Issue 6, 2001

Robotic enzyme amplification: a comparison of some kinetic properties of bovine liver, Candida utilis and Proteus sp. glutamic dehydrogenasesElectronic Supplementary Information available. See http://www.rsc.org/suppdata/an/b0/b008596k/

Abstract

NADP(H)-specific Bakers yeast glucose 6-phosphate dehydrogenase (BYG6PDH) was paired, in turn, with each of three different source glutamate dehydrogenases (GDHs): NAD(P)-specific bovine liver (BLGDH), NADP-specific Candida utilis (CUGDH) and NADP-specific Proteus sp. (PSGDH) to constitute three enzyme cycling systems; (i) BYG6PDH/BLGDH; (ii) BYG6PDH/CUGDH; and (iii) BYG6PDH/PSGDH. When incorporated into an enzymatic cycling/amplification system for NAD kinase and run on a centrifugal fast analyzer (CFA), the microbial source enzyme CUGDH gave rise to a seven-fold greater amplification rate [21.5 × 103 cycles−1 (cph)] relative to that realized (3 × 103 cph) using the BYG6PDH/BLGDH cycling pair previously reported. Either of these cycling systems can be used as a flexible and general-purpose module for robotic amplification and data collection of NADP(H) linked enzymes as a user’s requirements dictate. Although the BYG6PDH/PSGDH cycling pair produced a respectable cycling rate (14.4 × 103 cph), for reasons discussed the PSGDH enzyme was not considered a suitable replacement for BLGDH in an NADP(H) cycling system.

Supplementary files

Article information

Article type
Paper
Submitted
20 Oct 2000
Accepted
06 Apr 2001
First published
23 May 2001

Analyst, 2001,126, 855-860

Robotic enzyme amplification: a comparison of some kinetic properties of bovine liver, Candida utilis and Proteus sp. glutamic dehydrogenases

B. Lewis, M. Tallman and E. McGuinness, Analyst, 2001, 126, 855 DOI: 10.1039/B008596K

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