Novel determination system for urea in alcoholic beverages by using an FIA system with an acid urease column.

A novel determination method for urea using an acid urease column-FIA system was developed, and the system was applied to the determination of urea in rice wine. This novel FIA system was characterized by CO2 detection due to the property of acid urease and by a microfluidic gas-diffusion device with the use of an ultra-thin hollow fiber membrane. A biosensing system fabricated in this study was assembled with a double-plunger pump, a sample-injection valve, an immobilized acid urease column as a recognition element for the assay of urea, a gas-diffusion unit, and a flow-type spectrophotometer. The gas-diffusion unit consisted of a double-tubing structure in which the outer tubing was made of PTFE (i.d. 1.0 mm; o.d. 1.5 mm) and the inner tubing was of porous PTFE (i.d. 0.19 mm; o.d. 0.25 mm). Standard urea solutions (20 microl) were measured through monitoring variations in the absorbance of a coloring agent solution resulting from a pH shift due to carbon dioxide molecules being enzymatically generated. A wide and linear relationship was obtained between the concentration of urea (16 microM - 1.0 mM) and the change in absorbance. This FIA system has great advantages that the system did not suffer from ammonia and ethanol in samples. This system, armed with a microfluidic gas-diffusion device, was applicable to the determination of various substrates of many kinds of decarboxylase, amino-acid oxidase, and amino-acid oxygenase, producing CO2 and NH3 molecules.     

Flow-injection on-line oxidizing fluorimetry and solid phase extraction for determination of thioridazine hydrochloride in human plasma

A simple, sensitive and specific fluorimetric method has been developed for the determination of thioridazine hydrochloride in human plasma involving solid phase extraction (SPE). In a flow-injection system, thioridazine hydrochloride is on-line oxidized into a strongly fluorescent compound with a lead dioxide solid-phase reactor and the fluorescence intensity is measured with a fluorescence detector (λ_ex = 349 nm, λ_em = 429 nm). A comparison of plasma sample pretreatment between SPE procedure and precipitation method was made and the results showed that SPE procedure was better than precipitation method. Under the optimum conditions, the fluorescence intensity is proportional to the concentration of thioridazine hydrochloride in the range from 0.015 to 2.000 μg mL⁻¹. The detection limit is 5.5 ng mL⁻¹ of thioridazine hydrochloride and the relative standard deviation is 1.06%. This method has been applied to determination of thioridazine hydrochloride in real patients plasma samples with the results compared with those obtained by HPLC method.     

Preconcentration and decomposition of perfluorinated carboxylic acids on an activated charcoal cartridge with sodium biphenyl reagent and its determination at microg L(-1) level on the basis of flow injection-fluorimetric detection of fluoride ion

Perfluorinated surfactants of heptafluorobutylate and pentadecafluorooctanoate ions were adsorbed on an activated charcoal cartridge and decomposed with sodium biphenyl (SBP) reagent to form inorganic fluoride ion. The fluoride ion thus formed was determined by flow injection analysis (FIA) using quercetin-Zr complex as a fluorimetric reagent, where λ_ex and λ_em were 422 and 491 nm, respectively. The limit of detection for fluoride ion by the FIA system was developed to 1.1 × 10⁻⁶ M (signal to noise ratio of three), when 50% (v/v) tetrahydrofuran (THF) was used as a dissolving solvent for quercetin. The perfluorinated surfactants in the sample solution were quantitatively adsorbed on the cartridge containing 100 mg of activated charcoal and were decomposed with 0.5 mL of sodium biphenyl reagent after drying thoroughly by flowing through dry nitrogen gas. The fluoride ion formed was recovered with 3 mL of purified water as an eluent, and it was determined by the fluorimetric flow injection system. The blank fluorescence signal accompanied during the adsorption/decomposition on the cartridge was reduced by washing the activated charcoal with acetone. The blank signal was also observed from dimethoxyethane, which was used in sodium biphenyl reagent. When 600 mL sample solution was used and 200 times enrichment was applied, the heptafluorobutylate and pentadecafluorooctanoate ions at the concentrations of 2.1 μg L⁻¹ were quantitatively recovered as fluoride ion, and the limit of detections for the perfluorinated surfactants were 0.3 and 0.3 μg L⁻¹ for the two perfluorinated surfactants, respectively (3 sigma of the blank signal).     

Immobilization enzyme fluorescence capillary analysis for determination of lactic acid

A new method for the determination of lactic acid based on the immobilization enzyme fluorescence capillary analysis (IE-FCA) was proposed. Lactic dehydrogenase (LDH) was immobilized on inner surface of a capillary with glutaraldehyde, and an immobilized enzyme lactate capillary bioreactor (IE-LCBR) was formed for the determination of lactic acid. After nicotinamide adenine dinucleotide (NAD⁺) is mixed with lactic acid solution, it was sucked into the IE-LCBR and was detected at λ_ex 353 nm/λ_em 466 nm. Optimized conditions are as follows: the temperature is 38 °C; the reaction time is 15 min; the concentrations of Tris buffer (pH 8.8) and NAD⁺ are 0.1 mol L⁻¹ and 4 mmol L⁻¹, respectively; the concentration of LDH used for immobilization is 15 kU L⁻¹. The concentration of lactic acid is directly proportional to the fluorescence intensity measured from 0.50 to 2.0 mmol L⁻¹; and the analytical recovery of added lactic acid was 99–105%. The minimum detection limit of the method is 0.40 mmol L⁻¹ and sensitivity of the IE-CBR is 4.6 F mmol⁻¹ L⁻¹ lactate. Its relative standard deviation (R.S.D.) is ≤2.0%. This IE-FCA method was employed for determination of lactate in milk drink.     

A triple helical calcium-based coordination polymer with strong blue fluorescent emission

A hydrothermal reaction of 1,3-dicyanobenzene and Ca(OH)₂ yielded a triple helical calcium-based coordination polymer of the formula, C₂₀H₂₅Ca_2.50O_18.50 (1). The 1,3-benzenecarboxylate anion, found in the final product was generated in situ during the synthesis by the hydrolysis of 1,3-dicyanobenzene. X-ray diffraction study shows that the complex 1 crystallizes in the monoclinic system, C2/c space group, a=15.5701(5), b=21.4445(7), c=17.1601(6) Å, β=111.7400(7)°, V=5322.1(3) Å³, Z=8, D_c=1.651 Mg/m³. The calcium atoms show differences in the coordination environments. Complex 1 emits strong blue fluorescent light (λ_em(max)=419 nm) when it is excited by UV light (λ_ex(max)=316 nm) in the solid state at room temperature.     

Synthesis, structure, and fluorescence of two cadmium(II)-citrate coordination polymers with different coordination architectures

Two novel Cd(II)-citrate complexes were obtained with different metal/ligand ratios through hydrothermal method. Their structures were determined by single-crystal X-ray diffraction analysis. Although their topological structures are both 2-D layer network assemblies, both central Cd(II) ions and Hcit³⁻ ligands display completely different coordination modes. In polymeric complex 1, Hcit³⁻ serves as a μ₁₀-bridged and central Cd(II) ions adopt 6- and 8-coordinated configurations. In contrast, a μ₉-bridged and 6- and 7-coordinated environments between Cd(II) and Hcit³⁻ are established in the polymeric complex 2. Two Complexes remain stable up to approximately 300 °C. The complex 1 exhibits strong fluorescent emission band at 450 nm (λ=346 nm) as well as complex 2 exhibits strong fluorescent emission band at 430 (λ=346 nm).     

Determination of chromophore charge states in the low pH color transition of the fluorescent protein Rtms5 via time-dependent DFT

The red fluorescent protein Rtms5^H146S displays a transition from blue (absorbance λ_max 590 nm) to yellow (absorbance λ_max 453 nm) upon titration to low pH. The pK_a of the reaction depends on the concentration of halide, offering promise for new expressible halide sensors. The protonation state involved in the low pH form of the chromophore remains, however, ambiguous. We report calculated excitation energies of different protonation states of an RFP chromophore model. These suggest that the relevant titration site is the phenoxy moiety of the chromophore, and the relevant base and conjugate acid are anionic and neutral chromophore species, respectively.     

Determination of urea with an ammonia gas-sensitive semiconductor device in combination with urease

An ammonia gas-sensitive Ir/Pd MOS capacitor is used for urea determinations with the aid of urease in two different systems. One combination utilizes a reaction column with immobilized urease in a flow-injection system. The lower limit of urea detection for 150-μl samples was 0.2 μM. Urea in whole blood and blood serum was determined after a 500-fold dilution, and 15 samples per hour could be assayed. The relative standard deviation was 4.6% (n=10). Recovery tests were satisfactory. Values obtained for urea in serum correlated well with those from a spectrophotometric method. The other combination is based on a small flow cell with free urease enclosed between a dialysis membrane and a gas-permeable membrane. Urea was determined in the concentration range 0.01–50 mM. The enzyme probe could be used for up to four days without changes of behaviour.     

Structure of liquid 1-chloronaphthalene at 293 K

The structure of 1-chloronaphthalene, C₁₀H₇–Cl, at 293 K was investigated using the X-ray diffraction method. Monochromatic radiation MoK (λ=0.71069 Å) enabled the determination of the scattered radiation intensity between S₀=4πsin ₀/λ=0.430 Å⁻¹ and S_max=14.311 Å⁻¹. The interpretation of the results was carried out using the reduction method of Blum and Narten. Experimental distributions of X-ray scattered intensity were compared with theoretical results predicted for a proposed model of 1-chloronaphthalene molecule. The electron-density radial-distribution function was calculated and some intra- and intermolecular distances in liquid 1-chloronaphthalene were determined. X-ray structural analysis was applied to determine the packing coefficient of 1-chloronaphthalene molecules.     

A simple method for predicting the frequency of the infrared inactive carbonyl stretching mode in LM(CO)5 molecules with C4V symmetry

The paper presents a new method for predicting the frequency of the b₁ mode, which is infrared-inactive, in complexes of the type LM(CO)₅ belonging to C_4V point group. The method was based on the relation λ₃=λ₄+[(1−δ/δ)](λ₁−λ₂), where δ=(λ₁−λ₂)/(λ₁−λ₂+λ₃−λ₄), λ₁, λ₂, λ₃ and λ₄ are the λ parameters of the , , b₁ and e modes, respectively. For a large numbers of complexes of the type LM(CO)₅ the average value of δ was found to be 0.80, with a standard deviation of 0.02. With the use of average value of δ, the frequencies of b₁ mode were estimated. The result obtained indicated that there exists a rather good fit between observed and calculated frequencies, with a mean error of 2.7 cm⁻¹. In addition, it was shown that the δ parameter can be used as a criterion of the correct band assignment for the complexes understudy.     

Determination of adenosine disodium triphosphate using prulifloxacin-terbium(III) as a fluorescence probe by spectrofluorimetry

A new spectrofluorimetric method is developed for determination of adenosine disodium triphosphate (ATP). The interactions between prulifloxacin (PUFX)–Tb³⁺ complex and adenosine disodium triphosphate has been studied by using UV–vis absorption and fluorescence spectra. Using prulifloxacin–Tb³⁺ as a fluorescence probe, under the optimum conditions, ATP can remarkably enhance the fluorescence intensity of the prulifloxacin–Tb³⁺ complex at λ = 545 nm and the enhanced fluorescence intensity is in proportion to the concentration of ATP. Optimum conditions for the determination of ATP were also investigated. The dynamic range for the determination of ATP is 4.0 × 10⁻⁷ to 2.0 × 10⁻⁵ mol L⁻¹, and the detection limit (3 σ/k) is 1.7 × 10⁻⁸ mol L⁻¹. This method is simple, practical and relatively free interference from coexisting substances and can be successfully applied to determination of ATP in real pharmaceutical samples. The mechanism of fluorescence enhancement of prulifloxacin–Tb³⁺ complex by ATP was also discussed.     

Determination of boron in water and pharmaceuticals by sequential-injection analysis and fluorimetric detection

This work reports the application of a sequential-injection analysis (SIA) method for the determination of boron. The method relies on the enhancement of the fluorescence (λ_ex=313 nm, λ_em=360 nm) of chromotropic acid (4,5-dihydroxynaphthalene-2,7-disulphonic acid-CA) as a result of its complexation with boric acid (BA). Individual zones of the sample, the CA solution in a suitable buffer and a NaOH solution were aspirated in the holding coil of the SIA apparatus. As the zones were propelled towards the detector, zone penetration in the sample–CA interfaces occurred resulting in the formation of the strongly fluorescent BA–CA complex. The native fluorescence of the CA was quenched by the alkaline environment established as a result of the mixing at the CA–NaOH interface. The chemical and instrumental parameters affecting the fluorescence intensity were investigated and the influence of potential interferents was investigated. After selecting the most suitable conditions, the calibration plot for boron was linear in the range of 8–350 μg l⁻¹ with a 3σ limit of detection of 3 μg l⁻¹ and a relative standard deviation of 2.7% at the 90 μg l⁻¹ boron level (n=8). Finally, the method was applied to the determination of boron in natural waters and pharmaceutical products with revoveries in the range of 96–106%.     

Determination of urea in serum by a fiber-optic fluorescence biosensor

A new fiber-optic biosensor for urea has been developed, based on immobilized urease coupled to a fluorescence ammonia sensor. The enzymatically generated ammonia diffuses through the membrane into a solution of the fluorescent pH indicator trisodium 8-hydroxypyrene-1,3,6-trisulfonate. The sensor has been successfully used for the determination of urea in serum samples, with results in good agreement with those reported by a local hospital. The proposed sensor is reversible and selective to urea. The ease of construction of the sensor tip offers the possibility of designing disposable tips for use in clinical applications.     

Determination of trace amounts of vanadium by UV-vis spectrophotometric after separation and preconcentration with modified natural clinoptilolite as a new sorbent

Natural clinoptilolite was used as a sorbent material for solid phase extraction and preconcentration of vanadium. The clinoptilolite was first saturated with a cation such as nickel(II) and then modified with benzyldimethyltetradecyleammonium chloride (BDTA) for increasing sorption of 4-(2-pyridylazo)resorcinol (PAR). Vanadium–PAR complex was quantitatively retained on the sorbent by the column method at the pH range 6.2–7.0 at a flow rate of 1 mL min⁻¹. It was removed from the column with 5.0 mL of dimethylformamide solution at a flow rate of 0.8 mL min⁻¹ and determined by UV–vis spectrophotometry at λ_max = 550 nm. 0.031 μg of vanadium can be concentrated from 450 mL of aqueous sample (where detection limit as 0.07 ng mL⁻¹ with preconcentration factor of 90). Relative standard deviation for eight replicate determination of 5.0 μg of vanadium in final solution is 2.1%. The interference of number of anions and cations has been studied in detail to optimize the conditions and method was successfully applied for determination of all vanadium as V(IV) form in standard samples.     

Kinetic investigation of electronic energy transfer processes following the pulsed dye-laser generation of excited atomic barium, Ba[6s6p(P1)], in the presence of atomic strontium

The collisional behaviour of Ba[6s5d(³D_J)], 1.151 eV above the 6s²(¹S₀) electronic ground state, in the presence of atomic strontium, has been investigated in the ‘long-time domain' (ca. 100 μs–1 ms) following the pulsed dye-laser excitation of barium vapour at elevated temperature at λ = 553.5 nm (Ba[6s6p(¹P₁)] ← Ba[6s²(¹S₀)]. Ba(³D_J) is subsequently produced from the short-lived ¹P₁ state (τ_e = 8.37 ± 0.38 ns) by a number of radiative and collisional processes. It may then be monitored in the ‘long-time domain' by atomic spectroscopic marker methods involving either collisional activation of Ba(³D_J) by Ba(¹S₀) and He buffer gas to yield Ba[6s6p(³P_J)] with subsequent emission from the ³P₁ state (τ_e = 1.2 ± 0.1 μs): Ba[6s6p(³P₁)] → Ba[6s²(¹S₀)] + hv (λ = 791.1 nm). Alternatively, emission from Ba(¹P₁) may be monitored at long times following the generation of this short-lived state by energy pooling following self-annihilation of Ba(³D_J) + Ba(³D_J) from Ba[6s6p(¹P₁)] → Ba[6s²(¹S₀)] + hv (λ = 553.5 nm). The generation of Ba(³D_J) in the presence of atomic strontium yields emission in the long-time domain from Sr[5s5p(³P₁)] (τ_e = 19.6 μs): Sr[5s5p(³P₁)] → Sr[5s²(¹S₀)]  + hv (λ = 689.3 nm). Whilst the decay profiles at short times are complex in form, at long times all these atomic profiles show first-order kinetic removal with the decay coefficients for λ = 791.1 nm, 689.3 nm and 553.5 nm emissions in the ratio 1 : 2 : 2, consistent with overall third-order activation of the form: Ba(³D_J) + Ba(³D_J) + Sr(¹S₀) → Sr(³P_J) + 2Ba(¹S₀). The mechanism is modelled in detail, including measurement of integrated emission intensities, yielding kinetic data for fundamental collisional processes. The overall rate constant for the third-order collisional activation of Sr[5s5p(³P_J])from 2Ba[6s5d(³D_J)] + Sr[5s²(¹S₀)] takes the upper limit of 5.8 × 10⁻²⁷ cm⁶ atom⁻² s⁻¹ (T = 900 K). The rate constant for the two body collisional quenching of Ba[6s5d(³D_J)] by ground state atomic strontium, Sr[5s²(¹S₀)], is found to be (2.0 ± 0.1) × 10⁻¹² cm³ atom⁻¹ s⁻¹ (T = 900 K).     

Gas phase derivatization of ammonia with 4-fluoro-7-nitrobenzo-2-oxa-1,3-diazole and its application to urease assay.

An ammonia-specific and rapid fluorometric method for determination of ammonia and urease activity was developed. The method is designed to assay ammonia levels or urease activity for the rapid diagnosis of Helicobacter pylori infection. 4-Fluoro-7-nitrobenzo-2-oxa-1,3-diazole was used to derivatize ammonia and 4-amino-7-nitrobenzo-2-oxa-1,3-diazole was analysed by high performance liquid chromatography at an excitation wavelength of 455 nm and an emission wavelength of 520 nm. Derivatization was designed to react with ammonia gas produced in a strong alkaline pH sample. The fluorescent intensity was linear in the range of 0.1-10 mM ammonia per tube when the reaction was carried out for 15 min at 37 degrees C. Urease activity, judged as the amount of ammonia production from urea, could be measured at 25 ng per tube (S/N = 1.5) with Jack bean meal urease. Because of its rapidity, this assay is potentially superior to the current standard method in use in clinical settings.     

Flow-injection analysis for hypoxanthine in meat with dissolved oxygen detector and enzyme reactor

A low cost flow-injection analysis (FIA) with a dissolved oxygen (DO) detector and a xanthine oxidase immobilized column for the analysis of hypoxanthine as an index to determine degree of aging in meat was developed for quality control in the food industry. In this system, hypoxanthine is oxidized by an enzyme reaction with xanthine oxidase immobilized on the column to produce xanthine. Then the catalytic reaction between hypoxanthine and DO with xanthine oxidase proceeds with the DO concentration decreasing in the stream of the flow system. Decrease in the DO concentration was monitored by a DO detector located downstream of the flow system. This decrease in DO concentration was proportional to the hypoxanthine concentration. For detecting the decreased DO concentration efficiently a flow-through cell with a polarographic-type DO sensor was specially designed. As a result, a linear working curve was obtained from 3.68 × 10⁻⁵ to 1.84 × 10⁻³ M hypoxanthine concentrations with this FIA system. We applied the present system with a DO detector for the determination of hypoxanthine in meat samples and compared the results with those obtained by the conventional HPLC method. The data obtained with the present FIA method were in fairly good agreement with those obtained by the conventional HPLC method for the meat samples. Correlation factor and regression line between the two methods were 0.998 and Y= 1.51X-32.64 respectively. We concluded that the present FIA system with a DO detector was suitable as a simple, easy to handle and reliable instrument for quality control in the food industry.     

Determination of urea in serum by using naturally immobilized urease in a flow injection conductimetric system

A flow injection method was developed, aimed at the determination of urea in human serum. The system makes use of the naturally immobilized urease present in Canavalia ensiformis DC (jack bean). A column is filled with small pieces of this bean, and the sample (50 microliters) containing urea passes through it carried by a 1% NaCl solution. On leaving the column the stream is merged with an alkaline reagent (0.5 mol dm-3 NaOH; 0.5% disodium dihydrogen ethylenediaminetetraacetate). The ammonium ions, arising from the enzymatic reaction that occurs inside the column, are changed into the molecular form, which permeates a polytetrafluoroethylene membrane and is received in a de-ionized water acceptor stream. The ammonia ionizes causing an increase in the conductance, which is proportional to the urea content of the sample. About 40 samples can be processed in 1 h with negligible carry-over and with a relative standard deviation of 1% or less. The results are in agreement with those obtained by a standard spectrophotometric method.     

Application of enzyme-field effect transistor sensor arrays as detectors in a flow-injection analysis system for simultaneous monitoring of medium components. Part II. Monitoring of cultivation processes

Glucose, maltose, sucrose, lactose, ethanol and urea concentrations were monitored simultaneously during the cultivation of Escherichia coli and Saccharomyces cerevisiae by means of enzyme field effect transistors (EnFETs) applying glucose dehydrogenase (GDH), maltase (MAL)/GDH, invertase (INV)/GDH, β-galactosidase (β-GAL)/galactosedehydrogenase (GALDH), alcoholdehydrogenase (ADH)/aldehydedehydrogenase (ALDH), and urease. These enzymes were (co)immobilized on the pH sensitive gates of an eight-FET array. The FET array was integrated in a commercial FIA system.     

Flow injection determination of nitrite by fluorescence quenching

A simple, sensitive and selective fluorimetric method for the determination of nitrite ion in waters using a merging zones flow injection system is described. The fluorimetric determination is based on the measurement of the quenching effect produced by nitrite on proflavine (3,6-diaminoacridine) fluorescence (λ_ex/λ_em=290/519 nm).

The optimum experimental conditions were investigated by merging 0.5 ml of the sample and 0.5 ml of a solution of 5 mg l⁻¹ of proflavine (in 0.1 M HCl) in a flow injection system, on-line connected to a flow-cell placed in the conventional sample compartment of a spectrofluorimeter. The selected carrier solution and final flow rate were 0.1 M HCl and 0.5 ml min⁻¹, respectively. A reaction coil of 2 ml was used. As a result of the simplicity of this system, a sample throughput of about 50 samples h⁻¹ can be achieved with the proposed methodology.

The detection limit was 1.1 ng ml⁻¹ (3σ criterion) of nitrite. The repeatability for five sample injections containing 100 ng ml⁻¹ of nitrite was ±0.3% and the observed linear range extended up to 400 ng ml⁻¹. Also, the effect of interferences from various metals and anions commonly present in waters was also studied.

The method was successfully applied to the determination of low levels of nitrite in different water samples (river, fountain, tap and commercial drinking waters).