Molecular characterization of avrPphD, a widely-distributed gene from Pseudomonas syringae pv. phaseolicola involved in non-host recognition by pea (Pisum sativum)

Arnold, D. L.; Jackson, R. W.; Mansfield, J. W.; Taylor, J. D.; Vivian, A.; Arnold, Dawn L.; Jackson, Robert W.; Mansfield, John W.; Gibbon, M. J.; Taylor, John D.; Vivian, Alan; Wood, J. R.; Brown, J.

doi:10.1006/pmpp.2000.0315

Molecular characterization of avrPphD, a widely-distributed gene from Pseudomonas syringae pv. phaseolicola involved in non-host recognition by pea (Pisum sativum)

Arnold, D. L.; Jackson, R. W.; Mansfield, J. W.; Taylor, J. D.; Vivian, A.; Arnold, Dawn L.; Jackson, Robert W.; Mansfield, John W.; Gibbon, M. J.; Taylor, John D.; Vivian, Alan; Wood, J. R.; Brown, J.

Authors

D. L. Arnold

R. W. Jackson

J. W. Mansfield

J. D. Taylor

A. Vivian

Dawn L. Arnold

Robert W. Jackson

John W. Mansfield

M. J. Gibbon

John D. Taylor

Alan Vivian

J. R. Wood

J. Brown

Abstract

A genomic library clone, pPPY40, from Pseudomonas syringae pv. phaseolicola was previously shown to consist of two regions: region I potentially encoded an avirulence gene involved in non-host recognition in pea and region II contained a replicase gene. In this study, region I was sequenced and shown to contain a single open reading frame (ORF) of 2130 nt with a 55 % G + C ratio encoding a deduced peptide product of 710 amino acids with a predicted molecular mass of 75.4 kDa. Both the entire ORF and an ORF truncated by five residues were isolated by PCR amplification. The full length ORF was successfully cloned in the broad host range vector pBBR1MCS-2, but not in the RK2-based broad host range vector pLAFR3. Truncated ORFs were successfully cloned in both vectors. The constructs obtained were transferred to Pseudomonas syringae pv. pisi strain PT10 and the transconjugants tested for pathogenicity on pea plants. Only the full length ORF conferred avirulence and the gene was designated avrPphD. Inactivation of avrPphD by marker-exchange did not affect the ability of P. syringae pv. phaseolicola to cause a non-host hypersensitive reaction. PCR amplification using avrPphD-specific primers and hybridization analysis indicated that homologues of avrPphD occurred in a wide range of P. syringae pathovars. © 2001 Academic Press.

Journal Article Type	Article
Publication Date	Jan 1, 2001
Journal	Physiological and Molecular Plant Pathology
Print ISSN	0885-5765
Publisher	Elsevier
Peer Reviewed	Peer Reviewed
Volume	58
Issue	2
Pages	55-62
DOI	https://doi.org/10.1006/pmpp.2000.0315
Keywords	bean, Phaseolus spp., broad host range vectors, replication
Public URL	https://uwe-repository.worktribe.com/output/1088042
Publisher URL	http://dx.doi.org/10.1006/pmpp.2000.0315
Additional Information	Additional Information : Arnold was lead worker on this project and carried out the majority of the experimental work including cloning, sequencing and characterising this avirulence gene. She also investigated its distribution in a range of Pseudomonas plant pathogens. She co-wrote the paper and is corresponding author.

Authors

Abstract

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