4.8 Article

Redefining Protein Interfaces within Protein Single Crystals with DNA

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY (2021)

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Journal

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
Volume 143, Issue 23, Pages 8925-8934

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/jacs.1c04191

Keywords

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Categories

Chemistry, Multidisciplinary

Funding

  1. Vannevar Bush Faculty Fellowship program - Basic Research Office of the Assistant Secretary of Defense for Research and Engineering
  2. Office of Naval Research [N00014-15-1-0043]
  3. Air Force Office of Scientific Research [FA9550-16-1-0150]
  4. National Science Foundation [DMR-2104353]
  5. DOE Office of Science [DE-AC02-06CH11357]
  6. Michigan Economic Development Corporation
  7. Michigan Technology Tri-Corridor [085P1000817]
  8. Soft and Hybrid Nanotechnology Experimental (SHyNE) Resource [NSF ECCS-2025633]
  9. State of Illinois
  10. International Institute for Nanotechnology (IIN)
  11. NCI CCSG [P30 CA060553]

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This study found that introducing DNA-DNA interactions can alter protein packing within single crystals, allowing for changes in crystal structures by manipulating DNA design. It enhances our understanding of how DNA can be used to program protein packing within ordered materials.
Proteins are exquisite nanoscale building blocks: molecularly pure, chemically addressable, and inherently selective for their evolved function. The organization of proteins into single crystals with high positional, orientational, and translational order results in materials where the location of every atom can be known. However, controlling the organization of proteins is challenging due to the myriad interactions that define protein interfaces within native single crystals. Recently, we discovered that introducing a single DNA-DNA interaction between protein surfaces leads to changes in the packing of proteins within single crystals and the protein-protein interactions (PPIs) that arise. However, modifying specific PPIs to effect deliberate changes to protein packing is an unmet challenge. In this work, we hypothesized that disrupting and replacing a highly conserved PPI with a DNA-DNA interaction would enable protein packing to be modulated by exploiting the programmability of the introduced oligonucleotides. Using concanavalin A (ConA) as a model protein, we circumvent potentially deleterious mutagenesis and exploit the selective binding of ConA toward mannose to noncovalently attach DNA to the protein surface. We show that DNA association eliminates the major PPI responsible for crystallization of native ConA, thereby allowing subtle changes to DNA design (length, complementarity, and attachment position) to program distinct changes to ConA packing, including the realization of three novel crystal structures and the deliberate expansion of ConA packing along a single crystallographic axis. These findings significantly enhance our understanding of how DNA can supersede native PPIs to program protein packing within ordered materials.

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