2JWU

Solution NMR structures of two designed proteins with 88% sequence identity but different fold and function

PDB DOI: https://doi.org/10.2210/pdb2JWU/pdb
BMRB: 15537

Classification: DE NOVO PROTEIN
Organism(s): synthetic construct
Expression System: Escherichia coli BL21(DE3)
Mutation(s): No

Deposited: 2007-10-25 Released: 2008-09-09
Deposition Author(s): He, Y., Chen, Y., Alexander, P., Bryan, P., Orban, J.

Experimental Data Snapshot

Method: SOLUTION NMR
Conformers Calculated: 250
Conformers Submitted: 20
Selection Criteria: structures with acceptable covalent geometry

wwPDB Validation 3D Report Full Report

This is version 1.2 of the entry. See complete history.

Literature

NMR structures of two designed proteins with high sequence identity but different fold and function

He, Y., Chen, Y., Alexander, P., Bryan, P.N., Orban, J.

(2008) Proc Natl Acad Sci U S A 105: 14412-14417

PubMed: 18796611 Search on PubMedSearch on PubMed Central
DOI: https://doi.org/10.1073/pnas.0805857105
Primary Citation of Related Structures:
2JWS, 2JWU

PubMed Abstract:
How protein sequence codes for 3D structure remains a fundamental question in biology. One approach to understanding the folding code is to design a pair of proteins with maximal sequence identity but retaining different folds. Therefore, the nonidentities must be responsible for determining which fold topology prevails and constitute a fold-specific folding code. We recently designed two proteins, G(A)88 and G(B)88, with 88% sequence identity but different folds and functions [Alexander et al. (2007) Proc Natl Acad Sci USA 104:11963-11968]. Here, we describe the detailed 3D structures of these proteins determined in solution by NMR spectroscopy. Despite a large number of mutations taking the sequence identity level from 16 to 88%, G(A)88 and G(B)88 maintain their distinct wild-type 3-alpha and alpha/beta folds, respectively. To our knowledge, the 3D-structure determination of two monomeric proteins with such high sequence identity but different fold topology is unprecedented. The geometries of the seven nonidentical residues (of 56 total) provide insights into the structural basis for switching between 3-alpha and alpha/beta conformations. Further mutation of a subset of these nonidentities, guided by the G(A)88 and G(B)88 structures, leads to proteins with even higher levels of sequence identity (95%) and different folds. Thus, conformational switching to an alternative monomeric fold of comparable stability can be effected with just a handful of mutations in a small protein. This result has implications for understanding not only the folding code but also the evolution of new folds.

Organizational Affiliation

Center for Advanced Research in Biotechnology, University of Maryland Biotechnology Institute, 9600 Gudelsky Drive, Rockville, MD 20850, USA.

Macromolecule Content

Total Structure Weight: 6.46 kDa
Atom Count: 456
Modelled Residue Count: 56
Deposited Residue Count: 56
Unique protein chains: 1

Macromolecules

Find similar proteins by:

(by identity cutoff) | 3D Structure

Entity ID: 1
Molecule	Chains	Sequence Length	Organism	Details	Image
Gb88	A	56	synthetic construct	Mutation(s): 0
Entity Groups
Sequence Clusters	30% Identity50% Identity70% Identity90% Identity95% Identity100% Identity
Sequence Annotations Expand
Reference Sequence

Experimental Data & Validation

Experimental Data

Method: SOLUTION NMR
Conformers Calculated: 250
Conformers Submitted: 20
Selection Criteria: structures with acceptable covalent geometry

Structure Validation

View Full Validation Report

Entry History

Deposition Data

Released Date: 2008-09-09

Deposition Author(s):

Revision History (Full details and data files)

Version 1.0: 2008-09-09
Type: Initial release
Version 1.1: 2011-07-13
Changes: Version format compliance
Version 1.2: 2020-02-19
Changes: Data collection, Database references, Derived calculations, Other, Source and taxonomy