Lipophilicity determination of some 3,5-dinitro-benzoic-acid esters on unimepregnated cellulose layer

Unimpregnated cellulose layers proved to be suitable for the determination of the lipophilic character of 14 3,5-dinitro benzoic acid esters under reversed-phase, thin-layer chromatographic conditions. Lipophilic characters measured on unimpregnated cellulose layers correlated well with similar values determined on impregnated silica and on impregnated alumina. Minor differences in retention of the three types of layers were observed.     

Effect of some amino acids and peptides on silicic acid polymerization

The polymerization of silicic acid in aqueous solutions at different pH was followed by the colorimetric molybdosilicate method. The role of four amino acids (serine, lysine, proline and aspartic acid) and the corresponding homopeptides was studied. All four amino acids behave the same way and favor the condensation of silicic acid. Peptides exhibit a stronger catalytic effect than amino acids but they appear to behave in very different ways depending on the nature of side-groups and pH. Poly-lysine and poly-proline for instance lead to the precipitation of solid phases containing both silica and peptides. The role of these biomolecules on the polymerization of silicic acid is discussed in terms of electrostatic interactions, hydrogen bonds and solubility.     

Reversed-phase high-performance liquid chromatographic separation of theα- andβ-isomers of aspartyl peptides

Summary A high-performance liquid chromatography method is described for the separation of the - and -isomers of aspartyl-containing peptides such as N-benzyloxycarbonyl methyl aspartate, protected sweet dipeptide and delta sleep inducing peptide (DSIP, a nonapeptide). The - and -isomers were separated on a column containing octadecyl silica bonded-phase packing under reversed-phase conditions using methanol-water as the mobile phase containing a small amount of acetic acid. The resolution achieved meets the requirements of qualitative and quantitative analysis. This method is also suited for the determination of intermediates in the aspartyl peptide synthesis.     

Quantitative evaluation of amino acids using microwave accelerated hydrolysis

Summary An improved method for the quantitative determination of amino acids using HPLC, after preliminary derivatisation with o-phthalaldehyde, is described. Separation was carried out on a LiChrospher RP-18 column, using gradient elution and a fluorescence detector. Hydrolysis was performed with 6M HCl or with 3M p-toluenesulphonic acid depending on the amount of carbohydrates in the sample. In addition, the time required for total hydrolysis was shortened from 24 hours to 15 minutes by the use of a microwave oven. The results with these two hydrolytic methods are compared with regard to the extent of peptide bond cleavage and the percentage of decomposition of amino acids in a test mixture.     

TLC resolution of enantiomeric mixtures of amino acids

Summary Resolution of enantiomeric mixtures of DL-amino acids (Nine) using silica gel layers impregnated with (-)-bruncine is reported. The solvent system used was Butanol: Acetic acid: Chloroform (3∶1∶4). The diastereomers were formed and hydrolysed, by dilute HCl spray, on the chromatogram only and the amino acids thus resolved were located by ninhydrin spray. The cross resolution possibilities of enantiomers were also calculated.     

Synthesis of N,N-dimethyl-2,4-dinitro-5-fluorobenzylamine and its reactions with amino acids and peptides

A practical synthesis is described for N,N-dimethyl-2,4-dinitro-5-fluorobenzylamine (DMDNFB) and its -d₆ analog as an alternative Sanger's reagent (DNFB), for purposes of amino acid derivatization detectable by positive mode electrospray ionization mass spectrometry. DMDNFB is comparable to DNFB in its efficiency to derivatize amino acids and peptides. Various DMDNP (d₀/d₆) derivatives of (modified) lysine were synthesized to evaluate the potential use of isotope-edited LC-ESI-MS as a tool for structural definition of the posttranslational modification of protein-based lysines.     

Retention prediction of o-phthalaldehyde amino acid derivatives in reversed-phase liquid chromatography

Summary Retention prediction of o-phthalaldehyde amino acid derivatives in reversed-phase liquid chromatography has been investigated. The retention of all derivatives could be predicted within about 10% relative error under the appropriate separation conditions in both isocratic and gradient-elution modes.     

Effect of halides on the TLC resolution of amino acids below their isoelectric points

TLC of a fifteen component mixture of amino acids has been carried out in two ways; firstly, the amino acids were treated with halides below their isoelectric points and chromatographed on plain silica plates, and secondly the amino acids in their cationic forms were chromatographed on silica plates impregnated with halides, keeping the same solvent system. The resolution is considered to be affected by hydrophobic interactions between silica gel and amino acid molecule and by the polarity and the flow of the mobile phase. The method provides resolution of 10–11 amino acids from the fifteen component mixture.     

HPLC enantioseparation of amino acids and their protected derivatives used in peptide synthesis with pre-column chiral derivatization

Summary Indirect chiral separation methods based on enantiomeric derivatizations were developed in order to monitor optical purity of uncoded amino acids and a new series of amino acid derivatives. Marfey's reagent was used for derivatization of amino groups: whilst boxyl groups were derivatised with (1R, 2R)-or (1S, 2S)-2-amino-1(4-nitrophenyl)-1,3-propanediol reagents were used, respectively. The separations of diastereomeric derivatives formed via derivatization were optimized in RP-HPLC and NP-HPLC systems. Presented at Balaton Symposium on High Performance Separation Methods, Siófok, Hungary, September 1–3, 1999     

Lipophilicity determination of some new crown ethers by reversed-phase thin-layer chromatography

Summary The lipophilicity of 28 modified crown ether derivatives was determined by reversed-phase thin-layer chromatography (RPTLC) using various organic phases and supports. The lipophilicity values determined in different RPTLC systems showed good correlations, however the quality of the organic phase (methanol, acetone, acetonitrile) and the support characteristics influenced to a small extent the determination.     

Lipophilicity determination of some nitrostyrene derivatives on RP-2, PR-8 and RP-18 layers

Summary The lipophilicity of 33 nitrostyrene derivatives was determined by reversed-phase thin-layer chromatography on RP-2, RP-8 and RP-18 layers using methanol as the organic phase. The R_M value of each compound linearly decreased with increasing concentration of the organic solvent. The retention strength of RP-2 layer was lower than that of RP-8 and RP-18 layers. Between the retention strength of RP-8 and RP-18 layers no significant difference was detected. Minor differences among the selectivities of the layers were also observed. The impact of the change of methanol concentration on the retention was higher on RP-2 than on RP-18 layers probably due to the sterically favourable interaction of methanol with the shorter alkyl groups on the silica surface.     

Applications of hydrophilic interaction chromatography to amino acids,peptides, and proteins

This review summarizes the recent advances in the analysis of amino acids, peptides, and proteins using hydrophilic interaction chromatography. Various reports demonstrate the successful analysis of amino acids under such conditions. However, a baseline resolution of the 20 natural amino acids has not yet been published and for this reason, there is often a need to use mass spectrometry for detection to further improve selectivity. Hydrophilic interaction chromatography is also recognized as a powerful technique for peptide analysis, and there are a lot of papers showing its applicability for proteomic applications (peptide mapping). It is expected that its use for peptide mapping will continue to grow in the future, particularly because this analytical strategy can be combined with reversed‐phase liquid chromatography, in a two‐dimensional setup, to reach very high resolving power. Finally, the interest in hydrophilic interaction chromatography for intact proteins analysis is less evident due to possible solubility issues and a lack of suitable hydrophilic interaction chromatography stationary phases. To date, it has been successfully employed only for the characterization of membrane proteins, histones, and the separation of glycosylated isoforms of an intact glycoprotein. From our point of view, the number of hydrophilic interaction chromatography columns compatible with intact proteins (higher upper temperature limit, large pore size, etc.) is still too limited.     

Chemiluminescence determination of 20 amino acids and the mechanism study

<正>It was found that 20 amino acids could inhibit the intensity of the luminol-H_2O_2-CuSO_4 chemiluminescence system.Using this character,a rapid and sensitive method for the determination of 20 amino acids was developed with flow injection coupled with chemiluminescence detection.Under the optimal conditions,the detection limits of 20 amino acids were in the range of 4.5×10~(-7)- 4.3×10~(-10) mol/L,and the relative standard deviations were less than 3.2%.The proposed method was successfully applied to drug analysis.The possible mechanism was also discussed.     

Separation of DABS derivatives of amino acids by multiple gradient development (MGD) in thin-layer chromatography

Summary A mixture of 13 DABS-amino acids has been chromatographed on high-performance silica gel layers developed with eluents containing increasing concentrations of ethyl acetate in heptane + chloroform, using a modification of stepwise multiple development MGD described in a earlier paper. Densitograms were obtained at 485 nm. The MGD method was very efficient, separating all 13 DABS-amino acids, and rapid, owing to the use of a non-aqueous mobile phase.     

Simple conversion of fully protected amino acids to zwitterions

An operationally simple and efficient method under mild acidic conditions was developed to convert fully protected amino acids to the corresponding zwitterions without either isoelectric precipitation or ion exchange chromatography.     

New chromogenic reagents for labelling amino groups in peptides. Chromatographic and preparatives aspects

Summary A new type of chromogenic reagent for labelling the amino groups of peptides or amino acids, 5-substituted 2,4-dinitrofluorobenzenes, is presented. These reagents are characterized by a polarity determined by the function included in the substituent in the 5-position and by the nature of this substituent. Preparation and chromatographic behaviour of these reagents, of eventual by-products of reactions and of some N-(2,4-dinitro-5-diethylaminophenyl)-peptides or amino acids are described.Proportions in solvent mixtures are v/v except otherwise indicated. Abbreviations: lit=literature, TLC=thin-layer chromatography, TLE=TL electrophoresis, see also: Figs. 2, 3, 5.     

Enzymatic C-terminal amidation of amino acids and peptides

Herein, we describe two versatile and high yielding enzymatic approaches for the conversion of semi-protected amino acid and peptidyl C-terminal α-carboxylic acids into their corresponding amides. In the first approach, the lipase Candida antarctica lipase-B (Cal-B), and in the second approach, the protease Subtilisin A, are used, respectively. We found that by using the ammonium salt of the α-carboxylic acid instead of separate ammonia sources, the enzymatic amidation reactions proceeded much faster without side reactions and gave near to quantitative yields of products.     

Micellar-mediated shifts of ionization constants of amino acids and peptides

The acid-base dissociation constants, K_a, of amino acids and small peptides were determined in both aqueous and micellar solutions of sodium dodecyl sulfate and cetyltrimethylammonium bromide by potentiometric and chromatographic means. The observed differences in pK_a values between micellar media and aqueous solutions ranged between 0.23 and 2.21 units. The micellar-mediated pK_a shifts can be attributed to different solute-micelle interactions, mainly hydrophobic and electrostatic forces. The implications of the change in acid-base behavior on separation selectivity in micellar liquid chromatography and micellar electrokinetic capillary chromatography are discussed.     

Indirect determination of amino acids by molecular emission cavity analysis

An indirect method for the determination of ca. 10^?4 M amino acids is described which is based on the reaction of the latter with 2,4,6-trinitrobenzene-1-sulphonic acid at pH 11.7 and the measurement of the S₂ emission in a hydrogen-nitrogen flame that is produced from the resulting compound after the addition of hydrochloric acid. The optimum conditions for the determination of amino acids were investigated. The amino acids examined were glycine, alanine, valine, methionine, serine, threonine and histidine.