Derivatisation of sympathomimetics with primary amino groups on thin-layer plates by spotting the sample spots with fluorescamine

Summary A method has been developed for the quantitative determination of sympathomimetics containing a primary amino group on thin-layer plates with fluorescamine. The reaction is carried out by spotting fluorescamine solution in acetone on top of the sample spots. The fluorescamine derivatives are subsequently separated using appropriate solvent systems. Spotting a buffer before reaction and spraying with triethanolamine after development is unnecessary. The consumption of reagent is extremely low. For ten thin-layer plates with ten sample spots per plate only 0.2 cm³ reagent solution are needed. The method has been applied to the quantitative determination of some compounds with primary amino groups in pharmaceutical preparations.Dedicated to Prof. Dr. G. Zigeuner on his 60^th birthday.     

A Chemical Ionization Mass Spectrometric Study of Fluorescamine and Fluorescamine - Amino Acid Derivatives

Abstract

The chemical ionization mass spectra of fluorescamine and fluorescamine - amino acid derivatives have been studied using methane and ammonia as reagent gases. Major ions in the spectra are protonated molecular ions, adduct ions and ions formed by loss of an oxygen atom.

Fluorescamine, 4-phenyl-spiro[furan-2(3H),1′-phthalan]3,3′-dione, is a powerful new fluorogenic reagent for assaying primary amines.¹ and EI² and EI³ mass spectrometric investigations of fluorescamine and its derivatives were carried out. Our present study reports the CI mass spectral analysis of fluorescamine and some of its amino acid derivatives.     

Discrimination of Primary Amines from Other Fluorescent Compounds in Biological Fluids

Abstract

Experimental condition and parameters involved in HPLC distinction of primary amines from non-primary amine compounds with native fluorescence were investigated. The discrimination conditions were designed to enable utilization of the sensitive reagent fluorescamine as a means of monitoring primary amines in physiologic fluids.     

Studies on Fluorescamine. Part II - Thin-Layer Chromatographic Mobilities of Fluorescamine Positive Drugs

Abstract

Fluorescamine reacts with primary amines, it does not react with secondary or tertiary amines, to yield bright acquamarine fluorescent products. This reaction has been developed into a spot test useful for differentiation of amphetamine from methamphetamine; previous spot tests did not have this degree of specificity. The fluorescent products of several primary amines have been demonstrated to have sufficient stability to permit thin-layer chromatography comparisons with authentic materials. The fluorescent derivative of amphetamine has been demonstrated to be capable of differentiation from other fluorescent products formed from fluorescamine based on its unique migration in three different TLC systems.     

Optimization of analytical conditions and validation of a fluorescence method for the determination of sulfadiazine in milk

This paper describes optimization and validation of a method for sulfadiazine determination in milk samples based on sulfadiazine derivatization with fluorescamine followed by excitation–emission (fluorescence) measurement. For both the optimization and the validation, a comparison between zero-order and first-order signals has been made, showing the advantages of using first-order signals. In the optimization the effects of the temperature of the derivatization reaction, the amount of fluorescamine and the derivatization time on the instrumental signal (maximum intensity or the net analyte signal) are studied by a factorial experimental design, with the optimal values of these factors which give the highest signal being 22 °C for the reaction temperature, 50 μl fluorescamine and 20 min of derivatization time. The validation of the method under the optimal experimental conditions shows that the analytical method is fit-for-purpose, with values of the capability of detection (CCβ) of 4.3 μg l⁻¹ at a sulfadiazine concentration of zero and with probabilities of a false positive and a false negative of 5%. Around the permitted limit (established for the sulfonamides at 100 μg l⁻¹), CCβ is 112 μg l⁻¹. The precision, as the intermediate reproducibility, was established as 1.2 and 3.3 μg l⁻¹ around 0 and 100 μg l⁻¹, respectively. In the application to milk samples spiked with sulfadiazine a mean recovery of around 90% was obtained with a standard deviation of about 8% (14 samples of different concentrations).     

A biacylhydrazone-based chemosensor for fluorescence ‘turn-on’ detection of Al3+ with high selectivity and sensitivity

A simple Al³⁺ fluorescent chemosensor (1) based on diacylhydrazone has been designed and synthesized by the condensation reaction of 2-hydroxy naphthaldehyde and metaphthalic hydrazide. The chemosensor 1 displays a specific and sensitive response to Al³⁺ over other cations in DMSO solution. Upon the addition of DMSO solution of Al³⁺, the sensor 1 shows an immediate fluorescence ‘turn-on’ response and emitting strong blue emission with visible color change from colorless to green. The fluorescence quantum yield enhanced from 7.24% to 48.68%. Meanwhile, the fluorescence and UV absorption spectra detection limits of the chemosensor 1 for Al³⁺ were 2.0 × 10^?7 M and 5.6 × 10^?7 M respectively, indicating the high sensitivity of 1 to Al³⁺. Furthermore, test strips based on 1 were fabricated, which could be used as a convenient test kit for the detection of Al³⁺ and an efficient Al³⁺ controlled fluorescent security display materials.     

Urinary Tyramine Assay by High-Performance Liquid Chromatography

Abstract

An assay for urinary tyramine based on its reaction with fluorescamine and subsequent separation on reverse phase column has been described. The method is simple, sensitive and free from interferences. Patients with neuroblastoma, pheochromocytoma and Parkinson's disease have elevated levels of urinary tyramine.     

HPLC Assay for S-2-(3-Aminopropylamino)ethyl Phosphorothioate (WR 2721) in Plasma

Abstract

A specific HPLC assay has been developed for determination of the radioprotective drug WR 2721. The method is based on precolumn derivatization of plasma with fluorescamine, separation with a C-18 cartridge and detection by fluorescence. An external standard was used for calibration, and values were adjusted based upon recovery of added ¹⁴C-labeled WR 2721. WR 2721 had a retention time of about 13 minutes using a mobile phase of acetonitrile/water (22:78), 0.01 M in dibutylammonium phosphate, at a flow rate of 2 mL/min. Sensitivity of the assay was characterized to 2 μg/mL, and detector response was linear over the range of 2 to 1100 μg/mL. The assay requires 90 μL of plasma and has a total chromatography time of about 45 minutes. 2-(3-Aminopropylamino)ethanethiol (WR 1065) and bis- [2- (3-aminopropylamino)ethyl]disulfide (WR 33278), metabolites of the drug, and a variety of primary amines were shown not to interfere with the assay. Suitability of this assay for pharmacokinetic studies was demonstrated in preliminary experiments with a beagle dog.     

A Fluorometric Method for Cyanogen (C2N2) with No Cyanide Interference

Abstract

A fluorometric method for the analysis of cyanogen (C₂N₂, ethanedinitrile) without cyanide interference is described the procedure is based on the reaction of C₂N₂ with hexamethylenetetramine (HMTA) to produce a fluorophor. the fluorescence yield is linear over a range of 3–4 orders of magnitude. the method is comparable in detection limits to CN^? measurements done electrochemically; in this case >10^?2?<10^?5 M. Many anions and cations were examined for interference; only transition and heavy metal compounds reduced fluorescence. Certain amines may interfere, although all examined reacted much slower than the HMTA.     

双态发光三苯胺基有机硼配合物的设计、合成与应用

以三(4-溴苯)胺、4-氨基苯硼酸频哪醇酯、4-二乙氨基水杨醛和三氟化硼乙醚溶液为原料,经过Suzuki偶联反应、缩合反应和配位反应,设计、合成了一种新型三枝结构的三苯胺有机硼配合物(TPAB),使用 ¹H和 ¹³C NMR对 TPAB的结构进行了表征,通过紫外可见吸收光谱和荧光发射光谱详细研究了TPAB溶液和固体态的光物理性能以及不同的外部条件对其发光性能的影响。发现 TPAB溶液和固体态都具有较强的荧光发射,在四氢呋喃溶液中的吸收峰位于 417 nm,发射峰位于 548 nm,荧光量子产率为 40.49%,荧光寿命为 1.72 ns;TPAB 固体的荧光发射峰位于 582 nm,荧光量子产率为 11.43%,荧光寿命为 0.72ns,表明TPAB具有优良的双光发光性能。此外,TPAB具有良好的发光稳定性,不受pH、金属离子、氨基酸和压力的影响。基于化合物优异的发光性能,将其应用于荧光细胞成像,在肝癌细胞(HepG2)中表现出良好的单光子和双光子荧光成像效果。     

双态发光三苯胺基有机硼配合物的设计、合成与应用

以三(4-溴苯)胺、4-氨基苯硼酸频哪醇酯、4-二乙氨基水杨醛和三氟化硼乙醚溶液为原料,经过Suzuki偶联反应、缩合反应和配位反应,设计、合成了一种新型三枝结构的三苯胺有机硼配合物(TPAB),使用¹H和¹³C NMR对TPAB的结构进行了表征,通过紫外可见吸收光谱和荧光发射光谱详细研究了TPAB溶液和固体态的光物理性能以及不同的外部条件对其发光性能的影响。发现TPAB溶液和固体态都具有较强的荧光发射,在四氢呋喃溶液中的吸收峰位于417 nm,发射峰位于548 nm,荧光量子产率为40.49%,荧光寿命为1.72 ns; TPAB固体的荧光发射峰位于582 nm,荧光量子产率为11.43%,荧光寿命为0.72ns,表明TPAB具有优良的双态发光性能。此外,TPAB具有良好的发光稳定性,不受pH、金属离子、氨基酸和压力的影响。基于化合物优异的发光性能,将其应用于荧光细胞成像,在肝癌细胞(HepG2)中表现出良好的单光子和双光子荧光成像效果。     

A sequential injection fluorometric procedure for the determination of procaine in human blood and pharmaceuticals

An automated procedure for the assay of procaine hydrochloride in human blood and pharmaceuticals was developed using a sequential injection (SI) technique with fluorometric detection and fluorescamine as the fluorescence probe. A few microliters of fluorescamine and procaine hydrochloride solutions were used in the SI system leading to the formation of a derivative, which was then excited by a 400-nm LED and whose emitted fluorescence was monitored at a wavelength of 494 nm. A linear calibration graph was obtained with 10–200 ng mL⁻¹ (procaine) by loading 10.0 μL of sample solution and 5.0 μL of fluorescamine solution (both 0.125 % m/v). A detection limit of 2.6 ng mL⁻¹, defined as 3 times the blank standard deviation (3σ), was achieved along with a sampling frequency of 25 h⁻¹ and a precision of 2.1 % RSD at the 50.0 ng mL⁻¹ level. Procaine contents in injection solutions from various pharmaceutical manufactures were analyzed and reasonable agreement was achieved between the values obtained by using the present procedure and the documented spectrophotometry, and both were coincident with the nominal concentrations. In addition, the degradation of procaine in human blood was investigated. A fast degradation of procaine in human blood was observed for the first 30 min, while afterwards the degradation was retarded.     

Determination of 1-aminocyclopropane-1-carboxylic Acid in Apple and Peach Extracts by High Performance Liquid Chromatography Coupled to a Fluorescence Detector

A new, sensitive, and simple HPLC method was described for the determination of 1-aminocyclopropane-1-carboxylic acid (ACC) in apple and peach extracts. The method was based on the derivatization of ACC with fluorescamine in borate buffer systems of pH 8.0 to yield a highly fluorescent product. The experimental parameters affecting the derivatization reaction efficiency were optimized by fluorimetric analysis. Under optimum derivatization conditions, the derivative product of ACC in apple and peach extracts without extra purification was successfully chromatographed on a C-18 column by HPLC coupled to fluorescence detection. The derivative product of ACC with fluorescamine could be well separated from other concomitant substances or their derivatives that might interfere with the determination of ACC. The linearity of ACC was measured in the range of 23.82–238.82 µg · L^?1 with a good correlation coefficient of 0.9997. Based on signal-to-noise ratio of 3, a low detection limit of 5.0 µg · L^?1 could be reached. The proposed method was applied successfully to the determination of ACC in the crude apple and peach extracts without extra purification with low RSDs of 0.19–1.9% and good recoveries of 90.89–104.4%. The sensitive HPLC quantitative method is of great significance for the investigations of ACC metabolism in plants.     

A sequential injection fluorometric procedure for rapid determination of total protein in human serum

A sensitive procedure for the quantification of total protein bovine serum albumen (BSA) in human serum was presented with sequential injection sampling and fluorometric detection. A few microliters of sample and fluorescamine solutions were aspirated into the holding coil to facilitate the reaction of protein with fluorescamine by giving rise to a blue-green-fluorescent derivative. The derivative was afterwards excited by a 400 nm radiation from a UV radiator, and the emitted fluorescence was monitored at the wavelength of 470 nm. By loading 5.0 μl of sample and 4.0 μl of fluorescamine solution 0.075% (m/v), a linear calibration graph was obtained within 0.3-12.5 μg ml⁻¹, and a detection limit (3σ) of 0.1 μg ml⁻¹ was achieved, along with a sampling frequency of 40 h⁻¹ and a R.S.D. value of 2.1% at the 5.0 μg ml⁻¹ levels. Protein contents in human serums were analyzed by using the present procedure, and reasonable agreements were obtained with those obtained by a documented spectrophotometric (Biuret) method.     

Colorimetric Determination of Surfactants Using Lipase

Abstract

The inhibition effect of a surfactant on an enzymic reaction of lipase was investigated to determine small amounts of the surfactant. Surfactants could be determined by colori-metrically measuring the degree of their inhibition in the enzymic reaction. By the method studied, 10–200 ppm of LAS, 25–300 ppm of ABS, 10² ?10³ ppm of SDS, and 1–10% of polyethyleneglycol dodecyl ether and polyethylene glycol octylphenyl ether could be determined with coefficient of variance of about 2%.     

Methods for the determination of the number of polytetrahydrofuran branches in neoprene-g-polytetrahydrofuran

Methods for the determination of the number of the number of polytetrahydrofuran branches in neoprene-g-polytetrahydrofuran were examined. Only two suitable methods were found; namely, termination of oxonium ions by triphenylphosphine followed by ³¹P-NMR and termination with NH₄OH? NH₄Cl buffer and reaction with fluorescamine followed by fluorescence spectroscopy. Both methods led to the conclusion that Neoprene W has 9 ± 1 active halogens per mole that can be used to initiate tetrahydrofuran polymerization when silver salts are added. Among the methods examined in this study the fluorescence method was the most reliable, most reproducible, fastest, and simplest.     

A Simple Simultaneous Colorimetric Determination of Primary and Secondary Amines with Fluorescamine

Abstract

Primary and secondary amines react reproducibly with fluorescamine to form pyrrolinones or aminoenone type chromophores with long wavelength absorption maxima in the 375–410 and 310–320 nm regions, respectively. A simple procedure has been worked out for the simultaneous colorimetric determination of primary and secondary amines.     

Effect of Substituents on the Reaction of Aromatic Primary Amines with Fluorescamine

Abstract

The effects of substituents on the reactivity of the monosubstituted anilines with fluorescamine (FLA) and the fluorescent properties of the reaction products, FI (Ph), were investigated. Generally, the substituent at o-position markedly inhibited the reactivity of the amino group (ortho-effect). While the electron-donating substituent seemed to be favorable for the formation of FI (Ph), the electron-attracting one seemed to lower reactivity of the amino group. However, the presence of the latter substituent led to the enhanced fluorescence of FI (Ph). The highly significant correlation was observed between the wavelengths (nm) of the emission maxima and the Hammett's substituent constants.     

A Superacid-catalyzed Synthesis of Fluorescent Covalent Triazine Based Framework Containing Perylene Tetraanhydride Bisimide for Sensing to O-nitrophenol with Ultrahigh Sensitivity

Abstract

A mesoporous covalent triazine framework, PCPDI, was synthesized via an aromatic nitrile trimerization reaction of N,N′-di(4-cyanphenyl)- 3,4,9,10-tetracarboxydiimide (CPDI) by CF₃SO₃H catalyzed at 40?°C and this method avoids the use of noble metal catalyzers or high temperature reaction. PCPDI exhibits high thermal stability and strong fluorescence. The PCPDI shows ultrahigh sensitivity to tracing o-nitrophenol in chloroform with K_SV constant of 1.74?×?10⁵ L mol^?1 and detection limit (LOD) of 1.72?×?10^?11?mol L^?1.     

1-(水杨醛)-5-(香草醛)缩卡巴肼丁基锡配合物的合成、结构、谱学性质和除草活性

卡巴肼分别与水杨醛和香草醛缩合制备1,5-不对称二取代卡巴肼配体,在甲醇溶剂热中,正丁基三氯化锡与配体反应,合成1-(水杨醛)-5-(香草醛)缩卡巴肼丁基锡配合物(B1)和含N,N′-双水杨醛缩连氮分子的丁基锡配合物(B2),经元素分析,IR,1H、119Sn、13C NMR和X射线衍射晶体结构表征,配合物(B1)、(B2)晶体分别属单斜晶系、P21/n空间群和三斜晶系、P1空间群,中心锡与配基原子构成六配位畸形八面体构型,配合物(B1)在DMF-H2O溶剂体系中具有良好的荧光性质,当含水0~10%(V/V)时具有聚集荧光增强效应,含水量大于10%,随含水体积分数增加荧光强度减弱,以至最后淬灭。配体及其配合物(B1)对马齿苋、刺苋、决明子、四九菜心和苋菜5种靶标植物均具有一定生长抑制作用,尤其是配体对马齿苋、刺苋的生长有良好的抑制作用,配合物可以选择性抑制决明子的生长,可作为决明子除草剂的候选化合物。