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Mapping translocation breakpoints by next-generation sequencing
Author(s) -
Wei Chen,
Vera M. Kalscheuer,
Andreas Tzschach,
Corinna Menzel,
Reinhard Ullmann,
Marcel H. Schulz,
Fikret Erdogan,
Na Li,
Zofia Kijas,
Ger J. A. Arkesteijn,
I. López Pajares,
Margret Goetz-Sothmann,
Uwe Heinrich,
Imma Rost,
Andreas Dufke,
Ute Grasshoff,
Birgitta Glaeser,
Martin Vingron,
HansHilger Ropers
Publication year - 2008
Publication title -
genome research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 9.556
H-Index - 297
eISSN - 1549-5469
pISSN - 1088-9051
DOI - 10.1101/gr.076166.108
Subject(s) - breakpoint , biology , genetics , bacterial artificial chromosome , chromosomal translocation , computational biology , chromosome , fluorescence in situ hybridization , dna sequencing , multiplex , gene , genome
Balanced chromosome rearrangements (BCRs) can cause genetic diseases by disrupting or inactivating specific genes, and the characterization of breakpoints in disease-associated BCRs has been instrumental in the molecular elucidation of a wide variety of genetic disorders. However, mapping chromosome breakpoints using traditional methods, such as in situ hybridization with fluorescent dye-labeled bacterial artificial chromosome clones (BAC-FISH), is rather laborious and time-consuming. In addition, the resolution of BAC-FISH is often insufficient to unequivocally identify the disrupted gene. To overcome these limitations, we have performed shotgun sequencing of flow-sorted derivative chromosomes using "next-generation" (Illumina/Solexa) multiplex sequencing-by-synthesis technology. As shown here for three different disease-associated BCRs, the coverage attained by this platform is sufficient to bridge the breakpoints by PCR amplification, and this procedure allows the determination of their exact nucleotide positions within a few weeks. Its implementation will greatly facilitate large-scale breakpoint mapping and gene finding in patients with disease-associated balanced translocations.

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