RAPID ISOLATION OF HUMAN CHROMOSOME-SPECIFIC DNA PROBES FROM A SOMATIC-CELL HYBRID

被引：74

作者：

COTTER, FE ^{[1
]}

HAMPTON, GM ^{[1
]}

NASIPURI, S ^{[1
]}

BODMER, WF ^{[1
]}

YOUNG, BD ^{[1
]}

机构：

[1] IMPERIAL CANC RES FUND,DIRECTORS LAB,LONDON WC2A,ENGLAND

来源：

GENOMICS | 1990年 / 7卷 / 02期

关键词：

D O I：

10.1016/0888-7543(90)90548-9

中图分类号：

Q81 [生物工程学（生物技术）]; Q93 [微生物学];

学科分类号：

071005 ; 0836 ; 090102 ; 100705 ;

摘要：

A strategy for the rapid isolation from rodent hybrids of human chromosome-specific probes by enzymatic amplification is described. Synthetic oligonucleotide primers based on the consensus Alu sequence were used to amplify inter-Alu sequence from total human genomic DNA and from a somatic cell hybrid, PNTS-1, containing one homolog of chromosome 5 as its only human complement. Direct sequence analysis of the products from human genomic DNA confirmed their inter-Alu structure and provided a novel means for the examination of the 5′ end of the Alu consensus. The amplified sequences from the somatic cell hybrid DNA were cloned into a plasmid vector by blunt-end ligation, yielding clones with inserts in the range 300 to 1000 bp. More than 80% of these clones carried inserts that behaved essentially as single-copy human sequences. Hybridization of a selection of these clones to human DNA, hamster DNA, and the original hybrid DNA confirmed that they were derived from chromosome 5. Direct sequence analysis of the vector/insert boundaries in two clones confirmed that inter-Alu sequences had been cloned. This approach has significant advantages over other methods of isolating chromosome-specific probes from hybrid cells, enabling direct separation and cloning of human DNA probes that can be readily used for mapping studies. © 1990.

引用

页码：257 / 263

页数：7

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