Image_1_Regulation of R1 Plasmid Transfer by H-NS, ArcA, TraJ, and DNA Sequence Elements.JPEG (382.51 kB)

Image_1_Regulation of R1 Plasmid Transfer by H-NS, ArcA, TraJ, and DNA Sequence Elements.JPEG

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posted on 2020-06-12, 04:35 authored by Karin Bischof, Doris Schiffer, Sarah Trunk, Thomas Höfler, Anja Hopfer, Gerald Rechberger, Günther Koraimann

In conjugative elements such as integrating conjugative elements (ICEs) or conjugative plasmids (CPs) transcription of DNA transfer genes is a prerequisite for cells to become transfer competent, i.e., capable of delivering plasmid DNA via bacterial conjugation into new host bacteria. In the large family of F-like plasmids belonging to the MobF₁₂A group, transcription of DNA transfer genes is tightly controlled and dependent on the activation of a single promoter, designated P_Y. Plasmid encoded TraJ and chromosomally encoded ArcA proteins are known activators, whereas the nucleoid associated protein heat-stable nucleoid structuring (H-NS) silences the P_Y promoter. To better understand the role of these proteins in P_Y promoter activation, we performed in vitro DNA binding studies using purified H-NS, ArcA, and TraJ_R₁ (TraJ encoded by the conjugative resistance plasmid R1). All proteins could bind to R1P_Y DNA with high affinities; however, only ArcA was found to be highly sequence specific. DNase I footprinting studies revealed three H-NS binding sites, confirmed the binding site for ArcA, and suggested that TraJ contacts a dyad symmetry DNA sequence located between −51 and −38 in the R1P_Y promoter region. Moreover, TraJ_R₁ and ArcA supplied together changed the H-NS specific protection pattern suggesting that these proteins are able to replace H-NS from R1P_Y regions proximal to the transcription start site. Our findings were corroborated by P_Y-lacZ reporter fusions with a series of site specific R1P_Y promoter mutations. Sequential changes of some critical DNA bases in the TraJ binding site (jbs) from plasmid R1 to plasmid F led to a remarkable specificity switch: The P_Y promoter became activatable by F encoded TraJ whereas TraJ_R₁ lost its activation function. The R1P_Y mutagenesis approach also confirmed the requirement for the host-encoded response-regulator ArcA and indicated that the sequence context, especially in the −35 region is critical for P_Y regulation and function.