Your search keyword '"Dillman, Adler"' showing total 12 results

1. NilD CRISPR RNA contributes to Xenorhabdus nematophila colonization of symbiotic host nematodes.

Author

Veesenmeyer JL, Andersen AW, Lu X, Hussa EA, Murfin KE, Chaston JM, Dillman AR, Wassarman KM, Sternberg PW, and Goodrich-Blair H

Subjects

Animals, Bacterial Proteins metabolism, Base Sequence, DNA Transposable Elements, Intestines microbiology, Molecular Sequence Data, Mutagenesis, Insertional, RNA, Bacterial genetics, Rhabditida physiology, Xenorhabdus genetics, Bacterial Proteins genetics, Clustered Regularly Interspaced Short Palindromic Repeats, RNA, Bacterial metabolism, Rhabditida microbiology, Symbiosis, Xenorhabdus physiology

Abstract

The bacterium Xenorhabdus nematophila is a mutualist of entomopathogenic Steinernema carpocapsae nematodes and facilitates infection of insect hosts. X. nematophila colonizes the intestine of S. carpocapsae which carries it between insects. In the X. nematophila colonization-defective mutant nilD6::Tn5, the transposon is inserted in a region lacking obvious coding potential. We demonstrate that the transposon disrupts expression of a single CRISPR RNA, NilD RNA. A variant NilD RNA also is expressed by X. nematophila strains from S. anatoliense and S. websteri nematodes. Only nilD from the S. carpocapsae strain of X. nematophila rescued the colonization defect of the nilD6::Tn5 mutant, and this mutant was defective in colonizing all three nematode host species. NilD expression depends on the presence of the associated Cas6e but not Cas3, components of the Type I-E CRISPR-associated machinery. While cas6e deletion in the complemented strain abolished nematode colonization, its disruption in the wild-type parent did not. Likewise, nilD deletion in the parental strain did not impact colonization of the nematode, revealing that the requirement for NilD is evident only in certain genetic backgrounds. Our data demonstrate that NilD RNA is conditionally necessary for mutualistic host colonization and suggest that it functions to regulate endogenous gene expression., (© 2014 John Wiley & Sons Ltd.)

Published

2014

2. Nematode-bacterium symbioses--cooperation and conflict revealed in the "omics" age.

Author

Murfin KE, Dillman AR, Foster JM, Bulgheresi S, Slatko BE, Sternberg PW, and Goodrich-Blair H

Subjects

Animals, Bacteria chemistry, Bacteria genetics, Genomics methods, Metabolomics methods, Proteomics methods, Transcriptome, Bacteria growth & development, Bacterial Physiological Phenomena, Nematoda microbiology, Nematoda physiology, Symbiosis

Abstract

Nematodes are ubiquitous organisms that have a significant global impact on ecosystems, economies, agriculture, and human health. The applied importance of nematodes and the experimental tractability of many species have promoted their use as models in various research areas, including developmental biology, evolutionary biology, ecology, and animal-bacterium interactions. Nematodes are particularly well suited for the investigation of host associations with bacteria because all nematodes have interacted with bacteria during their evolutionary history and engage in a variety of association types. Interactions between nematodes and bacteria can be positive (mutualistic) or negative (pathogenic/parasitic) and may be transient or stably maintained (symbiotic). Furthermore, since many mechanistic aspects of nematode-bacterium interactions are conserved, their study can provide broader insights into other types of associations, including those relevant to human diseases. Recently, genome-scale studies have been applied to diverse nematode-bacterial interactions and have helped reveal mechanisms of communication and exchange between the associated partners. In addition to providing specific information about the system under investigation, these studies also have helped inform our understanding of genome evolution, mutualism, and innate immunity. In this review we discuss the importance and diversity of nematodes, "omics"' studies in nematode-bacterial systems, and the wider implications of the findings.

Published

2012

3. RNA-Sequencing of Heterorhabditis nematodes to identify factors involved in symbiosis with Photorhabdus bacteria

Author

Bhat, Chaitra G, Budhwar, Roli, Godwin, Jeffrey, Dillman, Adler R, Rao, Uma, and Somvanshi, Vishal S

Subjects

Biological Sciences, Bioinformatics and Computational Biology, Genetics, Infection, Animals, Photorhabdus, Rhabditoidea, Symbiosis, Sequence Analysis, RNA, RNA, Biofilm, Early-adult stage, Heterorhabditis, Immunity, RNA-sequencing, Transcriptome, Information and Computing Sciences, Medical and Health Sciences, Bioinformatics, Biological sciences, Biomedical and clinical sciences

Abstract

BackgroundNematodes are a major group of soil inhabiting organisms. Heterorhabditis nematodes are insect-pathogenic nematodes and live in a close symbiotic association with Photorhabdus bacteria. Heterorhabditis-Photorhabdus pair offers a powerful and genetically tractable model to study animal-microbe symbiosis. It is possible to generate symbiont bacteria free (axenic) stages in Heterorhabditis. Here, we compared the transcriptome of symbiotic early-adult stage Heterorhabditis nematodes with axenic early-adult nematodes to determine the nematode genes and pathways involved in symbiosis with Photorhabdus bacteria.ResultsA de-novo reference transcriptome assembly of 95.7 Mb was created for H. bacteriophora by using all the reads. The assembly contained 46,599 transcripts with N50 value of 2,681 bp and the average transcript length was 2,054 bp. The differentially expressed transcripts were identified by mapping reads from symbiotic and axenic nematodes to the reference assembly. A total of 754 differentially expressed transcripts were identified in symbiotic nematodes as compared to the axenic nematodes. The ribosomal pathway was identified as the most affected among the differentially expressed transcripts. Additionally, 12,151 transcripts were unique to symbiotic nematodes. Endocytosis, cAMP signalling and focal adhesion were the top three enriched pathways in symbiotic nematodes, while a large number of transcripts coding for various responses against bacteria, such as bacterial recognition, canonical immune signalling pathways, and antimicrobial effectors could also be identified.ConclusionsThe symbiotic Heterorhabditis nematodes respond to the presence of symbiotic bacteria by expressing various transcripts involved in a multi-layered immune response which might represent non-systemic and evolved localized responses to maintain mutualistic bacteria at non-threatening levels. Subject to further functional validation of the identified transcripts, our findings suggest that Heterorhabditis nematode immune system plays a critical role in maintenance of symbiosis with Photorhabdus bacteria.

Published

2022

4. A core set of venom proteins is released by entomopathogenic nematodes in the genus Steinernema.

Author

Chang, Dennis Z, Serra, Lorrayne, Lu, Dihong, Mortazavi, Ali, and Dillman, Adler R

Subjects

Venoms, Animals, Drosophila melanogaster, Lepidoptera, Rhabditida, Rhabditida Infections, Helminth Proteins, Gene Expression Profiling, Symbiosis, Host-Parasite Interactions, Microbiology, Immunology, Medical Microbiology, Virology

Abstract

Parasitic helminths release molecular effectors into their hosts and these effectors can directly damage host tissue and modulate host immunity. Excreted/secreted proteins (ESPs) are one category of parasite molecular effectors that are critical to their success within the host. However, most studies of nematode ESPs rely on in vitro stimulation or culture conditions to collect the ESPs, operating under the assumption that in vitro conditions mimic actual in vivo infection. This assumption is rarely if ever validated. Entomopathogenic nematodes (EPNs) are lethal parasites of insects that produce and release toxins into their insect hosts and are a powerful model parasite system. We compared transcriptional profiles of individual Steinernema feltiae nematodes at different time points of activation under in vitro and in vivo conditions and found that some but not all time points during in vitro parasite activation have similar transcriptional profiles with nematodes from in vivo infections. These findings highlight the importance of experimental validation of ESP collection conditions. Additionally, we found that a suite of genes in the neuropeptide pathway were downregulated as nematodes activated and infection progressed in vivo, suggesting that these genes are involved in host-seeking behavior and are less important during active infection. We then characterized the ESPs of activated S. feltiae infective juveniles (IJs) using mass spectrometry and identified 266 proteins that are released by these nematodes. In comparing these ESPs with those previously identified in activated S. carpocapsae IJs, we identified a core set of 52 proteins that are conserved and present in the ESPs of activated IJs of both species. These core venom proteins include both tissue-damaging and immune-modulating proteins, suggesting that the ESPs of these parasites include both a core set of effectors as well as a specialized set, more adapted to the particular hosts they infect.

Published

2019

5. The insect pathogenic bacterium Xenorhabdus innexi has attenuated virulence in multiple insect model hosts yet encodes a potent mosquitocidal toxin

Author

Kim, Il-Hwan, Aryal, Sudarshan K, Aghai, Dariush T, Casanova-Torres, Ángel M, Hillman, Kai, Kozuch, Michael P, Mans, Erin J, Mauer, Terra J, Ogier, Jean-Claude, Ensign, Jerald C, Gaudriault, Sophie, Goodman, Walter G, Goodrich-Blair, Heidi, and Dillman, Adler R

Subjects

Genetics, Infectious Diseases, Aetiology, 2.2 Factors relating to the physical environment, Infection, Aedes, Animals, Bacterial Proteins, Bacterial Toxins, Drosophila melanogaster, Genome, Bacterial, Green Fluorescent Proteins, Host-Pathogen Interactions, Lepidoptera, Male, Phylogeny, Quantitative Trait Loci, Symbiosis, Tylenchida, Virulence, Virulence Factors, Xenorhabdus, Toxin, Insect, Immunity, NRPS/PKS, Mosquito, Lipopeptide, Biological Sciences, Information and Computing Sciences, Medical and Health Sciences, Bioinformatics

Abstract

BACKGROUND:Xenorhabdus innexi is a bacterial symbiont of Steinernema scapterisci nematodes, which is a cricket-specialist parasite and together the nematode and bacteria infect and kill crickets. Curiously, X. innexi expresses a potent extracellular mosquitocidal toxin activity in culture supernatants. We sequenced a draft genome of X. innexi and compared it to the genomes of related pathogens to elucidate the nature of specialization. RESULTS:Using green fluorescent protein-expressing X. innexi we confirm previous reports using culture-dependent techniques that X. innexi colonizes its nematode host at low levels (~3-8 cells per nematode), relative to other Xenorhabdus-Steinernema associations. We found that compared to the well-characterized entomopathogenic nematode symbiont X. nematophila, X. innexi fails to suppress the insect phenoloxidase immune pathway and is attenuated for virulence and reproduction in the Lepidoptera Galleria mellonella and Manduca sexta, as well as the dipteran Drosophila melanogaster. To assess if, compared to other Xenorhabdus spp., X. innexi has a reduced capacity to synthesize virulence determinants, we obtained and analyzed a draft genome sequence. We found no evidence for several hallmarks of Xenorhabdus spp. toxicity, including Tc and Mcf toxins. Similar to other Xenorhabdus genomes, we found numerous loci predicted to encode non-ribosomal peptide/polyketide synthetases. Anti-SMASH predictions of these loci revealed one, related to the fcl locus that encodes fabclavines and zmn locus that encodes zeamines, as a likely candidate to encode the X. innexi mosquitocidal toxin biosynthetic machinery, which we designated Xlt. In support of this hypothesis, two mutants each with an insertion in an Xlt biosynthesis gene cluster lacked the mosquitocidal compound based on HPLC/MS analysis and neither produced toxin to the levels of the wild type parent. CONCLUSIONS:The X. innexi genome will be a valuable resource in identifying loci encoding new metabolites of interest, but also in future comparative studies of nematode-bacterial symbiosis and niche partitioning among bacterial pathogens.

Published

2017

6. Activated entomopathogenic nematode infective juveniles release lethal venom proteins.

Author

Lu, Dihong, Macchietto, Marissa, Chang, Dennis, Barros, Mirayana M, Baldwin, James, Mortazavi, Ali, and Dillman, Adler R

Subjects

Venoms, Animals, Drosophila melanogaster, Xenorhabdus, Nematode Infections, Pest Control, Biological, Symbiosis, Host-Parasite Interactions, Insecta, Pest Control, Biological, Virology, Microbiology, Immunology, Medical Microbiology

Abstract

Entomopathogenic nematodes (EPNs) are unique parasites due to their symbiosis with entomopathogenic bacteria and their ability to kill insect hosts quickly after infection. It is widely believed that EPNs rely on their bacterial partners for killing hosts. Here we disproved this theory by demonstrating that the in vitro activated infective juveniles (IJs) of Steinernema carpocapsae (a well-studied EPN species) release venom proteins that are lethal to several insects including Drosophila melanogaster. We confirmed that the in vitro activation is a good approximation of the in vivo process by comparing the transcriptomes of individual in vitro and in vivo activated IJs. We further analyzed the transcriptomes of non-activated and activated IJs and revealed a dramatic shift in gene expression during IJ activation. We also analyzed the venom proteome using mass spectrometry. Among the 472 venom proteins, proteases and protease inhibitors are especially abundant, and toxin-related proteins such as Shk domain-containing proteins and fatty acid- and retinol-binding proteins are also detected, which are potential candidates for suppressing the host immune system. Many of the venom proteins have conserved orthologs in vertebrate-parasitic nematodes and are differentially expressed during IJ activation, suggesting conserved functions in nematode parasitism. In summary, our findings strongly support a new model that S. carpocapsae and likely other Steinernema EPNs have a more active role in contributing to the pathogenicity of the nematode-bacterium complex than simply relying on their symbiotic bacteria. Furthermore, we propose that EPNs are a good model system for investigating vertebrate- and human-parasitic nematodes, especially regarding the function of excretory/secretory products.

Published

2017

7. Infective Juveniles of the Entomopathogenic Nematode Steinernema scapterisci Are Preferentially Activated by Cricket Tissue.

Author

Lu, Dihong, Sepulveda, Claudia, and Dillman, Adler R

Subjects

Animals, Insects, Gryllidae, Rhabditida, Xenorhabdus, Electrophoresis, Polyacrylamide Gel, Pest Control, Biological, Symbiosis, Species Specificity, Reproduction, Time Factors, Host-Parasite Interactions, Insecta, Electrophoresis, Polyacrylamide Gel, Pest Control, Biological, MD Multidisciplinary, General Science & Technology

Abstract

Entomopathogenic nematodes are a subgroup of insect-parasitic nematodes that are used in biological control as alternatives or supplements to chemical pesticides. Steinernema scapterisci is an unusual member of the entomopathogenic nematode guild for many reasons including that it is promiscuous in its association with bacteria, it can reproduce in the absence of its described bacterial symbiont, and it is known to have a narrow host range. It is a powerful comparative model within the species and could be used to elucidate parasite specialization. Here we describe a new method of efficiently producing large numbers of S. scapterisci infective juveniles (IJs) in house crickets and for quantifying parasitic activation of the IJs upon exposure to host tissue using morphological features. We found that parasite activation is a temporal process with more IJs activating over time. Furthermore, we found that activated IJs secrete a complex mixture of proteins and that S. scapterisci IJs preferentially activate upon exposure to cricket tissue, reaffirming the description of S. scapterisci as a cricket specialist.

Published

2017

8. Comparative genomics of Steinernema reveals deeply conserved gene regulatory networks

Author

Dillman, Adler R, Macchietto, Marissa, Porter, Camille F, Rogers, Alicia, Williams, Brian, Antoshechkin, Igor, Lee, Ming-Min, Goodwin, Zane, Lu, Xiaojun, Lewis, Edwin E, Goodrich-Blair, Heidi, Stock, S Patricia, Adams, Byron J, Sternberg, Paul W, and Mortazavi, Ali

Subjects

Genetics, Biotechnology, Human Genome, Infectious Diseases, Infection, Animals, Caenorhabditis, Conserved Sequence, Gene Regulatory Networks, Genome, Pest Control, Biological, Phylogeny, Protein Structure, Tertiary, Regulatory Sequences, Nucleic Acid, Rhabditida, Symbiosis, Environmental Sciences, Biological Sciences, Information and Computing Sciences, Bioinformatics

Abstract

BackgroundParasitism is a major ecological niche for a variety of nematodes. Multiple nematode lineages have specialized as pathogens, including deadly parasites of insects that are used in biological control. We have sequenced and analyzed the draft genomes and transcriptomes of the entomopathogenic nematode Steinernema carpocapsae and four congeners (S. scapterisci, S. monticolum, S. feltiae, and S. glaseri).ResultsWe used these genomes to establish phylogenetic relationships, explore gene conservation across species, and identify genes uniquely expanded in insect parasites. Protein domain analysis in Steinernema revealed a striking expansion of numerous putative parasitism genes, including certain protease and protease inhibitor families, as well as fatty acid- and retinol-binding proteins. Stage-specific gene expression of some of these expanded families further supports the notion that they are involved in insect parasitism by Steinernema. We show that sets of novel conserved non-coding regulatory motifs are associated with orthologous genes in Steinernema and Caenorhabditis.ConclusionsWe have identified a set of expanded gene families that are likely to be involved in parasitism. We have also identified a set of non-coding motifs associated with groups of orthologous genes in Steinernema and Caenorhabditis involved in neurogenesis and embryonic development that are likely part of conserved protein-DNA relationships shared between these two genera.

Published

2015

9. CRISPR required for host colonization

Author

Veesenmeyer, Jeff L, Andersen, Aaron W, Lu, Xiaojun, Hussa, Elizabeth A, Murfin, Kristen E, Chaston, John M, Dillman, Adler R, Wassarman, Karen M, Sternberg, Paul W, and Goodrich‐Blair, Heidi

Subjects

Microbiology, Biological Sciences, Infectious Diseases, Genetics, Digestive Diseases, Animals, Bacterial Proteins, Base Sequence, Clustered Regularly Interspaced Short Palindromic Repeats, DNA Transposable Elements, Intestines, Molecular Sequence Data, Mutagenesis, Insertional, RNA, Bacterial, Rhabditida, Symbiosis, Xenorhabdus, Agricultural and Veterinary Sciences, Medical and Health Sciences, Biological sciences

Abstract

The bacterium Xenorhabdus nematophila is a mutualist of entomopathogenic Steinernema carpocapsae nematodes and facilitates infection of insect hosts. X. nematophila colonizes the intestine of S. carpocapsae which carries it between insects. In the X. nematophila colonization-defective mutant nilD6::Tn5, the transposon is inserted in a region lacking obvious coding potential. We demonstrate that the transposon disrupts expression of a single CRISPR RNA, NilD RNA. A variant NilD RNA also is expressed by X. nematophila strains from S. anatoliense and S. websteri nematodes. Only nilD from the S. carpocapsae strain of X. nematophila rescued the colonization defect of the nilD6::Tn5 mutant, and this mutant was defective in colonizing all three nematode host species. NilD expression depends on the presence of the associated Cas6e but not Cas3, components of the Type I-E CRISPR-associated machinery. While cas6e deletion in the complemented strain abolished nematode colonization, its disruption in the wild-type parent did not. Likewise, nilD deletion in the parental strain did not impact colonization of the nematode, revealing that the requirement for NilD is evident only in certain genetic backgrounds. Our data demonstrate that NilD RNA is conditionally necessary for mutualistic host colonization and suggest that it functions to regulate endogenous gene expression.

Published

2014

10. NilD CRISPR RNA contributes to Xenorhabdus nematophila colonization of symbiotic host nematodes

Author

Veesenmeyer, Jeff L., Andersen, Aaron W., Lu, Xiaojun, Hussa, Elizabeth A., Murfin, Kristen E., Chaston, John M., Dillman, Adler R., Wassarman, Karen M., Sternberg, Paul W., and Goodrich-Blair, Heidi

Subjects

Base Sequence, Agricultural and Veterinary Sciences, Molecular Sequence Data, Bacterial, Biological Sciences, Medical and Health Sciences, Microbiology, Article, Xenorhabdus, Intestines, Mutagenesis, Insertional, RNA, Bacterial, Rhabditida, Infectious Diseases, Bacterial Proteins, Mutagenesis, Insertional, DNA Transposable Elements, Genetics, Animals, RNA, Clustered Regularly Interspaced Short Palindromic Repeats, Symbiosis, Digestive Diseases

Abstract

The bacterium Xenorhabdus nematophila is a mutualist of entomopathogenic Steinernema carpocapsae nematodes and facilitates infection of insect hosts. X. nematophila colonizes the intestine of S. carpocapsae which carries it between insects. In the X. nematophila colonization-defective mutant nilD6::Tn5, the transposon is inserted in a region lacking obvious coding potential. We demonstrate that the transposon disrupts expression of a single CRISPR RNA, NilD RNA. A variant NilD RNA also is expressed by X. nematophila strains from S. anatoliense and S. websteri nematodes. Only nilD from the S. carpocapsae strain of X. nematophila rescued the colonization defect of the nilD6::Tn5 mutant, and this mutant was defective in colonizing all three nematode host species. NilD expression depends on the presence of the associated Cas6e but not Cas3, components of the Type I-E CRISPR-associated machinery. While cas6e deletion in the complemented strain abolished nematode colonization, its disruption in the wild-type parent did not. Likewise, nilD deletion in the parental strain did not impact colonization of the nematode, revealing that the requirement for NilD is evident only in certain genetic backgrounds. Our data demonstrate that NilD RNA is conditionally necessary for mutualistic host colonization and suggest that it functions to regulate endogenous gene expression.

Published

2014

11. The insect pathogenic bacterium Xenorhabdus innexi has attenuated virulence in multiple insect model hosts yet encodes a potent mosquitocidal toxin.

Author

Il-Hwan Kim, Aryal, Sudarshan K., Aghai, Dariush T., Casanova-Torres, Ángel M., Hillman, Kai, Kozuch, Michael P., Mans, Erin J., Mauer, Terra J., Ogier, Jean-Claude, Ensign, Jerald C., Gaudriault, Sophie, Goodman, Walter G., Goodrich-Blair, Heidi, and Dillman, Adler R.

Subjects

XENORHABDUS, BACTERIAL toxins, VIRULENCE of bacteria, MOSQUITO control, POLYKETIDE synthases, HIGH performance liquid chromatography, STEINERNEMA

Abstract

Background: Xenorhabdus innexi is a bacterial symbiont of Steinernema scapterisci nematodes, which is a cricketspecialist parasite and together the nematode and bacteria infect and kill crickets. Curiously, X. innexi expresses a potent extracellular mosquitocidal toxin activity in culture supernatants. We sequenced a draft genome of X. innexi and compared it to the genomes of related pathogens to elucidate the nature of specialization. Results: Using green fluorescent protein-expressing X. innexi we confirm previous reports using culture-dependent techniques that X. innexi colonizes its nematode host at low levels (~3-8 cells per nematode), relative to other Xenorhabdus-Steinernema associations. We found that compared to the well-characterized entomopathogenic nematode symbiont X. nematophila, X. innexi fails to suppress the insect phenoloxidase immune pathway and is attenuated for virulence and reproduction in the Lepidoptera Galleria mellonella and Manduca sexta, as well as the dipteran Drosophila melanogaster. To assess if, compared to other Xenorhabdus spp., X. innexi has a reduced capacity to synthesize virulence determinants, we obtained and analyzed a draft genome sequence. We found no evidence for several hallmarks of Xenorhabdus spp. toxicity, including Tc and Mcf toxins. Similar to other Xenorhabdus genomes, we found numerous loci predicted to encode non-ribosomal peptide/polyketide synthetases. Anti-SMASH predictions of these loci revealed one, related to the fcl locus that encodes fabclavines and zmn locus that encodes zeamines, as a likely candidate to encode the X. innexi mosquitocidal toxin biosynthetic machinery, which we designated Xlt. In support of this hypothesis, two mutants each with an insertion in an Xlt biosynthesis gene cluster lacked the mosquitocidal compound based on HPLC/MS analysis and neither produced toxin to the levels of the wild type parent. Conclusions: The X. innexi genome will be a valuable resource in identifying loci encoding new metabolites of interest, but also in future comparative studies of nematode-bacterial symbiosis and niche partitioning among bacterial pathogens. [ABSTRACT FROM AUTHOR]

Published

2017

12. NilD CRISPR RNA contributes to X enorhabdus nematophila colonization of symbiotic host nematodes.

Author

Veesenmeyer, Jeff L., Andersen, Aaron W., Lu, Xiaojun, Hussa, Elizabeth A., Murfin, Kristen E., Chaston, John M., Dillman, Adler R., Wassarman, Karen M., Sternberg, Paul W., and Goodrich‐Blair, Heidi

Subjects

CRISPRS, XENORHABDUS nematophilus, NEMATODE-plant relationships, SYMBIOSIS, GENE expression, INSECT hosts

Abstract

The bacterium X enorhabdus nematophila is a mutualist of entomopathogenic S teinernema carpocapsae nematodes and facilitates infection of insect hosts. X . nematophila colonizes the intestine of S . carpocapsae which carries it between insects. In the X . nematophila colonization-defective mutant nilD6:: Tn 5, the transposon is inserted in a region lacking obvious coding potential. We demonstrate that the transposon disrupts expression of a single CRISPR RNA, NilD RNA. A variant NilD RNA also is expressed by X . nematophila strains from S . anatoliense and S . websteri nematodes. Only nilD from the S . carpocapsae strain of X . nematophila rescued the colonization defect of the nilD6:: Tn 5 mutant, and this mutant was defective in colonizing all three nematode host species. NilD expression depends on the presence of the associated Cas6e but not Cas3, components of the Type I- E CRISPR-associated machinery. While cas6e deletion in the complemented strain abolished nematode colonization, its disruption in the wild-type parent did not. Likewise, nilD deletion in the parental strain did not impact colonization of the nematode, revealing that the requirement for NilD is evident only in certain genetic backgrounds. Our data demonstrate that NilD RNA is conditionally necessary for mutualistic host colonization and suggest that it functions to regulate endogenous gene expression. [ABSTRACT FROM AUTHOR]

Published

2014