| Literature DB >> 25983246 |
Masoud Zamani Esteki1, Eftychia Dimitriadou1, Ligia Mateiu1, Cindy Melotte1, Niels Van der Aa1, Parveen Kumar1, Rakhi Das1, Koen Theunis1, Jiqiu Cheng2, Eric Legius1, Yves Moreau3, Sophie Debrock4, Thomas D'Hooghe4, Pieter Verdyck5, Martine De Rycke6, Karen Sermon7, Joris R Vermeesch8, Thierry Voet9.
Abstract
Methods for haplotyping and DNA copy-number typing of single cells are paramount for studying genomic heterogeneity and enabling genetic diagnosis. Before analyzing the DNA of a single cell by microarray or next-generation sequencing, a whole-genome amplification (WGA) process is required, but it substantially distorts the frequency and composition of the cell's alleles. As a consequence, haplotyping methods suffer from error-prone discrete SNP genotypes (AA, AB, BB) and DNA copy-number profiling remains difficult because true DNA copy-number aberrations have to be discriminated from WGA artifacts. Here, we developed a single-cell genome analysis method that reconstructs genome-wide haplotype architectures as well as the copy-number and segregational origin of those haplotypes by employing phased parental genotypes and deciphering WGA-distorted SNP B-allele fractions via a process we coin haplarithmisis. We demonstrate that the method can be applied as a generic method for preimplantation genetic diagnosis on single cells biopsied from human embryos, enabling diagnosis of disease alleles genome wide as well as numerical and structural chromosomal anomalies. Moreover, meiotic segregation errors can be distinguished from mitotic ones.Entities:
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Year: 2015 PMID: 25983246 PMCID: PMC4473724 DOI: 10.1016/j.ajhg.2015.04.011
Source DB: PubMed Journal: Am J Hum Genet ISSN: 0002-9297 Impact factor: 11.025