Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama

Detalhes bibliográficos
Autor(a) principal: Padoin, Licerio Vicente
Data de Publicação: 2019
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/8991
Resumo: Introduction: Breast cancer is probably the most feared among women, because of its high incidence and its psychological effects, which affect sexuality and personal image. It is considered serious public health problem worldwide, with approximately 2.1 million new cases and 627.000 deaths from the disease each year. Objective: To evaluate the integrity and quantification of the human epidermal growth factor 2 (HER2) receptor gene amplification in plasma free cell circulating DNA (cfDNA) in luminal breast cancers. Methodology: Plasma was collected for cfDNA analysis during core-biopsy (cancer diagnosis). Tumor size was obtained from ultrasound and mammography and immunohistochemistry was performed from core-biopsy samples. CfDNA levels of the Alu sequence, (Alu sequences can be considered genomic instability factors), and HER2 amplification levels were quantified by qPCR gene expression analysis. Results Paper 1: 19 patients and 14 controls were analyzed. Total and long (apoptosis) and short (necrosis) cfDNA amounts were significantly higher in patients than in controls, except for cfDNA integrity (ratio of long and short segments). There was a correlation between tumor size and the amount of long and short Alu fragments, as well as cfDNA integrity. No differences in Alu cfDNA levels were observed when compared to molecular subtypes. Results Paper 2: We analyzed 33 patients, 22 HER2- and 11 HER2 +,according to the mmunohistochemistry evaluated at the time of diagnosis. Tumor size had a positive correlation with cfDNA level, and this event was significant. HER2 amplification level in cfDNA was not associated with histological type or histological grade of tumors. An increase in HER2 amplification was observed in patients positive for immunohistochemical diagnosis of HER2 (p = 0.004). The ROC curve was significant (AUC = 0.76, p = 0.016). Discussion: The results indicate that cfDNA Alu quantification differentiates patients and controls, however, may not be useful in differentiating early diagnosis of breast cancer. Future studies using cfDNA are suggested in advanced cancer. Analysis of HER2 amplification in cfDNA appears to have potential for clinical use as it could prevent HER2 + tumors from being underdiagnosed by immunohistochemistry, probably due to histological heterogeneity, as well as to reveal other metastatic sites where HER2 amplification may occur.
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spelling Fay, Andre Poislhttp://lattes.cnpq.br/6858336633023217http://lattes.cnpq.br/6814140898573600Padoin, Licerio Vicente2019-10-29T19:20:27Z2019-08-30http://tede2.pucrs.br/tede2/handle/tede/8991Introduction: Breast cancer is probably the most feared among women, because of its high incidence and its psychological effects, which affect sexuality and personal image. It is considered serious public health problem worldwide, with approximately 2.1 million new cases and 627.000 deaths from the disease each year. Objective: To evaluate the integrity and quantification of the human epidermal growth factor 2 (HER2) receptor gene amplification in plasma free cell circulating DNA (cfDNA) in luminal breast cancers. Methodology: Plasma was collected for cfDNA analysis during core-biopsy (cancer diagnosis). Tumor size was obtained from ultrasound and mammography and immunohistochemistry was performed from core-biopsy samples. CfDNA levels of the Alu sequence, (Alu sequences can be considered genomic instability factors), and HER2 amplification levels were quantified by qPCR gene expression analysis. Results Paper 1: 19 patients and 14 controls were analyzed. Total and long (apoptosis) and short (necrosis) cfDNA amounts were significantly higher in patients than in controls, except for cfDNA integrity (ratio of long and short segments). There was a correlation between tumor size and the amount of long and short Alu fragments, as well as cfDNA integrity. No differences in Alu cfDNA levels were observed when compared to molecular subtypes. Results Paper 2: We analyzed 33 patients, 22 HER2- and 11 HER2 +,according to the mmunohistochemistry evaluated at the time of diagnosis. Tumor size had a positive correlation with cfDNA level, and this event was significant. HER2 amplification level in cfDNA was not associated with histological type or histological grade of tumors. An increase in HER2 amplification was observed in patients positive for immunohistochemical diagnosis of HER2 (p = 0.004). The ROC curve was significant (AUC = 0.76, p = 0.016). Discussion: The results indicate that cfDNA Alu quantification differentiates patients and controls, however, may not be useful in differentiating early diagnosis of breast cancer. Future studies using cfDNA are suggested in advanced cancer. Analysis of HER2 amplification in cfDNA appears to have potential for clinical use as it could prevent HER2 + tumors from being underdiagnosed by immunohistochemistry, probably due to histological heterogeneity, as well as to reveal other metastatic sites where HER2 amplification may occur.Introdução: O câncer de mama é provavelmente o mais temido entre as mulheres, por ser de alta incidência e pelos seus efeitos psicológicos, que afetam a sexualidade e a própria imagem pessoal. É considerado um grave problema de saúde pública no mundo, com aproximadamente 2,1 milhões de casos novos e 627 mil óbitos pela doença por ano. Objetivo: a avaliar a integridade e quantificar a amplificação do gene do receptor do fator de crescimento epidérmico humano 2 (HER2) no DNA circulante livre de células (cfDNA) no plasma (biópsia líquida) em cânceres mamários luminais. Metodologia: o plasma foi coletado para análise de cfDNA durante a core-biopsy (diagnóstico de câncer). O tamanho do tumor foi obtido a partir de ultrassom e mamografia e a imunoistoquímica foi realizada a partir de amostras de core-biopsy. Os níveis de cfDNA da sequência Alu, (as sequências Alu podem ser consideradas, fatores de instabilidade genômica), e os níveis de amplificação de HER2 foram quantificados por análise da expressão gênica via qPCR. Resultados artigo 1: foram analisados 19 pacientes e 14 controles. As quantidades de cfDNA total e de fragmentos longos (apoptose) e curtos (necrose) foram significativamente maiores em pacientes do que nos controles, com exceção da integridade cfDNA (relação de segmentos longos e curtos). Houve correlação entre o tamanho do tumor e a quantidade de fragmentos longos e curtos de Alu, bem como com a integridade do cfDNA. Nenhuma diferença nos níveis de Alu cfDNA foi observada quando comparada com os subtipos moleculares. Resultados artigo 2: Foram analisados 33 pacientes, sendo 22 HER2-e 11 HER2+, de acordo com a imunoistoquímica avaliada no momento do diagnóstico. O tamanho do tumor teve uma correlação positiva com o nível de cfDNA, e este evento foi significativo. O nível de amplificação do HER2 no cfDNA não se associou ao tipo histológico ou ao grau histológico dos tumores. Um aumento na amplificação de HER2 foi observado em pacientes positivas ao diagnóstico imunohistoquímico do HER2 (p = 0,004). A curva ROC foi significativa (AUC = 0,76, p = 0,016). Discussão: Os resultados indicam que a quantificação do Alu no cfDNA diferencia os pacientes e os controles, entretanto, pode não ser útil para diferenciar o diagnóstico precoce do câncer de mama. Futuros estudos usando o cfDNA são sugeridos em câncer avançado. A análise da amplificação do HER2 no cfDNA parece ter o potencial para uso clínico uma vez que poderia evitar que tumores HER2+ sejam sub diagnosticados pela imunoistoquímica, devido provavelmente à heterogeneidade histológica, bem como para revelar outros locais metastáticos onde possa ocorrer a amplificação do HER2.Submitted by PPG Medicina e Ciências da Saúde (medicina-pg@pucrs.br) on 2019-10-22T12:01:26Z No. of bitstreams: 1 tese final licerio PDF 26-09.pdf: 1174908 bytes, checksum: 76c7aa66dd5da48db9254809b51b9a2e (MD5)Approved for entry into archive by Sheila Dias (sheila.dias@pucrs.br) on 2019-10-29T19:02:01Z (GMT) No. of bitstreams: 1 tese final licerio PDF 26-09.pdf: 1174908 bytes, checksum: 76c7aa66dd5da48db9254809b51b9a2e (MD5)Made available in DSpace on 2019-10-29T19:20:27Z (GMT). No. of bitstreams: 1 tese final licerio PDF 26-09.pdf: 1174908 bytes, checksum: 76c7aa66dd5da48db9254809b51b9a2e (MD5) Previous issue date: 2019-08-30Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPESapplication/pdfhttp://tede2.pucrs.br:80/tede2/retrieve/177062/TES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.jpgporPontifícia Universidade Católica do Rio Grande do SulPrograma de Pós-Graduação em Medicina e Ciências da SaúdePUCRSBrasilEscola de MedicinaCfDNAImunoistoquímicaHER2Subtipos MolecularesCâncer de MamaImmunohistochemistryHER2Molecular SubtypesBreast CancerCIENCIAS DA SAUDE::MEDICINAIntegridade e amplificação do gene HER2 na biópsia líquida no câncer de mamainfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/doctoralThesisTrabalho será publicado como artigo ou livro60 meses29/10/2024-721401722658532398500500500600-224747486637135387-9693694523087866273590462550136975366info:eu-repo/semantics/openAccessreponame:Biblioteca Digital de Teses e Dissertações da PUC_RSinstname:Pontifícia Universidade Católica do Rio Grande do Sul (PUCRS)instacron:PUC_RSTHUMBNAILTES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.jpgTES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.jpgimage/jpeg4086http://tede2.pucrs.br/tede2/bitstream/tede/8991/4/TES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.jpgb640f219590f55301c8bdef9c51c26c7MD54TEXTTES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.txtTES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.txttext/plain1982http://tede2.pucrs.br/tede2/bitstream/tede/8991/3/TES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdf.txt328ea54331d33875bf2c1dd739ebee47MD53ORIGINALTES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdfTES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdfapplication/pdf589353http://tede2.pucrs.br/tede2/bitstream/tede/8991/2/TES_LUCERIO_VICENTE_PADOIN_CONFIDENCIAL.pdfa89250b84f23fe50169645a57e945fb8MD52LICENSElicense.txtlicense.txttext/plain; charset=utf-8590http://tede2.pucrs.br/tede2/bitstream/tede/8991/1/license.txt220e11f2d3ba5354f917c7035aadef24MD51tede/89912019-10-29 21:00:41.797oai:tede2.pucrs.br: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Biblioteca Digital de Teses e Dissertaçõeshttp://tede2.pucrs.br/tede2/PRIhttps://tede2.pucrs.br/oai/requestbiblioteca.central@pucrs.br||opendoar:2019-10-29T23:00:41Biblioteca Digital de Teses e Dissertações da PUC_RS - Pontifícia Universidade Católica do Rio Grande do Sul (PUCRS)false
dc.title.por.fl_str_mv Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
title Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
spellingShingle Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
Padoin, Licerio Vicente
CfDNA
Imunoistoquímica
HER2
Subtipos Moleculares
Câncer de Mama
Immunohistochemistry
HER2
Molecular Subtypes
Breast Cancer
CIENCIAS DA SAUDE::MEDICINA
title_short Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
title_full Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
title_fullStr Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
title_full_unstemmed Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
title_sort Integridade e amplificação do gene HER2 na biópsia líquida no câncer de mama
author Padoin, Licerio Vicente
author_facet Padoin, Licerio Vicente
author_role author
dc.contributor.advisor1.fl_str_mv Fay, Andre Poisl
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/6858336633023217
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/6814140898573600
dc.contributor.author.fl_str_mv Padoin, Licerio Vicente
contributor_str_mv Fay, Andre Poisl
dc.subject.por.fl_str_mv CfDNA
Imunoistoquímica
HER2
Subtipos Moleculares
Câncer de Mama
topic CfDNA
Imunoistoquímica
HER2
Subtipos Moleculares
Câncer de Mama
Immunohistochemistry
HER2
Molecular Subtypes
Breast Cancer
CIENCIAS DA SAUDE::MEDICINA
dc.subject.eng.fl_str_mv Immunohistochemistry
HER2
Molecular Subtypes
Breast Cancer
dc.subject.cnpq.fl_str_mv CIENCIAS DA SAUDE::MEDICINA
description Introduction: Breast cancer is probably the most feared among women, because of its high incidence and its psychological effects, which affect sexuality and personal image. It is considered serious public health problem worldwide, with approximately 2.1 million new cases and 627.000 deaths from the disease each year. Objective: To evaluate the integrity and quantification of the human epidermal growth factor 2 (HER2) receptor gene amplification in plasma free cell circulating DNA (cfDNA) in luminal breast cancers. Methodology: Plasma was collected for cfDNA analysis during core-biopsy (cancer diagnosis). Tumor size was obtained from ultrasound and mammography and immunohistochemistry was performed from core-biopsy samples. CfDNA levels of the Alu sequence, (Alu sequences can be considered genomic instability factors), and HER2 amplification levels were quantified by qPCR gene expression analysis. Results Paper 1: 19 patients and 14 controls were analyzed. Total and long (apoptosis) and short (necrosis) cfDNA amounts were significantly higher in patients than in controls, except for cfDNA integrity (ratio of long and short segments). There was a correlation between tumor size and the amount of long and short Alu fragments, as well as cfDNA integrity. No differences in Alu cfDNA levels were observed when compared to molecular subtypes. Results Paper 2: We analyzed 33 patients, 22 HER2- and 11 HER2 +,according to the mmunohistochemistry evaluated at the time of diagnosis. Tumor size had a positive correlation with cfDNA level, and this event was significant. HER2 amplification level in cfDNA was not associated with histological type or histological grade of tumors. An increase in HER2 amplification was observed in patients positive for immunohistochemical diagnosis of HER2 (p = 0.004). The ROC curve was significant (AUC = 0.76, p = 0.016). Discussion: The results indicate that cfDNA Alu quantification differentiates patients and controls, however, may not be useful in differentiating early diagnosis of breast cancer. Future studies using cfDNA are suggested in advanced cancer. Analysis of HER2 amplification in cfDNA appears to have potential for clinical use as it could prevent HER2 + tumors from being underdiagnosed by immunohistochemistry, probably due to histological heterogeneity, as well as to reveal other metastatic sites where HER2 amplification may occur.
publishDate 2019
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dc.publisher.none.fl_str_mv Pontifícia Universidade Católica do Rio Grande do Sul
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dc.publisher.country.fl_str_mv Brasil
dc.publisher.department.fl_str_mv Escola de Medicina
publisher.none.fl_str_mv Pontifícia Universidade Católica do Rio Grande do Sul
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