BACTERIOPHAGE-P1 CLONING SYSTEM FOR THE ISOLATION, AMPLIFICATION, AND RECOVERY OF DNA FRAGMENTS AS LARGE AS 100 KILOBASE PAIRS

被引：220

作者：

STERNBERG, N

机构：

来源：

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA | 1990年 / 87卷 / 01期

关键词：

DNA packaging; gene isolation; genome mapping; pac cleavage;

D O I：

10.1073/pnas.87.1.103

中图分类号：

O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];

学科分类号：

07 ; 0710 ; 09 ;

摘要：

The development of a bacteriophage P1 cloning system capable of accepting DNA fragments as large as 100 kilobase pairs (kbp) is described. The vectors used in this system contain a P1 packaging site (pac) to package vector and cloned DNA into phage particles, two P1 loxP recombination sites to cyclize the packaged DNA once it has been injected into a strain of Escherichia coli containing the P1 Cre recombinase, a kan(r) gene to select bacterial clones containing the cyclized DNA, a P1 plasmid replicon to stably maintain that DNA in E. coli at one copy per cell chromosome, and a lac promoter-regulated P1 lytic replicon to amplify the DNA before it is reisolated. An essential feature of the cloning system is a two-stage in vitro packaging reaction that packages vector DNA containing cloned inserts into phage particles that can deliver their DNA to E. coli with near unit efficiency. The packaging reaction can generate 105 clones with high molecular weight DNA inserts per μg of vector DNA. Using Not I fragments from E. coli DNA, it was shown that the system can clone 95- and 100-kbp fragments but not a 106-kbp fragment. Presumably, the combined size of the latter fragment and the vector DNA (13 kbp) exceeds the headful capacity of P1.

引用

页码：103 / 107

页数：5

共 26 条

[1] STUDIES ON THE PROPERTIES OF P1 SITE-SPECIFIC RECOMBINATION - EVIDENCE FOR TOPOLOGICALLY UNLINKED PRODUCTS FOLLOWING RECOMBINATION
ABREMSKI, K
HOESS, R
STERNBERG, N
[J]. CELL, 1983, 32 (04) : 1301 - 1311
[2] AUSTIN S, 1982, J BACTERIOL, V152, P63
[3] BIRNBOIM HC, 1979, NUCLEIC ACIDS RES, V7, P1513
[4] CLONING OF LARGE SEGMENTS OF EXOGENOUS DNA INTO YEAST BY MEANS OF ARTIFICIAL CHROMOSOME VECTORS
BURKE, DT
CARLE, GF
OLSON, MV
[J]. SCIENCE, 1987, 236 (4803) : 806 - 812
[5] ELECTROPHORETIC SEPARATIONS OF LARGE DNA-MOLECULES BY PERIODIC INVERSION OF THE ELECTRIC-FIELD
CARLE, GF
FRANK, M
OLSON, MV
[J]. SCIENCE, 1986, 232 (4746) : 65 - 68
[6] GENETIC-ANALYSIS OF THE LYTIC REPLICON OF BACTERIOPHAGE-P1 .1. ISOLATION AND PARTIAL CHARACTERIZATION
COHEN, G
STERNBERG, N
[J]. JOURNAL OF MOLECULAR BIOLOGY, 1989, 207 (01) : 99 - 109
[7] DIRECTIONAL CLONING OF DNA FRAGMENTS AT A LARGE DISTANCE FROM AN INITIAL PROBE - A CIRCULARIZATION METHOD
COLLINS, FS
WEISSMAN, SM
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1984, 81 (21): : 6812 - 6816
[8] A GENETIC-LINKAGE MAP OF THE HUMAN GENOME
DONISKELLER, H
GREEN, P
HELMS, C
CARTINHOUR, S
WEIFFENBACH, B
STEPHENS, K
KEITH, TP
BOWDEN, DW
SMITH, DR
LANDER, ES
BOTSTEIN, D
AKOTS, G
REDIKER, KS
GRAVIUS, T
BROWN, VA
RISING, MB
PARKER, C
POWERS, JA
WATT, DE
KAUFFMAN, ER
BRICKER, A
PHIPPS, P
MULLERKAHLE, H
FULTON, TR
NG, S
SCHUMM, JW
BRAMAN, JC
KNOWLTON, RG
BARKER, DF
CROOKS, SM
LINCOLN, SE
DALY, MJ
ABRAHAMSON, J
[J]. CELL, 1987, 51 (02) : 319 - 337
[9] CONTROL OF HOST-INDUCED MODIFICATION BY PHAGE P1
GLOVER, SW
SCHELL, J
SYMONDS, N
STACEY, KA
[J]. GENETICS RESEARCH, 1963, 4 (03) : 480 - +
[10] ROLE OF IS1 IN THE FORMATION OF HYBRIDS BETWEEN THE BACTERIOPHAGE-P1 AND THE R-PLASMID NR1
IIDA, S
ARBER, W
[J]. MOLECULAR AND GENERAL GENETICS, 1980, 177 (02): : 261 - 270

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