A method for targeting a specified segment of DNA to a bacterial microorganelle

Author:

Otoničar Jan1,Hostnik Maja1,Grundner Maja1,Kostanjšek Rok1,Gredar Tajda1,Garvas Maja2,Arsov Zoran2,Podlesek Zdravko1,Gostinčar Cene1,Jakše Jernej3,Busby Stephen J W4ORCID,Butala Matej1ORCID

Affiliation:

1. Department of Biology, Biotechnical Faculty, University of Ljubljana , 1000  Ljubljana ,  Slovenia

2. Jožef Stefan Institute, Condensed Matter Physics Department , 1000  Ljubljana ,  Slovenia

3. Department of Agronomy, Biotechnical Faculty, University of Ljubljana , 1000  Ljubljana ,  Slovenia

4. School of Biosciences, University of Birmingham , Birmingham  B15 2TT,  UK

Abstract

Abstract Encapsulation of a selected DNA molecule in a cell has important implications for bionanotechnology. Non-viral proteins that can be used as nucleic acid containers include proteinaceous subcellular bacterial microcompartments (MCPs) that self-assemble into a selectively permeable protein shell containing an enzymatic core. Here, we adapted a propanediol utilization (Pdu) MCP into a synthetic protein cage to package a specified DNA segment in vivo, thereby enabling subsequent affinity purification. To this end, we engineered the LacI transcription repressor to be routed, together with target DNA, into the lumen of a Strep-tagged Pdu shell. Sequencing of extracted DNA from the affinity-isolated MCPs shows that our strategy results in packaging of a DNA segment carrying multiple LacI binding sites, but not the flanking regions. Furthermore, we used LacI to drive the encapsulation of a DNA segment containing operators for LacI and for a second transcription factor.

Funder

Slovenian Research Agency

Publisher

Oxford University Press (OUP)

Subject

Genetics

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