Shaun Healey
Verenium Corporation
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Featured researches published by Shaun Healey.
Applied and Environmental Microbiology | 2004
Yali Brennan; Walter Callen; Leif Christoffersen; Paul Dupree; Florence Goubet; Shaun Healey; Myrian Hernández; Martin S. Keller; Ke Li; Nisha Palackal; Ana Sittenfeld; Giselle Tamayo; Steve Wells; Geoffrey P. Hazlewood; Eric J. Mathur; Jay M. Short; Dan E. Robertson; Brian Steer
ABSTRACT Recombinant DNA technologies enable the direct isolation and expression of novel genes from biotopes containing complex consortia of uncultured microorganisms. In this study, genomic libraries were constructed from microbial DNA isolated from insect intestinal tracts from the orders Isoptera (termites) and Lepidoptera (moths). Using a targeted functional assay, these environmental DNA libraries were screened for genes that encode proteins with xylanase activity. Several novel xylanase enzymes with unusual primary sequences and novel domains of unknown function were discovered. Phylogenetic analysis demonstrated remarkable distance between the sequences of these enzymes and other known xylanases. Biochemical analysis confirmed that these enzymes are true xylanases, which catalyze the hydrolysis of a variety of substituted β-1,4-linked xylose oligomeric and polymeric substrates and produce unique hydrolysis products. From detailed polyacrylamide carbohydrate electrophoresis analysis of substrate cleavage patterns, the xylan polymer binding sites of these enzymes are proposed.
Protein Science | 2004
Nisha Palackal; Yali Brennan; Walter Callen; Paul Dupree; Gerhard Frey; Florence Goubet; Geoffrey P. Hazlewood; Shaun Healey; Young E. Kang; Keith Kretz; Edd Lee; Xuqiu Tan; Geoffery L. Tomlinson; John Verruto; Vicky W.K. Wong; Eric J. Mathur; Jay M. Short; Dan E. Robertson; Brian Steer
Directed evolution technologies were used to selectively improve the stability of an enzyme without compromising its catalytic activity. In particular, this article describes the tandem use of two evolution strategies to evolve a xylanase, rendering it tolerant to temperatures in excess of 90°C. A library of all possible 19 amino acid substitutions at each residue position was generated and screened for activity after a temperature challenge. Nine single amino acid residue changes were identified that enhanced thermostability. All 512 possible combinatorial variants of the nine mutations were then generated and screened for improved thermal tolerance under stringent conditions. The screen yielded eleven variants with substantially improved thermal tolerance. Denaturation temperature transition midpoints were increased from 61°C to as high as 96°C. The use of two evolution strategies in combination enabled the rapid discovery of the enzyme variant with the highest degree of fitness (greater thermal tolerance and activity relative to the wild‐type parent).
Archive | 2004
Brian Steer; Walter Callen; Shaun Healey; Derrick Pulliam
Archive | 2003
Brian Steer; Walter Callen; Shaun Healey; Geoff Hazlewood; Di Wu; David Blum; Alireza Esteghlalian
Archive | 2003
Brian Steer; Walter Callen; Shaun Healey; Geoff Hazlewood; Di Wu; David Blum; Alireza Esteghlalian
Archive | 2012
Justin T. Stege; Alexander Varvak; John Poland; Chris S. Lyon; Shaun Healey; Peter Luginbuhl
Archive | 2012
David Weiner; Alexander Varvak; Toby Richardson; Mircea Podar; Ellen Burke; Shaun Healey
Archive | 2007
Brian Steer; Shaun Healey; Alireza Esteghlalian; Stacy Marie Miles; Kenneth Barrett; Rene Quadt
Archive | 2011
Justin T. Stege; Alexander Varvak; John Poland; Chris S. Lyon; Shaun Healey; Peter Luginbuhl
Archive | 2011
Justin T. Stege; Alexander Varvak; John Poland; Chris S. Lyon; Shaun Healey; Peter Luginbuhl