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Review
. 2015 Mar:78:59-64.
doi: 10.1016/j.plasmid.2014.11.002. Epub 2014 Nov 11.

Plasmids in the driving seat: The regulatory RNA Rcd gives plasmid ColE1 control over division and growth of its E. coli host

Affiliations
Review

Plasmids in the driving seat: The regulatory RNA Rcd gives plasmid ColE1 control over division and growth of its E. coli host

Hannah Gaimster et al. Plasmid. 2015 Mar.

Abstract

Regulation by non-coding RNAs was found to be widespread among plasmids and other mobile elements of bacteria well before its ubiquity in the eukaryotic world was suspected. As an increasing number of examples was characterised, a common mechanism began to emerge. Non-coding RNAs, such as CopA and Sok from plasmid R1, or RNAI from ColE1, exerted regulation by refolding the secondary structures of their target RNAs or modifying their translation. One regulatory RNA that seemed to swim against the tide was Rcd, encoded within the multimer resolution site of ColE1. Required for high fidelity maintenance of the plasmid in recombination-proficient hosts, Rcd was found to have a protein target, elevating indole production by stimulating tryptophanase. Rcd production is up-regulated in dimer-containing cells and the consequent increase in indole is part of the response to the rapid accumulation of dimers by over-replication (known as the dimer catastrophe). It is proposed that indole simultaneously inhibits cell division and plasmid replication, stopping the catastrophe and allowing time for the resolution of dimers to monomers. The idea of a plasmid-mediated cell division checkpoint, proposed but then discarded in the 1980s, appears to be enjoying a revival.

Keywords: Cell division checkpoint; Indole; Plasmid maintenance; Regulatory RNA; Signalling.

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Figures

Fig. 1
Fig. 1
Red-mediated response to the ColE1 dimer catastrophe. Plasmid dimers express the non-coding RNA, Red, from the cer site. Red binds to tryptophanase increasing the production of indole. High levels of indole inhibit plasmid replication, cell division and growth, allowing the Xer–cer recombination system to resolve plasmid dimers back to monomers.

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