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Dive into the research topics where Ar Clarke is active.

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Featured researches published by Ar Clarke.


Biochemical Society Transactions | 2007

Protein engineering applications of industrially exploitable enzymes: Geobacillus stearothermophilus LDH and Candida methylica FDH

Nevin Gül Karagüler; Richard B. Sessions; Barış Binay; Emel B. Ordu; Ar Clarke

Enzymes have become important tools in several industries due to their ability to produce chirally pure and complex molecules with interesting biological properties. The NAD(+)-dependent LDH (lactate dehydrogenase) [bsLDH [Geobacillus stearothermophilus (formerly Bacillus stearothermophilus) LDH] from G. stearothermophilus and the NAD(+)-dependent FDH (formate dehydrogenase) [cmFDH (Candida methylica FDH)] enzyme from C. methylica are particularly crucial enzymes in the pharmaceutical industry and are related to each other in terms of NADH use and regeneration. LDH catalyses the interconversion of pyruvate (oxo acid) and lactate (alpha-hydroxy acid) using the NADH/NAD(+) pair as a redox cofactor. Employing LDH to reduce other oxo acids can generate chirally pure alpha-hydroxy acids of use in the production of pharmaceuticals. One important use of FDH is to regenerate the relatively expensive NADH cofactor that is used by NAD(+)-dependent oxidoreductases such as LDH. Both LDH and FDH from organisms of interest were previously cloned and overproduced. Therefore they are available at a low cost. However, both of these enzymes show disadvantages in the large-scale production of chirally pure compounds. We have applied two routes of protein engineering studies to improve the properties of these two enzymes, namely DNA shuffling and site-directed mutagenesis. Altering the substrate specificity of bsLDH by DNA shuffling and changing the coenzyme specificity of cmFDH by site-directed mutagenesis are the most successful examples of our studies. The present paper will also include the details of these examples together with some other applications of protein engineering regarding these enzymes.


Biochemistry | 1999

EFFECTS OF CORE MUTATIONS ON THE FOLDING OF A BETA -SHEET PROTEIN : IMPLICATIONS FOR BACKBONE ORGANIZATION IN THE I-STATE

Mark Lorch; Jody M. Mason; Ar Clarke; Martin J. Parker


Protein Engineering | 1999

A general method for relieving substrate inhibition in lactate dehydrogenases

Co Hewitt; Cm Eszes; Richard B. Sessions; Kathleen M. Moreton; Tr Dafforn; Jiro Takei; Christopher E. Dempsey; Ar Clarke; J. John Holbrook


Journal of Physical Chemistry B | 2007

Absolute Free-Energy Calculations of Liquids Using a Harmonic Reference State

Tyka; Richard B. Sessions; Ar Clarke


Biochemistry | 1998

Self-Association of Disulfide-Dimerized Melittin Analogues†

Jiro Takei; Attila Reményi; Ar Clarke; Christopher E. Dempsey


Biochemistry | 2001

The A245K mutation exposes another stage of the bacterial L-lactate dehydrogenase reaction mechanism.

P Kedzierski; Kathleen M. Moreton; Ar Clarke; J. John Holbrook


American Chemical Society | 1992

Crystal City, VA, USA

Hm Wilks; Kathleen M. Moreton; Kw Hart; Jl Gelpi; Guy Casy; Richard B Sessions; Ar Clarke; J. John Holbrook


Archive | 2000

VIIth DBMS/IBS Workshop, from the structure and function to the design of modular proteins. Autrans, France, January

Ja Dando; Richard B Sessions; Mv Hayes; Ar Clarke; R L Brady


Archive | 2000

Dynamic assembly of IgSF modules via strand exchanging: Implications for module evolution, design and function

Ja Dando; Richard B Sessions; Mv Hayes; Ar Clarke; R L Brady


Proceedings of the 24th Meeting Federation of European Biochemical Societies, Barcelona, 1996 | 1996

Correction of substrate inhibition in dehydrogenases

N Bernard; J Delcour; A Alvarez; A Cortes; K Johnsen; Chris L Willis; Cr Dunn; Ar Clarke; J. John Holbrook

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Guy Casy

University of East Anglia

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Mv Hayes

University of Bristol

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R L Brady

University of Bristol

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Cm Eszes

University of Bristol

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Co Hewitt

University of Bristol

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