Abstract

Remarkable progress in single cell genomics rests on the polymerase chain reaction. There is no analogous tool to probe the cell-to-cell distribution of protein diversity and posttranslational modification (PTM) patterns at the few- or single-cell level. If protein-capture arrays can be synthesized on a molecular scale, then the arrays themselves become reagents suitable for incubation with the contents of even a single cell. Molecular arrays could be used in titrations, giving a potentially enormous dynamic detection range and facilitating quantification of the protein content and PTMs for each generation of the progeny of a single parent cell. Nanotechnology already provides the components for such a system, and we propose to integrate four new technologies to develop self-assembled nanoarrays for protein analysis. The first is construction of an array of single molecule probes arranged at nanometer density using nucleic acid self-assembly. The arrays are themselves giant molecules and are used like a reagent in a solution analysis, only being deposited onto a surface for a final readout. The second is a nanoscale readout using atomic force microscopy (AFM).The AFM is capable of reading out >30,000 array sites per minute. The third is the development of new molecular recognition elements based on aptamers and multivalent aptamers for proteins and their PTM variants. Because aptamers are synthetic and also nucleic acid sequences, individual aptamers can bind to a unique position on the array through nucleic acid hybridization and require no printing or lithography. The fourth is microfluidic technology to allow the nanoarrays to interact with lysed or intact cells, and to deliver the reacted arrays to predefined locations for readout. Our goal is to fill a unique niche in proteomics: parallel analysis of minute amounts of protein from small numbers of (potentially individual) cells. Can we make suitable ligands and will they work on arrays? Can we read the arrays accurately with AFM? Can we synthesize ligands that are highly selective for posttranslational modifications? What factors cause biodegradation of the arrays, and how can we control them while maintaining sensitivity and selectivity? What conditions are required to exploit the arrays for proteomics in a microfluidic system? What methodologies can we employ to deposit nanoliter solutions of reacted arrays at precise locations for AFM readout? These questions are the focus of this proposal. If successful, this work will make it possible to correlate nucleic acid diversity with the corresponding protein PTM diversity on a cell-by- cell basis, yielding, for the first time, data on the interplay between genome, gene expression, the environment and the spectrum of protein posttranslational modifications: the 'protein language'.

Public Health Relevance

Probing the cell-to-cell distribution of protein diversity will provide critical information for understanding the development of living organisms and many diseases. Our goal is to develop a water soluble nanoarray system to open up to single-cell analysis the protein realm of the biochemical universe, uncovering new knowledge that will impact our understanding of how cells work and of how pathologies like cancer develop. This new technology will afford us a fuller view of the systems biology of the cell.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
1R01GM088818-01
Application #
7697954
Study Section
Enabling Bioanalytical and Biophysical Technologies Study Section (EBT)
Program Officer
Edmonds, Charles G
Project Start
2009-08-01
Project End
2014-05-31
Budget Start
2009-08-01
Budget End
2010-05-31
Support Year
1
Fiscal Year
2009
Total Cost
$306,553
Indirect Cost

  Institution

Name
Arizona State University-Tempe Campus
Department
Engineering (All Types)
Type
Organized Research Units
DUNS #
943360412
City
Tempe
State
AZ
Country
United States
Zip Code
85287

  Publications

Lan, Xiang; Su, Zhaoming; Zhou, Yadong et al. (2017) Programmable Supra-Assembly of a DNA Surface Adapter for Tunable Chiral Directional Self-Assembly of Gold Nanorods. Angew Chem Int Ed Engl 56:14632-14636
Yang, Yang; Han, Dongran; Nangreave, Jeanette et al. (2012) DNA origami with double-stranded DNA as a unified scaffold. ACS Nano 6:8209-15
Fu, Jinglin; Liu, Minghui; Liu, Yan et al. (2012) Interenzyme substrate diffusion for an enzyme cascade organized on spatially addressable DNA nanostructures. J Am Chem Soc 134:5516-9
Li, Zhe; Wang, Lei; Yan, Hao et al. (2012) Effect of DNA hairpin loops on the twist of planar DNA origami tiles. Langmuir 28:1959-65
Fu, Jinglin; Liu, Minghui; Liu, Yan et al. (2012) Spatially-interactive biomolecular networks organized by nucleic acid nanostructures. Acc Chem Res 45:1215-26
Torring, Thomas; Voigt, Niels V; Nangreave, Jeanette et al. (2011) DNA origami: a quantum leap for self-assembly of complex structures. Chem Soc Rev 40:5636-46
Pinheiro, Andre V; Han, Dongran; Shih, William M et al. (2011) Challenges and opportunities for structural DNA nanotechnology. Nat Nanotechnol 6:763-72
Deng, Zhengtao; Tong, Ling; Flores, Marco et al. (2011) High-quality manganese-doped zinc sulfide quantum rods with tunable dual-color and multiphoton emissions. J Am Chem Soc 133:5389-96
Nangreave, Jeanette; Yan, Hao; Liu, Yan (2011) DNA nanostructures as models for evaluating the role of enthalpy and entropy in polyvalent binding. J Am Chem Soc 133:4490-7
Zhao, Zhao; Liu, Yan; Yan, Hao (2011) Organizing DNA origami tiles into larger structures using preformed scaffold frames. Nano Lett 11:2997-3002

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