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Titlebook: Gene Isolation and Mapping Protocols; Jacqueline Boultwood Book 1997 Humana Press 1997

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Use of Dinucleotide Polymorphism Analyses in Physical Mapping,ld be as frequent as one in approximately every 30–40 kb of the human genome. Thus, the entire genome can be represented by a large number of dC-dA or dG-dT repeat sequences. The repeat elements vary in size and can be analyzed by polymerase chain reaction (PCR) using unique primers; the high degree
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Mapping Expressed Sequence Tags (ESTs) by Multiplexing PCR Reactions from Hybrid Cell Panels and De.). Positional cloning of disease genes requires that previously uncharacterized transcripts be mapped to the smallest possible defined region. We have developed an efficient polymerase chain reaction (PCR)-based procedure for the rapid assignment of ESTs to human chromosome regions (.–.; .). The cr
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Isolation of Coding Sequences from Genomic Regions Using Direct Selection,ysis of mutations in these genes. Direct selection is an expression-based gene identification technique that can rapidly identify cDNAs within large genomic regions. It has been successfully used in numerous positional cloning projects (.–.). It can capture cDNAs that are expressed, temporally and s
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Gene Mapping and Isolation, differences will explain the nature of the variants. In practice, this is a daunting task in a genome the size of human (3000 Mb) and may take many years to achieve. Genome mapping and sequencing projects invert the problem by attempting the systematic discovery and ordering of all genes over a per
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