Database of articles cited by EMDB/PDB/SASBDB data

Keywords
Structure methods	All X-ray diffraction NMR electron microscopy small angle scattering neutron diffraction fiber diffraction powder diffraction infrared spectroscopy EPR fluorescence transfer theoretical model Hybrid
Author
Journal
IF	>30 >20 >10 >5 all

Title	Near-atomic cryo-EM imaging of a small protein displayed on a designed scaffolding system.
Journal, issue, pages	Proc Natl Acad Sci U S A, Vol. 115, Issue 13, Page 3362-3367, Year 2018
Publish date	Mar 27, 2018
Authors	Yuxi Liu / Shane Gonen / Tamir Gonen / Todd O Yeates /
PubMed Abstract	Current single-particle cryo-electron microscopy (cryo-EM) techniques can produce images of large protein assemblies and macromolecular complexes at atomic level detail without the need for crystal ...Current single-particle cryo-electron microscopy (cryo-EM) techniques can produce images of large protein assemblies and macromolecular complexes at atomic level detail without the need for crystal growth. However, proteins of smaller size, typical of those found throughout the cell, are not presently amenable to detailed structural elucidation by cryo-EM. Here we use protein design to create a modular, symmetrical scaffolding system to make protein molecules of typical size suitable for cryo-EM. Using a rigid continuous alpha helical linker, we connect a small 17-kDa protein (DARPin) to a protein subunit that was designed to self-assemble into a cage with cubic symmetry. We show that the resulting construct is amenable to structural analysis by single-particle cryo-EM, allowing us to identify and solve the structure of the attached small protein at near-atomic detail, ranging from 3.5- to 5-Å resolution. The result demonstrates that proteins considerably smaller than the theoretical limit of 50 kDa for cryo-EM can be visualized clearly when arrayed in a rigid fashion on a symmetric designed protein scaffold. Furthermore, because the amino acid sequence of a DARPin can be chosen to confer tight binding to various other protein or nucleic acid molecules, the system provides a future route for imaging diverse macromolecules, potentially broadening the application of cryo-EM to proteins of typical size in the cell.
External links	Proc Natl Acad Sci U S A / PubMed:29507202 / PubMed Central
Methods	EM (single particle)
Resolution	3.09 - 4.03 Å
Structure data	EMDB-7403: Single-particle reconstruction of DARP14 - A designed protein scaffold displaying ~17kDa DARPin proteins - Helical extension Method: EM (single particle) / Resolution: 4.03 Å 7436 6c9i EMDB-7436, PDB-6c9i: Single-Particle reconstruction of DARP14 - A designed protein scaffold displaying ~17kDa DARPin proteins - Scaffold Method: EM (single particle) / Resolution: 3.09 Å 7437 6c9k EMDB-7437, PDB-6c9k: Single-Particle reconstruction of DARP14 - A designed protein scaffold displaying ~17kDa DARPin proteins Method: EM (single particle) / Resolution: 3.49 Å
Source	synthetic construct (others) Pyrococcus horikoshii OT3 (archaea) Pseudomonas aeruginosa PAO1 (bacteria) pyrococcus horikoshii (strain atcc 700860 / dsm 12428 / jcm 9974 / nbrc 100139 / ot-3) (archaea) pseudomonas aeruginosa (strain atcc 15692 / dsm 22644 / cip 104116 / jcm 14847 / lmg 12228 / 1c / prs 101 / pao1) (bacteria) synthetic (others)
Keywords	DE NOVO PROTEIN / Designed Complex / DARPin / Scaffold / Single-Particle Cryo-EM