AUTHOR=Santillán Orlando , Ramírez-Romero Miguel A. , Lozano Luis , Checa Alberto , Encarnación Sergio M. , Dávila Guillermo 

TITLE=Region 4 of Rhizobium etli Primary Sigma Factor (SigA) Confers Transcriptional Laxity in Escherichia coli

JOURNAL=Frontiers in Microbiology

VOLUME=7

YEAR=2016

URL=https://www.frontiersin.org/journals/microbiology/articles/10.3389/fmicb.2016.01078

DOI=10.3389/fmicb.2016.01078

ISSN=1664-302X

ABSTRACT=<p>Sigma factors are RNA polymerase subunits engaged in promoter recognition and DNA strand separation during transcription initiation in bacteria. Primary sigma factors are responsible for the expression of <italic>housekeeping</italic> genes and are essential for survival. RpoD, the primary sigma factor of <italic>Escherichia coli</italic>, a γ-proteobacteria, recognizes consensus promoter sequences highly similar to those of some α-proteobacteria species. Despite this resemblance, RpoD is unable to sustain transcription from most of the α-proteobacterial promoters tested so far. In contrast, we have found that SigA, the primary sigma factor of <italic>Rhizobium etli</italic>, an α-proteobacteria, is able to transcribe <italic>E. coli</italic> promoters, although it exhibits only 48% identity (98% coverage) to RpoD. We have called this the <italic>transcriptional laxity phenomenon</italic>. Here, we show that SigA partially complements the thermo-sensitive deficiency of RpoD285 from <italic>E</italic>. <italic>coli</italic> strain UQ285 and that the SigA region σ4 is responsible for this phenotype. Sixteen out of 74 residues (21.6%) within region σ4 are variable between RpoD and SigA. Mutating these residues significantly improves SigA ability to complement <italic>E</italic>. <italic>coli</italic> UQ285. Only six of these residues fall into positions already known to interact with promoter DNA and to comprise a helix-turn-helix motif. The remaining variable positions are located on previously unexplored sites inside region σ4, specifically into the first two α-helices of the region. Neither of the variable positions confined to these helices seem to interact directly with promoter sequence; instead, we adduce that these residues participate allosterically by contributing to correct region folding and/or positioning of the HTH motif. We propose that transcriptional laxity is a mechanism for ensuring transcription in spite of naturally occurring mutations from endogenous promoters and/or horizontally transferred DNA sequences, allowing survival and fast environmental adaptation of α-proteobacteria.</p>