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Direct Cloning of Human Transcripts with HnRNA from Hybrid Cell Lines

1990; American Association for the Advancement of Science; Volume: 249; Issue: 4969 Linguagem: Inglês

10.1126/science.2382140

1095-9203

Laura Corbo, Julie A. Maley, David L. Nelson, C. Thomas Caskey,

CRISPR and Genetic Engineering

A library of human-derived complementary DNA from a human-hamster hybrid cell line containing the Xq24-qter region has been constructed. Complementary DNA synthesis was primed from heterogeneous nuclear (hn) RNA by oligonucleotides derived from conserved regions of human Alu repeats. At least 80% of these cloned sequences were of human origin, providing an enrichment of at least two orders of magnitude. Two clones, one containing a fragment of the primary transcript of the human hypoxanthine-guanine phosphoribosyltransferase (HPRT) gene at Xq26 and another recognizing a family of human genes mapping to two regions of Xq24-qter, were characterized. Additional hncDNA clones mapped to a variety of sites in the Xq24-qter region, demonstrating the isolation of many transcriptionally active loci. These clones provide probes for identification of genetic loci on the terminal region of the X chromosome long arm, which is the location of a number of inherited disorders.