High-performance hquid HPLC

Reversed-phase high performance Hquid chromatography has come into use for estimating the purity of proteins and peptides as weU. However, before employed, a high performance Hquid chromatographic (hplc) profile of a given protein must be completely vaHdated (43). 

Thin-Layer Chromatography. Chiral stationary phases have been used less extensively in tic as in high performance Hquid chromatography (hplc). This may, in large part, be due to lack of avakabiHty. The cost of many chiral selectors, as well as the accessibiHty and success of chiral additives, may have inhibited widespread commerciali2ation. Usually, nondestmctive visuali2ation of the sample spots in tic is accompHshed using iodine vapor, uv or fluorescence. However, the presence of the chiral selector in the stationary phase can mask the analyte and interfere with detection (43). 

High Performance Liquid Chromatography. Although chiral mobile phase additives have been used in high performance Hquid chromatography (hplc), the large amounts of solvent, thus chiral mobile phase additive, required to pre-equiUbrate the stationary phase renders this approach much less attractive than for dc and is not discussed here. 

Antioxidants (qv) have a positive effect on oils when present in the proper concentration. Sterols and tocopherols, which are natural antioxidants, may be analy2ed by gas-Hquid chromatography (glc), high performance Hquid chromatography (hplc), or thin-layer chromatography (tic). Synthetic antioxidants maybe added by processors to improve the performance or shelf life of products. These compounds include butylatedhydroxyanisole (BHA), butylated hydroxytoluene (BHT), / fZ-butyUiydroquinone (TBHQ), and propyl gallate. These materials may likewise be analy2ed by glc, hplc, or tic. Citric acid (qv), which functions as a metal chelator, may also be deterrnined by glc. 

The total phosphoms content of the sample is determined by method AOCS Ja 5-55. Analysis of phosphoUpid in lecithin concentrates (AOCS Ja 7-86) is performed by fractionation with two-dimensional thin-layer chromatography (tic) followed by acid digestion and reaction with molybdate to measure total phosphorous for each fraction at 310 nm. It is a semiquantitative method for PC, PE, PI, PA, LPC, and LPE. Method AOCS Ja 7b-91 is for the direct deterrnination of single phosphoHpids PE, PA, PI, PC in lecithin by high performance Hquid chromatography (hplc). The method is appHcable to oil-containing lecithins, deoiled lecithins, lecithin fractions, but not appHcable to lyso-PC and lyso-PE. 

Several new oxalates have been developed for use ia analytical appHcations. Bis(2,6-difluorophenyl) oxalate (72) and bis(4-nitro-2-(3,6,9-trioxadecylcarbonyl)phenyl) oxalate (97) have been used ia flow iajection and high performance Hquid chromatography (hplc) as activators for chemiluminescence detectors. These oxalates are generally more stable and show better water solubiUty ia mixed aqueous solvents yet retain the higher efficiencies ( ) of the traditional oxalates employed for chemiluminescence. 

High performance Hquid chromatography (hplc) may be used to determine nitroparaffins by utilizing a standard uv detector at 254 nm. This method is particularly appHcable to small amounts of nitroparaffins present, eg, in nitro alcohols (qv), which caimot be analyzed easily by gas chromatography. Suitable methods for monitoring and deterrnination of airborne nitromethane, nitroethane, and 2-nitropropane have been pubUshed by the National Institute of Occupational Safety and Health (NIOSH) (97). Ordinary sorbant tubes containing charcoal are unsatisfactory, because the nitroparaffins decompose on it unless the tubes are held in dry ice and analyzed as soon after collection as possible. 

Instmmental methods of analysis provide information about the specific composition and purity of the amines. QuaUtative information about the identity of the product (functional groups present) and quantitative analysis (amount of various components such as nitrile, amide, acid, and deterruination of unsaturation) can be obtained by infrared analysis. Gas chromatography (gc), with a Hquid phase of either Apiezon grease or Carbowax, and high performance Hquid chromatography (hplc), using siHca columns and solvent systems such as isooctane, methyl tert-huty ether, tetrahydrofuran, and methanol, are used for quantitative analysis of fatty amine mixtures. Nuclear magnetic resonance spectroscopy (nmr), both proton ( H) and carbon-13 ( C), which can be used for quaHtative and quantitative analysis, is an important method used to analyze fatty amines (8,81). 

Chromatographic Method. Progress in the development of chromatographic techniques (55), especially, in high performance Hquid chromatography, or hplc, is remarkable (56). Today, chiral separations are mainly carried out by three hplc methods chiral hplc columns, achiral hplc columns together with chiral mobile phases, and derivatization with optical reagents and separation on achiral columns. All three methods are usehil but none provides universal appHcation. 

Mixtures can be identified with the help of computer software that subtracts the spectra of pure compounds from that of the sample. For complex mixtures, fractionation may be needed as part of the analysis. Commercial instmments are available that combine ftir, as a detector, with a separation technique such as gas chromatography (gc), high performance Hquid chromatography (hplc), or supercritical fluid chromatography (96,97). Instmments such as gc/ftir are often termed hyphenated instmments (98). Pyrolyzer (99) and thermogravimetric analysis (tga) instmmentation can also be combined with ftir for monitoring pyrolysis and oxidation processes (100) (see Analytical methods, hyphenated instruments). 

Body fluids are analyzed for T and T by a variety of radioimmunoassay procedures (31) (see Immunoassays). The important clinical parameter for estimating thyroid function, the protein-bound iodine (PBI), is measured as described in treatises of clinical chemistry. High performance Hquid chromatographic (hplc) methods have replaced dc (32,33). 

Various aspects of the chromatography of vitamin B 2 and related corrinoids have been reviewed (59). A high performance Hquid chromatographic (hplc) method is reported to require a sample containing 20—100 p.g cyanocobalamin and is suitable for premixes, raw material, and pharmaceutical products (60). 

In addition, the appHcation of the mass spectrometer (ms) as a detector for gas—Hquid chromatography has made the positive identification of peaks possible. High performance Hquid chromatography (hplc), which involves various detectors, can be used to measure hydrophilic and hydrophobic organic compounds in water. 

The successful separation of xanthate-related compounds by high performance Hquid chromatography (hplc) methods has been reported (91—93). The thin-layer chromatography procedure has been used to determine the nature of the alcohols in a xanthate mixture. A short mn of 3 cm at a development time of 25 min gives a complete separation of C —alkanol xanthates (94). 

Chemical stabiUty studies are monitored by siUca gel thin-layer chromatography (dc) or by high performance Hquid chromatography (hplc) using a reverse-phase C g coated column (24). Hplc peaks or dc spots are visualized by thek uv absorption at 245 nm the tic spots can also be detected by ceric sulfate or phosphomolybdic acid staining. 

Immobilization. The abiUty of cyclodextrins to form inclusion complexes selectively with a wide variety of guest molecules or ions is well known (1,2) (see INCLUSION COMPOUNDS). Cyclodextrins immobilized on appropriate supports are used in high performance Hquid chromatography (hplc) to separate optical isomers. Immobilization of cyclodextrin on a soHd support offers several advantages over use as a mobile-phase modifier. For example, as a mobile-phase additive, P-cyclodextrin has a relatively low solubiUty. The cost of y- or a-cyclodextrin is high. Furthermore, when employed in thin-layer chromatography (tic) and hplc, cyclodextrin mobile phases usually produce relatively poor efficiencies. 

A high performance Hquid chromotography (hplc) method to determine citric acid and other organic acids has been developed (46). The method is an isocratic system using sulfuric acid to elute organic acids onto a specific hplc column. The method is sensitive for citric acid down to ppm levels and is capable of quantifying citric acid in clear aqueous systems. 

Determination of ethyleneamines in air can be accomplished by absorbing the amines on NITC (1-naphthyl isothiocyanate) treated XAD-2 resin, then desorbing the derivative from the treated tubes and quantifying the amount using high performance Hquid chromatography (hplc). Sensitivity is reported as 0.37 and 0.016 mg/m for EDA and DETA, respectively, pet sample (153,154). 

Both MS and NMR coupling to HPLC have been employed for the analysis of p-carotene isomers and determination of lutein and zeaxanthin isomers in spinach, sweet com, and in retina. Capillary high performance hquid chromatography with stop flow connected to NMR (600 MHz) was used for stracture elucidation of all-trans deoxylutein 11 and its isomers.Efforts are in progress to eliminate the remaining major drawbacks such as obligatory use of deuterated solvents in the mobile phase, poor sensitivity, and low throughput of HPLC-NMR analyses. 

Prado, M.A. and Godoy, H.T., Determination of synthetic dyes by high performance hquid chromatography (HPLC) in jelly powder, J. Liq. Chromatogr. Rel. TechnoL, 25, 2455, 2002. 

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