Molecular biology and biochemistry of regulation of Hrp/type III secretion genes in the corn pathogen Pantoea stewartii pv. stewartii

Merighi, Massimo.

January 2004

Thesis (Ph. D.)--Ohio State University, 2004. / Document formatted into pages; contains xxxiii, 421 p. Includes bibliographical references. Abstract available online via OhioLINK's ETD Center; full text release delayed at author's request until 2005 Dec. 2.

Corn Pantoea stewartii

Emerging diseases of maize and onion caused by bacteria belonging to the genus Pantoea

Goszczynska, Teresa

15 July 2008

Center rot of onion, caused by Pantoea ananatis, was first described in the USA, in 1997. P. ananatis is seed-borne in onions and it was suggested that it was introduced into the USA on infected seed lots from South Africa. Center rot has not been observed in South Africa and it was essential to determine if P. ananatis is present in local onion seed. Colonies resembling those of P. ananatis were isolated from four South African seed lots on PA 20, a new semi-selective medium. Pathogenicity tests demonstrated that the South African and America strains induced the same symptoms on onion. Phenotypic and genotypic analyses identified the strains from seed as P. ananatis. In 2004/2005, an unreported disease of maize, brown stalk rot, was observed on commercial fields in South Africa. The representative strains induced disease symptoms similar to those observed in the field. The phenotypic and genotyping tests showed that the strains belonged to the genus Pantoea and separated them into two groups. The first group was identified as P. ananatis. The F-AFLP genomic fingerprints generated by the second group of strains, were distinctly different from those generated by known Pantoea species. To resolve the taxonomic position of Pantoea isolated from onion and maize, sixty-seven strains were subjected to a polyphasic study. The methods used included phenotypic characterisation, genomic fingerprinting, 16S rRNA gene sequence analysis and DNA-DNA hybridisation. The results revealed that the strains belong to three different species within the genus Pantoea: P. ananatis, P. vagens and a novel species, Pantoea allii sp. nov. / Thesis (PhD (Microbiology))--University of Pretoria, 2009. / Microbiology and Plant Pathology / unrestricted

Seed-borne in onions

Pantoea ananatis

UCTD

Understanding the quorum-sensing bacterium Pantoea stewartii strain M009 with whole-genome sequencing analysis

Tan, W., Chang, Chien-Yi, Yin, W., Chan, K.

29 January 2015

Yes / Pantoea stewartii is known to be the causative agent of Stewart's wilt, which usually affects sweet corn (Zea mays) with the corn flea beetle as the transmission vector. In this work, we present the whole-genome sequence of Pantoea stewartii strain M009, isolated from a Malaysian tropical rainforest waterfall. / University of Malaya via High Impact Research Grants (UM C/625/1/HIR/MOHE/CHAN/01 no. A-000001- 50001 and UM C/625/1/HIR/MOHE/CHAN/14/1 no. H-50001-A000027)

Bacterial infection, immune responses, and autophagy in lutzomyia longipalpis sand flies

Heerman, Matthew C.

January 1900

Doctor of Philosophy / Department of Entomology / Marcelo Ramalho-Ortigao / Kun Yan Zhu / Microbial communities residing within the midgut of insect vectors play a critical role in the response to various zoonotic and human pathogens, and can directly alter the development and survival of the insects. Sand flies are the primary vector of Leishmania, the causative pathogen of leishmaniasis, a neglected tropical disease. Sand flies acquire many microbes from the soil where immature stages develop until emergence as adults. Gram-negative Pantoea agglomerans and gram-positive Bacillus subtilis are two bacteria commonly associated with sand fly populations. Here, I demonstrated that an EGFP- and a GFP-expressing version of these two bacteria localize to different compartments of the midgut; a phenomenon that is achieved, in part, to pH differences found across the length of the gut. Additionally, P. agglomerans is able to selectively induce midgut epithelial apoptosis while B. subtilis does not. This is accompanied by differential immune and homeostasis responses to both bacteria highlighted by immune pathway suppression via the Poor Immune Response upon Knock-in (Pirk) gene. These effects may actually be representative of a broader type of response to bacterial infection that might be present across several insect species. Finally, I demonstrated that during metamorphosis the sand fly relies, at least in part, upon the activation of multiple genes from the autophagy pathway to aid in generating adult tissues. More specifically, I demonstrate, using microscopy, the presence of ATG6 in the cytoplasm of developing midgut epithelial cells of the sand fly pupae.

Immunity

Autophagy

Leishmania

Sand flies

Metamorphosis

Pantoea agglomerans

Genome assembly and metabolic pathway reconstruction of Pantoea ananatis LMG 20103

Chan, Wai Yin

13 October 2012

Next generation of sequencing (NGS) technologies have taken life science research into a new era. With the rapid advances in these technologies and the associated reduction in overall costs, the sequencing and assembly of genomes have come within reach of most laboratories. Studies related to the evolution, ecology and biology of an organism now rely heavily on genomic data and obtaining a genome sequence has become an essential resource for the rapid progress and success of these studies. Pantoea ananatis is recognised as an emerging but rather unconventional pathogen capable of infecting a wide range of different hosts. Numerous plants of agricultural and economic importance including maize, rice, onion, pineapple, melon, sudan grass and Eucalyptus trees have been affected. With the outbreak of P. ananatis in a South African Eucalyptus nursery in 1998, it was realised that very little is known about this pathogen. A better understanding of the pathogenicity, metabolism and ecology of the bacterium is required to develop strategies for the control of the disease. During this study, the genome sequence of P. ananatis strain LMG 20103 was obtained using the Roche 454 technology. To aid in the assembly of this Eucalyptus pathogen’s genome sequence, the type strain of P. ananatis LMG 2665 was also sequenced using Illinima’s Genome Analyzer (GA). A draft assembly of P. ananatis LMG 20103, consisting of 117 contigs, was generated after optimization of the Newbler assembly parameters and comparison with other genome assemblies and genomes. This study demonstrated that the assembly could be completed using both in-vitro, and in-silico approaches such as contig scaffolding, gap closure with conventional PCR reactions and sequencing, manual curation and automated genome annotation. The final complete genome consisted of a 4 386 227 bp chromosome and a 317 146 bp mega-plasmid. With the complete genome sequence available, the reconstruction of metabolic network of P. ananatis LMG 20103 was attempted using two pathways reconstruction pipelines namely, Pathway Tools and Model SEED. It was found that missing metabolic reactions and incomplete pathways in the draft metabolic networks were mainly caused by incorrect gene annotations or bioinformatic errors during the automated network reconstruction. These two pipelines differed substantially in the way network reconstruction is undertaken. Performing a comparison between the two proposed networks, annotation errors could be detected and corrected. Although some improvement could be made to the predicted network further experimental data is still required to improve the accuracy of the draft metabolic network. Despite the amount of effort and cost, it is believed that the complete genome and a draft metabolic network of P. ananatis LMG 20103 will be a valuable resource for many subsequent studies to investigate the evolution and biology of this emerging plant pathogen. This information will be essential for the development of strategies to predict and control future disease outbreaks associated with this pathogen. / Dissertation (MSc)--University of Pretoria, 2012. / Microbiology and Plant Pathology / unrestricted

Genome assembly

Metabolic pathway

Reconstruction

Pantoea ananatis

Lmg 20103

UCTD

Pantoea agglomerans bacteremia: A rare case of spontaneous human infection by a plant pathogen in an immunocompromised host.

Panta, Utsab R, Joslyn, James A, Shah, Rupal D

05 April 2018

Introduction: Pantoea agglomerans is a Gram negative ubiquitous bacteria commonly isolated from plant surfaces, seeds, fruits and animal/human feces usually introduced to human by ingestion of infected fruits/vegetables, thorn pricks and gastrointestinal translocation in lack of stomach acidity. However, the pathogen can also cause opportunistic human infection especially when the immune system is impaired. The aim of this case report is to investigate clinical features in a patient with P. agglomerans bacteremia and bring attention the opportunistic infection by this rare bacteria. Case presentation: We present a case of 57 year old caucasian lady with past medical history of Chronic Obstructive Pulmonary Disease, Atrial fibrillation, Immunoglobulin (IgG) deficiency, recurrent pneumonia, urine infection, oral/vaginal candidiasis, Gastro-esophageal reflux disease who presents with one week history of increased shortness of breath, chest tightness and productive cough without fever/chills. She also had high INR of 4.7 (target 2-3) despite taking normal dose of warfarin. She denies plant exposure. Her vitals were stable, saturation maintained with oxygen supplementation. Chest exam revealed very poor air entry bilaterally suggesting exacerbation of COPD. Oral thrush was present. Recent IgG level within last 6 months was low. Blood culture grew Pantoea agglomerans, pan-sensitive to most of the antibiotics. Chest X ray, CT scan abdomen and urine studies could not localize the source of infection. She was treated with Ceftriaxone, INR normalized to therapeutic range and she improved to baseline after 10 days of treatment. Discussion and conclusion: P. agglomerans is a rare cause of bacteremia which usually presents as fever, chills and general toxicity, however could also present as a cause of exacerbation of chronic diseases. Spontaneous infection can occur in a immunocompromised host, however the pathogen is of low virulence. The link between upper GI symptoms along with antacid receipt and spontaneous P. agglomerans infection could be possible, however needs further study. Hence, P. agglomerans should be considered one of the possible cause of spontaneous bacteremia in a immunocompromised host.

Pantoea agglomerans

bacteremia

Immunocompromised hostinfection

atypical bacteremia

Bacteria

Genome Evolution During Development of Symbiosis in Extracellular Mutualists of Stink Bugs (Pentatomidae)

Otero Bravo, Alejandro

29 September 2020

No description available.

Biology

Bioinformatics

symbiosis

genomics

stink bug

Pantoea

gammaproteobacteria

genome reduction

Analysis of quorum-sensing Pantoea stewartii strain M073a through whole-genome sequencing

Mohamad, N.I., Tan, W., Chang, Chien-Yi, Tee, K.K., Yin, W., Chan, K.

19 February 2015

Yes / Pantoea stewartii strain M073a is a Gram-negative bacterium isolated from a tropical waterfall. This strain exhibits quorum-sensing activity. Here, the assembly and annotation of its genome are presented. / High Impact Research Grants from the University of Malaya (UM.C/625/1/HIR/MOHE/CHAN/01, grant no. A-000001-50001 and UM-MOHE HIR Grant UM.C/625/1/HIR/MOHE/ CHAN/14/1, no. H-50001-A000027)

The in planta role of the global regulator Lrp in the bacterial phytopathogen Pantoea stewartii subsp. stewartii

Reynoso, Guadalupe

19 January 2022

Pantoea stewartii subsp. stewartii is a bacterial phytopathogen that causes the disease Stewart's wilt in corn. The insect vector Chaetocnema pulicaria, the corn flea beetle, transmits P. stewartii into corn plants through wounds in the leaves. The bacteria can then move to the xylem of the plant where they form a biofilm that inhibits the flow of water. A previous in planta RNA-Seq study resulted in the selection of lrp as a gene of interest for further analyses. A reverse genetics approach was used for the creation of a strain containing the in-frame deletion of lrp, as well as a revertant strain. The strain with the deletion of the lrp gene showed reduced motility and capsule formation when in vitro assays were conducted. It has previously been demonstrated that these characteristics are both important for the bacteria's ability to form a biofilm in the xylem of corn plants and produce disease symptoms. The in planta virulence and competition assays demonstrated that the lrp gene deletion also results in reduced disease symptoms in infected corn plants, as well as an inability to outcompete wildtype P. stewartii in xylem colonization. In a bioinformatics approach, the transcriptional regulator Lrp of P. stewartii was present in the same node of the phylogeny as homologues from other closely related phytopathogens. This demonstrates that Lrp from P. stewartii and such homologues have evolved from a recent common ancestral gene. Examining the genomic islands present in P. stewartii, it is possible to begin to predict where some of the genes which have functions involved in plant colonization may have originated. Overall, the results collected from the studies in this thesis contribute to improving understanding of how P. stewartii is successful at colonizing the xylem of corn plants and cause disease. This research could result in the development of methods to decrease crop susceptibility to infection with P. stewartii. / Master of Science / Stewart's wilt is a disease of corn plants caused by the bacterium Pantoea stewartii subsp. stewartii via the insect vector Chaetocnema pulicaria, the corn flea beetle. This infection has proven to be costly as it impacts the health of corn crops and impedes the export of corn seeds from varieties that are susceptible to infection by P. stewartii. The focus of the research conducted for this thesis has been on learning more about how specific P. stewartii genes impact the ability of the bacterium to colonize corn plants and cause Stewart's wilt disease symptoms. The information collected from this study is important for developing a better understanding of how wilt disease-causing pathogens are able to successfully infect plants, as well as for developing future treatments to prevent further infection of corn plants. In addition, preliminary bioinformatics work has shown that some of the P. stewartii genes of interest share a common ancestor with select genes from other known plant pathogens. Additional preliminary bioinformatics work on regions of the DNA called genomic islands has revealed where some genes of importance to the bacterium's ability to colonize plants may have originated. Overall, the work presented in this thesis contributes to improving our understanding of the roles that different parts of the P. stewartii genome have in allowing the bacterium to successfully colonize and cause disease in corn plants.

corn

genomic islands

lrp

Pantoea stewartii

phytopathogen

Stewart's wilt

Development of Methods for Structural Characterization of Pantoea stewartii Quorum-Sensing Regulator EsaR

Pennerman, Kayla Kara

04 February 2014

The LuxR family of proteins serves as quorum-sensing transcriptional regulators in proteobacteria. At high population densities, a small acyl-homoserine lactone (AHL) molecule, produced by a LuxI homologue, accumulates in the environment. The LuxR proteins bind to their respective AHL when the ligand accumulates to sufficient levels. Once bound to AHL, the holoproteins usually become functional as transcriptional activators. However, there is a subset of LuxR homologues, the EsaR subfamily, which is active without the AHL ligand and becomes inactivated once bound to it. EsaR is the best understood member of this subfamily. It controls virulence in the corn pathogen Pantoea stewartii ssp. stewartii. Solubility issues have previously limited structural studies of LuxR homologues as the proteins could not be purified without the AHL ligand. A soluble recombinant EsaR protein, HMGE, is biologically active and can be purified in the absence and presence of AHL, unlike most other LuxR homologues. Using HMGE, amino acid substitutions and Förster resonance energy transfer (FRET), experimental methods were designed for determining the dimerization interface of EsaR and for testing the hypothesis that EsaR undergoes a conformational shift when presented with the AHL ligand. To identify residues of the dimerization interface, heterodimerization assays were designed, involving either coexpression or coincubation of wild-type EsaR and variant HMGE proteins. In this assay, the inability of the proteins to copurify by nickel affinity chromatography would indicate that the modified residue(s) are important for dimerization of EsaR. To determine the conformational change that EsaR undergoes when bound to the AHL ligand, a FRET assay was developed to estimate the distances between amino acid residues in the absence and presence of AHL. Future work will have to include a few modifications to the methods and/or control experiments. This study provides the basis upon which the present methods can be further developed and later used for structural studies of EsaR. / Master of Science

EsaR

LuxR homologue

Pantoea stewartii

quorum sensing

FRET