Neurotransmitter amino acid—oxobenzo[f]benzopyran conjugates: synthesis and photorelease studies

A series of fluorescent conjugates of neurotransmitter amino acids, such as β-alanine, tyrosine, 3,4-dihydroxyphenylalanine (DOPA) and glutamic acid, were prepared by reaction with a suitable fluorophore, namely 1-chloromethyl-9-methoxy-3-oxo-3H-benzo[f]benzopyran. The photophysical properties of the resulting ester bioconjugates were evaluated as well as the stability to photolysis at different wavelengths of irradiation (250, 300, 350 and 419 nm).     

Determination of Enantiomeric Excess of Glutamic Acids by Lab-made Capillary Array Electrophoresis

The techniques of combinatorial chemistry have recently been applied to the discovery of new asymmetric catalyst for a variety of organic transformations1-3. Using combina- torial methods, it is straightforward to generate thousands of potential asymmetri…     

2-(2-Pyridyl) benzimidazole based Co(II) complex as an efficient fluorescent probe for trace level determination of aspartic and glutamic acid in aqueous solution: a displacement approach

A weakly fluorescent cobalt(II) complex is synthesized using 2-(2-pyridyl)-benzimidazole (PBI) as a chelating fluorescent ligand and characterized by single crystal X-ray structure. This complex serves as an efficient fluorescent probe for trace level determination of aspartic acid (AspA) and glutamic acid (GluA) in aqueous solution. Rest of the naturally occurring amino acids did not interfere. Both aspartic acid and glutamic acid replaces PBI from the coordination sphere of Co(II)-PBI complex resulting appearance of strong fluorescence signal for the released free PBI. The signal response is very fast and the interaction of both the AspA and GluA with the Co(II) is strong enough as evident from their displacement equilibrium constant values, viz. 4357.8 M(-1) and 8333.33 M(-1) respectively.     

Thermoanalytical study of acid-treated clay containing amino acid immobilized on its surface

The aim of this study is to investigate the incorporation of amino acid molecules in an acid-activated montmorillonite by means of solid characterization after the incorporation of these biomolecules. The acid activation procedure was carried out for the purpose of increasing the acid sites in the clay as well as the impurity elimination in the mineral. Cysteine, aspartic, and glutamic acids were adsorbed on montmorillonite K10 which was previously treated with a hydrochloric acid solution. The clay was put in contact with amino acid solutions at two different concentrations. Each amino acid was adsorbed at identical conditions, with the pH fixed to ensure the charge of molecules and surface clay. The solid was characterized by means of X-ray diffraction, infrared spectroscopy, thermogravimetric analysis, and nitrogen adsorption at 77 K. After the amino acid adsorption, the powders showed changes in their characteristics as well as in their thermal behavior, which depended on both the concentration and the nature of the adsorbed amino acid. The thermal decomposition and elimination of cysteine occurred at a higher temperature than the aspartic and glutamic acid; the complete removal of glutamic acid molecules was not observed at 850 °C. The differences observed in the solid characteristic after the adsorption of each amino acid were discussed. Both the thermoanalytical study and characterization of materials after the interaction with amino acid molecules can be useful to understand the adsorption mechanism of biomolecules on solid surfaces.     

Rapid method for the assay of 4-aminobutyric acid (GABA), glutamic acid and aspartic acid in brain tissue and subcellular fractions

The thin-layer electrophoretic separation at pH 4.8 of brain extracts and a procedure for fluorescent staining of the plates with fluorescamine are described for the rapid routine determination of 4-aminobutyric acid (GABA), glutamic acid and aspartic acid in brain extracts and in particulate fractions of brain tissue. Automated sample application, electrophoretic separation using two chambers, and quantitation by in situ fluorescence scanning allows the assay of 280 samples within three working days. The method is reproducible (S.D. less than 8% of the mean) within the range of 0.2--2 nmole per spot. The staining procedure can be applied to a variety of related analytical problems. The method has proved useful for the determination of the specific radioactivities of GABA, glutamic acid and aspartic acid in metabolic studies.     

Enantioselective chromenone benzoxazole receptor for glutamic acid and its derivatives

Combination of a binaphthyl unit with chromenone benzoxazole fragments provided a chiral receptor that is enantioselective for glutamic acid and its derivatives. The receptor racemic mixture was resolved by TLCs impregnated with (R,R)-thiodilactic acid. High association constants were measured for dansylglutamic acid, using a fluorescent method. This receptor can be used for the resolution of the tosylglutamic acid racemic mixture.     

Carboxylate anion diminishes chloride transport through a synthetic, self-assembled transmembrane pore

Six amphiphilic heptapeptides with the structure (C18H37)2NCOCH2OCH2CO-(Gly)3-Pro-(Gly)n-(Glx)-(Gly)m-O(CH2)6CH3, in which Glx represents glutamic acid or its benzyl ester and n+m=2, have been studied. In addition, the glutamate residue in the GGGPGGE sequence was esterified by fluorescent 1-pyrenemethanol. These compounds insert into phospholipid bilayers and form anion-conducting pores. Hill plots based on carboxyfluorescein release indicate that the pores are at least dimeric. Studies that involved ion-selective electrode techniques showed that transport of chloride varied with the position of glutamate within the peptide chain and whether glutamic acid was present as the free acid or its benzyl ester. Chloride transport activity was significantly higher for the glutamate esters than for free carboxylates irrespective of the glutamate position. Activity was highest when the glutamate residue in approximately (Gly)3-Pro-(Xxx)3 approximately was closest to the C terminus of the peptide. A fluorescent pyrene residue was introduced to probe the aggregation state of the amphiphile. The selectivity of the pore for Cl(-) over K+ was maintained even when the carboxylate anion was present within it. Complexation of Cl(-) by the ionophoric peptides was confirmed by negative ion mass spectrometry. Planar bilayer voltage clamp experiments confirmed that pores with more than one conductance state may form in these dynamic, self-assembled pores.     

Preparation and adsorption properties of phospho‐L‐glutamic acid on hydroxyapatite

Phospho‐L‐glutamic acid was successfully prepared by the phosphorylation of glutamic acid, and its adsorption on synthetic hydroxyapatite (HAP) was studied together with glutamic. The adsorption behaviors of both adsorbates were adequately described by a Langmuirian model. From the comparison between two different adsorbates, the results of the investigation indicated that the phosphate group in phospho‐L‐glutamic acid can greatly enhanced the adsorption affinity for HAP, the improvement of which was achieved through replacing the same group on the surface of HAP and interacting with the surface calcium ion of HAP by electrostatic attraction. The results obtained laid the solid foundation for further research on the regulating function of phosphorylated amino acids with hydroxyapatite biological composites. Copyright © 2010 John Wiley & Sons, Ltd.     

Capillary electrophoretic enantioseparation of basic drugs using a new single‐isomer cyclodextrin derivative and theoretical study of the chiral recognition mechanism

A novel single‐isomer cyclodextrin derivative, heptakis {2,6‐di‐O‐[3‐(1,3‐dicarboxyl propylamino)‐2‐hydroxypropyl]}‐β‐cyclodextrin (glutamic acid‐β‐cyclodextrin) was synthesized and used as a chiral selector in capillary electrophoresis for the enantioseparation of 12 basic drugs, including terbutaline, clorprenaline, tulobuterol, clenbuterol, procaterol, carvedilol, econazole, miconazole, homatropine methyl bromide, brompheniramine, chlorpheniramine and pheniramine. The primary factors affecting separation efficiency, which include the background electrolyte pH, the concentration of glutamic acid‐β‐cyclodextrin and phosphate buffer concentration, were investigated. Satisfactory enantioseparations were obtained using an uncoated fused‐silica capillary of 50 cm (effective length 40 cm) × 50 μm id with 120 mM phosphate buffer (pH 2.5–4.0) containing 0.5–4.5 mM glutamic acid‐β‐cyclodextrin as background electrolyte. A voltage of 20 kV was applied and the capillary temperature was kept at 20°C. The results proved that glutamic acid‐β‐cyclodextrin was an effective chiral selector for studied 12 basic drugs. Moreover, the possible chiral recognition mechanism of brompheniramine, chlorpheniramine and pheniramine on glutamic acid‐β‐cyclodextrin was investigated using the semi‐empirical Parametric Method 3.     

谷氨酸在乳状液膜中的迁移行为

用氯化三等基·甲基铵（Ａｌｉｑｕａｔ ３３６）－Ｓｐａｎ８０－甲苯制成的乳状液膜体系对谷氨酸的迁移行为进行了研究,２ ｍｉｎ的迁移率可达９３％。在谷氨酸的最佳迁移条件下,油溶性好的苯丙氨酸迁移率较高,但油溶性低的甘氨酸和碱性氨基酸的迁移率明显较低。此法适用于微量氨基酸的提取和分离。     

Use of reversed-phase high-performance liquid chromatography for simultaneous determination of glutamine synthetase and glutamic acid decarboxylase in crude extracts

Glutamine and gamma-aminobutyric acid (GABA), formed from glutamic acid in crude tissue extracts by glutamine synthetase and glutamic acid decarboxylase respectively, were separated by derivatization with dansyl chloride followed by reversed-phase high-performance liquid chromatography on the Altex Ultrasphere ODS-5 column. The mobile phase was a gradient of 100 mM potassium dihydrogen phosphate (pH 2.1) with 0-40% acetonitrile. The amounts of glutamine and GABA formed from glutamic acid were determined under different reaction conditions.     

Effect of additives on the amination of 2-oxoglutaric acid by gamma-radiation

The effect of added substances was studied on the yield of glutamic acid produced by gamma-ray irradiation of 2-oxoglutaric acid and ammonia in aqueous solution. The contents of amino acids in the irradiated solutions were determined with amino acids analyzer. Sodium nitrate, allyl alcohol or sodium formate was used as an added substance. The yield of glutamic acid significantly decreased by the addition of nitrate, and it was little affected by the addition of allyl alcohol. In the presence of formate the yield increased from G = 0.4 (2-oxoglutaric acid 0.05M and ammonium hydroxide 2M) to G = 1.1. As a result, it was found that hydrated electron contributes on the formation of glutamic acid, but hydroxyl radical does not. The yield showed a maximum at ca. 0.1 M ammonium hydroxide concentration. These facts indicate that NH2 radical does not contribute to the formation of glutamic acid. As a reaction mechanism, it can be explained that 2-oxoglutaric acid which had been reduced by hydrated electron reacts with ammonia.     

Fragmentation pathway for glutamine identification: Loss of 73 da from dimethylformamidine glutamine isobutyl ester

A fragmentation mechanism for the neutral loss of 73 Da from dimethylformamidine glutamine isobutyl ester is investigated. Understanding this mechanism will allow to improve the identification and quantification of 15N-labeled and unlabeled glutamine and the distinguishing of glutamine and glutamic acid by electrospray ionization (ESI)-tandem mass spectrometry. Before mass spectrometry analysis, glutamine and glutamic acid are derivatized with dimethylformamide dimethyl acetal and isobutanol to form dimethylformamidine isobutyl ester. Derivatization conditions are modified based on an existing method to ensure complete derivatization of glutamic acid and to prevent the hydrolysis of glutamine. The fragmentation mechanism of dimethylformamidine glutamine isobutyl ester is studied and possible fragmentation pathways are proposed. Based on the fragmentation mechanism, a quantification method is developed to quantify both 15N-labeled and unlabeled glutamine and glutamic acid at a series of different neutral losses by performing multiple-reaction monitoring (MRM) scans in a triple-quadrupole mass spectrometer. Labeled glutamine includes 15N-amide labeled, 15N-amine labeled glutamine and glutamine 15N-labeled at both amide and amine positions. Deuterium labeled glutamine and glutamic acid are used as internal standards. Isotope effects are characterized for 15N labeled and deuterium labeled glutamine. It is found that the same method can be used to distinguish aspartic acid from asparagine. This study will improve the application of MS/MS for amino acid quantification and stable isotope labeling metabolism studies.     

Determination and comparison of stability constants of tungsten(VI) and molybdenum(VI) with nitrilotriacetic acid and glutamic acid at different ionic strengths

The formation constants of species formed in the systems H⁺?+?W(VI)?+?nitrilotriacetic acid (NTA) and H⁺?+?NTA have been determined in aqueous solution for pH?=?4–9 at 25°C and different ionic strengths ranging from 0.1 to 1.0?mol?dm^?3 NaClO₄, using potentiometric and spectrophotometric techniques. It was shown that tungsten(VI) forms a mononuclear 1?:?1 complex with NTA of the type WO₃L^3? at pH?=?7.5. The composition of the complex was determined by the continuous variations method. The complexation of molybdenum(VI) with glutamic acid was investigated in aqueous solution ranging in pH from 4 to 9, using polarimetric, potentiometric and spectrophotometric techniques. The composition of the complex was determined by the continuous variations method. It was shown that molybdenum(VI) forms a mononuclear 1?:?1 complex with glutamic acid of the type MoO₃L^2? at pH?=?6.0. The dissociation constants of glutamic acid and the stability constants of the complex were determined at 25°C and at ionic strengths ranging from 0.1 to 1.0?mol?dm^?3 sodium perchlorate. In both complex formation reactions the dependence of the dissociation and stability constants on ionic strength is described by a Debye-Huckel type equation. Finally, a comparison has been made between the patterns of ionic strength dependence for the two complexes and the results have been compared with data previously reported.     

Separation of bonito extract by composite UF membranes of sulfonated polysulfone coated on ceramics

Separation of ingredients in bonito extract was studied by a composite UF membrane of ceramic/sulfonated polysulfone (SPS). The bonito extract mainly contained inosine-5′-monophosphate (IMP), glutamic acid as a tasty ingredient and hypoxanthine, histidine as a putrefaction ingredient. The composite membrane showed a high rejection against negatively charged IMP, but permeated non-charged hypoxanthine. This is because of the negatively charged repulsion between the membrane and the solute. The permeation of amino acid could be controlled using the difference in isoelectric points of amino acids themselves. When the amino acid solution was filtrated by the composite membrane at pH 7, glutamic acid was rejected and no histidine was rejected. The charges of composite membrane were found to have an effect on the separation of ingredients in bonito extract.The composite membrane was stable within a wide pH range from 3 to 9, and had a thermal durability under 353 K.     

Enantiomeric separations using polymeric L-glutamate surfactant derivatives: effect of increasing steric factors

This study examines the role of steric hindrance near the stereogenic centers of four glutamic acid based polymeric surfactants. The single amino acid surfactants of glutamic acid, glutamic acid methyl ester, glutamic ethyl ester, and glutamic acid tert-butyl ester were investigated. The micellar electrokinetic chromatography (MEKC) separation of three binaphthyl derivatives and three benzodiazepines were used to study these steric factors. In addition, the hydrophobicity of these polymers as a function of pH was investigated by use of fluorescence measurements.     

Fast determination of lead in lake sediment samples using electrothermal atomic absorption spectrometry with slurry samples introduction

An analytical method for the determination of glutamic acid by the sequential perturbation caused by different amounts of glutamic acid on the oscillating chemical system involving the Cu(II)-catalyzed oscillating reaction between hydrogen peroxide and sodium thiocyanate in an alkaline medium is proposed. The method relies on the linear relationship between the changes in the oscillation amplitude of the chemical system and the concentration of glutamic acid. The reaction is implemented in a continuous-flow stirred-tank reactor, and changes in the oscillation amplitude on each perturbation are proportional to the glutamic acid concentration. The use of the analyte pulse perturbation (APP) technique permits sequential determinations on the same oscillating system owing to the expeditiousness with which the steady state is regained after each perturbation. The dynamic range lies between 2.5x10(-6) and 3.2x10(-4) M of glutamic acid, with the regression coefficient is 0.9987. The precision is excellent (less than 0.68% as relative standard deviation (R.S.D.)). Some aspects of the potential mechanism of action of glutamic acid on the oscillating system are discussed.     

聚谷氨酸修饰电极同时检测对苯二酚和邻苯二酚

以谷氨酸单体为初始试剂,利用电化学聚合方法制备得到聚谷氨酸修饰电极.考察了电化学聚合条件(电位、扫速及扫描圈数)对修饰电极的影响,运用电化学方法对所制备的修饰电极进行了表征.此修饰电极对对苯二酚和邻苯二酚的电化学氧化还原显示出很高的催化能力,显著降低了二者的氧化电位,改善了二者的电化学可逆性,同时增强了二者的氧化还原峰...     

Effect of chemical compounds on amino acid content of some Fusarium species and its significance to fungal chemotaxonomy

The cellular amino acid profiles of nine species of Fusarium; namely, Fusarium anthophilum, Fusarium avenaceum, Fusarium cerealis, Fusarium graminearum, Fusarium graminum, Fusarium oxysporum f. sp. conglutinans, Fusarium pseudograminearum, Fusarium roseum, and Fusariumsacchari var. elongatum growing on malt extract medium were determined. The amino acid profiles of the investigated fungi were varied and could be used for identification and characterisation of certain Fusarium species. Addition of certain chemical compounds including aspartic acid, glutamic acid, methionine, selenium, and urea to the growth medium affected the amino acid profiles. However, susceptibility of amino acid content to environmental conditions increased the variation of amino acid profiles among all the investigated Fusarium species. Some amino acids were only produced when certain chemical compounds were added to the growth medium. Valine was produced by F. anthophilum only in the presence of aspartic acid or selenium, while serine was produced in the presence of aspartic acid, glutamic acid, or methionine. Also, cysteine was produced by F. avenaceum in the presence of glutamic acid or urea. F. cerealis produced tryptophan only in the presence of aspartic acid or urea, while F. graminearum produced leucine in glutamic, methionine or urea. Similarly, many different amino acids were produced by each Fusarium species only in the presence of certain chemical compounds. The results revealed that the amino acid profiles will be more useful for characterisation and identification of fungi if they are determined under different conditions.     

Enzymatic Synthesis of γ-Glutamylmethylamide from Glutamic Acid γ-Methyl Ester and Methylamine Catalyzed by Escherichia coli Having γ-Glutamyltranspeptidase Activity

A new method for the synthesis of γ-glutamylmethylamide is presented. Glutamic acid γ-methyl ester was used as substrate for γ-glutamylmethylamide synthesis catalyzed by Escherichia coli with γ-glutamyltranspeptidase activity. Reaction conditions were optimized by using 300 mM glutamic acid γ-methyl ester and 3,000 mM methylamine at pH 10 and 40 °C. Bioconversion rate of γ-glutamylmethylamide reached 87 % after 10 h. γ-Glutamyltranspeptidase was reversibly inhibited only when glutamic acid γ-methyl ester was above 300 mM.