1988
DOI: 10.1016/0378-1119(88)90425-8
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A simple and rapid method for the selection of oligodeoxynucleotide-directed mutants

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Cited by 293 publications
(157 citation statements)
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“…[34] Mutations were introduced by PCR using the QuikChange TM site-directed mutagenesis kit from Stratagene according to the manufacturer's protocol. [43] High level protein expression was achieved using a slightly modified version of the protocol already published. [34] By incubating the starter culture for only 4 h, using terrific broth (TB)-medium for expression and prolonging cultivation time after induction to 16 h at 25°C, 800 to 1200 nmol (96 to 144 mg) of soluble CYP102A1 per litre of cell culture were obtained.…”
Section: Design Of Nadh-dependent Reductase Mutantsmentioning
confidence: 99%
“…[34] Mutations were introduced by PCR using the QuikChange TM site-directed mutagenesis kit from Stratagene according to the manufacturer's protocol. [43] High level protein expression was achieved using a slightly modified version of the protocol already published. [34] By incubating the starter culture for only 4 h, using terrific broth (TB)-medium for expression and prolonging cultivation time after induction to 16 h at 25°C, 800 to 1200 nmol (96 to 144 mg) of soluble CYP102A1 per litre of cell culture were obtained.…”
Section: Design Of Nadh-dependent Reductase Mutantsmentioning
confidence: 99%
“…Construction of point mutations in the core of attI by site-directed mutagenesis Directed point mutations in attI were introduced by the hemimethylation protection method described by Vandeyar et al (1988) in the integron fragment of plasmid 2273 cloned in M13mp18 or M13mp19, using synthetic degenerate mutagenesis primers according to Table 5. Three mutants out of each experiment were selected after sequencing 24 clones.…”
Section: Construction Of Deletion Mutationsmentioning
confidence: 99%
“…JM101 [A(lac-proAB)supE thi F'(traD36 proA +B+ lacIVZAM15)] (10) was used for cloning and propagating M13 derivatives. SDM [hsdRl7 mcrAB recAl supE44 Tetr A(lac-proAB) F'(traD36 proA+B+ lacIVZAM15)] was used to grow M13 derivatives which had undergone mutagenesis as described by Vandeyar et al (22). JP3923 (thr-1 leuB6 thi-1 lacZAM15 lacYl gal-351 supE44 tonA21 hsdR4 gyrA379 rpsL743 recA56 srl-1300::TnJO aroL513) was used for all f-galactosidase assays.…”
mentioning
confidence: 99%