Your search keyword '"Nilles, Matthew L."' showing total 39 results

1. Structure-function analysis of the C-terminal domain of LcrV from Yersinia pestis

Author

Hamad, Mohamad A. and Nilles, Matthew L.

Subjects

Yersinia pestis -- Physiological aspects, Bacterial proteins -- Properties, Biological sciences

Abstract

LcrV, a multifunctional protein, acts as a positive regulator of effector protein secretion for the type III secretion system (T3SS) in Yersinia pestis by interaction with the negative regulator LcrG. In this study, LcrV was analyzed to identify regions required for LcrG interaction. Random-linker insertion mutagenesis, deletion analysis, and site-directed mutagenesis of hydrophobic amino acids between residues 290 and 311 allowed the isolation of an LcrV mutant (LcrV L291R F308R) defective for LcrG interaction. The new residues identified in LcrG interaction lie in helix 12 of LcrV; residues in helix 7 of LcrV are known to be involved in LcrG interaction. Helix 7 and helix 12 of LcrV interact to form an intramolecular coiled coil; these new results suggest that the intramolecular coiled coil in LcrV is required for LcrG interaction and activation of the T3SS.

Published

2007

2. Bile salts and fatty acids induce the expression of Escherichia coli AcrAB multidrug efflux pump through their interaction with Rob regulatory protein

Author

Rosenberg, Emiko Y., Bertenthal, Dan, Nilles, Matthew L., Bertrand, Kevin P., and Nikaido, Hiroshi

Published

2003

3. LcrG secretion is not required for blocking of Yops secretion in Yersinia pestis

Author

Matson Jyl S, O'Bryant Deanna M, Reina Laura D, and Nilles Matthew L

Subjects

Microbiology, QR1-502

Abstract

Abstract Background LcrG, a negative regulator of the Yersinia type III secretion apparatus has been shown to be primarily a cytoplasmic protein, but is secreted at least in Y. pestis. LcrG secretion has not been functionally analyzed and the relevance of LcrG secretion on LcrG function is unknown. Results An LcrG-GAL4AD chimera, originally constructed for two-hybrid analyses to analyze LcrG protein interactions, appeared to be not secreted but the LcrG-GAL4AD chimera retained the ability to regulate Yops secretion. This result led to further investigation to determine the significance of LcrG secretion on LcrG function. Additional analyses including deletion and substitution mutations of amino acids 2–6 in the N-terminus of LcrG were constructed to analyze LcrG secretion and LcrG's ability to control secretion. Some changes to the N-terminus of LcrG were found to not affect LcrG's secretion or LcrG's secretion-controlling activity. However, substitution of poly-isoleucine in the N-terminus of LcrG did eliminate LcrG secretion but did not affect LcrG's secretion controlling activity. Conclusion These results indicate that secretion of LcrG, while observable and T3SS mediated, is not relevant for LcrG's ability to control secretion.

Published

2008

4. Immunization of mice with YscF provides protection from Yersinia pestis infections

Author

Bradley David S, Durick Kelly A, Matson Jyl S, and Nilles Matthew L

Subjects

Microbiology, QR1-502

Abstract

Abstract Background Yersinia pestis, the causative agent of plague, is a pathogen with a tremendous ability to cause harm and panic in populations. Due to the severity of plague and its potential for use as a bioweapon, better preventatives and therapeutics for plague are desirable. Subunit vaccines directed against the F1 capsular antigen and the V antigen (also known as LcrV) of Y. pestis are under development. However, these new vaccine formulations have some possible limitations. The F1 antigen is not required for full virulence of Y. pestis and LcrV has a demonstrated immunosuppressive effect. These limitations could damper the ability of F1/LcrV based vaccines to protect against F1-minus Y. pestis strains and could lead to a high rate of undesired side effects in vaccinated populations. For these reasons, the use of other antigens in a plague vaccine formulation may be advantageous. Results Desired features in vaccine candidates would be antigens that are conserved, essential for virulence and accessible to circulating antibody. Several of the proteins required for the construction or function of the type III secretion system (TTSS) complex could be ideal contenders to meet the desired features of a vaccine candidate. Accordingly, the TTSS needle complex protein, YscF, was selected to investigate its potential as a protective antigen. In this study we describe the overexpression, purification and use of YscF as a protective antigen. YscF immunization triggers a robust antibody response to YscF and that antibody response is able to afford significant protection to immunized mice following challenge with Y. pestis. Additionally, evidence is presented that suggests antibody to YscF is likely not protective by blocking the activity of the TTSS. Conclusion In this study we investigated YscF, a surface-expressed protein of the Yersinia pestis type III secretion complex, as a protective antigen against experimental plague infection. Immunization of mice with YscF resulted in a high anti-YscF titer and provided protection against i.v. challenge with Y. pestis. This is the first report to our knowledge utilizing a conserved protein from the type III secretion complex of a gram-negative pathogen as a candidate for vaccine development.

Published

2005

5. Interaction of the Yersinia pestis type III regulatory proteins LcrG and LcrV occurs at a hydrophobic interface: correction

Author

Nilles Matthew L and Matson Jyl S

Subjects

Microbiology, QR1-502

Published

2002

6. Dengue virus specific IgY provides protection following lethal dengue virus challenge and is neutralizing in the absence of inducing antibody dependent enhancement.

Author

Fink, Ashley L., Williams, Katherine L., Harris, Eva, Alvine, Travis D., Henderson, Thomas, Schiltz, James, Nilles, Matthew L., and Bradley, David S.

Subjects

DENGUE virus genetics, ANTIBODY-dependent enhancement, DENGUE hemorrhagic fever, FC receptors, ANTIGENS, DISEASE risk factors, THERAPEUTICS

Abstract

Dengue hemorrhagic fever (DHF) and dengue shock syndrome (DSS) are severe disease manifestations that can occur following sequential infection with different dengue virus serotypes (DENV1-4). At present, there are no licensed therapies to treat DENV-induced disease. DHF and DSS are thought to be mediated by serotype cross-reactive antibodies that facilitate antibody-dependent enhancement (ADE) by binding to viral antigens and then Fcγ receptors (FcγR) on target myeloid cells. Using genetically engineered DENV-specific antibodies, it has been shown that the interaction between the Fc portion of serotype cross-reactive antibodies and FcγR is required to induce ADE. Additionally, it was demonstrated that these antibodies were as neutralizing as their non-modified variants, were incapable of inducing ADE, and were therapeutic following a lethal, antibody-enhanced infection. Therefore, we hypothesized that avian IgY, which do not interact with mammalian FcγR, would provide a novel therapy for DENV-induced disease. We demonstrate here that goose-derived anti-DENV2 IgY neutralized DENV2 and did not induce ADE in vitro. Anti-DENV2 IgY was also protective in vivo when administered 24 hours following a lethal DENV2 infection. We were also able to demonstrate via epitope mapping that both full-length and alternatively spliced anti-DENV2 IgY recognized different epitopes, including epitopes that have not been previously identified. These observations provide evidence for the potential therapeutic applications of goose-derived anti-DENV2 IgY. [ABSTRACT FROM AUTHOR]

Published

2017

7. Interaction of the Yersinia pestis type III regulatory proteins LcrG and LcrV occurs at a hydrophobic interface: correction

Author

Matson, Jyl S and Nilles, Matthew L

Subjects

lcsh:QR1-502, Correction, lcsh:Microbiology

Published

2002

8. Antiviral Biologic Produced in DNA Vaccine/Goose Platform Protects Hamsters Against Hantavirus Pulmonary Syndrome When Administered Post-exposure.

Author

Haese, Nicole, Brocato, Rebecca L., Henderson, Thomas, Nilles, Matthew L., Kwilas, Steve A., Josleyn, Matthew D., Hammerbeck, Christopher D., Schiltz, James, Royals, Michael, Ballantyne, John, Hooper, Jay W., and Bradley, David S.

Subjects

DNA vaccines, IMMUNE serums, HANTAVIRUS diseases, VIRAL antibodies, HAMSTERS, VIRAL tropism, HUMORAL immunity

Abstract

Andes virus (ANDV) and ANDV-like viruses are responsible for most hantavirus pulmonary syndrome (HPS) cases in South America. Recent studies in Chile indicate that passive transfer of convalescent human plasma shows promise as a possible treatment for HPS. Unfortunately, availability of convalescent plasma from survivors of this lethal disease is very limited. We are interested in exploring the concept of using DNA vaccine technology to produce antiviral biologics, including polyclonal neutralizing antibodies for use in humans. Geese produce IgY and an alternatively spliced form, IgYΔFc, that can be purified at high concentrations from egg yolks. IgY lacks the properties of mammalian Fc that make antibodies produced in horses, sheep, and rabbits reactogenic in humans. Geese were vaccinated with an ANDV DNA vaccine encoding the virus envelope glycoproteins. All geese developed high-titer neutralizing antibodies after the second vaccination, and maintained high-levels of neutralizing antibodies as measured by a pseudovirion neutralization assay (PsVNA) for over 1 year. A booster vaccination resulted in extraordinarily high levels of neutralizing antibodies (i.e., PsVNA80 titers >100,000). Analysis of IgY and IgYΔFc by epitope mapping show these antibodies to be highly reactive to specific amino acid sequences of ANDV envelope glycoproteins. We examined the protective efficacy of the goose-derived antibody in the hamster model of lethal HPS. α-ANDV immune sera, or IgY/IgYΔFc purified from eggs, were passively transferred to hamsters subcutaneously starting 5 days after an IM challenge with ANDV (25 LD50). Both immune sera, and egg-derived purified IgY/IgYΔFc, protected 8 of 8 and 7 of 8 hamsters, respectively. In contrast, all hamsters receiving IgY/IgYΔFc purified from normal geese (n=8), or no-treatment (n=8), developed lethal HPS. These findings demonstrate that the DNA vaccine/goose platform can be used to produce a candidate antiviral biological product capable of preventing a lethal disease when administered post-exposure. Author Summary: Our studies show the utility of combining DNA vaccination with the goose platform for the development of polyclonal avian antibodies for use as candidate medical countermeasures. We demonstrate that these antibodies have potent anti-viral neutralizing activity in cell culture and are efficacious in preventing hantavirus pulmonary syndrome in Syrian hamsters when administered as a post-exposure prophylactic. The polyclonal anti-Andes virus antibodies were not effective if administered late in the disease course indicating that the effective use of an avian polyclonal antibody-based approach to preventing hantavirus disease will require rapid diagnosis and treatment of persons presenting signs of hantavirus disease. [ABSTRACT FROM AUTHOR]

Published

2015

9. HLA-DQ8ab transgenic mice demonstrate an increased resistance to the plague

Author

O'Bryant, Deanna M., Nilles, Matthew L., and Bradley, David S.

Subjects

T cells -- Research -- Physiological aspects, Genetically modified mice -- Physiological aspects -- Research, Drug resistance in microorganisms -- Research, Science and technology, Physiological aspects, Research

Abstract

The number of different antigenic peptides that can be presented by a Major Histocompatibility Complex (MHC) Class II molecule varies greatly from allele to allele. The more restricted the presentation, [...]

Published

2005

10. Roles of YopN, LcrG and LcrV in Controlling Yops Secretion by Yersinia pestis.

Author

Back, Nathan, Cohen, Irun R., Kritchevsky, David, Lajtha, Abel, Paoletti, Rodolfo, Perry, Robert D., Fetherston, Jacqueline D., Hamad, Mohamad A., and Nilles, Matthew L.

Abstract

Control of Yops secretion in pathogenic Yersinia is achieved at several levels. These levels likely include transcriptional, post-transcriptional, translational and secretional controls. Secretion control appears to be mediated by two pathways. One pathway involves YopN and proteins that interact with YopN. The second pathway consists of LcrG and its interaction with LcrV. LcrV is a postive regulator of Yops secretion that exerts control over Yops secretion by negating the secretion blocking role of LcrG. However, the intersection of these two control pathways is not understood. Recent work has allowed the development of a speculative model that brings YopN-mediated and LcrG-LcrV-mediated control together in the context of the ability of the needle complex to respond to Ca2+. [ABSTRACT FROM AUTHOR]

Published

2008

11. SECTION II TOXIN BIOGENESIS: CROSSING BACTERIAL MEMBRANE BARRIERS: Chapter 7: Type III Secretion Systems.

Author

Plano, Gregory V., Schesser, Kurt, and Nilles, Matthew L.

Published

2003

12. LcrG secretion is not required for blocking of Yops secretion in Yersinia pestis.

Author

Reina, Laura D., O'Bryant, Deanna M., Matson, Jyl S., and Nilles, Matthew L.

Subjects

SECRETION, PROTEINS, YERSINIA pestis, MICROBIAL mutation, AMINO acids

Abstract

Background: LcrG, a negative regulator of the Yersinia type III secretion apparatus has been shown to be primarily a cytoplasmic protein, but is secreted at least in Y. pestis. LcrG secretion has not been functionally analyzed and the relevance of LcrG secretion on LcrG function is unknown. Results: An LcrG-GAL4AD chimera, originally constructed for two-hybrid analyses to analyze LcrG protein interactions, appeared to be not secreted but the LcrG-GAL4AD chimera retained the ability to regulate Yops secretion. This result led to further investigation to determine the significance of LcrG secretion on LcrG function. Additional analyses including deletion and substitution mutations of amino acids 2-6 in the N-terminus of LcrG were constructed to analyze LcrG secretion and LcrG's ability to control secretion. Some changes to the N-terminus of LcrG were found to not affect LcrG's secretion or LcrG's secretion-controlling activity. However, substitution of poly-isoleucine in the N-terminus of LcrG did eliminate LcrG secretion but did not affect LcrG's secretion controlling activity. Conclusion: These results indicate that secretion of LcrG, while observable and T3SS mediated, is not relevant for LcrG's ability to control secretion. [ABSTRACT FROM AUTHOR]

Published

2008

13. Immunization of mice with YscF provides protection from Yersinia pestis infections.

Author

Matson, Jyl S., Durick, Kelly A., Bradley, David S., and Nilles, Matthew L.

Subjects

YERSINIA pestis, PLAGUE, PATHOGENIC microorganisms, BIOLOGICAL weapons, VACCINES, PROTEINS, THERAPEUTICS

Abstract

Background: Yersinia pestis, the causative agent of plague, is a pathogen with a tremendous ability to cause harm and panic in populations. Due to the severity of plague and its potential for use as a bioweapon, better preventatives and therapeutics for plague are desirable. Subunit vaccines directed against the F1 capsular antigen and the V antigen (also known as LcrV) of Y. pestis are under development. However, these new vaccine formulations have some possible limitations. The F1 antigen is not required for full virulence of Y. pestis and LcrV has a demonstrated immunosuppressive effect. These limitations could damper the ability of F1/LcrV based vaccines to protect against F1-minus Y. pestis strains and could lead to a high rate of undesired side effects in vaccinated populations. For these reasons, the use of other antigens in a plague vaccine formulation may be advantageous. Results: Desired features in vaccine candidates would be antigens that are conserved, essential for virulence and accessible to circulating antibody. Several of the proteins required for the construction or function of the type III secretion system (TTSS) complex could be ideal contenders to meet the desired features of a vaccine candidate. Accordingly, the TTSS needle complex protein, YscF, was selected to investigate its potential as a protective antigen. In this study we describe the overexpression, purification and use of YscF as a protective antigen. YscF immunization triggers a robust antibody response to YscF and that antibody response is able to afford significant protection to immunized mice following challenge with Y. pestis. Additionally, evidence is presented that suggests antibody to YscF is likely not protective by blocking the activity of the TTSS. Conclusion: In this study we investigated YscF, a surface-expressed protein of the Yersinia pestis type III secretion complex, as a protective antigen against experimental plague infection. Immunization of mice with YscF resulted in a high anti-YscF titer and provided protection against i.v. challenge with Y. pestis. This is the first report to our knowledge utilizing a conserved protein from the type III secretion complex of a gram-negative pathogen as a candidate for vaccine development. [ABSTRACT FROM AUTHOR]

Published

2005

14. LcrG-LcrV Interaction Is Required for Control of Yops Secretion in Yersinia pestis.

Author

Matson, Jyl S. and Nilles, Matthew L.

Subjects

*YERSINIA pestis, *BACTERIAL proteins, *GENETICS

Abstract

Examines the effect of disrupting the interaction between the LcrG and LcrV proteins in Yersinia pestis. Creation of a stable LcrG mutant that does not interact with LcrV; Role of LcrG A16R in blocking secretion of Yops in vitro; Role of LcrG A16R in repressing expression of Yops; Role of LcrG in blocking translocation of Yops into HeLa cells.

Published

2001

15. The V antigen of Yersinia pestis regulates yop vectorial targeting as well as yop secretion...

Author

Nilles, Matthew L., Fields, Kenneth A., and Straley, Susan C.

Subjects

*YERSINIA pestis, *PROTEINS, *SECRETION

Abstract

Presents a study where Yersinia pestis expresses a set of secreted proteins referred to as Yops and the bifunctional low positive ion response virulence (lcrV) which have regulatory and antihost functions. Regulation of Yops and LcrV expression and the activity of the type III mechanism for their secretion; Description of the secretion process of Yops and LcrV; Information on Yersinia pestis.

Published

1998

16. Yersinia pestis LcrV forms a stable complex with LcrG and may have a secretion-related regulatory...

Author

Nilles, Matthew L. and Williams, Andrew W.

Subjects

*CELL membranes

Abstract

Presents information which shows that the cell-associated LcrG is cytoplasmically localized. Interaction of LcrG with LcrV to form a heterodimeric complex; Detection of small amounts of LcrG abnd YopE in periplasmic fractions.

Published

1997

17. Zika Virus-Specific IgY Results Are Therapeutic Following a Lethal Zika Virus Challenge without Inducing Antibody-Dependent Enhancement.

Author

O'Donnell, Kyle L., Meberg, Bernadette, Schiltz, James, Nilles, Matthew L., and Bradley, David S.

Subjects

ZIKA virus infections, FLAVIVIRUSES, MICROCEPHALY, IMMUNOGLOBULINS, VIRUS diseases

Abstract

The Zika virus (ZIKV) is a newly emerged pathogen in the Western hemisphere. It was declared a global health emergency by the World Health Organization in 2016. There have been 223,477 confirmed cases, including 3720 congenital syndrome cases since 2015. ZIKV infection symptoms range from asymptomatic to Gullain–Barré syndrome and extensive neuropathology in infected fetuses. Passive and active vaccines have been unsuccessful in the protection from or the treatment of flaviviral infections due to antibody-dependent enhancement (ADE). ADE causes an increased viral load due to an increased monocyte opsonization by non-neutralizing, low-avidity antibodies from a previous dengue virus (DENV) infection or from a previous exposure to ZIKV. We have previously demonstrated that polyclonal avian IgY generated against whole-killed DENV-2 ameliorates DENV infection in mice while not inducing ADE. This is likely due to the inability of the Fc portion of IgY to bind to mammalian Fc receptors. We have shown here that ZIKV oligoclonal IgY is able to neutralize the virus in vitro and in IFNAR−/− mice. The concentration of ZIKV-specific IgY yielding 50% neutralization (NT50) was 25 µg/mL. The exposure of the ZIKV, prior to culture with ZIKV-specific IgY or 4G2 flavivirus-enveloped IgG, demonstrated that the ZIKV-specific IgY does not induce ADE. ZIKV IgY was protective in vivo when administered following a lethal ZIKV challenge in 3-week-old IFNAR−/− mice. We propose polyclonal ZIKV-specific IgY may provide a viable passive immunotherapy for a ZIKV infection without inducing ADE. [ABSTRACT FROM AUTHOR]

Published

2019

18. Dissecting the Structure of LcrV from Yersinia pestis, a Truly Unique Virulence Protein

Author

Nilles, Matthew L.

Subjects

*YERSINIA pestis, *PLAGUE, *PATHOGENIC microorganisms, *MICROBIAL virulence

Abstract

Last month in the February issue, Structure published the crystal structure of LcrV from Yersinia pestis, the infectious agent that causes plague. LcrV activity is essential for disease, and the structure of this protein provides a valuable tool to dissect the nature of its pathogenicity. [Copyright &y& Elsevier]

Published

2004

19. Genome Sequence of Yersinia pestis KIM.

Author

Wen Deng, Burland, Valerie, Plunkett III, Guy, Boutin, Adam, Mayhew, George F., Liss, Paul, Perna, Nicole T., Rose, Debra J., Mau, Bob, Zhou, Shiguo, Schwartz, David C., Fetherston, Jacqueline D., Lindler, Luther E., Brubaker, Robert R., Plano, Gregory V., Straley, Susan C., McDonough, Kathleen A., Nilles, Matthew L., and Matson, Jyl S.

Subjects

*GENOMES, *YERSINIA pestis

Abstract

Examines the complete genome sequence of Yersinia (Y.) pestis KIM. List of diseases associated with Y. pestis; Comparison of genome proteins; Identification of ribosomal RNA operons.

Published

2002

20. Avian anti-NS1 IgY antibodies neutralize dengue virus infection and protect against lethal dengue virus challenge.

Author

O'Donnell, Kyle L., Espinosa, Diego A., Puerta-Guardo, Henry, Biering, Scott B., Warnes, Colin M., Schiltz, James, Nilles, Matthew L., Li, Jeffrey, Harris, Eva, and Bradley, David S.

Subjects

*DENGUE viruses, *VIRUS diseases, *ARBOVIRUS diseases, *ZIKA virus infections, *IMMUNOGLOBULINS, *GLYCOCALYX, *EGG yolk, *ZIKA virus

Abstract

Dengue is the most prevalent arboviral disease in humans and a continually increasing global public health burden. To date, there are no approved antiviral therapies against dengue virus (DENV) and the only licensed vaccine, Dengvaxia, is exclusively indicated for individuals with prior DENV infection. Endothelial hyperpermeability and vascular leak, pathogenic hallmarks of severe dengue disease, can be directly triggered by DENV non-structural protein 1 (NS1). As such, anti-NS1 antibodies can prevent NS1-triggered endothelial dysfunction in vitro and pathogenesis in vivo. Recently, goose-derived anti-DENV immunoglobulin Y (IgY) antibodies were shown to neutralize DENV and Zika virus (ZIKV) infection without adverse effects, such as antibody-dependent enhancement (ADE). In this study, we used egg yolks from DENV-immunized geese to purify IgY antibodies specific to DENV NS1 epitopes. We determined that 2 anti-NS1 IgY antibodies, NS1-1 and NS1-8, were capable of neutralizing DENV infection in vitro. In addition, these antibodies did not cross-react with the DENV Envelope (E) protein nor enhance DENV or ZIKV infection in vitro. Intriguingly, NS1-8, but not NS1-1, partially blocked NS1-induced endothelial dysfunction in vitro while neither antibody blocked binding of soluble NS1 to cells. Finally, prophylactic treatment of mice with NS1-8 conferred significant protection against lethal DENV challenge. Although further research is needed to define the mechanism of action of these antibodies, our findings highlight the potential of anti-NS1 IgY as a promising prophylactic approach against DENV infection. • DENV NS1-specific IgY antibodies were purified from egg yolks obtained from DENV2-immunized geese. • Two anti-NS1 IgY antibodies neutralized DENV2 infection in vitro and did not mediate antibody-dependent enhancement. • One of these anti-NS1 IgY antibodies partially blocked NS1-induced endothelial dysfunction and protected mice from lethal DENV2 infection. [ABSTRACT FROM AUTHOR]

Published

2020

21. Difference in Strain Pathogenicity of Septicemic Yersinia pestis Infection in a TLR2 -/- Mouse Model.

Author

O'Donnell KL, Knopick PL, Larsen R, Sarkar S, Nilles ML, and Bradley DS

Subjects

Animals, Bacterial Load, Bacterial Proteins genetics, Cytokines metabolism, Disease Models, Animal, Female, Granulocytes metabolism, Liver immunology, Macrophages immunology, Macrophages metabolism, Mice, Mice, Inbred C57BL, Mice, Knockout, Neutrophils immunology, Neutrophils metabolism, Plague metabolism, Plague microbiology, Reactive Nitrogen Species metabolism, Reactive Oxygen Species metabolism, Spleen immunology, Spleen microbiology, Toll-Like Receptor 2 immunology, Virulence genetics, Yersinia pestis genetics, Plague immunology, Toll-Like Receptor 2 deficiency, Yersinia pestis pathogenicity

Abstract

Yersinia pestis is the causative agent of bubonic, pneumonic, and septicemic plague. We demonstrate that Toll-like receptor 2-deficient (TLR2 -/- ) mice are resistant to septicemic infection by the KIM5 strain of Y. pestis but not to infection by the CO92 Δpgm strain. This resistance is dependent on TLR2, the route of infection, and the isoform of YopJ. Elevated bacterial burdens were found in the spleens of CO92 Δpgm -infected animals by 24 h postinfection and in the livers by 4 days. The YopJ isoform present contributed directly to cytotoxicity and inflammatory cytokine production of bone marrow-derived macrophages from TLR2 -/- mice. Immune cell trafficking is altered in CO92 Δpgm infections, with an increased neutrophil infiltration to the spleen 5 days postinfection. Immune cell infiltration to the liver was greater and earlier in KIM5-infected TLR2 -/- mice. The functionality of the immune cells was assessed by the ability to develop reactive oxygen and nitrogen species. Our data suggest an inhibition of granulocytes in forming these species in CO92 Δpgm -infected TLR2 -/- mice. These findings suggest that resistance to KIM5 in TLR2 -/- mice is dependent on early immune cell trafficking and functionality., (Copyright © 2020 American Society for Microbiology.)

Published

2020

22. Necroptosis of infiltrated macrophages drives Yersinia pestis dispersal within buboes.

Author

Arifuzzaman M, Ang WXG, Choi HW, Nilles ML, St John AL, and Abraham SN

Subjects

Animals, Bacterial Proteins metabolism, Cell Death, Cell Line, Disease Models, Animal, Lysophospholipids metabolism, Macrophages microbiology, Mice, Mice, Inbred C57BL, Receptor-Interacting Protein Serine-Threonine Kinases metabolism, Sphingosine analogs & derivatives, Sphingosine metabolism, Virulence Factors, Apoptosis, Macrophages immunology, Plague immunology, Yersinia pestis pathogenicity

Abstract

When draining lymph nodes become infected by Yersinia pestis (Y. pestis), a massive influx of phagocytic cells occurs, resulting in distended and necrotic structures known as buboes. The bubonic stage of the Y. pestis life cycle precedes septicemia, which is facilitated by trafficking of infected mononuclear phagocytes through these buboes. However, how Y. pestis convert these immunocytes recruited by host to contain the pathogen into vehicles for bacterial dispersal and the role of immune cell death in this context are unknown. We show that the lymphatic spread requires Yersinia outer protein J (YopJ), which triggers death of infected macrophages by downregulating a suppressor of receptor-interacting protein kinase 1-mediated (RIPK1-mediated) cell death programs. The YopJ-triggered cell death was identified as necroptotic, which released intracellular bacteria, allowing them to infect new neighboring cell targets. Dying macrophages also produced chemotactic sphingosine 1-phosphate, enhancing cell-to-cell contact, further promoting infection. This necroptosis-driven expansion of infected macrophages in buboes maximized the number of bacteria-bearing macrophages reaching secondary lymph nodes, leading to sepsis. In support, necrostatins confined bacteria within macrophages and protected mice from lethal infection. These findings define necrotization of buboes as a mechanism for bacterial spread and a potential target for therapeutic intervention.

Published

2018

23. Detection of Protein Interactions in T3S Systems Using Yeast Two-Hybrid Analysis.

Author

Nilles ML

Subjects

Gene Expression, Genes, Reporter, Protein Binding, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Transformation, Genetic, beta-Galactosidase metabolism, Bacterial Proteins metabolism, Protein Interaction Mapping methods, Two-Hybrid System Techniques, Type III Secretion Systems metabolism

Abstract

Two-hybrid systems, sometimes termed interaction traps, are genetic systems designed to find and analyze interactions between proteins. The most common systems are yeast based (commonly Saccharomyces cerevisae) and rely on the functional reconstitution of the GAL4 transcriptional activator. Reporter genes, such as the lacZ gene of Escherichia coli (encodes β-galactosidase), are placed under GAL4-dependent transcriptional control to provide quick and reliable detection of protein interactions. In this method the use of a yeast-based two-hybrid system is described to study protein interactions between components of type III secretion systems.

Published

2017

24. Blue Native Protein Electrophoresis to Study the T3S System Using Yersinia pestis as a Model.

Author

Henderson TA and Nilles ML

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Blotting, Western, Mass Spectrometry, Proteome, Proteomics methods, Type III Secretion Systems genetics, Electrophoresis methods, Type III Secretion Systems metabolism, Yersinia pestis physiology

Abstract

Since the introduction of blue native, clear native, and high-resolution clear native electrophoresis to study protein complexes of eukaryotic, bacterial, and archaeal cells, the technique has been used primarily to study physiological systems that are found in abundance within the cell. Systems involved in oxidative phosphorylation, electron transport, membrane transporters, and secretion systems have been studied using these techniques. These microscale techniques are ideal due to the minimal perturbations caused to these protein complexes. The utility of the blue native electrophoresis method was determined in a study described here of protein complexes identified in the plague causing bacteria, Yersinia pestis. In addition, the technique was used to observe how LcrG, a negative regulator of the pathogenic Type III secretion system (T3SS), interacts with the T3SS and other protein complexes.

Published

2017

25. In Vivo Photo-Cross-Linking to Study T3S Interactions Demonstrated Using the Yersinia pestis T3S System.

Author

Henderson TA and Nilles ML

Subjects

Bacterial Proteins genetics, Bacterial Proteins isolation & purification, Blotting, Western, Carrier Proteins metabolism, Chromatography, Affinity, Leucine metabolism, Methionine metabolism, Pore Forming Cytotoxic Proteins chemistry, Pore Forming Cytotoxic Proteins isolation & purification, Pore Forming Cytotoxic Proteins metabolism, Protein Binding, Type III Secretion Systems genetics, Bacterial Proteins metabolism, Protein Interaction Mapping methods, Type III Secretion Systems metabolism, Yersinia pestis physiology

Abstract

Cross-linking of proteins is effective in determining protein-protein interactions. The use of photo-cross-linkers was developed to study protein interactions in several manners. One method involved the incorporation of photo-activatable cross-linking groups into chemically synthesized peptides. A second approach relies on incorporation of photo-activatable cross-linking groups into proteins using tRNAs with chemically bound photo-activatable amino acids with suppressor tRNAs translational systems to incorporate the tags into specific sites. A third system was made possible by the development of photoreactive amino acids that use the normal cellular tRNAs and aminoacyl tRNA synthetases. In this method, the third system is used to demonstrate its utility for the study of T3S system interactions. This method describes how two photo-activatable amino acids, photo-methionine and photo-leucine, that use the normal cellular machinery are incorporated into Yersinia pestis and used to study interactions in the T3S system. To demonstrate the system, the method was used to cross-link the T3S regulatory proteins LcrG and LcrV.

Published

2017

26. Analysis of Type III Secretion System Secreted Proteins.

Author

Condry DL and Nilles ML

Subjects

Bacterial Outer Membrane Proteins genetics, Bacterial Outer Membrane Proteins metabolism, Bacterial Proteins genetics, Blotting, Western, Protein Transport, Type III Secretion Systems genetics, Yersinia genetics, Yersinia metabolism, Bacterial Proteins metabolism, Type III Secretion Systems metabolism

Abstract

Secreted proteins of the T3SS vary from genus to genus. How secretion is induced in vitro also depends on the genus of bacteria. However, once those proteins are isolated the method for analyzing those proteins is largely the same. The following chapter outlines the specific induction of Yersinia secreted proteins and uniform analysis of those secreted proteins.

Published

2017

27. Identification of the Targets of Type III Secretion System Inhibitors.

Author

Condry DL and Nilles ML

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Blotting, Western, Electrophoresis, Polyacrylamide Gel, Gene Knockout Techniques, Gram-Negative Bacteria drug effects, Gram-Negative Bacteria metabolism, Hemolysis drug effects, Mutation, Type III Secretion Systems genetics, Type III Secretion Systems metabolism, Anti-Bacterial Agents pharmacology, Bacterial Proteins antagonists & inhibitors, Drug Discovery, Type III Secretion Systems antagonists & inhibitors

Abstract

A type III secretion system (T3SS) Inhibitor can be utilized for study in the research lab but also progressed into drug development. Since many pathogenic Gram-negative bacteria utilize this highly conserved system as a virulence factor, the prospect of the T3SS as a drug target is promising. To effectively move a T3SS inhibitor into the route of either research or pharmaceuticals an understanding of the target and mechanism of the inhibitor is required. Several methods can be utilized to identify the target. Included here is the use of knockout mutations, tagged inhibitor pull-down assays, and targeted identification methods.

Published

2017

28. Isolation of Type III Secretion System Needle Complexes by Shearing.

Author

Nilles ML, Condry DL, and Osei-Owusu P

Subjects

Blotting, Western, Electrophoresis, Bacterial Proteins metabolism, Gram-Negative Bacteria metabolism, Multiprotein Complexes isolation & purification, Multiprotein Complexes metabolism, Type III Secretion Systems metabolism

Abstract

Type III secretion (T3S) needle proteins are essential for the pathogenesis of many gram-negative bacteria. The needle component of the T3S system serves as the conduit for the translocation of effector proteins from the cytoplasm of many gram-negative bacteria into their target eukaryotic cells. Despite substantial advances that have been made in their characterization, a lot is still unknown about their interactions with other T3S system proteins and their roles in modulating host immune responses during infections. Critical to achieving this knowledge is the ability to isolate these needle proteins in their stable, native form. In this chapter, we describe a modified, streamlined isolation strategy for native forms of these T3S system needle proteins. We also present assays to detect the presence and quantification of these needle proteins.

Published

2017

29. Mouse Immunization with Purified Needle Proteins from Type III Secretion Systems and the Characterization of the Immune Response to These Proteins.

Author

Alvine TD, Bradley DS, and Nilles ML

Subjects

Animals, Antibodies, Bacterial immunology, Cytokines metabolism, Enzyme-Linked Immunosorbent Assay, Immunization, Immunoglobulin G immunology, Mice, Recombinant Proteins administration & dosage, Bacterial Proteins immunology, Recombinant Proteins immunology, Type III Secretion Systems immunology

Abstract

Many Gram-negative pathogens utilize a type III secretion (T3S) system to directly deliver effector molecules into host eukaryotic cells to manipulate cellular processes. These surface-exposed syringe-like structures are highly conserved, necessary for pathogenesis, and hence are therapeutic targets against a number of Gram-negative pathogens. Here we describe a protocol for using purified needle proteins to immunize mice, and subsequently, ways to characterize the immune response to immunization.

Published

2017

30. A Method for Characterizing the Type III Secretion System's Contribution to Pathogenesis: Homologous Recombination to Generate Yersinia pestis Type III Secretion System Mutants.

Author

Osei-Owusu P, Nilles ML, Bradley DS, and Alvine TD

Subjects

Animals, Bacterial Proteins genetics, Bacterial Proteins metabolism, Blotting, Western, Disease Models, Animal, Electrophoresis, Polyacrylamide Gel, Female, HeLa Cells, Homologous Recombination, Humans, Mice, Mutation, Plague microbiology, Protein Transport, Yersinia pestis pathogenicity, Type III Secretion Systems genetics, Type III Secretion Systems metabolism, Yersinia pestis genetics, Yersinia pestis metabolism

Abstract

The type III (T3S) secretion system of many gram-negative bacteria is a surface-exposed protein secretion apparatus used to directly inject bacterial effector molecules into eukaryotic cells. These effector molecules contribute to bacterial pathogenesis in many ways, and have been shown to be crucial for infectivity. Here, we describe a protocol for using homologous recombination to generate T3S system mutants to assess the role of different T3S system proteins in bacterial pathogenesis.

Published

2017

31. Introduction to Type III Secretion Systems.

Author

Condry DL and Nilles ML

Subjects

Animals, Gram-Negative Bacterial Infections diagnosis, Gram-Negative Bacterial Infections transmission, Humans, Plants microbiology, Virulence Factors genetics, Virulence Factors metabolism, Gram-Negative Bacteria physiology, Gram-Negative Bacterial Infections microbiology, Host-Pathogen Interactions, Type III Secretion Systems physiology

Abstract

Type III secretion (T3S) systems are found in a large number of gram-negative bacteria where they function to manipulate the biology of infected hosts. Hosts targeted by T3S systems are widely distributed in nature and are represented by animals and plants. T3S systems are found in diverse genera of bacteria and they share a common core structure and function. Effector proteins are delivered by T3S systems into targeted host cells without prior secretion of the effectors into the environment. Instead, an assembled translocon structure functions to translocate effectors across eukaryotic cell membranes. In many cases, T3S systems are essential virulence factors and in some instances they promote symbiotic interactions.

Published

2017

32. Expression and Purification of N-Terminally His-Tagged Recombinant Type III Secretion Proteins.

Author

Alvine TD, Osei-Owusu P, Condry DL, and Nilles ML

Subjects

Chromatography, Cloning, Molecular, Polymerase Chain Reaction, Transformation, Bacterial, Bacterial Proteins genetics, Bacterial Proteins isolation & purification, Recombinant Fusion Proteins, Type III Secretion Systems genetics

Abstract

The ability to express and purify recombinant needle proteins from the Type III Secretion System (T3SS) of many gram-negative bacteria has allowed us to develop novel experimental approaches, both in vitro and in vivo, to identify unique roles for T3SS in bacterial pathogenesis. In addition, these purified needle proteins have shown to be promising immunotherapies acting as both protective antigens and adjuvants, presumably due to their immune activating properties. Here, we describe the expression and purification of recombinant T3SS needle proteins.

Published

2017

33. The N terminus of type III secretion needle protein YscF from Yersinia pestis functions to modulate innate immune responses.

Author

Osei-Owusu P, Jessen Condry DL, Toosky M, Roughead W, Bradley DS, and Nilles ML

Subjects

Amino Acid Sequence, Bacterial Proteins pharmacology, Bacterial Secretion Systems immunology, Cell Line, Cytokines biosynthesis, HeLa Cells, Humans, Immune Evasion genetics, Inflammation immunology, Membrane Proteins genetics, Membrane Proteins metabolism, Monocytes immunology, NF-kappa B metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins pharmacology, Salmonella enterica genetics, Salmonella enterica immunology, Salmonella enterica pathogenicity, Sequence Alignment, Sequence Deletion genetics, Signal Transduction immunology, Transcription Factor AP-1 metabolism, Yersinia pestis genetics, Yersinia pestis immunology, Yersinia pestis pathogenicity, Bacterial Proteins genetics, Bacterial Proteins immunology, Cytokines metabolism, Membrane Proteins immunology, Recombinant Fusion Proteins immunology

Abstract

The type III secretion system is employed by many pathogens, including the genera Yersinia, Shigella, Pseudomonas, and Salmonella, to deliver effector proteins into eukaryotic cells. The injectisome needle is formed by the polymerization of a single protein, e.g., YscF (Yersinia pestis), PscF (Pseudomonas aeruginosa), PrgI (Salmonella enterica SPI-1), SsaG (Salmonella enterica SPI-2), or MxiH (Shigella flexneri). In this study, we demonstrated that the N termini of some needle proteins, particularly the N terminus of YscF from Yersinia pestis, influences host immune responses. The N termini of several needle proteins were truncated and tested for the ability to induce inflammatory responses in a human monocytic cell line (THP-1 cells). Truncated needle proteins induced proinflammatory cytokines to different magnitudes than the corresponding wild-type proteins, except SsaG. Notably, N-terminally truncated YscF induced significantly higher activation of NF-κB and/or AP-1 and higher induction of proinflammatory cytokines, suggesting that a function of the N terminus of YscF is interference with host sensing of YscF, consistent with Y. pestis pathogenesis. To directly test the ability of the N terminus of YscF to suppress cytokine induction, a YscF-SsaG chimera with 15 N-terminal amino acids from YscF added to SsaG was constructed. The chimeric YscF-SsaG induced lower levels of cytokines than wild-type SsaG. However, the addition of 15 random amino acids to SsaG had no effect on NF-κB/AP-1 activation. These results suggest that the N terminus of YscF can function to decrease cytokine induction, perhaps contributing to a favorable immune environment leading to survival of Y. pestis within the eukaryotic host., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published

2015

34. Type III secretion needle proteins induce cell signaling and cytokine secretion via Toll-like receptors.

Author

Jessen DL, Osei-Owusu P, Toosky M, Roughead W, Bradley DS, and Nilles ML

Subjects

Escherichia coli physiology, HEK293 Cells, Humans, Signal Transduction immunology, Bacterial Secretion Systems physiology, Cytokines metabolism, Escherichia coli Proteins physiology, Membrane Proteins physiology, Signal Transduction physiology, Toll-Like Receptors physiology

Abstract

Pathogens are recognized by hosts by use of various receptors, including the Toll-like receptor (TLR) and Nod-like receptor (NLR) families. Ligands for these varied receptors, including bacterial products, are identified by the immune system, resulting in development of innate immune responses. Only a couple of components from type III secretion (T3S) systems are known to be recognized by TLR or NLR family members. Known T3S components that are detected by pattern recognition receptors (PRRs) are (i) flagellin, detected by TLR5 and NLRC4 (Ipaf); and (ii) T3S rod proteins (PrgJ and homologs) and needle proteins (PrgI and homologs), detected by NAIP and the NLRC4 inflammasome. In this report, we characterize the induction of proinflammatory responses through TLRs by the Yersinia pestis T3S needle protein, YscF, the Salmonella enterica needle proteins PrgI and SsaG, and the Shigella needle protein, MxiH. More specifically, we determine that the proinflammatory responses occur through TLR2 and -4. These data support the hypothesis that T3S needles have an unrecognized role in bacterial pathogenesis by modulating immune responses.

Published

2014

35. A type III secretion system inhibitor targets YopD while revealing differential regulation of secretion in calcium-blind mutants of Yersinia pestis.

Author

Jessen DL, Bradley DS, and Nilles ML

Subjects

Bacterial Outer Membrane Proteins genetics, Bacterial Outer Membrane Proteins metabolism, Bacterial Secretion Systems genetics, Biological Transport drug effects, Calcium metabolism, Mutation, Pseudomonas aeruginosa drug effects, Pseudomonas aeruginosa genetics, Pseudomonas aeruginosa metabolism, Yersinia pestis genetics, Yersinia pestis metabolism, Yersinia pseudotuberculosis drug effects, Yersinia pseudotuberculosis genetics, Yersinia pseudotuberculosis metabolism, Bacterial Outer Membrane Proteins antagonists & inhibitors, Bacterial Secretion Systems drug effects, Cresols pharmacology, Gene Expression Regulation, Bacterial, Yersinia pestis drug effects

Abstract

Numerous Gram-negative pathogens rely upon type III secretion (T3S) systems to cause disease. Several small-molecule inhibitors of the type III secretion systems have been identified; however, few targets of these inhibitors have been elucidated. Here we report that 2,2'-thiobis-(4-methylphenol) (compound D), inhibits type III secretion in Yersinia pestis, Yersinia pseudotuberculosis, and Pseudomonas aeruginosa. YopD, a protein involved in the formation of the translocon and regulatory processes of the type III secretion system, appears to play a role in the inhibition of secretion by compound D. The use of compound D in T3S regulatory mutants demonstrated a difference in secretion inhibition in the presence and absence of calcium. Interestingly, compound D was effective only under conditions without calcium, indicating that a secretion-active needle structure may be necessary for compound D to inhibit secretion.

Published

2014

36. Resistance to Yersinia pestis infection decreases with age in B10.T(6R) mice.

Author

Lambert ND, Langfitt DM, Nilles ML, and Bradley DS

Subjects

Animals, Chemokines genetics, Chemokines metabolism, Female, Gene Expression Regulation immunology, Granuloma microbiology, Granuloma pathology, Interleukin-6 genetics, Interleukin-6 metabolism, Male, Mice, Mice, Inbred Strains, Spleen pathology, Stem Cells, Time Factors, Aging immunology, Disease Susceptibility immunology, Plague immunology, Yersinia pestis immunology

Abstract

We demonstrate that 2-month-old female B10.T(6R) mice are highly resistant to systemic infection with the KIM5 strain of Yersinia pestis and that B10.T(6R) mice become susceptible to Y. pestis infection by the age of 5 months. In this study, young (2-month-old) and middle-aged (5- to 12-month-old) B10.T(6R) mice were infected with equal CFU counts of Y. pestis. The 50% lethal dose (LD(50)) for young B10.T(6R) mice was ∼1.4 × 10(4) CFU, while middle-aged B10.T(6R) mice exhibited an LD(50) of ∼60 CFU. Elevated bacterial burdens were found in the spleens of middle-aged mice at 24 and 60 h and in the livers at 60 h postinfection. Immune cell infiltration was greater in the livers of resistant young mice than in those of middle-aged mice and mice of the susceptible C57BL/6N strain. Unlike susceptible mice, young B10.T(6R) mice did not develop necrotic lesions throughout the liver. Instead, livers from young B10.T(6R) mice contained granuloma-like structures. Immunohistochemical staining of liver sections from these mice at 60 h postinfection revealed that the majority of immune cells present in these structures were neutrophils. These findings suggest that resistance to plague in B10.T(6R) mice correlates with early formation of neutrophilic lesions in the liver.

Published

2011

37. Resistance of Yersinia pestis to complement-dependent killing is mediated by the Ail outer membrane protein.

Author

Bartra SS, Styer KL, O'Bryant DM, Nilles ML, Hinnebusch BJ, Aballay A, and Plano GV

Subjects

Animals, Bacterial Outer Membrane Proteins biosynthesis, Bacterial Outer Membrane Proteins genetics, Caenorhabditis elegans microbiology, Escherichia coli genetics, Escherichia coli immunology, Escherichia coli Infections, Female, Gene Deletion, Gene Expression, Mice microbiology, Microbial Viability, Siphonaptera microbiology, Survival Analysis, Temperature, Virulence Factors biosynthesis, Virulence Factors genetics, Yersinia pestis genetics, Bacterial Outer Membrane Proteins physiology, Complement System Proteins immunology, Virulence Factors physiology, Yersinia pestis immunology, Yersinia pestis pathogenicity

Abstract

Yersinia pestis, the causative agent of plague, must survive in blood in order to cause disease and to be transmitted from host to host by fleas. Members of the Ail/Lom family of outer membrane proteins provide protection from complement-dependent killing for a number of pathogenic bacteria. The Y. pestis KIM genome is predicted to encode four Ail/Lom family proteins. Y. pestis mutants specifically deficient in expression of each of these proteins were constructed using lambda Red-mediated recombination. The Ail outer membrane protein was essential for Y. pestis to resist complement-mediated killing at 26 and 37 degrees C. Ail was expressed at high levels at both 26 and 37 degrees C, but not at 6 degrees C. Expression of Ail in Escherichia coli provided protection from the bactericidal activity of complement. High-level expression of the three other Y. pestis Ail/Lom family proteins (the y1682, y2034, and y2446 proteins) provided no protection against complement-mediated bacterial killing. A Y. pestis ail deletion mutant was rapidly killed by sera obtained from all mammals tested except mouse serum. The role of Ail in infection of mice, Caenorhabditis elegans, and fleas was investigated.

Published

2008

38. Roles of YopN, LcrG and LcrV in controlling Yops secretion by Yersinia pestis.

Author

Hamad MA and Nilles ML

Subjects

Animals, Antigens, Bacterial genetics, Bacterial Proteins genetics, Genes, Bacterial, Humans, Membrane Proteins genetics, Models, Biological, Mutation, Pore Forming Cytotoxic Proteins genetics, Quorum Sensing, Signal Transduction, Yersinia pestis genetics, Yersinia pestis pathogenicity, Antigens, Bacterial physiology, Bacterial Proteins physiology, Membrane Proteins physiology, Pore Forming Cytotoxic Proteins physiology, Yersinia pestis physiology

Abstract

Control of Yops secretion in pathogenic Yersinia is achieved at several levels. These levels likely include transcriptional, post-transcriptional, translational and secretional controls. Secretion control appears to be mediated by two pathways. One pathway involves YopN and proteins that interact with YopN. The second pathway consists of LcrG and its interaction with LcrV. LcrV is a postive regulator of Yops secretion that exerts control over Yops secretion by negating the secretion blocking role of LcrG. However, the intersection of these two control pathways is not understood. Recent work has allowed the development of a speculative model that brings YopN-mediated and LcrG-LcrV-mediated control together in the context of the ability of the needle complex to respond to Ca2+.

Published

2007

39. Genome sequence of Yersinia pestis KIM.

Author

Deng W, Burland V, Plunkett G 3rd, Boutin A, Mayhew GF, Liss P, Perna NT, Rose DJ, Mau B, Zhou S, Schwartz DC, Fetherston JD, Lindler LE, Brubaker RR, Plano GV, Straley SC, McDonough KA, Nilles ML, Matson JS, Blattner FR, and Perry RD

Subjects

Bacteriophages, Biological Transport genetics, Bodily Secretions, Chemotaxis genetics, DNA Replication genetics, DNA Transposable Elements genetics, Energy Metabolism genetics, Escherichia coli genetics, Gene Expression Regulation, Bacterial, Genes, rRNA genetics, Operon genetics, Plasmids genetics, Protein Biosynthesis genetics, Repetitive Sequences, Nucleic Acid, Virulence, Yersinia pestis metabolism, Yersinia pestis pathogenicity, Genome, Bacterial, Yersinia pestis genetics

Abstract

We present the complete genome sequence of Yersinia pestis KIM, the etiologic agent of bubonic and pneumonic plague. The strain KIM, biovar Mediaevalis, is associated with the second pandemic, including the Black Death. The 4.6-Mb genome encodes 4,198 open reading frames (ORFs). The origin, terminus, and most genes encoding DNA replication proteins are similar to those of Escherichia coli K-12. The KIM genome sequence was compared with that of Y. pestis CO92, biovar Orientalis, revealing homologous sequences but a remarkable amount of genome rearrangement for strains so closely related. The differences appear to result from multiple inversions of genome segments at insertion sequences, in a manner consistent with present knowledge of replication and recombination. There are few differences attributable to horizontal transfer. The KIM and E. coli K-12 genome proteins were also compared, exposing surprising amounts of locally colinear "backbone," or synteny, that is not discernible at the nucleotide level. Nearly 54% of KIM ORFs are significantly similar to K-12 proteins, with conserved housekeeping functions. However, a number of E. coli pathways and transport systems and at least one global regulator were not found, reflecting differences in lifestyle between them. In KIM-specific islands, new genes encode candidate pathogenicity proteins, including iron transport systems, putative adhesins, toxins, and fimbriae.

Published

2002