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      Direct cloning of human 10q25 neocentromere DNA using transformation-associated recombination (TAR) in yeast.

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          Abstract

          The transformation-associated recombination (TAR) procedure allows rapid, site-directed cloning of specific human chromosomal regions as yeast artificial chromosomes (YACs). The procedure requires knowledge of only a single, relatively small genomic sequence that resides adjacent to the chromosomal region of interest. We applied this approach to the cloning of the neocentromere DNA of a marker chromosome that we have previously shown to have originated through the activation of a latent centromere at human chromosome 10q25. Using a unique 1.4-kb DNA fragment as a "hook" in TAR experiments, we achieved single-step isolation of the critical neocentromere DNA region as two stable, 110- and 80-kb circular YACs. For obtaining large quantities of highly purified DNA, these YACs were retrofitted with the yeast-bacteria-mammalian-cells shuttle vector BRV1, electroporated into Escherichia coli DH10B, and isolated as bacterial artificial chromosomes (BACs). Extensive characterization of these YACs and BACs by PCR and restriction analyses revealed that they are identical to the corresponding regions of the normal chromosome 10 and provided further support for the formation of the neocentromere within the marker chromosome through epigenetic activation.

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          Author and article information

          Journal
          Genomics
          Genomics
          Elsevier BV
          0888-7543
          0888-7543
          Feb 01 1998
          : 47
          : 3
          Affiliations
          [1 ] The Murdoch Institute for Research into Birth Defects, Royal Children's Hospital, Flemington Road, Parkville, 3052, Australia.
          Article
          S0888-7543(97)95129-6
          10.1006/geno.1997.5129
          9480754
          46433a19-b234-4e51-8167-628dc848983a
          Copyright 1998 Academic Press.
          History

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