Literature DB >> 21387408

Introduction of a disulfide bond leads to stabilization and crystallization of a ricin immunogen.

Jaimee R Compton1, Patricia M Legler, Benjamin V Clingan, Mark A Olson, Charles B Millard.   

Abstract

RTA1-33/44-198 is a catalytically inactive, single-domain derivative of the <span class="Gene">ricin toxin A-chain (RTA) engineered to serve as a stable protein scaffold for presentation of native immunogenic epitopes (Olson et al., Protein Eng Des Sel 2004;17:391-397). To improve the stability and solubility of RTA1-33/44-198 further, we have undertaken the design challenge of introducing a disulfide (SS) bond. Nine pairs of residues were selected for placement of the SS-bond based on molecular dynamics simulation studies of the modeled single-domain chain. Disulfide formation at either of two positions (R48C/T77C or V49C/E99C) involving a specific surface loop (44-55) increased the protein melting temperature by ~5°C compared with RTA1-33/44-198 and by ~13°C compared with RTA. Prolonged stability studies of the R48C/T77C variant (> 60 days at 37°C, pH 7.4) confirmed a > 40% reduction in self-aggregation compared with RTA1-33/44-198 lacking the SS-bond. The R48C/T77C variant retained affinity for anti-RTA antibodies capable of neutralizing ricin toxin, including a monoclonal that recognizes a human B-cell epitope. Introduction of either R48C/T77C or V49C/E99C promoted crystallization of RTA1-33/44-198, and the X-ray structures of the variants were solved to 2.3 A or 2.1 A resolution, respectively. The structures confirm formation of an intramolecular SS-bond, and reveal a single-domain fold that is significantly reduced in volume compared with RTA. Loop 44 to 55 is partly disordered as predicted by simulations, and is positioned to form self-self interactions between symmetry-related molecules. We discuss the importance of RTA loop 34 to 55 as a nucleus for unfolding and aggregation, and draw conclusions for ongoing structure-based minimalist design of RTA-based immunogens.
© 2011 Wiley-Liss, Inc

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Year:  2011        PMID: 21387408      PMCID: PMC3332088          DOI: 10.1002/prot.22933

Source DB:  PubMed          Journal:  Proteins        ISSN: 0887-3585


  55 in total

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4.  The geometry of the ribosomal polypeptide exit tunnel.

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5.  The crystallographically determined structures of atypical strained disulfides engineered into subtilisin.

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