The Composite Protocol Text: An Effective Strengthening of the Biological and Toxin Weapons Convention

Pearson, Graham S., Dando, Malcolm R., Sims, N.A.

January 2001

Yes

BTWC

Biological and Toxin Weapons Convention

Protocol

Towards a New Implementation Mechanism for the BTWC

Pearson, Graham S.

January 2007

No description available.

BTWC

Biological and Toxin Weapons Convention

Implementation Mechanism

2001 Review Conference: The Future - What can be done?

Sims, N.A., Whitby, Simon M.

January 2001

Yes / In this final Review Conference Video Nicholas A. Sims describes strategies that both governmenal and non-governmental groups might adopt prior to the reconveneing of the Review Conference process in November 2002.

BTWC

Biological and Toxin Weapons Convention

Review Conference

The BTWC: An Evolving Regime

Sims, N.A., Whitby, Simon M.

January 2001

Yes / In this video Nicholas A. Sims describes the way in which the BTWC treaty regimes has evolved since its entry into force in 1975.

BTWC

Biological and Toxin Weapons Convention

Regime

Developments

ASSEMBLY AND SECRETION OF PERTUSSIS TOXIN BY <i>BORDETELLA PERTUSSIS</i>

RAMBOW-LARSEN, AMY ALISON

January 2003

No description available.

Biology, Microbiology

pertussis

toxin

secretion

bacteria

pathogen

Synthesis of Multivalent Glycoconjugates for the Detection of Pathogens

Vermillion, Rebecca Marie

02 October 2006

No description available.

Chemistry, Organic

influenza

botulinum toxin

carbohydrate

sensor

ANTHRAX TOXIN: IMMUNITY AND RECEPTOR ACTIVITY

TAFT, SARAH C.

January 2007

No description available.

Biology, Microbiology

Bacillus anthracis

anthrax toxin

AVA

Characterization and Molecular Analysis of Fragilysin: The Bacteroides fragilis Toxin

Obiso, Richard J. Jr.

05 June 1997

Bacteroides fragilis is a gram negative, anaerobic rod, that is a member of the normal colonic microflora of most mammals, and it is the anaerobe most commonly isolated from human soft tissue infections. During the past decade, strains of B. fragilis that produce an enterotoxin have been implicated as the cause of diarrhea in a number of animals, including humans. The extracellular enterotoxin has been purified and characterized as a single polypeptide (Mr~ 20,600) that causes rapid morphological changes in human colon carcinoma cell lines, particularly, HT-29. This dissertation research began in 1993 with the purpose of determining how this enterotoxin, termed fragilysin, causes diarrhea. The deduced amino acid sequence revealed a signature zinc binding consensus motif (His-Glu-Xx-Xxx-His-Xxx-Xxx-Gly-Xxx-Xxx-His/Met) characteristic of metalloproteinases. Sequence analysis showed close identity with metalloproteinases within the zinc-binding and Met-turn regions. Purified fragilysin contained 1 gram atom of zinc per molecule, and it hydrolyzed a number of proteins, including gelatin. Optimal proteolytic activity occurred at 37° C and pH 6.5. Activity was inhibited by metal chelators but not by inhibitors of other classes of proteinases. When fragilysin is injected into ligated ileal and colonic loops of animals, there is significant tissue damage and a subsequent dose dependent fluid response. Histological examination revealed mild necrosis of epithelial cells, crypt elongation, villus attenuation, and hyperplasia. There was extensive detachment and rounding of surface epithelial cells and an infiltration of neutrophils. Enterotoxic activity was inhibited by the metal chelators EDTA and 1,10-phenanthroline; and, to some degree, the enterotoxic activity could be reconstituted by the addition of zinc to chelated toxin. Fragilysin rapidly increased the permeability of the paracellular barrier of epithelial cells to ions (decrease in electrical resistance across monolayers) and to larger molecules (increase in mannitol flux across monolayers). Furthermore, there is a direct effect on the tight junction proteins. Fragilysin appears to cause diarrhea by proteolytically degrading the paracellular barrier of epithelial cells. Fragilysin is a recently discovered virulence factor that could contribute to the pathogenesis of B. fragilis in both intestinal and soft tissue infections. This research was supported by a Public Health Service grants AI 322940 and AI 32940-03 from the National Institute of Allergy and Infectious Diseases, and by the Commonwealth of Virginia project 6127250 / Ph. D.

Bacteroides fragilis

virulence

toxin

metalloproteinases

enterotoxin

Development of a targeted proteomic assay for rapid detection of Shiga-like toxins 1 and 2 in Shiga toxin-producing Escherichia coli

Scharikow, Leanne Gene

05 January 2017

Shiga toxin-producing Escherichia coli (STEC) are extensive contributors to foodborne illness, causing renal and central nervous system damage due to production of Shiga toxin (Stx). Rapid Stx detection is important to distinguish STEC from other enteric pathogens. Current detection techniques are time consuming, expensive, and lack sensitivity. We have developed and evaluated a novel targeted mass spectrometry-based assay for detection of Stx using parallel reaction monitoring (PRM). The PRM assay used 11 target tryptic peptides and was validated using STEC and non-STEC bacterial cultures. Stx was detected in 56 of 62 STEC isolates and did not detect Stx in any of the 29 non-STEC isolates. The PRM assay successfully determined the Stx2 subtype in 32 of 46 Stx2-positive isolates. By applying a targeted proteomics assay, we were able to simultaneously detect Stx toxins 1 and 2 and subtype Stx2 into six toxin subgroups in Stx2-positive isolates. / February 2017

Mass spectrometry

Targeted proteomics

Shiga toxin-producing Escherichia coli

Shiga toxin

Příprava a charakterizace rekombinantního adenylát cyklázového toxoidu bakterie Bordetella pertussis nesoucího mykobakteriální antigen TB7.7 / Construction and characterization of recombinant adenylate cyclase toxoid of bacterium Bordetella pertussis carrying mycobacterial antigen TB7.7

Mikulecký, Pavel

January 2010

Bacterium Mycobacterium tuberculosis is an etiological agent of a deadly disease called tuberculosis that presents a global problem. According to The World Health Organization there are more than 2 billions people infected with latent tuberculosis all over the world. There is still need of specific, sensitive, quick and economic available method for identification of infected individuals. Currently in vitro blood tests are considered to be the best way of diagnosis. They are based on restimulation of specific T lymphocytes by mycobacterial antigens derived from virulent strains. There are several different approaches for enhancing of direct antigen delivery into antigen presenting cells and promising one is a genetically detoxified adenylate cyclase toxin (CyaA) of bacteria Bordetella pertussis. The main aim of the thesis includes construction and subsequent characterization of biological properties of CyaA protein carrying specific mycobacterial antigen TB7.7 in translocating domain. Here is shown that fusion protein CyaA-TB7.7 can form cation selective pores in target cell membranes and is able to deliver antigens into the cytosol of APC to be presented on surface with molecules MHC class II. Genetically detoxified CyaA- TB7.7 protein will be used to supplement current approaches such as also in vitro...