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Abstract

Grant Number: 1R01GM081817-01

Project Title: Membrane Protein Structure by Electron Crystallography

PI Information: Name Email Title

STOKES, DAVID L. stokes@nyu.edu ASSOCIATE PROFESSOR

Abstract: DESCRIPTION (provided by applicant): The overall goal of this proposal is to promote structure determination of integral membrane proteins by cryoelectron microscopy (cryo-EM) of 2D crystals. Membrane proteins are essential to all cells and favored drug targets, yet their 3D structures have proven difficult to ascertain. Cryo-EM has a demonstrated capability for structure determination at atomic resolution and the important advantage of maintaining integral membrane proteins within their native membrane environment. Nevertheless, the proliferation of high- throughput screening for 3D crystallization trials has given a distinct advantage to X-ray crystallography. We propose to implement analogous technologies for screening 2D crystallization trials of integral membrane proteins within lipid bilayers in order to reestablish cryo-EM as a viable alternative in the high-throughput, post-genomic era. We will form a partnership with the New York Consortium on Membrane Protein Structure (NYCOMPS), which is a Specialized Center of the NIH Protein Structure Initiative operating out of the New York Structural Biology Center. NYCOMPS will provide requested expression vectors from a large database of membrane proteins that they are screening for expression levels and homogeneity. After scaling up expression, we will use a robotic liquid handler to set up 2D crystallization trials by dialysis and prepare EM samples by negative stain in a 96-well format. Imaging currently represents a critical bottleneck for screening 2D crystal trials and we will implement technologies to automatically acquire images from these samples in the electron microscope. Thus, we expect to assess -50 different protein targets per year. The resulting information will be used to establish general principles governing the 2D crystallization process and, importantly, to produce 2D crystals that are suitable for structure determination at atomic resolution. Given a workable method to systematically search for and optimize 2D crystals, cryo-EM will become generally viable for high resolution structure determination and offer an important alternative to X-ray crystallography and NMR spectroscopy. In particular, the modest requirements for quantity and purity of proteins, as well as the natural environment provided by the lipid membrane, make cryo-EM an attractive alternative, especially as we move from bacterial proteomes towards large membrane protein complexes from eukaryotic cells that have proven more difficult to express and to maintain in a detergent solubilized state.
Public Health Relevance:
This Public Health Relevance is not available.
Thesaurus Terms:
cryoelectron microscopy, membrane protein, protein structure, structural biology, technology /technique development
NIH Roadmap Initiative tag

Institution: NEW YORK STRUCTURAL BIOLOGY CENTER

89 CONVENT AVE

NEW YORK, NY 10027

Fiscal Year: 2007

Department:

Project Start: 21-SEP-2007

Project End: 31-JUL-2010

ICD: NATIONAL INSTITUTE OF GENERAL MEDICAL SCIENCES

IRG: ZRG1

Grant Number:	1R01GM081817-01
Project Title:	Membrane Protein Structure by Electron Crystallography

PI Information:	Name	Email	Title
	STOKES, DAVID L.	stokes@nyu.edu	ASSOCIATE PROFESSOR

Institution:	NEW YORK STRUCTURAL BIOLOGY CENTER
	89 CONVENT AVE
	NEW YORK, NY 10027
Fiscal Year:	2007
Department:
Project Start:	21-SEP-2007
Project End:	31-JUL-2010
ICD:	NATIONAL INSTITUTE OF GENERAL MEDICAL SCIENCES
IRG:	ZRG1