Construction and characterization of new cloning vehicles I. Ampicillin-resistant derivatives of the plasmid pMB9

Construction and characterization of new cloning vehicles I. Ampicillin-resistant derivatives of the plasmid pMB9

In vitro recombination via restriction endonucleases and the in vivo genetic translocation of the Ap resistance (Apr) gene resulted in the construction of a new cloning vehicle, the plasmid pBR313. This vector was derived from a ColE1-like plasmid and, while it does not produce colicon E1, it still...

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Veröffentlicht in:Gene 1977, Vol.2 (2), p.75-91
Hauptverfasser: Bolivar, Francisco, Rodriguez, Raymond L., Betlach, Mary C., Boyer, Herbert W.
Format: Artikel
Sprache:eng
Schlagworte:
Ampicillin - pharmacology
DNA Restriction Enzymes - metabolism
DNA, Bacterial - analysis
DNA, Recombinant
Escherichia coli - genetics
Molecular Weight
R Factors
Tetracycline - pharmacology
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container_end_page 91
container_issue 2
container_start_page 75
container_title Gene
container_volume 2
creator Bolivar, Francisco
Rodriguez, Raymond L.
Betlach, Mary C.
Boyer, Herbert W.
description In vitro recombination via restriction endonucleases and the in vivo genetic translocation of the Ap resistance (Apr) gene resulted in the construction of a new cloning vehicle, the plasmid pBR313. This vector was derived from a ColE1-like plasmid and, while it does not produce colicon E1, it still retains colicin E1 immunity. The Apr and tetracycline resistance (Tcr) markers carried in pBR313 were derived from the ampicillin transposon (TnA) of pRSF2124 and pSC101 respectively. During the construction of pBR313, the TnA component was altered and the Apr gene in pBR313 can no longer be translocated. This plasmid has a molecular weight of 5.8 Mdalton and has been characterized using thirteen restriction enzymes, six of which (EcoRI, SmaI, HpaI, HindIII, BamHI and SalI) cleave the plasmid at unique restriction sites. This allows the molecular cloning of DNA fragments generated by these six enzymes. The restriction sites for the latter three enzymes, HindIII, BamHI and SalI, are located in the Tcr gene(s). Cloning DNA fragments into these sites alters the expression of the Tcr mechanisms thus providing a selection for cells carrying recombinant plasmid molecules. An enrichment method for AprTcS cells carrying recombinant plasmid molecules is described.
doi_str_mv 10.1016/0378-1119(77)90074-9
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source MEDLINE; Elsevier ScienceDirect Journals
subjects Ampicillin - pharmacology
DNA Restriction Enzymes - metabolism
DNA, Bacterial - analysis
DNA, Recombinant
Escherichia coli - genetics
Molecular Weight
R Factors
Tetracycline - pharmacology
title Construction and characterization of new cloning vehicles I. Ampicillin-resistant derivatives of the plasmid pMB9
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