Interaction of bacteriophage P1 with an epiphytic Pantoea agglomerans strain-the role of the interplay between various mobilome elements

Katarzyna Giermasińska-Buczek; Jan Gawor; Emil Stefańczyk; Urszula Gągała; Karolina Żuchniewicz; Hanna Rekosz-Burlaga; Robert Gromadka; Małgorzata Łobocka

doi:10.3389/fmicb.2024.1356206

Interaction of bacteriophage P1 with an epiphytic Pantoea agglomerans strain-the role of the interplay between various mobilome elements

Front Microbiol. 2024 Mar 25:15:1356206. doi: 10.3389/fmicb.2024.1356206. eCollection 2024.

Authors

Katarzyna Giermasińska-Buczek^{1

2}, Jan Gawor², Emil Stefańczyk², Urszula Gągała¹, Karolina Żuchniewicz², Hanna Rekosz-Burlaga¹, Robert Gromadka², Małgorzata Łobocka²

Affiliations

¹ Department of Biochemistry and Microbiology, Institute of Biology, Warsaw University of Life Sciences (SGGW-WULS), Warsaw, Poland.
² Institute of Biochemistry and Biophysics of the Polish Academy of Sciences, Warsaw, Poland.

Abstract

P1 is a model, temperate bacteriophage of the 94 kb genome. It can lysogenize representatives of the Enterobacterales order. In lysogens, it is maintained as a plasmid. We tested P1 interactions with the biocontrol P. agglomerans L15 strain to explore the utility of P1 in P. agglomerans genome engineering. A P1 derivative carrying the Tn9 (cm^R) transposon could transfer a plasmid from Escherichia coli to the L15 cells. The L15 cells infected with this derivative formed chloramphenicol-resistant colonies. They could grow in a liquid medium with chloramphenicol after adaptation and did not contain prophage P1 but the chromosomally inserted cm^R marker of P1 Tn9 (cat). The insertions were accompanied by various rearrangements upstream of the Tn9 cat gene promoter and the loss of IS1 (IS1L) from the corresponding region. Sequence analysis of the L15 strain genome revealed a chromosome and three plasmids of 0.58, 0.18, and 0.07 Mb. The largest and the smallest plasmid appeared to encode partition and replication incompatibility determinants similar to those of prophage P1, respectively. In the L15 derivatives cured of the largest plasmid, P1 with Tn9 could not replace the smallest plasmid even if selected. However, it could replace the smallest and the largest plasmid of L15 if its Tn9 IS1L sequence driving the Tn9 mobility was inactivated or if it was enriched with an immobile kanamycin resistance marker. Moreover, it could develop lytically in the L15 derivatives cured of both these plasmids. Clearly, under conditions of selection for P1, the mobility of the P1 selective marker determines whether or not the incoming P1 can outcompete the incompatible L15 resident plasmids. Our results demonstrate that P. agglomerans can serve as a host for bacteriophage P1 and can be engineered with the help of this phage. They also provide an example of how antibiotics can modify the outcome of horizontal gene transfer in natural environments. Numerous plasmids of Pantoea strains appear to contain determinants of replication or partition incompatibility with P1. Therefore, P1 with an immobile selective marker may be a tool of choice in curing these strains from the respective plasmids to facilitate their functional analysis.

Keywords: Pantoea agglomerans complete genome sequence; Tn9 and mobile antibiotic resistance marker; bacteriophage P1; lysogeny; plasmid curing; plasmid-prophage; replication and partition incompatibility; transduction.

Grants and funding

The author(s) declare financial support was received for the research, authorship, and/or publication of this article. This work was supported by funds from the Warsaw University of Life Sciences (SGGW) internal grants no. 505-10-012400-A01080-99, 505-10-012400-K00394-99-40002, 505-10-012400-L00356-99, and 505-10-012400-M00289-99, for Ph.D. students; from the yearly Mazovian Voivodeship Marschal fellowship for KG-B in 2014, and the statutory funds of the Institute of Biochemistry and Biophysics of the Polish Academy of Sciences.