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用于摇瓶高密度培养的自诱导培养基
12/20/07
Recipes and stock solutions described in Protein Expression and Purification 41: 207-234 (2005)
Protein Production by Auto-Induction in High-Density Shaking Cultures
F. William Studier
Biology Department, Brookhaven National Laboratory, Upton, NY 11973
studier@bnl.gov
Abstract. Inducible expression systems in which T7 RNA polymerase transcribes
coding sequences cloned under control of a T7lac promoter efficiently produce a wide variety of
proteins in Escherichia coli. Investigation of factors that affect stability, growth and induction of
T7 expression strains in shaking vessels led to the recognition that sporadic, unintended
induction of expression in complex media, previously reported by others, is almost certainly
caused by small amounts of lactose. Glucose prevents induction by lactose by well-studied
mechanisms. Amino acids also inhibit induction by lactose during log-phase growth, and high
rates of aeration inhibit induction at low lactose concentrations. These observations, and
metabolic balancing of pH, allowed development of reliable non-inducing and auto-inducing
media in which batch cultures grow to high densities. Expression strains grown to saturation in
non-inducing media retain plasmids and remain fully viable for weeks in the refrigerator, making
it easy to prepare many freezer stocks in parallel and use working stocks for an extended period.
Auto-induction allows efficient screening of many clones in parallel for expression and
solubility, as cultures have only to be inoculated and grown to saturation, and yields of target
protein are typically several-fold higher than obtained by conventional IPTG induction. Auto-
inducing media have been developed for labeling proteins with selenomethioni
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