Pioneering precision in markerless strain development for Synechococcus sp. PCC 7002

Author:

Tsuji Ayaka1,Inabe Kosuke1,Hidese Ryota1,Kato Yuichi1,Domingues Lucília2,Kondo Akihiko1,Hasunuma Tomohisa1

Affiliation:

1. Kobe University

2. LABBELS-Associate Laboratory

Abstract

Abstract

Marine cyanobacteria such as Picosynechococcus sp. (formerly called Synechococcus sp.) PCC 7002 are promising chassis for photosynthetic production of commodity chemicals with low environmental burdens. Genetic engineering of cyanobacteria conventionally employs antibiotic resistance markers. However, limited availability of antibiotics is a problem for highly multigenic strain engineering. Although several markerless transformation methods have been developed for PCC 7002, they often lack versatility due to the requirement of gene disruption in the host strain. To achieve markerless transformation in Synechococcus sp. with no requirements for the host strain, this study developed a method in which temporarily introduces a mutated phenylalanyl-tRNA synthetase gene (pheS) into the genome for counter selection. Amino acid substitutions in the PheS that cause high susceptibility of PCC 7002 to the phenylalanine analogue p-chlorophenylalanine were examined, and the combination of T261A and A303G was determined as the most suitable mutation. The mutated PheS-based selection was utilized for the markerless knockout of the nblA gene in PCC 7002. In addition, the genetic construct containing the lldD and lldP genes from Escherichia coli was introduced into the ldhA gene site using the counter selection strategy, resulting in a markerless recombinant strain. The repeatability of this method was also demonstrated, suggesting it will be a powerful tool for multigenic strain engineering of cyanobacteria.

Publisher

Springer Science and Business Media LLC

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