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Mechanism of lac repressor function EMBO J 2011
Mechanism of transcriptional repression at a
bacterial promoter by analysis of single molecules
Alvaro Sanchez1,4, Melisa L Osborne2,
Larry J Friedman2, Jane Kondev3,*
and Jeff Gelles2,*
1Graduate program in Biophysics and Structural Biology, Brandeis
University, Waltham, MA, USA, 2Department of Biochemistry, Brandeis
University, Waltham, MA, USA and 3Department of Physics, Brandeis
University, Waltham, MA, USA
The molecular basis for regulation of lactose metabolism
in Escherichia coli is well studied. Nonetheless, the physi-
cal mechanism by which the Lac repressor protein pre-
vents transcription of the lactose promoter remains
unresolved. Using multi-wavelength single-molecule
fluorescence microscopy, we visualized individual com-
plexes of fluorescently tagged RNA polymerase holoen-
zyme bound to promoter DNA. Quantitative analysis of the
single-molecule observations, including use of a novel
statistical partitioning approach, reveals highly kinetically
stable binding of polymerase to two different sites on the
DNA, only one of which leads to transcription. Addition of
Lac repressor directly demonstrates that bound repressor
prevents the formation of transcriptionally productive
open promoter complexes; discrepancies in earlier studies
may be attributable to transcriptionally inactive polymer-
ase binding. The single-molecule statistical partitioning
approach is broadly applicable to elucidating mechanisms
of regulatory systems including those that are kinetically
rather than thermodynamically controlled.
The EMBO Journal (2011) 30, 3940–3946. doi:10.1038/
emboj.2011.273; Published online 9 August 2011
Subject Categories: chromatin transcription
Keywords: Lac promoter; open complexes; single-molecule
imaging
Introduction
In all organisms, messenger RNAs are synthesized by a multi-
subunit RNA polymerase (RNAP) that binds to promoter
regions of DNA, separates the DNA strands to form an ‘open’
promoter complex and then escapes from the promoter,
moving along the
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