Cloning of bacteriophage fd gene 2 and construction of a plasmid dependent on fd gene 2 protein. | Zendy

Thomas F. Meyer | Zendy; Klaus Geider | Zendy

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Cloning of bacteriophage fd gene 2 and construction of a plasmid dependent on fd gene 2 protein.

Author(s) -

Thomas F. Meyer,

Klaus Geider

Publication year - 1981

Publication title -

proceedings of the national academy of sciences

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 5.011

H-Index - 771

eISSN - 1091-6490

pISSN - 0027-8424

DOI - 10.1073/pnas.78.9.5416

Subject(s) - plasmid , replicon , biology , bacteriophage , microbiology and biotechnology , phagemid , gene , cloning vector , origin of replication , in vitro recombination , dna replication , cloning (programming) , genetics , molecular cloning , gene expression , escherichia coli , computer science , programming language

Bacteriophage fd gene 2 was cloned in plasmid pBR325. Cells carrying the hybrid plasmid produce about 200 times more enzymatically active fd gene 2 protein than did cells infected with phage fd wild type, as measured by replication of phage fd replicative form I in vitro. Cloned gene 2 supports replication of an artificial phage fd miniplasmid consisting of the origin of bacteriophage fd replication and a gene coding for kanamycin resistance. This plasmid occurs in high copy numbers and is viable only in cells carrying the cloned fd gene 2 or in cells infected with phage fd. Because the miniplasmid is not propagated in natural hosts, it can be considered a safe cloning vector. Its fusion with the gene 2 hybrid plasmid provides an autonomous replicon independent of the polA function of the host cell. fd gene 2 is the only phage-encoded trans-acting function required for replication of double-stranded fd DNA in vivo.

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