Creation and characterisation of a high-copy-number version of the pAL5000 mycobacterial replicon - 15/08/11

Doi : 10.1016/j.tube.2007.08.003

William R. Bourn ^a, Yvette Jansen ^a, Helen Stutz ^b, Robin M. Warren ^a, Anna-Lise Williamson ^b,^c, Paul D. van Helden ^a,^⁎
^a DST/NRF Centre of Excellence for Biomedical Tuberculosis Research, MRC Centre for Molecular and Cellular Biology, Division of Molecular Biology and Human Genetics, Faculty of Health Sciences, Stellenbosch University, P.O. Box 19063, Tygerberg, 7505, South Africa
^b Institute of Infectious Disease and Molecular Medicine, Faculty of Health Sciences, University of Cape Town, Observatory, 7925, Cape Town, South Africa
^c National Health Laboratory Service, Groote Schuur Hospital, Observatory, 7925, Cape Town, South Africa

Corresponding author. Tel.: +27219389401; fax: +27219389476.

Abstract

The majority of mycobacterial plasmid vectors are derived from the pAL5000 replicon and maintained at approximately five copies per cell. We have devised a method that directly selects for high-copy-number plasmids. This involves enriching for high copy number plasmids by repeatedly isolating and retransforming plasmids from a mutant library. Using this method we have selected a copy-up version of the pAL5000 replicon. In Mycobacterium smegmatis the copy-number was shown to have increased 7-fold to between 32 and 64 copies/cell, and the plasmid remained relatively stable after 100 generations in the absence of antibiotic selection. The plasmid also has a high-copy-number phenotype in M. bovis BCG and can be used to increase expression of cloned genes, as we have demonstrated with the green fluorescent protein. The mutation was found to be the deletion of an alanine residue in the C-terminal end of the RepA replication protein. We argue that the mutation exerts its effect through altered RNA folding, thereby affecting the translationally coupled RepA-RepB expression.

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Keywords : Mycobacterial replicon, Plasmid copy number, Recombinant mycobacterial expression, Plasmid replication

Plan

Introduction

Methods

Strains, growth conditions and transformation

Reference plasmids

DNA isolation and treatment

Mutagenesis

High-copy-number mutant plasmid selection

Copy-number determination

Protein extraction and quantitation

GFP quantitation by ELISA

Plasmid stability

Results

Construction and isolation of a high-copy-number plasmid

Identification of the causative mutation

Plasmid copy-number and stability determination

Copy-number and expression levels in M. bovis BCG

Discussion

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Vol 87 - N° 6

P. 481-488 - novembre 2007 Retour au numéro

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Creation and characterisation of a high-copy-number version of the pAL5000 mycobacterial replicon - 15/08/11

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