Acinetobacter sp. ADP1: an ideal model organism for genetic analysis and genome engineering

doi:10.1093/nar/gkh881

Nucleic Acids Research 2004 32(19):5780-5790; doi:10.1093/nar/gkh881

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Published online 28 October 2004

Acinetobacter sp. ADP1: an ideal model organism for genetic analysis and genome engineering

David Metzgar¹, Jamie M. Bacher¹, Valérie Pezo¹^,2, John Reader¹, Volker Döring², Paul Schimmel¹, Philippe Marlière² and Valérie de Crécy-Lagard¹^,*

¹ The Scripps Research Institute, BCC-379, 10550 N. Torrey Pines Road, La Jolla, CA 92037, USA and ² Evologic SA, 2 rue Gaston Crémieux, 91000 Evry, France

^* To whom correspondence should be addressed at Department of Microbiology and Cell Science, University of Florida, P.O. Box 110700, Gainesville, FL 32611-0700, USA. Tel: +1 352 392 9416; Fax: +1 352 392 5922; Email: vcrecy{at}ufl.edu

Received July 1, 2004; Revised August 30, 2004; Accepted September 21, 2004

Acinetobacter sp. strain ADP1 is a naturally transformable gram-negativebacterium with simple culture requirements, a prototrophic metabolismand a compact genome of 3.7 Mb which has recently been sequenced.Wild-type ADP1 can be genetically manipulated by the directaddition of linear DNA constructs to log-phase cultures. Thismakes it an ideal organism for the automation of complex strainconstruction. Here, we demonstrate the flexibility and versatilityof ADP1 as a genetic model through the construction of a broadvariety of mutants. These include marked and unmarked insertionsand deletions, complementary replacements, chromosomal expressiontags and complex combinations thereof. In the process of theseconstructions, we demonstrate that ADP1 can effectively expressa wide variety of foreign genes including antibiotic resistancecassettes, essential metabolic genes, negatively selectablecatabolic genes and even intact operons from highly divergentbacteria. All of the described mutations were achieved by thesame process of splicing PCR, direct transformation of growingcultures and plating on selective media. The simplicity of thesetools make genetic analysis and engineering with AcinetobacterADP1 accessible to laboratories with minimal microbial geneticsexpertise and very little equipment. They are also compatiblewith complete automation of genetic analysis and engineeringprotocols.

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