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DNA Dynamics and Chromosome Structure

The One-Kilobase DNA Fragment Upstream of the ardC Actin Gene of Physarum polycephalum Is Both a Replicator and a Promoter

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Pages 3506-3514 | Received 28 Sep 1998, Accepted 08 Feb 1999, Published online: 28 Mar 2023
 

Abstract

The 1-kb DNA fragment upstream of the ardC actin gene of Physarum polycephalum promotes the transcription of a reporter gene either in a transient-plasmid assay or as an integrated copy in an ectopic position, defining this region as the transcriptional promoter of the ardC gene (PardC). Since we mapped an origin of replication activated at the onset of S phase within this same fragment, we examined the pattern of replication of a cassette containing the PardCpromoter and the hygromycin phosphotransferase gene, hph, integrated into two different chromosomal sites. In both cases, we show by two-dimensional agarose gel electrophoresis that an efficient, early activated origin coincides with the ectopic PardC fragment. One of the integration sites was a normally late-replicating region. The presence of the ectopic origin converted this late-replicating domain into an early-replicating domain in which replication forks propagate with kinetics indistinguishable from those of the native PardC replicon. This is the first demonstration that initiation sites for DNA replication in Physarum correspond to cis-acting replicator sequences. This work also confirms the close proximity of a replication origin and a promoter, with both functions being located within the 1-kb proximal region of the ardC actin gene. A more precise location of the replication origin with respect to the transcriptional promoter must await the development of a functional autonomously replicating sequence assay in Physarum.

ACKNOWLEDGMENTS

We thank Yvette Florentin for providing dedicated technical assistance, Tim Burland for kindly providing the transformed amoebal strains, Claire Lagnel for performing their differentiation into plasmodia, and Helmut Sauer for critically reading the manuscript.

This work was supported by general funding from the CNRS; by grant 1301 from the “Association de la Recherche sur le Cancer”, Villejuif, France; by the CRSNG of Canada; and by the Cancer Research Society of Canada. This study was initiated during a France-Québec cooperation project.

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