Crystallization of recombinant Bacteroides fragilis glutamine synthetase (GlnN) isolated using a novel and rapid purification protocol

Journal Article

2010

Permanent link to this Item
http://hdl.handle.net/11427/20674
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van_Rooyen_Crystallization_2010.pdf (744.36 KB)
Authors
van Rooyen, J M
Abratt, V R
Belrhali, H
Sewell, B T
Journal Title

Protein Expression and Purification

Link to Journal
http://www.journals.elsevier.com/protein-expression-and-purification
Journal ISSN
Volume Title
Publisher

Elsevier

Publisher

University of Cape Town

License

https://creativecommons.org/licenses/by-nc-nd/4.0/

Series
Abstract
Glutamine synthetase enzymes (GSs) are large oligomeric enzymes that play a critical role in nitrogen metabolism in all forms of life. To date, no crystal structures exist for the family of large (1 MDa) type III GS enzymes, which only share 9% sequence identity with the well characterized GSI and GSII enzymes. Here we present a novel protocol for the isolation of untagged Bacteroides fragilis GlnN expressed in an auxotrophic Escherichia coli strain. The rapid and scalable two-step protocol utilized differential precipitation by divalent cations followed by affinity chromatography to produce suitable quantities of homogenous material for structural characterization. Subsequent optimizations to the sample stability and solubility led to the discovery of conditions for the production of the first diffraction quality crystals of a type III GS enzyme.
Description
Keywords
Glutamine synthetase type III GSIII Structure Bacteroides fragilis X-ray crystallography Protein pur

Reference:

Van Rooyen, J. M., Abratt, V. R., Belrhali, H., & Sewell, B. T. (2010). Crystallization of recombinant Bacteroides fragilis glutamine synthetase (GlnN) isolated using a novel and rapid purification protocol. Protein expression and purification, 74(2), 211-216.

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