PKSS - A 2ND-GENERATION GENERAL-PURPOSE CLONING VECTOR FOR EFFICIENT POSITIVE SELECTION OF RECOMBINANT CLONES

被引：81

作者：

KAST, P ^{[1
]}

机构：

[1] ETH ZENTRUM,LFV,INST MIKROBIOL,CH-8092 ZURICH,SWITZERLAND

来源：

GENE | 1994年 / 138卷 / 1-2期

关键词：

ALTERED SUBSTRATE SPECIFICITY; AMPICILLIN RESISTANCE; DIRECT SELECTION PLASMIC; ESCHERICHIA COLI HOST STRAIN INDEPENDENCE; PBLUSCRIPT; P-CHLORO-PHENYLALANINE SENSITIVITY; PHENYLALANYL-TRANSFER-RNA SYNTHETASE;

D O I：

10.1016/0378-1119(94)90790-0

中图分类号：

Q3 [遗传学];

学科分类号：

071007 ; 090102 ;

摘要：

A new small plasmid vector (pKSS) for the direct selection of insert-containing plasmid clones is presented. The selection strategy is based on the acquired sensitivity of Escherichia coli cells to p-chloro-phenylalanine (p-Cl-Phe) if they carry a pheS allele encoding a phenylalanyl-tRNA synthetase alpha subunit with relaxed substrate specificity. This pheS allele is present on pKSS. Insertion into, or replacement of, the plasmidial pheS gene by a cloned fragment enables transformed pheS wild-type cells to survive on agar plates containing p-Cl-Phe plus ampicillin. This host strain-independent positive selection of recombinant clones proved to be highly efficient (>99%) and did not require purification of the vector fragment prior to cloning. The high-copy-number vector pKSS offers a multitude of restriction sites and all of the features for analysis of cloned fragments that stem from the cloning vector pBluescript (Stratagene, La Jolla, CA, USA). Thus, pKSS represents a valuable alternative to previously reported positive-selection vectors; it should prove particularly useful for cloning when expecting a high fraction of cells transformed with non-recombinant vector, and for construction of DNA libraries.

引用

页码：109 / 114

页数：6

共 32 条

[1]

ALTENBUCHNER J, 1992, METHOD ENZYMOL, V216, P457

[2]

ALTINGMEES MA, 1992, METHOD ENZYMOL, V216, P483

[3] PLASMID VECTOR PBR322 AND ITS SPECIAL-PURPOSE DERIVATIVES - A REVIEW [J].

BALBAS, P ;

SOBERON, X ;

MERINO, E ;

ZURITA, M ;

LOMELI, H ;

VALLE, F ;

FLORES, N ;

BOLIVAR, F .

GENE, 1986, 50 (1-3) :3-40

[4] GENBANK [J].

BENSON, D ;

LIPMAN, DJ ;

OSTELL, J .

NUCLEIC ACIDS RESEARCH, 1993, 21 (13) :2963-2965

[5] ALLELIC EXCHANGE IN ESCHERICHIA-COLI USING THE BACILLUS-SUBTILIS SACB GENE AND A TEMPERATURE-SENSITIVE PSC101 REPLICON [J].

BLOMFIELD, IC ;

VAUGHN, V ;

REST, RF ;

EISENSTEIN, BI .

MOLECULAR MICROBIOLOGY, 1991, 5 (06) :1447-1457

[6] CONSTRUCTION AND CHARACTERIZATION OF NEW CLONING VEHICLES .2. MULTIPURPOSE CLONING SYSTEM [J].

BOLIVAR, F ;

RODRIGUEZ, RL ;

GREENE, PJ ;

BETLACH, MC ;

HEYNEKER, HL ;

BOYER, HW ;

CROSA, JH ;

FALKOW, S .

GENE, 1977, 2 (02) :95-113

[7] A COMPLEMENTATION ANALYSIS OF RESTRICTION AND MODIFICATION OF DNA IN ESCHERICHIA COLI [J].

BOYER, HW ;

ROULLAND.D .

JOURNAL OF MOLECULAR BIOLOGY, 1969, 41 (03) :459-&

[8]

BROSIUS J, 1992, METHOD ENZYMOL, V216, P469

[9] ESTABLISHMENT OF A GENOMIC BANK OF BOVINE HERPESVIRUS-1 USING A NOVEL POSITIVE SELECTION PLASMID VECTOR [J].

CHRISTENSEN, LS ;

BOYE, M .

JOURNAL OF VIROLOGICAL METHODS, 1992, 36 (03) :277-282

[10] A PLASMID CLONING VECTOR FOR THE DIRECT SELECTION OF STRAINS CARRYING RECOMBINANT PLASMIDS [J].

DEAN, D .

GENE, 1981, 15 (01) :99-102

← 1 2 3 4 →