Comparison between complete genomes of an isolate of Pseudomonas syringae pv. actinidiae from Japan and a New Zealand isolate of the pandemic lineage

Poulter, Russell T. M.; Ho, Joycelyn; Handley, Thomas N. G.; Taiaroa, George; Butler, Margaret I.

doi:10.1038/s41598-018-29261-5

Cited by 27 publications

(27 citation statements)

References 54 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Our Psa2 and Psa3 strains featured the canonical EEL structure (including tRNA Leu , queA and tgt sequences) although two of the three Psa2 genomes (ICMP 19071 and ICMP 19072) contained a phage insertion within the EEL, supporting the observation that tRNA genes are often found at phage integration sites (75). Multiple rearrangements have been reported in Psa1 and Psa3 biovars (76), and accordingly we found that the tRNA Leu , queA and tgt sequences were dispersed to other chromosomal locations in Psa1 (ICMP9617 and ICMP9853). Such rearrangements may be selectively neutral, but the genome structure may affect transcriptional regulation (76).…”

Section: Genomic Analysis Reveals New Features Of the Ttss-related Pasupporting

confidence: 78%

Transcriptional profiling of threePseudomonas syringaepv.actinidiaebiovars reveals different responses to apoplast-like conditions related to strain virulence

Vandelle

Colombo

Regaiolo

et al. 2020

Preprint

View full text Add to dashboard Cite

Pseudomonas syringae pv. actinidiae (Psa) is a phytopathogen that causes devastating bacterial canker in kiwifruit. Among five biovars defined by genetic, biochemical and virulence traits, Psa3 is the most aggressive and is responsible for the most recent reported outbreaks, but the molecular basis of its heightened virulence is unclear. We therefore designed the first P. syringae multi-strain whole-genome microarray, encompassing biovars Psa1, Psa2 and Psa3 and the well-established model P. syringae pv. tomato , and analyzed early bacterial responses to an apoplast-like minimal medium. Transcriptomic profiling revealed (i) the strong activation in Psa3 of all hrp / hrc cluster genes, encoding components of the type III secretion system required for bacterial pathogenicity and involved in responses to environmental signals; (ii) potential repression of the hrp / hrc cluster in Psa2; and (iii) activation of flagellum-dependent cell motility and chemotaxis genes in Psa1. The detailed investigation of three gene families encoding upstream regulatory proteins (histidine kinases, their cognate response regulators, and proteins with diguanylate cyclase and/or phosphodiesterase domains) indicated that c-di-GMP may be a key regulator of virulence in Psa biovars. The gene expression data were supported by the quantification of biofilm formation. Our findings suggest that diverse early responses to the host apoplast, even among bacteria belonging to the same pathovar, can lead to different virulence strategies and may explain the differing outcomes of infections. Based on our detailed structural analysis of hrp / hrc operons, we also propose a revision of hrp / hrc cluster organization and operon regulation in P. syringae.

show abstract

Section: Genomic Analysis Reveals New Features Of the Ttss-related Pasupporting

confidence: 78%

Transcriptional profiling of threePseudomonas syringaepv.actinidiaebiovars reveals different responses to apoplast-like conditions related to strain virulence

Vandelle

Colombo

Regaiolo

et al. 2020

Preprint

View full text Add to dashboard Cite

show abstract

“…Genome sequencing yielded an average of 1.05 million paired sequence reads for each genome, equivalent to an average 40-fold read coverage. The sequence reads from the Psa3 isolates were mapped to the completely assembled 6 555 571 bp chromosome and 74 432 bp plasmid of a pandemic Psa3 strain from New Zealand, ICMP18708 (GenBank accessions CP012179-chromosome and CP012180-plasmid [26]), using Geneious 11.0.3 [39]. Read mapping was performed with the Geneious 6.0.3 Read Mapper [40] using the following parameter values: maximum mismatches per read=10 %, minimum mapping quality=Phred 30, maximum gaps per read=10 % read length, maximum gap length=3 bp and minimum overlap=25 bp.…”

Section: Wgs Analysismentioning

confidence: 99%

“…The genomes of several isolates of Psa have been fully sequenced using the PacBio platform [26,41]. This permitted the identification of RM systems specific to different types of Psa.…”

Section: Rm Systems In Psa3mentioning

confidence: 99%

“…The sequence of pJH1 has been submitted to GenBank and assigned the accession number MN346704. To confirm the activity and specificity of the type I RM system suggested by the PacBio methylation data [26], a modified version of the pJH1 was constructed. This plasmid, designated pMZ5-103, has a single base change that generated a restriction site for the type I enzyme (AGCANNNNNGTC).…”

Section: Pjh1mentioning

confidence: 99%

“…More recently, Pseudomonas putida was also found to employ NHEJ to repair DNA during the stationary phase [24]. A variety of Psa strains have now been fully sequenced and annotated [6,25,26]. This has revealed the presence of Ku-and ATPdependent ligase genes arranged in an operon in these Psa genomes.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

The application of the CRISPR–Cas9 system in Pseudomonas syringae pv. actinidiae

Zhao

Wojcik

et al. 2020

Journal of Medical Microbiology

Self Cite

View full text Add to dashboard Cite

Introduction. Pseudomonas syringae pv. actinidiae (Psa) has emerged as a major bacterial pathogen of kiwifruit cultivation throughout the world. Aim. We aim to introduce a CRISPR–Cas9 system, a commonly used genome editing tool, into Psa. The protocols may also be useful in other Pseudomonas species. Methodology. Using standard molecular biology techniques, we modified plasmid pCas9, which carries the CRISPR–Cas9 sequences from Streptococcus pyogenes, for use in Psa. The final plasmid, pJH1, was produced in a series of steps and is maintained with selection in both Escherichia coli and Psa. Results. We have constructed plasmids carrying a CRISPR–Cas9 system based on that of S. pyogenes , which can be maintained, under selection, in Psa. We have shown that the gene targeting capacity of the CRISPR–Cas9 system is active and that the Cas9 protein is able to cleave the targeted sites. The Cas9 was directed to several different sites in the P. syringae genome. Using Cas9 we have generated Psa transformants that no longer carry the native plasmid present in Psa, and other transformants that lack the integrative, conjugative element, Pac_ICE1. Targeting of a specific gene, a chromosomal non-ribosomal peptide synthetase, led to gene knockouts with the transformants having deletions encompassing the target site. Conclusion. We have constructed shuttle plasmids carrying a CRISPR–Cas9 system that are maintained in both E. coli and P. syringae pv. actinidiae. We have used this gene editing system to eliminate features of the accessory genome (plasmids or ICEs) from Psa and to target a single chromosomal gene.

show abstract

Kiwifruit bacterial canker: an integrative view focused on biocontrol strategies

Pereira

Costa

Pinheiro

et al. 2021

Planta

View full text Add to dashboard Cite

Comparison between complete genomes of an isolate of Pseudomonas syringae pv. actinidiae from Japan and a New Zealand isolate of the pandemic lineage

Cited by 27 publications

References 54 publications

Transcriptional profiling of threePseudomonas syringaepv.actinidiaebiovars reveals different responses to apoplast-like conditions related to strain virulence

Transcriptional profiling of threePseudomonas syringaepv.actinidiaebiovars reveals different responses to apoplast-like conditions related to strain virulence

The application of the CRISPR–Cas9 system in Pseudomonas syringae pv. actinidiae

Kiwifruit bacterial canker: an integrative view focused on biocontrol strategies

Contact Info

Product

Resources

About