7—[（4—甲基2—胂酸基苯）偶氮]—8—羟基喹啉—5—磺酸荧光光度法测定氟

本文介绍了７－［（４－甲基－２－胂酸基苯）偶氮］－８－羟基喹啉－５－磺酸的合成方法以及性能，详细研究了氟对该试剂与铝形成的荧光的熄灭作用，建立了荧光法测定微量氟的新方法。应用于水样和牙膏中的氟的测定，效果良好。     

Fluorometric determination of fluoride ion by reagent tablets containing 3-hydroxy-2'-sulfoflavone and zirconium(IV) ethylenediamine tetraacetate

A reagent tablet for determination of fluoride ion has been prepared using ethylenediamine-N,N,N′,N′-tetraacetate complex of zirconium (Zr-EDTA), 3-hydroxy-2′-flavone (FS) and an appropriate pH buffer. Dissolving of the tablet into water exhibits an intense blue fluorescence (λ_max = 460 nm) upon excitation at 377 nm and the fluorescence intensity decreases with the presence of fluoride ion. Hence, a simple fluorescent detection procedure for fluoride ion in aqueous media was successfully constructed with this tablet. The principle of this detection system is the ligand exchange reaction of FS bound to Zr-EDTA with fluoride ion. The present system provides an easy, rapid and selective determination method of fluoride ion ranging from 5 × 10⁻⁶ to 1 × 10⁻³ mol dm⁻³. The measurement of real samples with this tablet showed the similar results as those by the common method with the Alfusone reagent.     

Terbium chelate labels for fluorescence immunoassays

Bovine serum albumin was labelled with a terbium complex by means of a reagent prepared from diethylenetriaminepentaacetic acid or diethylenetriaminepentaphosphonic acid and p-aminosalicylic acid. The ternary mixed ligand complexes showed strong fluorescence and were stable in very dilute solution (10(-10)M). The fluorescence of the conjugated products was compared with regard to their application in the fluoroimmunoassay of bovine serum albumin.     

Determination of agmatine in biological samples by capillary electrophoresis with optical fiber light-emitting-diode-induced fluorescence detection

A capillary electrophoresis (CE)/optical fiber light-emitting diode (LED)-induced fluorescence detection method is developed for the determination of agmatine in biological samples. The agmatine was precolumn-derivatized with fluorescence tagging reagent, fluorescein isothiocyanate (FITC). Optimal separation and determination for agmatine were obtained with an electrophoretic buffer of 20 mM sodium borate (pH 9.2). Under the optimal conditions, the determination of agmatine was achieved in less than 4 min, and the detection limit was 4.1x10(-9) M (S/N = 3). The relative standard deviation (RSD) for 11 parallel determination of agmatine was less than 3.0%. The present CE-LED induced fluorescence detection method has been applied to detect agmatine in rat brain tissue, rat stomach tissue, human serum, and human urine. The level of agmatine in human urine was quantified by CE for the first time and found to be in the range 2.5-4.1x10(-7) M.     

A fluorescent fluoride ion probe based on a self-organized ensemble of 5-hydroxyflavone-Al(III) complex

In the presence of Al(III) ions, 5-hydroxyflavone (5HF) through a complexation reaction in MeOH, shows dual fluorescence, characterized by a newly developed peak at 554nm upon excitation at 363nm. In this communication, the subsequent ligand exchange reaction of the complex with fluoride ion causing a fluorescence enhancement followed by a decrease in fluorescence intensity involving an intermediate mechanistic pathway, delivering a quantitative estimation route for fluoride ion in the concentration range from 5x10(-5) to 7x10(-4)M, has been reported. The ligand exchange reaction, without interference from other common anions, has been investigated by UV-vis and fluorescence spectroscopies combined with the AM1 semi-empirical self-consistent field quantum chemical calculations within UHF formalism in their ground state.     

A water-soluble fluorescent fluoride ion probe based on Alizarin Red S-Al(III) complex

A new water-soluble fluorescent fluoride ion signaling system has been developed based on the ligand exchange mechanism in aqueous medium. This procedure is based on the exchange of two Alizarin Red S (ARS) molecules coordinated to Al(III) by fluoride ion without interference from other common anions. The binary complex of ARS with Al(III) provides a sensitive signaling system for fluoride ion in the concentration range from 5x10(-6) to 3x10(-4) M. The ligand exchange reaction of ARS-Al(III) complex with fluoride ion has been investigated by UV-vis and fluorescence spectroscopies combined with the AM1 semi-empirical quantum chemical calculations. The pale orange fluorescence (lambdamax=575 nm) exhibited by the complex upon excitation at 435 nm decreases in intensity with fluoride addition with a detection limit of 0.1 mg L-1.     

Determination of phenylalanine in serum using reversed-phase liquid chromatography and fluorescence detection

A liquid chromatography procedure is reported for determining phenylalanine in small volumes of serum. A 10-microliter volume of serum was deproteinized with ethanol and an aliquot was derivatized with dansyl chloride reagent. The dansylated phenylalanine and the norleucine internal standard were separated using reversed-phase chromatography and measured with a fluorescence detector. Linearity was excellent over the range 50-800 mg/l. Within-run precision was better than 4%. Total analysis time including chromatography was approximately 40 min. As little as 300 pg of dansylated phenylalanine was detected.     

Fluorimetric determination of kynurenine in human serum by high-performance liquid chromatography coupled with post-column photochemical reaction with hydrogen peroxide

A high-performance liquid chromatographic method involving post-column photochemical reaction and fluorimetric detection has been developed for the determination of kynurenine in serum. Kynurenine was separated on a column of Capcell Pak C18 (resistant to pH 10). The mobile phase consisted of 0.05 M Na2B4O7-0.1 M KH2PO4 buffer (pH 8.5)-ethanol (97:3, v/v) containing 60 mM hydrogen peroxide. The post-column reagent, containing 60% (v/v) ethanol, was mixed with the mobile phase, which was irradiated with ultraviolet light to induce fluorescence. The recovery of kynurenine was 95.9 +/- 5.0% (n = 6). The method allows the determination of as little as 2 pmol of kynurenine.     

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).     

Optical-fibre sensing of fluoride ions in a flow-stream

The Alizarin Fluorine Blue method for the determination of fluoride has been adapted for use with optical fibres. The reagent was immobilized on a polymer matrix, Amberlite XAD-2, and the reflectance of this reagent phase was measured as a function of fluoride concentration by use of a flow-cell assembly and a bifurcated fibre-optic system. A linear response was obtained for 0.16-0.95mM fluoride at a pH of 4.1, with a response time of approximately 12 min.     

Indirect Spectrophotometric Determination of Fluoride In Water With Zirconium-Spadns By Flow Injection Analysis

Abstract

The zirconium-SPADNS method for the determination of fluoride based on the effect of fluoride ion on the color system (Zr-SPADNS), has been adapted to the continuous flow spectrophotometry. A manifold consisting of two lines was used. the decrease in the absorbance of Zr-SPADNS reagent at 590 nm is linear with fluoride concentration in the range 0.00-3.5 ppm. the method has a detection limit of 0.02 ppm fluoride. At a sampling rate of 50 determinations per hour, the precision was about 1% relative standard deviation. the method is applied to the determination of fluoride in natural water samples. the good agreement between the results obtained by this method and those obtained by a potentiometric method using a fluoride ion-selective electrode, show that the new method is potentially suitable for routine analysis. the effects of reaction conditions, flow parameters, and interferences on the FIA-spectrophotometric signals are reported. amount of interfering ion is present in quantity great enough to produce an error of 0.1 ppm or more, the sample must be distilled¹⁷     

Chemiluminescence investigation of NH(2)OH-fluorescein-Cu(2+) system and its application to copper analysis in serum

A novel chemiluminescent system, fluorescein-NH(2)OHOH(-), was developed for the determination of copper(II) in serum. A weak light emission arises from hydroxylamine in the presence of the organic reagent fluorescein in basic aqueous solution. Under the conditions of 1.2 x 10(-3) mol l(-1) NH(2)OH and 5 x 10(-3) mol l(-3) fluorescein, the light intensity is linearly dependent upon the concentration of copper(II) within the range 1-20 ppb. The relative standard deviation of the determination of copper(II) is 4.2% (n = 13) and the detection limit is 0.5 ppb. The system is highly selective for copper except in the presence of iron(II,III) and cobalt(II). In conjunction with potassium fluoride as masking agent, the method was successfully applied to the determination of microamounts of copper(II) in serum. A mechanistic study of the chemiluminescence reaction is also discussed.     

A novel method for the determination of total protein in human serum by near infrared fluorescence recovery

A novel fluorometric method has been developed for the determination of total protein in human serum with a new near-IR reagent as a fluorescence probe, based on the fluorescence recovery of the cyanine-CTAB system in the presence of protein. Maximum fluorescence is produced with maximum excitation and emission wave-lengths at 765 and 812 nm, respectively. Under optimal conditions, the calibration graphs are linear over the range 0.4-12.0 microg/mL for protein. The detection limit is 70 ng/mL, and the relative standard deviation of six replicate measurements is 1.14% for 6.0 microg/mL protein. The results are satisfactory.     

Determination of salbutamol using on-line solid-phase extraction and sequential injection analysis. Comparison of chemiluminescence and fluorescence detection

Determination of salbutamol using sequential injection analysis (SIA) with chemiluminescence and fluorescence detection has been devised. The chemiluminescence signal was emitted during the oxidation of salbutamol by potassium permanganate in sulfuric acid medium. Sodium polyphosphate was used as chemiluminescence enhancer. The fluorescence signal (excitation wavelength 230 nm) was also measured in sulfuric acid medium. Both detection techniques were compared with respect to the application of the methods to the determination of salbutamol in biological materials. The sample pre-treatment takes place directly in the SIA system, when salbutamol is adsorbed on the solid-phase (Baker-carboxylic acid) microcolumn integrated into the system. Sulfuric acid serves both as the reagent and the eluent. The lab-made SIA system consisted of a 2.5-mL Cavro syringe pump, ten-port Vici Valco selection valve and Spectra-Physics FS 970 fluorescence detector, which was lab-modified for chemiluminescence detection. The system was controlled by a PC using originally compiled LabVIEW-supported software. Concentrations, volumes of reagents and flow rates were optimised by a simplex method. Salbutamol was determined in the linear range 0.05-10 microg mL(-1) (RSD 1.53%), with the detection limit (3 sigma) 0.03 microg mL(-1) and sample throughput of 42 samples per hour with chemiluminescence detection in standard solutions. The fluorescence detection enabled the determination of salbutamol in standard solutions in the linear range 0.5-100 microg mL(-1) (RSD 2.69%), with the detection limit 0.2 microg mL(-1) and sample throughput of 24 h(-1). The proposed methods were applied to the determination of salbutamol in human serum and urine. However, serum is a very complicated matrix and the SIA-SPE analysis did not provide satisfactory results. It was possible to determine salbutamol in human urine using this technique. Better recovery was achieved with fluorescence detection.     

Determination of microgram amounts of metals by chronometric analysis

The reaction between peroxidisulphate and iodide, modified by the addition of thiosulphate to show the Landolt effect, has been used for the determination of copper and iron in the range 1-100 mug ml , based on the catalytic effect of these ions. The procedure is rapid and simple, and the errors are less than 10%. The interference from iron in the determination of copper may be overcome by the addition of a masking reagent such as fluoride.     

Fluorometric determination of khellin in human urine and serum by high-performance liquid chromatography using postcolumn photoirradiation.

For the determination of khellin in urine and serum, fluorometry using HPLC-postcolumn photoirradiation has been developed. Khellin and visnagin of similar structure were separated on a column of Capcell Pak C8. The mobile phase consisted of 40%(v/v) ethanol containing 75 mmol l(-1) H2O2. The postcolumn reagent, 70 mmol l(-1) KH2PO4-NaOH buffer (pH 12.7) containing 50%(v/v) ethanol, were mixed with the mobile phase, which was irradiated with ultraviolet light to induce fluorescence. The fluorescence was monitored with excitation at 378 nm and emission at 480 nm. The calibration graph for khellin was linear over the range of 65 - 2620 ng ml(-1) using an injection volume of 20 microl. The pretreatment of the urine or serum samples consisted of diluting steps or deproteinizing steps using perchloric acid, respectively.     

以1,4-二甲基咔唑-9-丙酸为荧光衍生化试剂高效液相色谱法测定醇

1,4-二甲基咔唑-9-丙酸与间苯二磺酰氯反应生成混合酸酐,该混合酸酐能够衍生化18个碳以下的直链脂肪伯醇、6个碳以下的仲醇,以及叔丁醇和胆固醇;将荧光衍生物用反相C18液相色谱柱进行分离,在室温下10min完成衍生化反应,衍生物24h内基本稳定.基于此,建立了血清中醇的高效液相色谱测定方法.     

基于无标记的核酸适配体荧光生物传感器检测凝血酶

设计了一个简单、通用、基于核酸适配体无标记的高敏感、高专一检测凝血酶的荧光方法。以无标记凝血酶核酸适配体单链DNA为识别元素,Pico Green染料传导互补双链的荧光信号。Pico Green是一种不对称菁,当其单独存在时不产生荧光信号,而当其被吸附到互补的双链DNA上时,可产生很强的荧光信号,但被吸附到单链DNA上时,却无明显的信号改变。基于该性质,将其用于凝血酶的检测。该方法对凝血酶的响应线性范围为1.0×10~(-14)~1.0×10~(-7)mol/L,相关系数(r~2)为0.99,检出限为1.0×10~(-14)mol/L。1.0×10~(-8)mol/L两种干扰物质(牛血清蛋白和细胞色素C)的存在不影响凝血酶的检测,表明该方法对凝血酶具有非常好的专一性。该方法成功应用于对人血清样品的检测,其平均回收率为97%~102%。方法可简单、灵敏、特异性地检测凝血酶,有望用于医学临床诊断等领域。     

荧光猝灭法测定超氧阴离子自由基的研究

合成了一种新的荧光探针试剂香草醛缩苯胺,利用元素分析、红外光谱等手段对探针试剂进行结构表征;结合邻苯三酚的自氧化作用,建立了一种荧光法测定超氧阴离子自由基(O_2~(-·))的新方法.该方法具有操作简单、灵敏度高和选择性好等特点.邻苯三酚线性范围为4.0×10~(-6)～1.0×10~(-5) mol·~(-1).检出限为2.0×10~(-7) mol·~(-1).方法用于大蒜等样品中超氧化物歧化酶(SOD)活性检测,结果满意.     

An enzymatic assay of chloramphenicol coupled with fluorescence reaction

An alternative method for the assay of chloramphenicol using an enzymatic reaction coupled with a fluorescence detection system has been developed. Chloramphenicol was enzymatically acetylated by chloramphenicol acetyltransferase in the presence of acetyl-coenzyme A (acetyl-CoA) as the acetyl-donor, after which the liberated CoA-SH was derivatized with a fluorogenic reagent, 4-(aminosulfonyl)-7-fluoro-2,1,3-benzoxadiazole. The assay was linear over the range of 2.5-40 micrograms/ml. Analytical recoveries of chloramphenicol at concentrations of 7.5 and 22.5 micrograms/ml, added to human serum, plasma, or a slightly hemolyzed serum, were in the range of 93.3 to 106.2%. The enzymatic assay was not affected by the presence of ten other antibiotics tested.