Electrophoretic assay for penicillinase: Substrate specificity screening by parallel CE with an active pixel sensor

We report application of a new UV imaging detector incorporating an active pixel sensor in an electrophoretic enzyme assay for penicillinase (β‐lactamase) with multiple substrates. The method based on electrophoretically mediated microanalysis was developed on a standard CE system with a single‐poin...

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Bibliographic Details
Published in:Electrophoresis 2007-06, Vol.28 (12), p.1926-1936
Main Authors: Urban, Pawel L., Goodall, David M., Bergström, Edmund T., Bruce, Neil C.
Format: Article
Language:English
Subjects:
Active pixel sensor
Anti-Bacterial Agents - analysis
Buffers
Clinical Laboratory Techniques
Electrophoresis, Capillary - instrumentation
Electrophoresis, Capillary - methods
Enzyme Inhibitors - analysis
Fiber Optic Technology - instrumentation
Flow Injection Analysis
Indicators and Reagents
Microchemistry
On-capillary enzyme assay
Online Systems
Penicillinase
Penicillinase - metabolism
Screening
Spectrophotometry, Ultraviolet - instrumentation
Substrate Specificity
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Summary:We report application of a new UV imaging detector incorporating an active pixel sensor in an electrophoretic enzyme assay for penicillinase (β‐lactamase) with multiple substrates. The method based on electrophoretically mediated microanalysis was developed on a standard CE system with a single‐point diode array detector and 200 nm UV wavelength, then transferred to a parallel capillary setup with the UV imaging detector for screening of penicillinase substrate specificity. One capillary is used for the assay and the other for reference, with an enzyme solution plug introduced into the first at the same time as a water plug into the second capillary. A mixture of antibiotics and markers is subsequently introduced as a sample plug to both capillaries, and driven through the enzyme (or water) plug by application of voltage. Most individual reactant and product peaks were separated and compounds amenable to β‐lactam hydrolysis could readily be identified and the extent of the reaction quantified within a single electrophoretic run.
ISSN:0173-0835
1522-2683
DOI:10.1002/elps.200600626