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J. Biol. Chem., Vol. 264, Issue 14, 7821-7825, 05, 1989
SB Jovanovich, MT Record Jr and RR Burgess
We have studied the in vitro expression of the osmoregulated proU promoter
in Escherichia coli coupled transcription-translation (S-30) extracts as a
function of the osmolality of the culture medium used to grow the cells and
of the salt concentration added to the extract. These variables represent
novel extensions of the use of S-30 extracts to investigate gene regulatory
phenomena in vitro. The concentrations of potassium acetate and of the
physiologically relevant osmolyte potassium glutamate for maximal
expression of the proU promoter are approximately 2-fold higher than the
concentrations of these salts providing maximal expression of the lacUV5
promoter. The relative promoter activity of proU with respect to lacUV5
increases more than 30- fold with an increase in salt concentration from 50
to 300 mM. In comparative studies with S-30 extracts prepared from cells
grown at high and low osmolalities, we find that at fixed salt
concentrations expression of proU is increased 10-fold in the S-30 extract
prepared from high osmolality-grown cells, whereas the expression of lacUV5
is increased less than 2-fold. Addition of anti-sigma 70 monoclonal
antibodies or purified sigma 70 to the S-30 extract demonstrated that the
major proU promoter(s) used in the S-30 extracts is sigma 70- dependent.
In an Escherichia coli coupled transcription-translation system, expression of the osmoregulated gene proU is stimulated at elevated potassium concentrations and by an extract from cells grown at high osmolality
McArdle Laboratory for Cancer Research, University of Wisconsin, Madison 53706.
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