M. Pilar Castañeda-Ojeda scite author profile

Pseudomonas savastanoi pv. savastanoi NCPPB 3335 causes olive knot disease and is a model pathogen for exploring bacterial infection of woody hosts. The type III secretion system (T3SS) effector repertoire of this strain includes 31 effector candidates plus two novel candidates identified in this study which have not been reported to translocate into plant cells. In this work, we demonstrate the delivery of seven NCPPB 3335 effectors into Nicotiana tabacum leaves, including three proteins from two novel families of the P. syringae complex effector super-repertoire (HopBK and HopBL), one of which comprises two proteins (HopBL1 and HopBL2) that harbor a SUMO protease domain. When delivered by P. fluorescens heterologously expressing a P. syringae T3SS, all seven effectors were found to suppress the production of defense-associated reactive oxygen species. Moreover, six of these effectors, including the truncated versions of HopAA1 and HopAZ1 encoded by NCPPB 3335, suppressed callose deposition. The expression of HopAZ1 and HopBL1 by functionally effectorless P. syringae pv. tomato DC3000D28E inhibited the hypersensitive response in tobacco and, additionally, expression of HopBL2 by this strain significantly increased its competitiveness in N. benthamiana. DNA sequences encoding HopBL1 and HopBL2 were uniquely detected in a collection of 31 P. savastanoi pv. savastanoi strains and other P. syringae strains isolated from woody hosts, suggesting a relevant role of these two effectors in bacterial interactions with olive and other woody plants.

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Bacterial multispecies studies and microbiome analysis of a plant disease

Silva

Castañeda-Ojeda

Moretti

et al. 2014

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Although the great majority of bacteria found in nature live in multispecies communities, microbiological studies have focused historically on single species or competition and antagonism experiments between different species. Future directions need to focus much more on microbial communities in order to better understand what is happening in the wild. We are using olive knot disease as a model to study the role and interaction of multispecies bacterial communities in disease establishment/development. In the olive knot, non-pathogenic bacterial species (e.g. Erwinia toletana) co-exist with the pathogen (Pseudomonas savastanoi pv. savastanoi); we have demonstrated cooperation among these two species via quorum sensing (QS) signal sharing. The outcome of this interaction is a more aggressive disease when co-inoculations are made compared with single inoculations. In planta experiments show that these two species co-localize in the olive knot, and this close proximity most probably facilitates exchange of QS signals and metabolites. In silico recreation of their metabolic pathways showed that they could have complementing pathways also implicating sharing of metabolites. Our microbiome studies of nine olive knot samples have shown that the olive knot community possesses great bacterial diversity; however. the presence of five genera (i.e. Pseudomonas, Pantoea, Curtobacterium, Pectobacterium and Erwinia) can be found in almost all samples.

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A New Bacterial Disease on Mandevilla sanderi, Caused by Pseudomonas savastanoi: Lessons Learned for Bacterial Diversity Studies

Eltlbany

Prokscha

Castañeda-Ojeda

et al. 2012

Appl Environ Microbiol

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Leaf lesions of Mandevilla sanderi were shown to be caused by Pseudomonas savastanoi. While BOX fingerprints were similar for P. savastanoi isolates from different host plants, plasmid restriction patterns and sequencing of plasmid-located pathogenicity determinants revealed that Mandevilla isolates contained similar plasmids distinct from those of other isolates. A repA-based detection method was established.T he ornamental plant Mandevilla sanderi (Dipladenia sanderi [family Apocynaceae]) originating from Middle and South America has become increasingly popular over the last decade, mainly because of its copiously formed red flowers. In 2008, breeders of Mandevilla sanderi observed for the first time large necrotic lesions with chlorotic rings on leaves and tumor formation on stems (see Fig. 1). The potential causal agents isolated from the lesions of leaves of diseased plant material were identified initially by metabolic profiling (Biolog) as Pseudomonas savastanoi pv. glycinea or pv. nerii (data not shown), pathogens of soybean (Glycine max) or oleander (Nerium oleander), respectively. Stem and leaf inoculation of healthy Mandevilla plants with these isolates indeed caused identical symptoms ( Fig. 1) fulfilling Koch's postulates.P. savastanoi strains are Gammaproteobacteria which belong to genomospecies 2 of the Pseudomonas syringae complex (6). Although the species P. savastanoi was established only in 1992 (5), sequencing of the genomes and plasmids of several P. syringae and P. savastanoi isolates reinforced the discussion about the taxonomic affiliation of P. savastanoi, as the core genome is clearly shared by P. syringae and P. savastanoi strains. Several pathovars of P. savastanoi infect woody plants, e.g., P. savastanoi pv. savastanoi is known as an important pathogen of olive trees (Olea europaea) in the Mediterranean area (11). The typical symptoms of olive knot disease, the formation of tumors in the stem and branches, were already described by Theobrast Eresos in the year 300 BC. The disease causes massive yield losses, and breeding for tolerant varieties is the main strategy to overcome the commercial losses due to infections with P. savastanoi pv. savastanoi (16).Taking into account that other known hosts of P. savastanoi are oleander (Nerium oleander) and privet (Liguster vulgare), leaf and stem inoculations of Mandevilla isolates were done also on oleander, olive, and privet plants. Nine weeks after inoculation, the response patterns of oleander were similar to those observed on Mandevilla plants; however, while no symptoms were observed for olive plants, privet plants displayed only leaf lesions (unpublished results). Thus, it was hypothesized that the most likely causal agent of the novel bacterial disease of Mandevilla sanderi might have originated from infested oleander plantations in the vicinity of the Mandevilla sanderi-producing companies in the South of France. To shed light on this hypothesis, P. savastanoi isolates from Mandevilla sanderi were characterized and compared to isolate...

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Suppression of Plant Immune Responses by the Pseudomonas savastanoi pv. savastanoi NCPPB 3335 Type III Effector Tyrosine Phosphatases HopAO1 and HopAO2

et al. 2017

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The effector repertoire of the olive pathogen P. savastanoi pv. savastanoi NCPPB 3335 includes two members of the HopAO effector family, one of the most diverse T3E families of the P. syringae complex. The study described here explores the phylogeny of these dissimilar members, HopAO1 and HopAO2, among the complex and reveals their activities as immune defense suppressors. Although HopAO1 is predominantly encoded by phylogroup 3 strains isolated from woody organs of woody hosts, both HopAO1 and HopAO2 are phylogenetically clustered according to the woody/herbaceous nature of their host of isolation, suggesting host specialization of the HopAO family across the P. syringae complex. HopAO1 and HopAO2 translocate into plant cells and show hrpL-dependent expression, which allows their classification as actively deployed type III effectors. Our data also show that HopAO1 and HopAO2 possess phosphatase activity, a hallmark of the members of this family. Both of them exert an inhibitory effect on early plant defense responses, such as ROS production and callose deposition, and are able to suppress ETI responses induced by the effectorless polymutant of P. syringae pv. tomato DC3000 (DC3000D28E) in Nicotiana. Moreover, we demonstrate that a ΔhopAO1 mutant of P. savastanoi NCPBB 3335 exhibits a reduced fitness and virulence in olive plants, which supports the relevance of this effector during the interaction of this strain with its host plants. This work contributes to the field with the first report regarding functional analysis of HopAO homologs encoded by P. syringae or P. savastanoi strains isolated from woody hosts.

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Differential modulation of plant immune responses by diverse members of the Pseudomonas savastanoi pv. savastanoi HopAF type III effector family

Castañeda-Ojeda

López‐Solanilla²,

Ramos

2016

Molecular Plant Pathology

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The Pseudomonas savastanoi pv. savastanoi NCPPB 3335 type III secretion system (T3SS) effector repertoire includes 33 candidates, seven of which translocate into host cells and interfere with plant defences. The present study was performed to investigate the co-existence of both plasmid- and chromosomal-encoded members of the HopAF effector family, HopAF1-1 and HopAF1-2, respectively, in the genome of NCPPB 3335. Here, we show that the HopAF1 paralogues are widely distributed in the Pseudomonas syringae complex, where HopAF1-1 is most similar to the homologues encoded by other P. syringae pathovars infecting woody hosts that belong to phylogroups 1 and 3. We show that the expression of both HopAF1-1 and HopAF-2 is transcriptionally dependent on HrpL and demonstrate their delivery into Nicotiana tabacum leaves. Although the heterologous delivery of either HopAF1-1 or HopAF1-2 significantly suppressed the production of defence-associated reactive oxygen species levels, only HopAF1-2 reduced the levels of callose deposition. Moreover, the expression of HopAF1-2 by functionally effectorless P. syringae pv. tomato DC3000D28E completely inhibited the hypersensitive response in tobacco and significantly increased the competitiveness of the strain in Nicotiana benthamiana. Despite their functional differences, subcellular localization studies reveal that green fluorescent protein (GFP) fusions to either HopAF1-1 or HopAF1-2 are targeted to the plasma membrane when they are expressed in plant cells, a process that is completely dependent on the integrity of their N-myristoylation motif. Our results further support the notion that highly similar T3SS effectors might differentially interact with diverse plant targets, even when they co-localize in the same cell compartment.

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