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Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR

The analysis of rare cells is not an easy task. This is especially true when cells representing a fetal microchimerism are to be utilized for the purpose of non-invasive prenatal diagnosis because it is both imperative and difficult to avoid contaminating the minority of fetal cells with maternal on...

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Autores principales: Kroneis, Thomas, Gutstein-Abo, Liat, Kofler, Kristina, Hartmann, Michaele, Hartmann, Petra, Alunni-Fabbroni, Marianna, Walcher, Wolfgang, Dohr, Gottfried, Petek, Erwin, Guetta, Esther, Sedlmayr, Peter
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Blackwell Publishing Ltd 2010
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3823127/
https://www.ncbi.nlm.nih.gov/pubmed/19453769
http://dx.doi.org/10.1111/j.1582-4934.2009.00784.x
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author Kroneis, Thomas
Gutstein-Abo, Liat
Kofler, Kristina
Hartmann, Michaele
Hartmann, Petra
Alunni-Fabbroni, Marianna
Walcher, Wolfgang
Dohr, Gottfried
Petek, Erwin
Guetta, Esther
Sedlmayr, Peter
author_facet Kroneis, Thomas
Gutstein-Abo, Liat
Kofler, Kristina
Hartmann, Michaele
Hartmann, Petra
Alunni-Fabbroni, Marianna
Walcher, Wolfgang
Dohr, Gottfried
Petek, Erwin
Guetta, Esther
Sedlmayr, Peter
author_sort Kroneis, Thomas
collection PubMed
description The analysis of rare cells is not an easy task. This is especially true when cells representing a fetal microchimerism are to be utilized for the purpose of non-invasive prenatal diagnosis because it is both imperative and difficult to avoid contaminating the minority of fetal cells with maternal ones. Under these conditions, even highly specific biochemical markers are not perfectly reliable. We have developed a method to verify the genomic identity of rare cells that combines automatic screening for enriched target cells (based on immunofluorescence labelling) with isolation of single candidate microchimeric cells (by laser microdissection and subsequent laser catapulting) and low-volume on-chip multiplex PCR for DNA fingerprint analysis. The power of the method was tested using samples containing mixed cells of related and non-related individuals. Single-cell DNA fingerprinting was successful in 74% of the cells analysed (55/74), with a PCR efficiency of 59.2% (860/1452) for heterozygous loci. The identification of cells by means of DNA profiling was achieved in 100% (12/12) of non-related cells in artificial mixtures and in 86% (37/43) of cells sharing a haploid set of chromosomes and was performed on cells enriched from blood and cells isolated from tissue. We suggest DNA profiling as a standard for the identification of microchimerism on a single-cell basis.
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spelling pubmed-38231272015-04-20 Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR Kroneis, Thomas Gutstein-Abo, Liat Kofler, Kristina Hartmann, Michaele Hartmann, Petra Alunni-Fabbroni, Marianna Walcher, Wolfgang Dohr, Gottfried Petek, Erwin Guetta, Esther Sedlmayr, Peter J Cell Mol Med Articles The analysis of rare cells is not an easy task. This is especially true when cells representing a fetal microchimerism are to be utilized for the purpose of non-invasive prenatal diagnosis because it is both imperative and difficult to avoid contaminating the minority of fetal cells with maternal ones. Under these conditions, even highly specific biochemical markers are not perfectly reliable. We have developed a method to verify the genomic identity of rare cells that combines automatic screening for enriched target cells (based on immunofluorescence labelling) with isolation of single candidate microchimeric cells (by laser microdissection and subsequent laser catapulting) and low-volume on-chip multiplex PCR for DNA fingerprint analysis. The power of the method was tested using samples containing mixed cells of related and non-related individuals. Single-cell DNA fingerprinting was successful in 74% of the cells analysed (55/74), with a PCR efficiency of 59.2% (860/1452) for heterozygous loci. The identification of cells by means of DNA profiling was achieved in 100% (12/12) of non-related cells in artificial mixtures and in 86% (37/43) of cells sharing a haploid set of chromosomes and was performed on cells enriched from blood and cells isolated from tissue. We suggest DNA profiling as a standard for the identification of microchimerism on a single-cell basis. Blackwell Publishing Ltd 2010-04 2009-05-19 /pmc/articles/PMC3823127/ /pubmed/19453769 http://dx.doi.org/10.1111/j.1582-4934.2009.00784.x Text en © 2009 The Authors Journal compilation © 2010 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
spellingShingle Articles
Kroneis, Thomas
Gutstein-Abo, Liat
Kofler, Kristina
Hartmann, Michaele
Hartmann, Petra
Alunni-Fabbroni, Marianna
Walcher, Wolfgang
Dohr, Gottfried
Petek, Erwin
Guetta, Esther
Sedlmayr, Peter
Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR
title Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR
title_full Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR
title_fullStr Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR
title_full_unstemmed Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR
title_short Automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex PCR
title_sort automatic retrieval of single microchimeric cells and verification of identity by on-chip multiplex pcr
topic Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3823127/
https://www.ncbi.nlm.nih.gov/pubmed/19453769
http://dx.doi.org/10.1111/j.1582-4934.2009.00784.x
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