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Enzyme-amplified immunoassays |
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| Authors: | Stanley C J Ellis D H Bates D L Johannsson A |
| Affiliation: | IQ(Bio) Ltd., Downham House, Downham's Lane, Milton Road, Cambridge CB4 1XG, England |
| Abstract: | The sensitivity of enzyme immunoassays may be enhanced by the use of enzyme-amplification. This technique uses the enzyme label in the immunoassay to provide a trigger substance for a secondary system that can generate a large quantity of coloured product. Two examples of enzyme amplifiers are described, using either a substrate cycle with phosphorylated hexose sugars, or a redox cycle involving the coenzyme NAD+. The redox enzyme-amplifier has a detection limit of less than one attomole for the enzyme label, alkaline phosphatase. The limited dynamic range of enzyme-amplified immunoassays may be overcome by kinetic analysis of the colour development in the enzyme-amplifier, to add at least a further order of magnitude to the range of directly measured analyte concentrations in the immunoassay. This is illustrated in an enzyme-amplified immunoassay for human thyroid stimulating hormone. Amperometric measurement of the enzyme-amplifier provides a method to extend the dynamic range still further and compares favourably with the performance of a gamma counter, a luminometer or a fluorimeter. |
| Keywords: | Ultrasensitive non-isotopic immunoassay amplification by enzyme modulation dynamic range extension by kinetic analysis amperometric detection of enzyme labels thyroid stimulating hormone. |
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