Amperometric sensor based on the alkaline phosphatase activity

The construction and response of an immobilized enzyme electrode as an amperometric sensor are described. Alkaline phosphatase was covalently bonded to a nylon filter mesh using glutaraldehyde and bovine serum albumin (BSA) as crosslinkers. This modified membrane was then attached to the surface of a glassy-carbon (GC) electrode. Substrate mass transport and enzymatic catalysis control were investigated in a rotating disk electrode. Various response characteristics and kinetic parameters were evaluated and are compared to those of a previously reported amperometric alkaline phosphatase electrode.     

Amperometric assay for collagenase

A sensitive and rapid amperometric assay for collagenase has been developed. The substrate for the assay is glucose oxidase covalently linked to insoluble collagen with dimethylsuberimidate. The collagenase cleaves the insoluble collagen-glucose oxidase conjugate into smaller, soluble fragments that have glucose oxidase activity. That activity is proportional to the collagenase activity hydrolyzing the insoluble conjugate. In the absence of collagenase, no glucose oxidase activity is found in the soluble phase. Glucose oxidase activity was assayed by measuring amperometrically the rate at which hydrogen peroxide is produced. The kinetics follow that proposed for a soluble enzyme acting on an insoluble substrate.     

Small luminescent molecular probe for developing as assay for alkaline phosphatase

Alkaline phosphatase (ALP) is an important biomarker in clinical diagnostics, and the abnormal level of ALP enzyme in serum is closely related to various diseases such as bone metastases, bone or liver cancer, and extrahepatic biliary obstruction. Recognizing the location and expression level of ALP in live cells has a substantial importance in early-stage cancer diagnosis, as well as an important parameter for studying the recovery of the patients after liver transplantation. With the advent of the newer and advanced fluorescence imaging techniques, small-molecule fluorescent probes have become a very powerful tool for mapping the subtle changes in the enzyme expression level in living cells and tissues in real-time. In this account, we provide an overview of recent advances in small-molecule ALP fluorescent probes, mainly during the last few years, including the design strategies and applications for biological applications.     

High-performance liquid chromatographic assay for acid and alkaline phosphatase in serum.

High-performance liquid chromatography was used to assay serum acid and alkaline phosphatase. Samples were incubated with adenosine-5'-monophosphoric acid (AMP) in a buffer of required pH, 5'-nucleotidase was inhibited with Ni2+ ions, and the phosphatase activity was determined by measuring the concentration of the reaction product, adenosine. The analysis time, after the incubation is terminated, is short (7 min), and the assay is quantitative and reproducible. Complete separation of the reaction product from the substrate and the naturally occurring serum constituents and the high sensitivity of the ultraviolet detection system eliminate some of the problems commonly encountered in spectrophotometric assays.     

Photometric and fluorimetric assay of alkaline phosphatase with new coumarin-derived substrates

Summary Two new coumarin-derived synthetic substrates for use in the direct and continuous kinetic assay of alkaline phosphatase are presented. They have been studied with respect to optimum pH (9.5) and rate of enzymatic hydrolysis (1.5–1.8 nmol/min at pH 9.5) by alkaline phosphatase from calf intestine. Detection limits were 0.0005 units/ml for the photometric assay, and 0.00001 units/ml for the fluorimetric one. The relatively longwave shifted absorption and emission maxima of the new substrates in addition to the large Stoke's shifts allow the determination of enzyme activities in a spectral range distinctly outside the intrinsic fluorescence of biological matter such as serum.     

Amperometric assay for the ketone body 3-hydroxybutyrate

A stable dry-strip electrochemical sensor for the direct measurement of 3-hydroxybutyrate in blood is described. The sensor utilizes the electrocatalytic oxidation of enzymically generated NADH by the redox mediator 4-methyl-o-quinone. The enzyme 3-hydroxybutyrate dehydrogenase, cofactor NAD⁺ and 4-methyl-o-quinone were incorporated into single-use disposable strip electrodes.     

Online assay of bone specific alkaline phosphatase with a flow injection-bead injection system

Alkaline phosphatase (ALP) has been used as one of the biomarkers for bone resorption and liver diseases. Normally, total alkaline phosphatase is quantified along with other symptoms to determine the releasing source of the alkaline phosphatase. A semi-automated flow injection-bead injection system was proposed to conveniently and selectively assay bone alkaline phosphatase (BALP) based on its specific binding to wheat germ coated beads. Amount of BALP in serum was determined from the intensity of the yellow product produced from bound BALP on the retained beads and its substrate pNPP. The used beads were discarded and the fresh ones were introduced for the next analysis. The reaction cell was designed to be opened and closed using a computer controlled solenoid valve for a precise incubation time. The performance of the proposed system was evaluated by using it to assay BALP in human serum. The results were compared to those obtained by using a commercial ELISA kit. The system is proposed to be an easy and cost effective system for quantification of BALP as an alternative to batch wise wheat germ specific binding technique.     

Highly sensitive assay for alkaline and acid phosphatase activities by high-performance liquid chromatography with electrochemical detection

A highly sensitive and specific assay for alkaline and acid phosphatases in biological materials, such as plasma and saliva, has been established. Phenol, formed enzymatically from the substrate phenylphosphate, was determined by high-performance liquid chromatography with electrochemical detection. The retention time of phenol was 7 min and no other peaks were observed. The method is rapid and sensitive with a detection limit for phenol of as little as 5 pmol. Thus, as little as 0.5 microliter of rat plasma or 10 microliters of human saliva is required for both alkaline and acid phosphatase assays. The assay is accurate and reproducible. Using this assay, alkaline and acid phosphatase activities in saliva were found to be 1.12 +/- 0.12 nmol/min/ml and 9.79 +/- 1.23 nmol/min/ml, respectively. This new assay method should be applicable to extremely small biological samples.     

Rapid electrochemical assay for theophylline in whole blood based on the inhibition of bovine liver alkaline phosphatase

A disposable electrochemical test strip for determining clinically relevant concentrations of theophylline (0–300 μM) in whole blood is described, based on the generation of p-aminophenol from p-aminophenyl phosphate by the action of bovine liver alkaline phosphatase. Theophylline is an uncompetitive inhibitor of alkaline phosphatase and thus inhibits this process. The test strip consists of a screen-printed, carbon-based electrode system containing the enzyme and substrate in separate layers. Application of a 20-μl blood sample to the strip initiates the enzymic reaction, which will proceed to an extent that is inversely dependent on the amount of theophylline in the sample. After a 2-min incubation, the p-aminophenol generated is quantified by its electrochemical oxidation at + 150 mV (vs. Ag/AgCl) on the underlying carbon electrode. Caffeine and theobromine (0–1 mM), phenylalanine (< mM) and endogenous alkaline phosphatase (<2 U ml ^?1) do not interfere.     

Amperometric detection of sulfur-containing compounds in alkaline media

A copper-based chemically modified glassy carbon electrode (GC-Cu) was developed to be used as an amperometric sensor for electrochemically detecting several sulfur-containing compounds in alkaline media. Under optimised flow injection conditions the calibration curves for sulfite, sulfide, thiosulfate, cysteine, cystine, etc., were linear over three orders of magnitude of concentration. Detection limits were of the order of 0.04-1.5 microM. A simple and rapid method for determining sulfite in red and white wines by anion-exchange chromatography with electrochemical detection is described.     

Amperometric complex-formation titration of traces of alkaline earths

Alkaline earth metals were determined in microgram quantities by complexometric titration with EDTA, EGTA and DTPA. The end-point was detected by following the anodic wave of the chelating agent at the rotating mercury electrode. All the alkaline earths can be titrated at the microgram level with reasonable accuracy, and calcium may be titrated with EGTA in the presence of a 1000-fold excess of magnesium.     

Amperometric biosensor based on D-aminoacid oxidase for the R-perindopril assay

A new amperometric biosensor based on D-aminoacid oxidase is described for the assay of R-perindopril. R-perindopril can be determined in the 400–¶20 nmol/L concentration range; the detection limit is ¶10 nmol/L. The selectivity was checked with S-perindopril, D- and L-proline, and polyvinylpyrrolidone. The main interfering species was D-proline. An automated system for the assay of R-perindopril based on the concept of flow injection with an amperometric biosensor (based on D-aminoacid oxidase) as detector is also described. The system is suitable for the on-line monitoring of R-perindopril at a sampling rate of 72 samples/h, in the linear range: 100 nmol/L –20 nmol/L with an RSD better than 0.09% (n = 10).     

Amperometric biosensor based on D-aminoacid oxidase for the R-perindopril assay

A new amperometric biosensor based on D-aminoacid oxidase is described for the assay of R-perindopril. R-perindopril can be determined in the 400-20 nmol/L concentration range; the detection limit is 10 nmol/L. The selectivity was checked with S-perindopril, D- and L-proline, and polyvinylpyrrolidone. The main interfering species was D-proline. An automated system for the assay of R-perindopril based on the concept of flow injection with an amperometric biosensor (based on D-aminoacid oxidase) as detector is also described. The system is suitable for the on-line monitoring of R-perindopril at a sampling rate of 72 samples/h, in the linear range: 100 nmol/L -20 nmol/L with an RSD better than 0.09% (n = 10).     

A ratiometric fluorescent probe for alkaline phosphatase with high sensitivity

Alkaline phosphatase(ALP)is one of essential biomarkers in mammalian tissue.Here we report a ratiometric probe for ALP,which is rationally designed and synthesized by employing ESIPT fluorophore N-(3-(benzo[d]thiazol-2-yl)-4-hydroxyphenyl)benzamide(BTHPB).The enzymatic dephosphorylation converts the probe to BTHPB,which exhibits a large spectral red-shift(120 nm),allowing extremely high sensitivity of ALP sensing at 0.004 mU/mL.The probe also shows excellent biocompatibility and has been applied for monitoring the endogenic ALP in living cells.     

Potentiometric flow-injection system for determination of alkaline phosphatase in human serum

A flow-injection system for detection of alkaline phosphatase (ALP) activity in human serum samples has been developed. As a specific and inexpensive ALP substrate for this kinetic assay monofluorophosphate (MFP) was applied. For detection of fluoride ions, generated in the course of the biocatalytic hydrolysis of MFP, conventional fluoride ion-selective electrode based on LaF₃-crystalline membrane was applied. After optimization the system allows analysis of human serum with high selectivity and relatively short time of analysis (5–6 samples h⁻¹). Volume of serum required for analysis is 0.05 mL. The system is useful for determination of the enzyme activity in human serum samples at physiological and pathological levels as well as for detection of isoenzymatic forms of ALP.