COMPLEMENT-STABILIZED D-LOOP - RECA-CATALYZED STABLE PAIRING OF LINEAR DNA-MOLECULES AT INTERNAL SITES

被引:28
作者
JAYASENA, VK [1 ]
JOHNSTON, BH [1 ]
机构
[1] SRI INT,CELL & MOLEC BIOL LAB,333 RAVENSWOOD AVE,MENLO PK,CA 94025
关键词
4-STRANDED COMPLEXES; HOMOLOGOUS BASE-PAIRING; DNA TARGETING;
D O I
10.1006/jmbi.1993.1216
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The RecA protein (RecA) of Escherichia coli has the ability to pair a single-stranded DNA to a homologous sequence in a duplex DNA without requiring denaturation of the duplex. This ability has stimulated interest in the use of RecA for targeting probes to genomic DNA. However, because pairing generally requires that the double-stranded DNA either have a homologous end or be negatively supercoiled, the application of RecA to targeting has been very limited. Here, we show that if the sequence complementary to the probe is also included in the reaction, RecA can pair the two single strands to sites distant from any ends on linear DNA. The resulting structure, termed a complement-stabilized D-loop (csD-loop), is cleavable by restriction endonucleases and, upon removal of RecA, remains stable to temperatures up to the t(m) of the double-stranded probe. These results indicate that the csD-loop probably consists of two side-by-side Watson-Crick duplexes, much like a replication bubble. This novel reaction of RecA may be useful in gene mapping and isolation, as well as in sequence-specific cleavage of genomic DNA, and might have functions in vivo. © 1993 Academic Press Limited.
引用
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页码:1015 / 1024
页数:10
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