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Abstract

Grant Number: 1R21NS053740-01

Project Title: Inhibitors of Yersinia Yop Type III Secretion(RMI)

PI Information: Name Email Title

MECSAS, JOAN C. joan.mecsas@tufts.edu ASSISTANT PROFESSOR

Abstract: DESCRIPTION (provided by applicant): Pneumonic plague, caused by Yersinia pestis, is highly virulent and frequently causes lethal infection even when diagnosed correctly and antibiotics are given. One (1) of the key virulence features of Y. pestis is the type secretion system and the toxins, called Yops, that are translocated into mammalian cell cytoplasm by the type III secretion system. In mouse model systems of infection, the translocation of Yops is essential for productive infection of Yersinia in lungs. We have generated a reporter system in which Yop translocation signals of YopE are fused to a gene, b-lactamase, which encodes TEM. When TEM is delivered into mammalian cells, it cleaves a fluorescent substrate, CCF2, such that CCF2 emits light at a different wavelength. We can easily detect translocation of YopE-TEM fusion proteins by loading HEp-2 cells withCCF2-AM and detecting the 450 versus 520 emission spectrum of cells with by fluorescence microscopy. We propose to adapt this technology to use in a high through-put screen to identifying small molecular inhibitors of translocation of Yops. Ultimately, CCR-2 loaded HEp-2 cells will be infected with Yersinia strains expressing YopE-TEM fusion proteins in the presence of small molecules. The ratio of 460 versus 520 emissions will be read in a Fluorescence ELISA plate reader. Cells exposed to compounds which inhibit translocation should fluoresce at 520. These compounds will'be tested in several secondary screens to confirm that the compounds inhibit type III secretion and translocation processes. Such inhibitors should provide a novel class of therapeutics against pneumonic plague as well as other pathogens that use type III secretion systems to overcome host defenses, including other pathogens on the Priority pathogens list such as Salmonella, and Y. enterocolitica. Potentially these molecules could be used either prophylatically during an outbreak of pneumonic plague or after initial signs of infection are apparent. In addition, these inhibitors will be valuable tools to probe the structure and function of type III secretion systems encoded by Yersinia species and other Gram-negative bacterial pathogens.
Public Health Relevance:
This Public Health Relevance is not available.
Thesaurus Terms:
Yersinia pestis, bacterial protein, bacterial toxin, drug screening /evaluation, high throughput technology, inhibitor /antagonist, protein transport, technology /technique development
beta lactamase, chimeric protein, small molecule
biotechnology, enzyme linked immunosorbent assay, fluorescence microscopy

Institution: TUFTS UNIVERSITY BOSTON

Office of the Vice Provost

BOSTON, MA 02111

Fiscal Year: 2005

Department: MOLECULAR BIOLOGY AND MICROBIOLOGY

Project Start: 30-SEP-2005

Project End: 28-FEB-2007

ICD: NATIONAL INSTITUTE OF NEUROLOGICAL DISORDERS AND STROKE

IRG: ZNS1

Grant Number:	1R21NS053740-01
Project Title:	Inhibitors of Yersinia Yop Type III Secretion(RMI)

PI Information:	Name	Email	Title
	MECSAS, JOAN C.	joan.mecsas@tufts.edu	ASSISTANT PROFESSOR

Institution:	TUFTS UNIVERSITY BOSTON
	Office of the Vice Provost
	BOSTON, MA 02111
Fiscal Year:	2005
Department:	MOLECULAR BIOLOGY AND MICROBIOLOGY
Project Start:	30-SEP-2005
Project End:	28-FEB-2007
ICD:	NATIONAL INSTITUTE OF NEUROLOGICAL DISORDERS AND STROKE
IRG:	ZNS1