Screening fetal losses for monosomy X with a simple PCR-based procedure

Detalhes bibliográficos
Autor(a) principal: Pereira, Rinaldo Wellerson
Data de Publicação: 2000
Outros Autores: Sturzeneker, Rosane, Pena, Sérgio Danilo Junho
Tipo de documento: Artigo
Idioma: eng
Título da fonte: Repositório Institucional da UCB
Texto Completo: http://twingo.ucb.br:8080/jspui/handle/10869/453
https://repositorio.ucb.br:9443/jspui/handle/123456789/7658
Resumo: To screen for monosomy X in spontaneous fetal losses we explored a simple molecular strategy based on loss of heterozygosity at highly polymorphic X-linked loci. We developed a multiplex fluorescent procedure that allows the simultaneous amplification of five dinucleotide repeat polymorphisms in a large low-recombination region in the long arm of the X chromosome. Analysis was performed by computer-assisted laser densitometry. We did not find any instances of homozygosity at all five loci in 30 normal females tested, nor among 37 women whose typing data were retrieved from the Fondation Jean Dausset - CEPH genotype database. In addition, all cases of monosomy X previously diagnosed by conventional cytogenetics presented the anticipated loss of heterozygosity at all loci. We studied 19 spontaneously aborted female fetuses and we found four samples homozygous for the five loci (21%), in good agreement with the expected rate of monosomy X in first trimester spontaneous abortions. We conclude that the loci have high diversity and high efficiency in PCR-amplification and that our multiplex procedure constitutes a simple and useful molecular screening test for monosomy X in abortions and stillbirths.
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spelling Pereira, Rinaldo WellersonSturzeneker, RosanePena, Sérgio Danilo Junho2016-10-10T03:52:15Z2016-10-10T03:52:15Z2000PEREIRA, Rinaldo Wellerson; STURZENEKER, Rosane; PENA, Sérgio Danilo Junho. Screening fetal losses for monosomy X with a simple PCR-based procedure. Genetics and Molecular Biology, v. 23, n.1, p.11-14, 2000.1415-4757http://twingo.ucb.br:8080/jspui/handle/10869/453https://repositorio.ucb.br:9443/jspui/handle/123456789/7658To screen for monosomy X in spontaneous fetal losses we explored a simple molecular strategy based on loss of heterozygosity at highly polymorphic X-linked loci. We developed a multiplex fluorescent procedure that allows the simultaneous amplification of five dinucleotide repeat polymorphisms in a large low-recombination region in the long arm of the X chromosome. Analysis was performed by computer-assisted laser densitometry. We did not find any instances of homozygosity at all five loci in 30 normal females tested, nor among 37 women whose typing data were retrieved from the Fondation Jean Dausset - CEPH genotype database. In addition, all cases of monosomy X previously diagnosed by conventional cytogenetics presented the anticipated loss of heterozygosity at all loci. We studied 19 spontaneously aborted female fetuses and we found four samples homozygous for the five loci (21%), in good agreement with the expected rate of monosomy X in first trimester spontaneous abortions. We conclude that the loci have high diversity and high efficiency in PCR-amplification and that our multiplex procedure constitutes a simple and useful molecular screening test for monosomy X in abortions and stillbirths.Made available in DSpace on 2016-10-10T03:52:15Z (GMT). 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dc.title.pt_BR.fl_str_mv Screening fetal losses for monosomy X with a simple PCR-based procedure
title Screening fetal losses for monosomy X with a simple PCR-based procedure
spellingShingle Screening fetal losses for monosomy X with a simple PCR-based procedure
Pereira, Rinaldo Wellerson
title_short Screening fetal losses for monosomy X with a simple PCR-based procedure
title_full Screening fetal losses for monosomy X with a simple PCR-based procedure
title_fullStr Screening fetal losses for monosomy X with a simple PCR-based procedure
title_full_unstemmed Screening fetal losses for monosomy X with a simple PCR-based procedure
title_sort Screening fetal losses for monosomy X with a simple PCR-based procedure
author Pereira, Rinaldo Wellerson
author_facet Pereira, Rinaldo Wellerson
Sturzeneker, Rosane
Pena, Sérgio Danilo Junho
author_role author
author2 Sturzeneker, Rosane
Pena, Sérgio Danilo Junho
author2_role author
author
dc.contributor.author.fl_str_mv Pereira, Rinaldo Wellerson
Sturzeneker, Rosane
Pena, Sérgio Danilo Junho
dc.description.abstract.por.fl_txt_mv To screen for monosomy X in spontaneous fetal losses we explored a simple molecular strategy based on loss of heterozygosity at highly polymorphic X-linked loci. We developed a multiplex fluorescent procedure that allows the simultaneous amplification of five dinucleotide repeat polymorphisms in a large low-recombination region in the long arm of the X chromosome. Analysis was performed by computer-assisted laser densitometry. We did not find any instances of homozygosity at all five loci in 30 normal females tested, nor among 37 women whose typing data were retrieved from the Fondation Jean Dausset - CEPH genotype database. In addition, all cases of monosomy X previously diagnosed by conventional cytogenetics presented the anticipated loss of heterozygosity at all loci. We studied 19 spontaneously aborted female fetuses and we found four samples homozygous for the five loci (21%), in good agreement with the expected rate of monosomy X in first trimester spontaneous abortions. We conclude that the loci have high diversity and high efficiency in PCR-amplification and that our multiplex procedure constitutes a simple and useful molecular screening test for monosomy X in abortions and stillbirths.
dc.description.version.pt_BR.fl_txt_mv Sim
dc.description.status.pt_BR.fl_txt_mv Publicado
description To screen for monosomy X in spontaneous fetal losses we explored a simple molecular strategy based on loss of heterozygosity at highly polymorphic X-linked loci. We developed a multiplex fluorescent procedure that allows the simultaneous amplification of five dinucleotide repeat polymorphisms in a large low-recombination region in the long arm of the X chromosome. Analysis was performed by computer-assisted laser densitometry. We did not find any instances of homozygosity at all five loci in 30 normal females tested, nor among 37 women whose typing data were retrieved from the Fondation Jean Dausset - CEPH genotype database. In addition, all cases of monosomy X previously diagnosed by conventional cytogenetics presented the anticipated loss of heterozygosity at all loci. We studied 19 spontaneously aborted female fetuses and we found four samples homozygous for the five loci (21%), in good agreement with the expected rate of monosomy X in first trimester spontaneous abortions. We conclude that the loci have high diversity and high efficiency in PCR-amplification and that our multiplex procedure constitutes a simple and useful molecular screening test for monosomy X in abortions and stillbirths.
publishDate 2000
dc.date.issued.fl_str_mv 2000
dc.date.accessioned.fl_str_mv 2016-10-10T03:52:15Z
dc.date.available.fl_str_mv 2016-10-10T03:52:15Z
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dc.identifier.citation.fl_str_mv PEREIRA, Rinaldo Wellerson; STURZENEKER, Rosane; PENA, Sérgio Danilo Junho. Screening fetal losses for monosomy X with a simple PCR-based procedure. Genetics and Molecular Biology, v. 23, n.1, p.11-14, 2000.
dc.identifier.uri.fl_str_mv http://twingo.ucb.br:8080/jspui/handle/10869/453
https://repositorio.ucb.br:9443/jspui/handle/123456789/7658
dc.identifier.issn.none.fl_str_mv 1415-4757
identifier_str_mv PEREIRA, Rinaldo Wellerson; STURZENEKER, Rosane; PENA, Sérgio Danilo Junho. Screening fetal losses for monosomy X with a simple PCR-based procedure. Genetics and Molecular Biology, v. 23, n.1, p.11-14, 2000.
1415-4757
url http://twingo.ucb.br:8080/jspui/handle/10869/453
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