Carbon Paste Electrode Incorporating 1‐[4‐(Ferrocenyl Ethynyl) Phenyl]‐1‐Ethanone for Electrocatalytic and Voltammetric Determination of Tryptophan

A carbon paste electrode spiked with 1‐[4‐ferrocenyl ethynyl) phenyl]‐1‐ethanone (4FEPE) was constructed by incorporation of 4FEPE in graphite powder‐paraffin oil matrix. It has been shown by direct current cyclic voltammetry and double step chronoamperometry that this electrode can catalyze the oxidation of tryptophan (Trp) in aqueous buffered solution. It has been found that under optimum condition (pH 7.00), the oxidation of Trp at the surface of such an electrode occurs at a potential about 200 mV less positive than at an unmodified carbon paste electrode. The kinetic parameters such as electron transfer coefficient, α and rate constant for the chemical reaction between Trp and redox sites in 4FEPE modified carbon paste electrode (4FEPEMCPE) were also determined using electrochemical approaches. The electrocatalytic oxidation peak current of Trp showed a linear dependent on the Trp concentrations and linear calibration curves were obtained in the ranges of 6.00×10^?6 M–3.35×10^?3 M and 8.50×10^?7 M–6.34×10^?5 M of Trp concentration with cyclic voltammetry (CV) and differential pulse voltammetry (DPV) methods, respectively. The detection limits (3σ) were determined as 1.80×10^?6 M and 5.60×10^?7 M by CV and DPV methods. This method was also examined as a selective, simple and precise new method for voltammetric determination of tryptophan in real sample.     

Simultaneous determination of tyrosine and tryptophan by mesoporous silica nanoparticles modified carbon paste electrode using H-point standard addition method

A simple, selective and sensitive sensor based on mesoporous silica nanoparticles modified carbon paste electrode (MSNs/CPE) is introduced for electrochemical determination of tyrosine (Tyr) and tryptophan (Trp). Compared with the unmodified electrode and commercial SiO₂ modified electrode (SiO₂/CPE), the oxidation peak current significantly improved for both amino acids. Under optimized experimental conditions, the oxidation peak current of Trp was linear over a concentration range of 5.0 × 10⁻⁸ to 4.0 × 10⁻⁴ M with a detection limit of 3.4 × 10⁻⁸ M. The oxidation peak current of Tyr was linear over a concentration range from 5.0 × 10⁻⁷ to 6.0 × 10⁻⁴ M with a detection limit of 1.5 × 10⁻⁷ M. For simultaneous determination Trp and Tyr, H-point standard addition method was applied to resolve the overlapping of differential pulse voltammetric peaks of Trp and Tyr. The results showed that the method was successfully applied to the simultaneous determination of Trp and Tyr in some synthetic samples. Moreover, the applicability of the method was demonstrated by the recovery tests of Trp and Tyr in artificial urine.     

A fluorescence spectroscopic study of a coagulating protein extracted from Moringa oleifera seeds

The fluorescence studies of coagulating protein extracted from Moringa oleifera seeds have been studied using steady-state intrinsic fluorescence. The fluorescence spectra are dominated by tryptophan emission and the emission peak maximum (lambda(max)=343+ or -2nm) indicated that the tryptophan residue is not located in the hydrophobic core of the protein. Changes in solution pH affected the protein conformation as indicated by changes in the tryptophan fluorescence above pH 9 whereas the ionic strength had minimal effect. The exposure and environments of the tryptophan residue were determined using collisional quenchers.     

Construction of Protein Probe with a His-tag and an Electron-transfer Peptide for a Target Protein Sensing

A protein probe with an electron-transfer peptide and a His-tag was designed to electrochemically sense a target protein. We selected tyrosine-rich (Y₄C) and tryptophan-rich (W₄C) peptides for use as electron-transfer agents. The peak for oxidation was based on the oxidations of the phenolic hydroxy groups in Y₄C and on the indole rings in W₄C. Asialofetuin (ASF) with galactose residues was the protein probe, and a galactose recognition protein, soybean agglutinin (SBA), was the target protein. A protein probe composed of an amino acid and carbohydrate residue was expected to be biocompatible. When voltammetric measurements were performed using a glassy carbon electrode, the oxidation peaks of H₆Y₄C and ASF-H₆Y₄C appeared at the same potential. The peak current of ASF-H₆Y₄C was 4-fold that of H₆Y₄C because of the stronger adsorption of ASF-H₆Y₄C onto the electrode. The electrode response of ASF-H₆Y₄C with SBA was half that of ASF-H₆Y₄C alone. By contrast, the peak current of ASF-Y₄CH₆ was higher than that of ASF-H₆Y₄C, which was the result of a greater degree of contact between the Y₄C moieties and an electrode. On the other hand, the voltammetric behaviors of ASF with W₄C and a His-tag were similar to those with Y₄C and a His-tag. The sensitivity of SBA using ASF-Y₄CH₆ was at the 10⁻¹³ M level. To confirm the function of the sensing system, measurements were performed in human serum with SBA and ASF-Y₄CH₆. When SBA was added, the serum had a concentration that ranged between 5.0×10⁻¹³ and 4.0×10⁻¹² M, and the amount of SBA that could be recovered ranged from 97 to 101%. Consequently, this system could be applied to the detection of SBA in serum.     

乙腈-水和乙二醇-水均相溶液中光诱导杜醌激发三重态与色氨酸、酪氨酸的氢原子转移反应

本文用激光闪光光解技术研究了光诱导生物醌杜醌激发三重态(³DQ^*)和色氨酸(Trp)与酪氨酸(Tyr)在乙腈-水(MeCN-H₂O)及乙二醇-水(EG-H₂O)均相溶液中的光化学反应,分析了反应的机理,并基于Stern-Volmer方法测量了反应速率常数. 光解DQ体系可以生成³DQ^*,³DQ^*与Trp、Tyr发生的氢原子转移反应占主导地位. 对于DQ/Trp/MeCN-H₂O和DQ/Trp/EG-H₂O溶液,³DQ^*与Trp反应生成杜醌中性自由基DQH^·、以碳为中心的色氨酸中性自由基Trp^·/NH和以氮为中心的色氨酸中性自由基Trp/N^·. 对于DQ/Tyr/MeCN-H₂O和DQ/Tyr/EG-H₂O溶液,³DQ^*与Tyr反应生成DQH^·和酪氨酸中性自由基Tyr/O^·. ³DQ^*与Trp、Tyr的氢原子转移反应速率常数都在10⁹ L·mol^-1·s^-1量级,反应近似受扩散控制. MeCN/H₂O均相溶液中³DQ^*与Trp、Tyr的反应速率常数要明显高于EG/H₂O均相溶液中的反应速率常数,这与Stokes-Einstein方程定性一致.     

Simultaneous determination of aromatic amino acids in human blood plasma by capillary electrophoresis with UV‐absorption detection

Phenylalanine, tyrosine, and tryptophan, also known as aromatic amino acids, are involved in many physiological and pathophysiological conditions and are indicative of the liver and kidney function. In this work, we describe a simple and accurate method for their simultaneous quantification, in a single capillary electrophoresis run. This method requires minimal sample manipulation, no derivatization procedures, and methyl tryptophan as internal standard. The human blood plasma sample was precipitated using sulfosalicylic acid and the supernatant was used for the analysis. All the analytes were baseline resolved within 16 min and detected at 200 nm using Tris phosphate 80 mmol/L at pH 1.4 as the background electrolyte. The proposed method showed good linearity (r = 0.998) and repeatability (intra‐assay RSD < 2.78%, interassay RSD < 5.4%) for all the analytes. The limit of quantification was 13 μmol/L for phenylalanine and 5 μmol/L for tyrosine and tryptophan. The method suitability was tested measuring aromatic amino acids level in 20 chronic kidney disease patients at basal level and after simvastatin/ezetimibe treatment.     

辅酶NADH与色氨酸共振能量转移的荧光动力学研究

采用时间相关单光子计数技术, 结合紫外-可见吸收光谱和稳态荧光光谱, 对不同环境下的色氨酸和辅酶还原型烟酰胺腺嘌呤二核苷酸(NADH)之间的共振能量转移荧光动力学进行了研究. 单体色氨酸、 牛血清白蛋白以及乳酸脱氢酶蛋白与NADH之间相互作用的光谱数据表明, 只有存在NADH结合位点的乳酸脱氢酶和NADH之间发生了荧光共振能量转移. 进一步通过加入丙酮酸来阻断乳酸脱氢酶和NADH之间的荧光共振能量转移通道, 时间分辨荧光光谱和衰减相关光谱(DAS)证实, 蛋白结合位点的存在是NADH和色氨酸之间发生荧光共振能量转移的前提条件. DAS揭示了乳酸脱氢酶平均荧光寿命的减小主要是源于色氨酸中7.35 ns的荧光寿命成分与NADH之间的荧光共振能量转移, 同时给出了NADH和色氨酸之间的能量转移效率, 为研究NADH和蛋白之间的相互作用提供了新思路.     

Simultaneous determination of tryptophan, kynurenine, kynurenic and xanthurenic acids in honey by liquid chromatography with diode array, fluorescence and tandem mass spectrometry detection

A liquid chromatography method using diode array-fluorescence detection and atmospheric pressure chemical ionization mass spectrometry (LC-DAD-FLD and LC–APCI-MS/MS) was developed to quantify the levels of tryptophan (TRP), kynurenine (KYN), kynurenic (KYNA) and xanthurenic (XA) acids in honey. This procedure involved isolating the compounds of interest via solid-phase extraction (SPE) with mixed-mode polymeric cartridges. Chromatographic separation of the analytes was performed in isocratic mode on a Synergi 4μ Hydro-RP 80Å (150 × 4.60 mm i.d.) analytical column at 30 °C. The mobile phase of 20 mM ammonium formate (pH 4) and methanol was passed at a flow rate of 0.5 mL/min. In replicate sets of spiked honey samples, the average analyte recoveries ranged from 60 to 98% for TRP, 55 to 120% for KYN, 65 to 106.5 for KYNA and 56 to 114% for XA. Detection limits ranged from 4 to 36 μg/kg for LC-DAD-FLD to 0.2 and 1.0 μg/kg for LC–APCI-MS/MS. A strong matrix effect was found when MS/MS was employed, necessitating calibration using the standard addition method on matrix-matched standards for each honey type. The method was used to quantify each of the compounds of interest in 17 honey samples of distinct botanical origins.     

Simultaneous determination of ascorbic acid,dopamine, uric acid and tryptophan on gold nanoparticles/overoxidized-polyimidazole composite modified glassy carbon electrode

A novel electrode was developed through electrodepositing gold nanoparticles (GNPs) on overoxidized-polyimidazole (PImox) film modified glassy carbon electrode (GCE). The combination of GNPs and the PImox film endowed the GNPs/PImox/GCE with good biological compatibility, high selectivity and sensitivity and excellent electrochemical catalytic activities towards ascorbic acid (AA), dopamine (DA), uric acid (UA) and tryptophan (Trp). In the fourfold co-existence system, the peak separations between AA–DA, DA–UA and UA–Trp were large up to 186, 165 and 285 mV, respectively. The calibration curves for AA, DA and UA were obtained in the range of 210.0–1010.0 μM, 5.0–268.0 μM and 6.0–486.0 μM with detection limits (S/N = 3) of 2.0 μM, 0.08 μM and 0.5 μM, respectively. Two linear calibrations for Trp were obtained over ranges of 3.0–34.0 μM and 84.0–464.0 μM with detection limit (S/N = 3) of 0.7 μM. In addition, the modified electrode was applied to detect AA, DA, UA and Trp in samples using standard addition method with satisfactory results.     

Synthesis of Ruthenium Xanthate Complex and Its Electrocatalytic Activity for Tryptophan Oxidation

A new ruthenium complex containing bidentate xanthate ligands was synthesized in a good yield. This complex was characterized by elemental analysis, proton nuclear magnetic resonance(¹H NMR), Fourier transform infrared(FTIR) and UV-Vis spectroscopies. The cyclic voltammetry of the complex revealed one quasi-redox wave centered at Ru(Ⅲ)/ Ru(Ⅱ) couple, indicating its catalytic potential. So the preparation of a glass carbon electrode modified with ruthenium xanthate complex and its electrocatalytic activity toward the oxidation of tryptophan(Trp) were also studied. The experimental results show that the modified electrode had excellent electrocatalytic activity for the oxidation of tryptophan. Moreover, under the optimized conditions, the oxidation peak current was proportional to tryptophan concentration in a range of 2.5×10^-7 to 5.0×10^-5 mol/L with a correlation coefficient of 0.9928 and a detection limit of 8.3×10^-8 mol/L(S/N=3). Using the proposed method, tryptophan was successfully determined in pharmaceutical samples with standard addition method.