εφήβους και νεαρούς ενήλικες με ΣΔ1. Τα επίπεδα sRAGE και CML προσδιορίστηκαν με ELISA και η πρωτεϊνική έκφραση του RAGE στα μονοπύρηνα του περιφερικού αίματος με ανοσοαποτύπωση κατά Western σε 74 παιδιά, εφήβους και νεαρούς ενήλικες με ΣΔ1 (13± 4 χρονών) και 43 μάρτυρες αντίστοιχης ηλικίας, φύλου και σταδίου Tanner. Σ’ αυτή την εργασία τα αυξημένα επίπεδα sRAGE στα παιδιά με ΣΔ1 και πιο ειδικά, σ’ αυτά ηλικίας κάτω από 13 ετών και με διάρκεια διαβήτη κάτω από 5 έτη, μπορεί να είναι ένα προσωρινό προστατευτικό μέτρο ενάντια στην κυτταρική βλάβη και πιθανόν να είναι επαρκές για να εξουδετερώσει επαρκώς τα κυκλοφορούντα CML, εμποδίζοντας έτσι τις διαβητικές αγγειακές επιπλοκές. Επίσης, μια ήπια αύξηση της LDL θα μπορούσε να είναι ένα ερέθισμα για την αύξηση του sRAGE, οδηγώντας στη δέσμευση του CML και τελικά τη μείωση των επιπέδων CML στην κυκλοφορία. Τα μειωμένα επίπεδα της πρωτεϊνικής έκφρασης του RAGE 55 kd (υποδοχέα πλήρους μήκους) μπορεί να αντανακλούν την αυξημένη έκφραση του sRAGE στους ασθενείς με ΣΔ1 συνολικά λόγω της αποκοπής του RAGE με μεταλλοπρωτεϊνάσες. Με την παρουσία κάποιου παράγοντα κινδύνου, όπως αύξηση ηλικίας, περιμέτρου κοιλίας, BMI, συστολικής ή διαστολικής αρτηριακής πίεσης ή επιδείνωση λιπιδαιμικού προφίλ αυξάνεται η πρωτεϊνική έκφραση της ισομορφής αυτής, ενώ φαίνεται αντίστοιχα να μειώνονται τα επίπεδα του sRAGE. Φαίνεται τελικά ότι συνολικά στα παιδιά, τους εφήβους και τους νεαρούς ενήλικες με ΣΔ1 υπάρχει μια υποκλινική διαταραχή του άξονα sRAGE-RAGE-CML, η οποία δύναται να μετατραπεί σε κλινικά εμφανείς αγγειακές βλάβες, αν προστεθούν περαιτέρω επιβαρυντικοί παράγοντες. / The binding of Advanced Glycation Endproducts (AGEs) to their receptor (RAGE) plays a major role in the development of diabetic vascular complications. This work is based on the relation between circulating soluble RAGE (sRAGE) levels in children, adolescents and young adults with IDDM and RAGE protein expression in association with N-(carboxymethyl)lysine (CML), a major antigenic AGEs component. Circulating sRAGE and CML levels were determined by ELISA and RAGE protein expression was evaluated in peripheral blood mononuclear cells by western immunoblotting in 74 children, adolescents and young adults with IDDM (134 years old) and 43 age, sex and Tanner stage-matched controls. Serum sRAGE levels were significantly higher in IDDM than in controls, inversely correlated to diabetes duration and directly correlated to LDL levels. Furthermore, circulating CML levels were not significantly different between IDDM and controls. Also, the protein expression of the RAGE isoforms 55 kd (full-length), 64 kd and 100 kd, measured by western immunoblotting, was significantly lower in IDDM than in controls, whereas RAGE 37 kd levels were not significantly different between IDDM and controls. Finally, when there was a risk factor, such as increased age, poor lipid profile, increased BMI or waist circumference or increased systolic or diastolic pressure, then it seemed that isoforms RAGE 55, 64 and 100 kd were increased. Isoform RAGE 64 kd could be RAGE-v5, a splice variant which resulted in a change of amino acid sequence in the extracellular ligand-binding domain of RAGE. Isoform RAGE 37 kd seemed to be Δ8-RAGE, a soluble splice variant with probably protective function, which had been found increased in patients with increased HDL. Finally, isoform RAGE 100 kd seemed to be some other splice variant in peripheral mononuclear cells. In conclusion, increased serum levels of sRAGE seen in IDDM children may be a temporary protective measure against cell damage and may be sufficient to efficiently eliminate excessive circulating CML. Moreover, the lower protein expression of the full-length RAGE in IDDM may also reflect the increased sRAGE expression in patients due to RAGE cleavage by metalloproteases. Consequently, in IDDM children, adolescents and young adults there may be a subclinical perturbation of the sRAGE-RAGE-CML axis, which could lead to future clinical vascular damage if additional risk factors are added over time.

Εναλλακτικό μάτισμα

Μεταλλοπρωτεϊνάσες

618.924 622

Insulin dependent diabetes mellitus

Advanced glycation endproducts (AGEs)

Microvascular complications

Alternative splicing

Metalloproteases