Detecção e caracterização molecular de talassemia alfa

Detalhes bibliográficos
Autor(a) principal: PENNA, Karlla Greick Batista Dias
Data de Publicação: 2009
Tipo de documento: Tese
Idioma: por
Título da fonte: Repositório Institucional da UFG
dARK ID: ark:/38995/00130000043f2
Texto Completo: http://repositorio.bc.ufg.br/tede/handle/tde/1013
Resumo: Alpha thalassemia is a syndrome resulting from disturbances in the synthesis of alpha globin chain that forms the tetramer of the hemoglobin molecule. Alpha thalassemia is classified into four types according to the number of alpha genes affected: silent carrier (-α/αα), alpha thalassemia trait (--/αα or -α/-α) Hemoglobin H disease (-- /-α), and fetalis hydrops (--/--). The decrease in synthesis of alpha globin causes inadequate production of hemoglobin resulting in hypochromic and microcytic anaemia. Also it causes accumulation of beta chains, inside the erythrocytes, resulting in formation of beta chain tetramer of hemoglobin called Hb H. Clinically the individual with thalassemia can be asymptomatic or present severe anemia. Asymptomatic forms of thalassemia, silent carrier and alpha thalassemia trait, are more difficult to diagnose because of the inclusions bodies of Hb H are not always present. In these situations it is necessary to research the molecular characterization of the genotype and confirming the presence of alpha thalassemia. This is mainly because the diagnosis by conventional methods, although important, is limited and imprecise. This study evaluated some of the traditional laboratory methods in the detection of alpha thalassemia and associated molecular characterization of the more prevalent deletion forms α3,7 and α4,2. For confirmation and characterization of alpha thalassemia, new oligonucleotides were designed. By conventional PCR technique, using 3.7F/KGB01 primers it was possible to detect the deletion α3,7, differentiating the normal genotype (αα/αα), the heterozygote (-α3,7/αα), and homozygous (-- α3,7/- α3,7). Although it was designed to detect the deletion α3,7, this primers also identified the deletion α4,2 when in homozigose (-α4,2/- α4,2). The primers KGB04/KGB05 detected the deletion α4,2, but without differentiating between the heterozygous and homozygous genotype. The most prevalent deletion founded was the α4,2 (20.0%) which represents 9.2% in the homozygous form (- α4,2/-α4,2). The deletion α3,7 in the heterozygous form was detected in 12.3% of patients. The data demonstrate that the importance of molecular detection for alpha thalassemia is not limited only to the definition of the genotype, but also confirmation of the presence in patients with abnormal erythrogram values, with regular erythrogram values, with values closed to the boundary values and in neonates.
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spelling BATAUS, Luiz Artur Mendeshttp://lattes.cnpq.br/5637230378599476http://lattes.cnpq.br/4356233663135923PENNA, Karlla Greick Batista Dias2014-07-29T15:10:32Z2011-02-252009-03-27PENNA, Karlla Greick Batista Dias. Detection and molecular characterization of alpha thalassemia. 2009. 144 f. Tese (Doutorado em Ciencias Biologicas) - Universidade Federal de Goiás, Goiânia, 2009.http://repositorio.bc.ufg.br/tede/handle/tde/1013ark:/38995/00130000043f2Alpha thalassemia is a syndrome resulting from disturbances in the synthesis of alpha globin chain that forms the tetramer of the hemoglobin molecule. Alpha thalassemia is classified into four types according to the number of alpha genes affected: silent carrier (-α/αα), alpha thalassemia trait (--/αα or -α/-α) Hemoglobin H disease (-- /-α), and fetalis hydrops (--/--). The decrease in synthesis of alpha globin causes inadequate production of hemoglobin resulting in hypochromic and microcytic anaemia. Also it causes accumulation of beta chains, inside the erythrocytes, resulting in formation of beta chain tetramer of hemoglobin called Hb H. Clinically the individual with thalassemia can be asymptomatic or present severe anemia. Asymptomatic forms of thalassemia, silent carrier and alpha thalassemia trait, are more difficult to diagnose because of the inclusions bodies of Hb H are not always present. In these situations it is necessary to research the molecular characterization of the genotype and confirming the presence of alpha thalassemia. This is mainly because the diagnosis by conventional methods, although important, is limited and imprecise. This study evaluated some of the traditional laboratory methods in the detection of alpha thalassemia and associated molecular characterization of the more prevalent deletion forms α3,7 and α4,2. For confirmation and characterization of alpha thalassemia, new oligonucleotides were designed. By conventional PCR technique, using 3.7F/KGB01 primers it was possible to detect the deletion α3,7, differentiating the normal genotype (αα/αα), the heterozygote (-α3,7/αα), and homozygous (-- α3,7/- α3,7). Although it was designed to detect the deletion α3,7, this primers also identified the deletion α4,2 when in homozigose (-α4,2/- α4,2). The primers KGB04/KGB05 detected the deletion α4,2, but without differentiating between the heterozygous and homozygous genotype. The most prevalent deletion founded was the α4,2 (20.0%) which represents 9.2% in the homozygous form (- α4,2/-α4,2). The deletion α3,7 in the heterozygous form was detected in 12.3% of patients. The data demonstrate that the importance of molecular detection for alpha thalassemia is not limited only to the definition of the genotype, but also confirmation of the presence in patients with abnormal erythrogram values, with regular erythrogram values, with values closed to the boundary values and in neonates.A talassemia alfa é uma síndrome resultante de distúrbios na síntese da cadeia da globina alfa que formam o tetrâmero da molécula da hemoglobina. A talassemia alfa é classificada em quatro tipos de acordo com o número de genes alfa afetado: portador silencioso (-α/αα); traço alfa talassêmico (--/αα ou - α/-α); doença de hemoglobina H (--/-α) e hidropsia fetal (--/--). A diminuição na síntese de globina alfa causa a produção inadequada de hemoglobina que resulta em anemia microcítica e hipocrômica. Causa também o acúmulo de cadeias do tipo beta, no interior do eritrócito, pela falta de balanceamento com a síntese da globina alfa afetada. O resultado deste desbalanceamento é a formação de tetrâmeros de cadeias beta denominados Hb H. Clinicamente o indivíduo portador de talassemia alfa pode ser assintomático ou apresentar anemia severa. As formas assintomáticas da talassemia alfa, o portador silencioso e o traço alfa talassêmico, são mais difíceis de diagnosticar, pois os corpúsculos de Hb H nem sempre estão presentes. Para estas situações faz-se necessária a investigação molecular visando a caracterização do genótipo e a confirmação da presença da talassemia alfa. Este fato se deve principalmente porque o diagnóstico através de métodos clássicos não moleculares, apesar de importantes, é limitado e impreciso. O presente trabalho avaliou alguns dos métodos laboratoriais clássicos na detecção de talassemia alfa e associou a caracterização molecular das formas delecionais mais prevalentes α3,7 e α4,2. Para a confirmação e caracterização da talassemia alfa, foram desenhados novos oligonucleotídeos. Através da técnica convencional da PCR, utilizando o par de oligonucleotídeos 3.7F/KGB01 foi possível detectar a deleção α3,7, diferenciando o genótipo normal (αα/αα), do heterozigoto ( α3,7/αα) e do homozigoto ( α3,7/ α3,7). Apesar de ter sido desenhado para detectar a deleção α3,7, este par também permitiu detectar a deleção α4,2 quando em homozigose ( α4,2/ α4,2). Utilizando o par KGB04/KGB05 foi possível detectar a deleção α4,2, porém sem diferenciar entre o genótipo heterozigoto e homozigoto. A deleção mais prevalente encontrada foi a α4,2 (20,0%) sendo que destas podemos afirmar que 9,2% estão na forma homozigótica ( α4,2/ α4,2). A deleção do tipo α3,7 na forma heterozigótica foi detectada em 12,3% dos pacientes. Os dados obtidos revelam que a importância da detecção molecular para talassemia alfa não se restringe apenas na definição do genótipo, mas também na detecção deste tipo de talassemia em pacientes que apresentam: quadros hematológicos alterados, quadros hematológicos normais, mas com valores próximos aos valores limítrofes e em neonatos.Made available in DSpace on 2014-07-29T15:10:32Z (GMT). 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dc.title.por.fl_str_mv Detecção e caracterização molecular de talassemia alfa
dc.title.alternative.eng.fl_str_mv Detection and molecular characterization of alpha thalassemia
title Detecção e caracterização molecular de talassemia alfa
spellingShingle Detecção e caracterização molecular de talassemia alfa
PENNA, Karlla Greick Batista Dias
Hemoglobinopatias
Talassemia alfa
Hemoglobina H
Detecção laboratorial
Análise Molecular
Hemoglobinopathies
Alpha thalassemia
Hemoglobin H
Laboratorial detection
Molecular characterization
CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA::BIOLOGIA MOLECULAR
title_short Detecção e caracterização molecular de talassemia alfa
title_full Detecção e caracterização molecular de talassemia alfa
title_fullStr Detecção e caracterização molecular de talassemia alfa
title_full_unstemmed Detecção e caracterização molecular de talassemia alfa
title_sort Detecção e caracterização molecular de talassemia alfa
author PENNA, Karlla Greick Batista Dias
author_facet PENNA, Karlla Greick Batista Dias
author_role author
dc.contributor.advisor1.fl_str_mv BATAUS, Luiz Artur Mendes
dc.contributor.advisor1Lattes.fl_str_mv http://lattes.cnpq.br/5637230378599476
dc.contributor.authorLattes.fl_str_mv http://lattes.cnpq.br/4356233663135923
dc.contributor.author.fl_str_mv PENNA, Karlla Greick Batista Dias
contributor_str_mv BATAUS, Luiz Artur Mendes
dc.subject.por.fl_str_mv Hemoglobinopatias
Talassemia alfa
Hemoglobina H
Detecção laboratorial
Análise Molecular
topic Hemoglobinopatias
Talassemia alfa
Hemoglobina H
Detecção laboratorial
Análise Molecular
Hemoglobinopathies
Alpha thalassemia
Hemoglobin H
Laboratorial detection
Molecular characterization
CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA::BIOLOGIA MOLECULAR
dc.subject.eng.fl_str_mv Hemoglobinopathies
Alpha thalassemia
Hemoglobin H
Laboratorial detection
Molecular characterization
dc.subject.cnpq.fl_str_mv CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA::BIOLOGIA MOLECULAR
description Alpha thalassemia is a syndrome resulting from disturbances in the synthesis of alpha globin chain that forms the tetramer of the hemoglobin molecule. Alpha thalassemia is classified into four types according to the number of alpha genes affected: silent carrier (-α/αα), alpha thalassemia trait (--/αα or -α/-α) Hemoglobin H disease (-- /-α), and fetalis hydrops (--/--). The decrease in synthesis of alpha globin causes inadequate production of hemoglobin resulting in hypochromic and microcytic anaemia. Also it causes accumulation of beta chains, inside the erythrocytes, resulting in formation of beta chain tetramer of hemoglobin called Hb H. Clinically the individual with thalassemia can be asymptomatic or present severe anemia. Asymptomatic forms of thalassemia, silent carrier and alpha thalassemia trait, are more difficult to diagnose because of the inclusions bodies of Hb H are not always present. In these situations it is necessary to research the molecular characterization of the genotype and confirming the presence of alpha thalassemia. This is mainly because the diagnosis by conventional methods, although important, is limited and imprecise. This study evaluated some of the traditional laboratory methods in the detection of alpha thalassemia and associated molecular characterization of the more prevalent deletion forms α3,7 and α4,2. For confirmation and characterization of alpha thalassemia, new oligonucleotides were designed. By conventional PCR technique, using 3.7F/KGB01 primers it was possible to detect the deletion α3,7, differentiating the normal genotype (αα/αα), the heterozygote (-α3,7/αα), and homozygous (-- α3,7/- α3,7). Although it was designed to detect the deletion α3,7, this primers also identified the deletion α4,2 when in homozigose (-α4,2/- α4,2). The primers KGB04/KGB05 detected the deletion α4,2, but without differentiating between the heterozygous and homozygous genotype. The most prevalent deletion founded was the α4,2 (20.0%) which represents 9.2% in the homozygous form (- α4,2/-α4,2). The deletion α3,7 in the heterozygous form was detected in 12.3% of patients. The data demonstrate that the importance of molecular detection for alpha thalassemia is not limited only to the definition of the genotype, but also confirmation of the presence in patients with abnormal erythrogram values, with regular erythrogram values, with values closed to the boundary values and in neonates.
publishDate 2009
dc.date.issued.fl_str_mv 2009-03-27
dc.date.available.fl_str_mv 2011-02-25
dc.date.accessioned.fl_str_mv 2014-07-29T15:10:32Z
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dc.identifier.citation.fl_str_mv PENNA, Karlla Greick Batista Dias. Detection and molecular characterization of alpha thalassemia. 2009. 144 f. Tese (Doutorado em Ciencias Biologicas) - Universidade Federal de Goiás, Goiânia, 2009.
dc.identifier.uri.fl_str_mv http://repositorio.bc.ufg.br/tede/handle/tde/1013
dc.identifier.dark.fl_str_mv ark:/38995/00130000043f2
identifier_str_mv PENNA, Karlla Greick Batista Dias. Detection and molecular characterization of alpha thalassemia. 2009. 144 f. Tese (Doutorado em Ciencias Biologicas) - Universidade Federal de Goiás, Goiânia, 2009.
ark:/38995/00130000043f2
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dc.publisher.program.fl_str_mv Doutorado em Biologia
dc.publisher.initials.fl_str_mv UFG
dc.publisher.country.fl_str_mv BR
dc.publisher.department.fl_str_mv Ciencias Biologicas
publisher.none.fl_str_mv Universidade Federal de Goiás
dc.source.none.fl_str_mv reponame:Repositório Institucional da UFG
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