Minimum handling method for the analysis of phosphorous inhibitors of urolithiasis (pyrophosphate and phytic acid) in urine by SPE-ICP techniques

Pyrophosphate (PPi) and phytic acid (IP6) are natural phosphorous compounds with growing interest in the biomedical field due to their ability as potential inhibitors of urolithiasis among others. Existing methodologies for their evaluation show inconveniences mainly associated with sample treatment, matrix interferences and lack of resolution. The objective of the present work is the validation of a new method to determine both inhibitors in urine samples selectively and its application to the diagnosis of lithiasic patients. After urine purification by an off-line anion exchange solid phase extraction (SPE), based in an appropriate acidic elution gradient, the phosphorous compounds were analyzed by ³¹P measurements by inductively coupled plasma mass spectrometry (ICP-MS) in the purified urine extracts. Linear range and limit of detection obtained were adequate for the analysis of the physiological amounts of the compounds in urine. The method was successfully applied to human urine samples, resulting in adequate accuracy and precision and allowing for the analysis of phosphorus inhibitors of urolithiasis in urine. The method simplicity and high sample throughput leads to a clear alternative to current determinations of the mentioned species in urine. Moreover, PPi and IP6 concentrations found in patients suffering from oxalocalcic urolithiasic were significantly lower than those for healthy controls, supporting the fact that the risk for oxalocalcic urolithiasis increases when urinary phosphorus inhibitors decrease. Thus, speciation of phosphorus inhibitors of urolithiasis in urine of stone formers can be performed, which is of unquestionable value in diagnostic, treatment and monitoring of urolithiasis.     

浓硫酸颜色反应荧光分析法测定甲芬那酸

提出了浓硫酸颜色反应用于甲芬那酸荧光测定的新方法.甲芬那酸为弱荧光物质,与浓硫酸反应后荧光显著增强.体系最大激发波长和最大发射波长分别为385.0和471.9nm,甲芬那酸浓度在9.0×10-9～7.5×10-5 g·mL-1范围内与荧光强度呈良好的线性关系,方法检出限为3.1×10-9 g· mL-1,回收率为99.3％ ～ 102％.方法操作简单,灵敏度高,选择性好,用于甲芬那酸胶囊中甲芬那酸含量测定,结果满意.     

Enzymatic—spectrophotometric determination of phytic acid with phytase from Aspergillus ficuum

A method to determine phytic acid in the range 3–60 μM based on the spectrophotometric determination of inorganic phosphate with vanadate and molybdate, after liberation by enzymatic hydrolysis of phytic acid with phytase from Aspergillus ficuum at pH 2.5 and 37 °C is reported. The method has been applied successfully to determine phytic acid in wheat flour and in a pharmaceutical product.     

Fluorimetric determination of nucleic acid using the enhancement of terbium-gadolinium-nucleic acid-cetylpyridine bromide system

It is found that the fluorescence intensity of Tb-cetylpyridine bromide (CPB)-nucleic acid system can be enhanced by La³⁺, Gd³⁺, Lu³⁺, Sc³⁺ and Y³⁺, of which Gd³⁺ has the greatest enhancement. The experiments indicate that under the optimum condition, the fluorescence intensity of the system is in proportion to the concentration of nucleic acids in the range from 9×10⁻⁸ to 1×10⁻⁵ g ml⁻¹ for yeast RNA, from 1×10⁻⁷ to 1×10⁻⁵ g ml⁻¹ for fish sperm DNA. The detection limits are 3.2 and 4.1 ng ml⁻¹, respectively. This method has been used satisfactorily for the determination of both synthetic and actual samples. In comparison with most fluorescence method for the determination of nucleic acids, this method has higher sensitivity and stability.     

Modified platinum electrode with phytic acid and single-walled carbon nanotube: Application to the selective determination of dopamine in the presence of ascorbic and uric acids

A platinum (Pt) electrode modified by single-walled carbon nanotubes (SWNTs) and phytic acid (PA) was investigated by voltammetric methods in buffer solution. The PA-SWNTs/Pt-modified electrode demonstrated substantial enhancements in electrochemical sensitivity and selectivity towards dopamine (DA) in the presence of L-ascorbic acid (AA) and uric acid (UA). The PA-SWNTs films promoted the electron transfer reaction of DA, while the PA film, acting as a negatively charged linker, combined with the positively charged DA to induced DA accumulation in the film at pH under 7.4. However, the PA film restrained the electrochemical response of the negatively charged AA due to the electrostatic repulsion. The anodic peak potentials of DA, AA and UA could be separated by electrochemical techniques, and the interferences from AA and UA were effectively eliminated in the DA determination. Linear calibration plots were obtained in the DA concentration range of 0.2-10 μM and the detection limit of the DA oxidation current was determined to be 0.08 μM at a signal-to-noise ratio of 3. The results indicated that the modified electrode can be used to determine DA without interference from AA and UA, while ensuring good sensitivity, selectivity, and reproducibility.     

Fluorimetric determination of peroxynitrite based on an enzymatic reaction.

A novel fluorimetric method for the determination of peroxynitrite (ONOO-) using hemoglobin (Hb) as a catalyst is described. The method employs the reaction of ONOO with thiamine (TM), a colorless, non-fluorescent reagent in a glycine-NaCl-NaOH buffer solution (pH 12.7), to generate a highly fluorescent product, thiochrome (TC). The fluorescent product was monitored by fluorimetry. A linear calibration graph was obtained over an ONOO- concentration range from 4.95 x 10(-7) mol L(-1) to 2.97 x 10(-5) mol L(-1), with a detection limit of 9.78 x 10(-9) mol L(-1) ONOO-. The relative standard deviation at an ONOO- concentration of 2.11 x 10(-6) mol L(-1) was 4.15% (n = 9).     

Fluorogenic derivatization of aryl halides based on the formation of biphenyl by Suzuki coupling reaction with phenylboronic acid

The fluorogenic derivatization method for aryl halide was developed for the first time. This method was based on the formation of fluorescent biphenyl structure by Suzuki coupling reaction between aryl halides and non-fluorescent phenylboronic acid (PBA). We measured the fluorescence spectra of the products obtained by the reaction of p-substituted aryl bromides (i.e., 4-bromobenzonitrile, 4-bromoanisole, 4-bromobenzoic acid ethyl ester and 4-bromotoluene) with PBA in the presence of palladium (II) acetate as a catalyst. The significant fluorescence at excitation maximum wavelength of 275–290 nm and emission maximum wavelength of 315–350 nm was detected in all the tested aryl bromides. This result demonstrated that non-fluorescent aryl bromides could be converted to the fluorescent biphenyl derivatives by the coupling reaction with non-fluorescent PBA. We tried to determine these aryl bromides by HPLC-fluorescence detection with pre-column derivatization. The aryl bromide derivatives were detected on the chromatogram within 30 min without any interfering peak derived from the reagent blank. The detection limits (S/N = 3) for aryl bromides were 13–157 fmol/injection.     

Determination of ascorbic acid in pharmaceutical dosage forms and urine by means of an oscillatory reaction system using the pulse perturbation technique

A simple and reliable method for the determination of ascorbic acid (AA) is proposed and validated. It is based on potentiometric monitoring of the concentration perturbations of an oscillatory reaction system in a stable nonequilibrium stationary state close to the bifurcation point. The response of the Bray–Liebhafsky (BL) oscillatory reaction as a matrix, to the perturbation by different concentrations of AA, is followed by a Pt electrode. The linear relationship between maximal potential shift and the logarithm of the amount of AA is obtained between 0.01 and 1.0 μmol. The sensitivity of the proposed method (as the limit of detection) is 0.009 μmol and the method has excellent sample throughput (30 samples per hour). The procedure was used for AA determination in pharmaceutical formulations and urine. The results are in agreement with those obtained using the official method. Some aspects of the possible mechanism of AA action on the BL oscillating chemical system are discussed.     

The microstructure and anticorrosion performance of phytic acid-catalyzed polysilsesquioxane coatings

In this paper, the polysilsesquioxanes were prepared via the hydrolysis and condensation of methyltriethoxysilane, 3-glycidoxypropyltrimethoxysilane and tetraethoxysilane under the catalysis of phytic acid for the first time. Their microstructure and corrosion resistant performance were investigated by ¹³C NMR, ²⁹Si NMR, GPC, SEM, electrochemical techniques and salt spray test, respectively. It was found that phytic acid could catalyze the sol–gel reaction more efficiently than hydrochloric acid, causing more T³ structures, and the phytic acid-catalyzed polysilsesquioxane coatings had excellent corrosion resistance performance.     

Fluorimetric determination of ascorbic acid with o-phenylenediamine

A simple and sensitive fluorimetric method for the determination of ascorbic acid (AA) is described. The method is based on the condensation reaction between AA and o-phenylenediamine (OPDA) in the absence of the oxidant. The fluorescence intensity is measured at excitation and emission wavelengths of 360 and 430 nm, respectively. Under optimum condition, a linear relationship is obtained between the fluorescence intensity and the concentration of AA in the range of 0.05-40 μg ml⁻¹. The detection limit is 0.006 μg ml⁻¹, which is obviously lower than that of other fluorimetric methods reported.     

动力学荧光法测定抗坏血酸

基于在pH 10.7的NH3-NH4Cl缓冲溶液中,抗坏血酸能活化氯化血红素酶催化H2O2氧化L-酪氨酸的反应,使其反应速率增大,将时间驱动技术和动力学中斜率法相结合,建立了一种新的测定抗坏血酸的动力学荧光分析方法。在最佳实验条件下,方法的线性范围为0.1~4.8μg/mL,相对标准偏差3.8%,检出限为1.48μg/L。并考察了环境介质和常见物质的干扰情况。方法可用于实际样品的测定。     

A specific micromethod for the determination of phytic acid in biological material

A method for the quantitative determination of phytic acid in biological material is described. The method permits a determination of phytic acid in quantities below 0.1 mg even if the material contains closely related compounds includingmyo-inositol pentakisphosphate.

---

Eine spezifische Mikromethode für die Bestimmung von Phytinsäure in biologischem Material

Zusammenfassung Es wird eine Methode zur quantitativen Bestimmung von Phytinsäure in biologischem Material beschrieben. Die Methode erlaubt die Bestimmung von Phytinsäure in Mengen von weniger als 0.1 mg, selbst wenn das Untersuchungsmaterial nahe verwandte Substanzen wie z. B.myo-Inositpentakisphosphat enthält.

     

Removal of metal ions from aqueous solution by chelating polymeric microspheres bearing phytic acid derivatives

The aim of this study was to investigate the possibility to synthesize new chelating polymeric microspheres owing immobilized biocompatible agent as chelating functional groups and to evaluate their performance in metal ions removal from aqueous solution.The microparticles were synthesized via precipitation polymerization of 4-O-(4-vinylbenzyl)-myo-inositol 1,3,5-orthoformate with ethylene glycol dimethacrylate (EGDMA) and subsequent exhaustive phosphorylation of myo-inositol groups using phosphoric acid.Spherical geometry with monodisperse nature of the polymeric microparticles was confirmed by scanning electron micrographs (SEM) and dimensional analysis. A large surface area of the microspheres provided a maximum interaction of metal ions and the chelating functional groups on the surface. Absorption capacity of the beads for the selected metal ions, i.e., Cu(II), Ni(II), Fe(III), was investigated in detail in aqueous solution at pH 5.0 utilizing UV/Vis spectroscopy. This study showed that the macromolecular systems are very effective in chelating these metal ions and the affinity order of the microbeads toward metal ions is: Fe(III) > Ni(II) > Cu(II).The chelating beads can be easily regenerated by 1.0 M HNO₃ with high effectiveness. These features make the synthesized beads a potential candidate for metal ions removal at high capacity.     

Separation of phytic acid and other related inositol phosphates by high-performance ion chromatography and its applications

A high-performance anion-exchange chromatographic method was developed for the separation of phytic acid and other inositol phosphates (myo-inositol bis-, tris-, tetrakis-, and pentakisphosphates) with gradient elution and ultraviolet absorbance detection after post-column derivatization. With the acidic eluents, the combination of anion-exchange and ion suppression retention mechanisms led to the separation of 35 inositol phosphates (excluding enantiomers) into 27 peaks for the first time, and the retention behaviors of all myo-inositol bis- to hexakisphosphate isomers were studied. The whole separation procedure was completed within 65 min. Based on the investigations of nonenzymatic hydrolysis of phytic acid under different conditions by using this method, an in-house reference standard solution was produced, which can be used for method development. In addition, by applying this method to in vitro kinetic studies, at least one new enzymatic hydrolysis pathway of phytic acid was found, and one rule of enzymatic dephosphorylation of inositol phosphates (position effect) was proposed and another one (neighboring effect) was confirmed. The principle of the proposed identification approach for several inositol phosphate isomers based on hydrolysis products study will be applicable to other natural products analysis, for which standards are very expensive or not available.     

乳酸的液态酶荧光毛细分析法研究

基于乳酸脱氢酶(LDH)和烟酰胺腺嘌呤二核苷酸(NADH)氧化还原体系,提出了乳酸的液态酶荧光毛细分析方法(LE-FCA).在激发波长350nm、发射波长460nm奈件下,用LE-FCA法对乳酸进行了测定;其线性范围为0.2～1.0 mmol/L,r>0.9932,检出限为0.022 mmol/L,RSD<4.2%.LE-FCA能节省贵重的酶试剂,样品用量仅为18μL;可用于医药、卫生、工业、食品等含乳酸样品的测定.     

Fluorimetric determination of phytic acid based on the activation of the oxidation of 2,2'-dipyridyl ketone hydrazone catalysed by Cu(II)

Phytic acid exerts an activation effect on the oxidation of 2,2'-dipyridyl ketone hydrazone catalysed by Cu(II) ion and the oxidation product is highly fluorescent. A fixed time method for the fluorimetric determination of phytic acid based on this effect is described. The calibration graph is linear over the range 0.05-0.6 mg l-1 phytic acid, resulting in a limit of detection of 0.03 mg l-1 phytic acid. The relative standard deviation is in the range 1.4-1.8%, depending on the sample analysed. The method was successfully applied to the determination of phytic acid in human urine (20 samples) and food samples (nine different products). The results obtained for urine samples ranged from 0.31 to 3.6 mg l-1 phytic acid and for food samples from 3.8 to 22 mg g-1 phytic acid. This is the first procedure to be reported for the determination of phytic acid based on fluorimetric measurements.     

Fluorimetric determination of vanadium based on its reaction with 1-amino-4-hydroxyanthraquinone

A fluorimetric method for the determination of vanadium(V) (0.06–0.36 ppm) is described. The 1-amino-4-hydroxyanthraquinone is oxidized by this ion which yields a product exhibiting an intense yellow fluorescence in acidic solution. The experimental variables and interferences in this determination have been studied.     

Fluorimetric determination of danthron in pharmaceutical tablets and in urine

A simple, rapid determination is reported for danthron (1,8-dihydroxyanthraquinone) in pharmaceutical tablets. In a flow-injection system, danthron is reduced by sodium dithionite in $\text{1}\text{1}$ methanol/borate buffer to give a fluorescent complex. Linearity ranges from 30 μg ml^?1 to below 0.1 μg ml^?1. In urine samples, danthron is separated from other fluorescing species by reversed-phase high-performance liquid chromatography before its reduction by dithionite in a post-column reactor. Urine preparation requires no extraction. Spiked urine samples were studied in the working range of 0.02–2.0 μg ml^?1 danthron.     

Trace determination of thiosulphate and thioglycolic acid using novel inhibitory kinetic spectrophotometric method

Sulphur containing compounds such as sodium thiosulphate (STS) and thioglycolic acid (TGA) inhibit the rate of cyanide substitution by nitroso-R-salt (NRS) in hexacyanoruthenate(II) catalysed by Hg(II) ions due to their strong binding tendencies with Hg(II) catalyst. This inhibitory effect of sodium thiosulphate and thioglycolic acid is used as the basis for their determination at micro levels. The reaction was followed spectrophotometrically at 525 nm (λ_max of [Ru(CN)₅NRS]³⁻ complex) under optimised reaction conditions at 8.75 × 10^− 5 M [Ru(CN)₆⁴⁻], 3.50 × 10^− 4 M [NRS], pH 7.00 ± 0.02, ionic strength (µ) 0.1 M (KCl) and temp 45.0 ±0.1 °C. The modified mechanistic scheme is proposed to understand the inhibition caused by sulphur containing compounds (STS and TGA) on Hg(II) catalysed substitution of cyanide by NRS in [Ru(CN)₆]⁴⁻. The range of analytical concentration of inhibitor depends upon two factors; the amount of Hg(II) catalyst present in the indicator reaction and the stability of the Hg(II)-inhibitor complex under consideration. Under optimum conditions STS and TGA have been determined in the range of 0.98-7.0 × 10^− 6 M and 0.30-7.0 × 10^− 6 M. The detection limits for STS and TGA were found to be 3.0 × 10^− 7 M and 1.0 × 10^− 7 M respectively.