Alu-PCR: Characterization of a chromosome 6-specific hybrid mapping panel and cloning of chromosome-specific markers

The Alu-polymerase chain reaction ( Alu-PCR) was applied to selectively amplify DNA sequences from human chromosome 6 using a single primer (A1) directed to the human Alu consensus sequence. A specific amplification pattern was demonstrated for a panel of eight somatic cell hybrids containing differ...

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Veröffentlicht in:Genomics (San Diego, Calif.) Calif.), 1992-03, Vol.12 (3), p.549-554
Hauptverfasser: Meese, Eckart U., Meltzer, Paul S., Ferguson, Paul W., Trent, Jeffrey M.
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Sprache:eng
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Zusammenfassung:The Alu-polymerase chain reaction ( Alu-PCR) was applied to selectively amplify DNA sequences from human chromosome 6 using a single primer (A1) directed to the human Alu consensus sequence. A specific amplification pattern was demonstrated for a panel of eight somatic cell hybrids containing different portions of chromosome 6. This PCR pattern permits the identification of submicroscopic DNA alterations and can be utilized as a reference for additional chromosome 6-specific hybrids. To obtain new chromosome 6-specific markers we established two libraries from PCR-amplified sequences using two somatic cell hybrids (MCH381.2D and 640-5A). Out of a total of 109 clones that were found to be chromosome 6 specific, 13 clones were regionally assigned. We also included a procedure that allows the isolation of chromosome 6-specific markers from hybrids that contain human chromosomes other than 6. Our results will contribute to the molecular characterization of chromosome 6 by fostering characterization of somatic cell hybrids and by the generation of new regicnally assigned DNA markers.
ISSN:0888-7543
1089-8646
DOI:10.1016/0888-7543(92)90447-Z