Biological membranes surround all cells and mediate their interactions with the outside world. Depending on the biological context, membrane proteins act as receptors, enzymes, channels, transporters, structural proteins and cell adhesion molecules and, as such, contribute to a wide variety of essential cellular functions. Structural information for membrane proteins is relatively scarce, despite the fact that they represent the target of 60% of therapeutic drugs sold in the United States. We propose to establish a pipeline for determining membrane protein structures by electron crystallography, which is the application of cryo-electron microscopy to two-dimensional crystals. To prepare such crystals, the membrane bilayer is reconstituted with a high density of purified membrane proteins, thus providing a native membrane environment and fewer crystallization constraints for the constituent proteins. Electron crystallography has an established track record in producing structures at both atomic and intermediate resolutions and represents a valuable alternative to X-ray crystallography and NMR spectroscopy, which are generally constrained to studying detergent-solubilized species. To date, electron crystallography remains a low-throughput operation, which has significantly reduced its contribution to membrane protein biology. We have developed some tools to overcome the bottlenecks in screening crystallization conditions, which we seek to expand in the current application. Specifically, we propose further developments for crystallization on a 96-well format by implementing a microfluidic device for dialysis that minimizes sample volumes and by using cyclodextrins to control detergent removal rates in an effort to optimize crystal quality. By studying a wide range of different target proteins, we will empirically establish factors that are most critical to influencing the crystallization process and develop a set of conditions that are generally effective for screening new proteins with unknown crystallization behaviors. We will continue developing our methods for robotic imaging of crystallization screens. The process of preparing samples and imaging them within the electron microscope currently represents the most significant bottleneck limiting the number of conditions that can be explored. We have built a robot for sample insertion and have interfaced it with automated image acquisition software, but we propose to add shape recognition to this software to maximize its efficiency. We will integrate the resulting images within an established LIMS database for keeping track of the structure determination pipeline and will implement shape recognition to enable automated assignment of scores to crystallization trials. Finally, we propose to develop an application for high resolution data collection from well-ordered crystals, thus facilitating the optimization of crystal size and order and, ultimately, acquisition of the data required for structure determination. We are convinced that by applying high- throughput methods to 2D crystallization and image acquisition, electron crystallography can make a substantial contribution to our understanding of membrane protein biology.

Public Health Relevance

Membranes surround all cells and proteins within these membrane mediate the flow ofinformation and materials. As a result; membrane proteins are implicated in manydiseases. Structural information about these proteins is critical to understanding thebiology behind the disease and for designing drugs to ameliorate the problems.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
7R01GM095747-05
Application #
8991232
Study Section
Special Emphasis Panel (ZRG1-BCMB-S (50))
Program Officer
Chin, Jean
Project Start
2010-09-30
Project End
2015-07-31
Budget Start
2015-01-01
Budget End
2015-07-31
Support Year
5
Fiscal Year
2013
Total Cost
$90,652
Indirect Cost
$37,170
Name
New York University
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
121911077
City
New York
State
NY
Country
United States
Zip Code
10016
Lopez-Redondo, Maria Luisa; Coudray, Nicolas; Zhang, Zhening et al. (2018) Structural basis for the alternating access mechanism of the cation diffusion facilitator YiiP. Proc Natl Acad Sci U S A 115:3042-3047
Coudray, Nicolas; L Seyler, Sean; Lasala, Ralph et al. (2017) Structure of the SLC4 transporter Bor1p in an inward-facing conformation. Protein Sci 26:130-145
Coudray, Nicolas; Lasala, Ralph; Zhang, Zhening et al. (2016) Deducing the symmetry of helical assemblies: Applications to membrane proteins. J Struct Biol 195:167-178
Lasala, R; Coudray, N; Abdine, A et al. (2015) Sparse and incomplete factorial matrices to screen membrane protein 2D crystallization. J Struct Biol 189:123-34
Stokes, David L; Ubarretxena-Belandia, Iban; Gonen, Tamir et al. (2013) High-throughput methods for electron crystallography. Methods Mol Biol 955:273-96
Allen, Gregory S; Stokes, David L (2013) Modeling, docking, and fitting of atomic structures to 3D maps from cryo-electron microscopy. Methods Mol Biol 955:229-41
Coudray, Nicolas; Valvo, Salvatore; Hu, Minghui et al. (2013) Inward-facing conformation of the zinc transporter YiiP revealed by cryoelectron microscopy. Proc Natl Acad Sci U S A 110:2140-5
Ubarretxena-Belandia, Iban; Stokes, David L (2012) Membrane protein structure determination by electron crystallography. Curr Opin Struct Biol 22:520-8
Stokes, David L; Rice, William J; Hu, Minghui et al. (2010) Two-dimensional crystallization of integral membrane proteins for electron crystallography. Methods Mol Biol 654:187-205
Kim, Changki; Vink, Martin; Hu, Minghui et al. (2010) An automated pipeline to screen membrane protein 2D crystallization. J Struct Funct Genomics 11:155-66

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