Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose
Autor(a) principal: | |
---|---|
Data de Publicação: | 2014 |
Tipo de documento: | Tese |
Idioma: | por |
Título da fonte: | Biblioteca Digital de Teses e Dissertações da PUC_RS |
Texto Completo: | http://tede2.pucrs.br/tede2/handle/tede/1793 |
Resumo: | Endometriosis is a well know estrogen dependent disease and it´s most common symptoms are severe pelvic pain and infertility. It affects up to 15% of patients on reproductive age and up to 50% of infertile patients. Its pathogenesis still unclear and there is evidence for a role of genetic components. The microRNA135a and 135b (miR135) silence gene expression and increased miR135 down-regulated HOXA 10, a key mediator of endometrial receptivity and implantation. MiRNA are aberrantly regulated in the endometrium of women with endometriosis when compared to the endometrium of disease free women. Considering that several genes are known to be differentially expressed in eutopic and ectopic endometrium of women with endometriosis, we analyzed the expression of miR135 in the ectopic endometrium, compared with the expression in the eutopic from the same patients, and also evaluate if there is different levels of expression during the menstrual cycle. We evaluated thirty one subjects who underwent surgery from March 2013 through May 2014 for diagnosis or treatment of endometriosis, they had endometrium and endometriosis lesions biopsies taken. Approval was obtained from the PUCRS and Santa Casa Hospital Investigations Committee. Eight subjects were excluded due to low levels of mRNA. The samples were divided according to the menstrual cycle as follows: proliferative, day 1-14 (n=11) and secretory, day 15-28 (n=12). For miRNA detection, we used the poly (A) RT-PCR method using Invitrogen NCode miRNA first-strand cDNA synthesis MIRC-50 kit (Invitrogen, California, USA). Gene transcripts were amplified by real-time PCR using the AB 7500 (Applied Biosystems, California, USA) with the forward specific primers to miR135a and miR135b and the universal reverse primer complementary to the anchor primer. U6 small nuclear RNA was used as a control to determine relative miRNA expression. Relative mRNA level was presented using the formula 2−ΔΔCt. Statistical analysis was performed using unpaired Mann Whitney test for the ectopic vs. eutopic endometrium samples and for comparison between different phases of the menstrual cycle. All the analyses considered a p< 0.05 as significant. Tweenty three patients submitted to laparoscopic surgery for diagnosis or treatment of endometriosis had endometrium biopsy taken and excision of endometriosis lesions. All endometriosis lesions samples expressed miR135a and miR135b. Comparing with the eutopic endometrium, there weren´t difference on its expression. When the subjects were divided by the menstrual cycle phase, during the secretory phase the expression of mir135a and 135b was lower in the ectopic endometrium comparing to the proliferative phase. MicroRNA is involved in endometrial receptivity, and there is evidence of a relation between miR135a and miR135b with HOXA10, a well know gene that is down regulated in women with endometriosis and has a strong influence on embryo implantation. Here we showed similar expression levels of miR135a and miR135b in the ectopic endometrium when compared with eutopic endometrium. However, we detected a lower expression of miR135 during the secretory phase that is likely due to physiological lower levels of estrogen and higher levels of progesterone during this phase. |
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Machado, Denise CantarelliCPF:29466911015http://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4788589H0CPF:97305626015http://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4778155Y7Petracco, Rafaella Gehm2015-04-14T13:36:02Z2014-12-232014-10-14PETRACCO, Rafaella Gehm. Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose. 2014. 95 f. Tese (Doutorado em Medicina e Ciências da Saúde) - Pontifícia Universidade Católica do Rio Grande do Sul, Porto Alegre, 2014.http://tede2.pucrs.br/tede2/handle/tede/1793Endometriosis is a well know estrogen dependent disease and it´s most common symptoms are severe pelvic pain and infertility. It affects up to 15% of patients on reproductive age and up to 50% of infertile patients. Its pathogenesis still unclear and there is evidence for a role of genetic components. The microRNA135a and 135b (miR135) silence gene expression and increased miR135 down-regulated HOXA 10, a key mediator of endometrial receptivity and implantation. MiRNA are aberrantly regulated in the endometrium of women with endometriosis when compared to the endometrium of disease free women. Considering that several genes are known to be differentially expressed in eutopic and ectopic endometrium of women with endometriosis, we analyzed the expression of miR135 in the ectopic endometrium, compared with the expression in the eutopic from the same patients, and also evaluate if there is different levels of expression during the menstrual cycle. We evaluated thirty one subjects who underwent surgery from March 2013 through May 2014 for diagnosis or treatment of endometriosis, they had endometrium and endometriosis lesions biopsies taken. Approval was obtained from the PUCRS and Santa Casa Hospital Investigations Committee. Eight subjects were excluded due to low levels of mRNA. The samples were divided according to the menstrual cycle as follows: proliferative, day 1-14 (n=11) and secretory, day 15-28 (n=12). For miRNA detection, we used the poly (A) RT-PCR method using Invitrogen NCode miRNA first-strand cDNA synthesis MIRC-50 kit (Invitrogen, California, USA). Gene transcripts were amplified by real-time PCR using the AB 7500 (Applied Biosystems, California, USA) with the forward specific primers to miR135a and miR135b and the universal reverse primer complementary to the anchor primer. U6 small nuclear RNA was used as a control to determine relative miRNA expression. Relative mRNA level was presented using the formula 2−ΔΔCt. Statistical analysis was performed using unpaired Mann Whitney test for the ectopic vs. eutopic endometrium samples and for comparison between different phases of the menstrual cycle. All the analyses considered a p< 0.05 as significant. Tweenty three patients submitted to laparoscopic surgery for diagnosis or treatment of endometriosis had endometrium biopsy taken and excision of endometriosis lesions. All endometriosis lesions samples expressed miR135a and miR135b. Comparing with the eutopic endometrium, there weren´t difference on its expression. When the subjects were divided by the menstrual cycle phase, during the secretory phase the expression of mir135a and 135b was lower in the ectopic endometrium comparing to the proliferative phase. MicroRNA is involved in endometrial receptivity, and there is evidence of a relation between miR135a and miR135b with HOXA10, a well know gene that is down regulated in women with endometriosis and has a strong influence on embryo implantation. Here we showed similar expression levels of miR135a and miR135b in the ectopic endometrium when compared with eutopic endometrium. However, we detected a lower expression of miR135 during the secretory phase that is likely due to physiological lower levels of estrogen and higher levels of progesterone during this phase.Endometriose é uma doença estrogênio dependente que, entre seus sintomas mais comuns, estão dor pélvica e infertilidade. Afeta até 15% das pacientes em idade reprodutiva e até 50% das pacientes inférteis. A etiopatogenia ainda não é bem clara, mas há evidências do envolvimento de componentes genéticos. O microRNA 135a e 135b (miR135) silencia a expressão gênica e o aumento na expressão do miR135 diminui a expressão do HOXA 10, um importante mediador da receptividade endometrial e implantação. MicroRNAs têm sua expressão alterada no endométrio de mulheres com endometriose quando comparado com o endométrio de mulheres sem a doença. Considerando que vários genes são conhecidos por terem sua expressão alterada no endométrio tópico quando comparado ao endométrio ectópico das pacientes com endometriose, foi analisado a expressão do miR135 neste dois tecidos endometriais na mesma paciente em diferentes fases do ciclo menstrual. Após aprovação pelos Comitês de Ética em Pesquisa do Hospital São Lucas da PUCRS e da Santa Casa de Porto Alegre, foram realizadas biopsias endometriais e exérese de lesões de endometriose de trinta e uma pacientes submetidas à cirurgia no período de março de 2013 a maio 2014 para diagnóstico ou tratamento de endometriose Oito pacientes foram excluídas devido a níveis de mRNA muito baixos. As amostras foram divididas de acordo com o ciclo menstrual, fase proliferativa, dia 1 a 14 (n=11) e fase secretora, dia 15 a 28 (n=12). Para a detecção de miRNA foi utilizado o método poly (A) RT-PCR utilizando o kit Invitrogen NCode miRNA first-strand cDNA synthesis MIRC-50 kit (Invitrogen, California, USA). A transcrição gênica foi amplificada por PCR em tempo real, utilizando o aparelho AB 7500 (Applied Biosystems, Califórnia, USA). Foram utilizados oligonucleotídeos iniciadores específicos para o miR135a e 135b e oligonucleotídeo iniciador universal. Para determinar a expressão relativa, foi utilizado o gene U6. Níveis relativos de mRNA foram apresentados utilizando a formula 2−ΔΔCt. Análise estatística foi realizada utilizando o teste de Mann Whitney, considerando como significativo um p<0,05. Vinte e três pacientes tiveram suas amostras analisadas. Todas as amostras expressavam níveis de miR135a e miR135b. Comparando o endométrio ectópico com o endométrio tópico não houve diferença na expressão do microRNA. Quando as pacientes foram divididas nas diferentes fases do ciclo menstrual, observou-se que durante a fase secretora, a expressão do miR135a e miR135b foi menor do que na fase proliferativa. Em conclusão, microRNAs estão envolvidos na receptividade endometrial e há evidência da relação entre o miR135a e miR135b com HOXA10, um gene sabidamente diminuído na endometriose e relacionado à implantação embrionária. Neste trabalho, foi demonstrado uma expressão semelhante do miR135 no endométrio ectópico em comparação com o endométrio tópico e uma diminuição nesta expressão quando comparado a fase secretora com a proliferativa, provavelmente devido a baixos níveis de estrogênio e altos níveis de progesterona presentes nesta fase.Made available in DSpace on 2015-04-14T13:36:02Z (GMT). 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dc.title.por.fl_str_mv |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
title |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
spellingShingle |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose Petracco, Rafaella Gehm MEDICINA ENDOMETRIOSE MENSTRUAÇÃO ÚTERO - DOENÇAS CNPQ::CIENCIAS DA SAUDE::MEDICINA |
title_short |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
title_full |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
title_fullStr |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
title_full_unstemmed |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
title_sort |
Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose |
author |
Petracco, Rafaella Gehm |
author_facet |
Petracco, Rafaella Gehm |
author_role |
author |
dc.contributor.advisor1.fl_str_mv |
Machado, Denise Cantarelli |
dc.contributor.advisor1ID.fl_str_mv |
CPF:29466911015 |
dc.contributor.advisor1Lattes.fl_str_mv |
http://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4788589H0 |
dc.contributor.authorID.fl_str_mv |
CPF:97305626015 |
dc.contributor.authorLattes.fl_str_mv |
http://buscatextual.cnpq.br/buscatextual/visualizacv.do?id=K4778155Y7 |
dc.contributor.author.fl_str_mv |
Petracco, Rafaella Gehm |
contributor_str_mv |
Machado, Denise Cantarelli |
dc.subject.por.fl_str_mv |
MEDICINA ENDOMETRIOSE MENSTRUAÇÃO ÚTERO - DOENÇAS |
topic |
MEDICINA ENDOMETRIOSE MENSTRUAÇÃO ÚTERO - DOENÇAS CNPQ::CIENCIAS DA SAUDE::MEDICINA |
dc.subject.cnpq.fl_str_mv |
CNPQ::CIENCIAS DA SAUDE::MEDICINA |
description |
Endometriosis is a well know estrogen dependent disease and it´s most common symptoms are severe pelvic pain and infertility. It affects up to 15% of patients on reproductive age and up to 50% of infertile patients. Its pathogenesis still unclear and there is evidence for a role of genetic components. The microRNA135a and 135b (miR135) silence gene expression and increased miR135 down-regulated HOXA 10, a key mediator of endometrial receptivity and implantation. MiRNA are aberrantly regulated in the endometrium of women with endometriosis when compared to the endometrium of disease free women. Considering that several genes are known to be differentially expressed in eutopic and ectopic endometrium of women with endometriosis, we analyzed the expression of miR135 in the ectopic endometrium, compared with the expression in the eutopic from the same patients, and also evaluate if there is different levels of expression during the menstrual cycle. We evaluated thirty one subjects who underwent surgery from March 2013 through May 2014 for diagnosis or treatment of endometriosis, they had endometrium and endometriosis lesions biopsies taken. Approval was obtained from the PUCRS and Santa Casa Hospital Investigations Committee. Eight subjects were excluded due to low levels of mRNA. The samples were divided according to the menstrual cycle as follows: proliferative, day 1-14 (n=11) and secretory, day 15-28 (n=12). For miRNA detection, we used the poly (A) RT-PCR method using Invitrogen NCode miRNA first-strand cDNA synthesis MIRC-50 kit (Invitrogen, California, USA). Gene transcripts were amplified by real-time PCR using the AB 7500 (Applied Biosystems, California, USA) with the forward specific primers to miR135a and miR135b and the universal reverse primer complementary to the anchor primer. U6 small nuclear RNA was used as a control to determine relative miRNA expression. Relative mRNA level was presented using the formula 2−ΔΔCt. Statistical analysis was performed using unpaired Mann Whitney test for the ectopic vs. eutopic endometrium samples and for comparison between different phases of the menstrual cycle. All the analyses considered a p< 0.05 as significant. Tweenty three patients submitted to laparoscopic surgery for diagnosis or treatment of endometriosis had endometrium biopsy taken and excision of endometriosis lesions. All endometriosis lesions samples expressed miR135a and miR135b. Comparing with the eutopic endometrium, there weren´t difference on its expression. When the subjects were divided by the menstrual cycle phase, during the secretory phase the expression of mir135a and 135b was lower in the ectopic endometrium comparing to the proliferative phase. MicroRNA is involved in endometrial receptivity, and there is evidence of a relation between miR135a and miR135b with HOXA10, a well know gene that is down regulated in women with endometriosis and has a strong influence on embryo implantation. Here we showed similar expression levels of miR135a and miR135b in the ectopic endometrium when compared with eutopic endometrium. However, we detected a lower expression of miR135 during the secretory phase that is likely due to physiological lower levels of estrogen and higher levels of progesterone during this phase. |
publishDate |
2014 |
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2014-12-23 |
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2014-10-14 |
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PETRACCO, Rafaella Gehm. Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose. 2014. 95 f. Tese (Doutorado em Medicina e Ciências da Saúde) - Pontifícia Universidade Católica do Rio Grande do Sul, Porto Alegre, 2014. |
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http://tede2.pucrs.br/tede2/handle/tede/1793 |
identifier_str_mv |
PETRACCO, Rafaella Gehm. Diminuição da expressão do miRNA 135 na fase secretora do ciclo menstrual em pacientes com endometriose. 2014. 95 f. Tese (Doutorado em Medicina e Ciências da Saúde) - Pontifícia Universidade Católica do Rio Grande do Sul, Porto Alegre, 2014. |
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