Hquid chromatography

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. 

Fig. 7. A tethered cyclodextrin and the structure of P-cyclodextrin, the most common cyclodextrin used as a bonded ligand in Hquid chromatography.

Gas chromatography or Hquid chromatography (23) are commonly used to measure impurities such as acetic, dichloroacetic, and trichloroacetic acids. High purity 99+% chloroacetic acid will contain less than 0.5% of either acetic acid or dichloroacetic acid. Other impurities that may be present in small amounts are water and hydrochloric acid. 

Higher or lower quaUty at more or less cost will meet the needs of some consumers. Acetone is often produced under contract to meet customer specifications which are different from those of ASTM D329. Some specialty grades are analy2ed reagent, isotopicaHy labeled, clean room, Hquid chromatography, spectroscopic, ACS reagent (48), semiconductor (low metals), and Federal Specification 0-A-51G. 

Hydroquinone can be deterrnined spectrophotometricaHy at 292 nm in methanol after a sample is evaporated to dryness to remove the interference of acrolein. An alternative method is high performance Hquid chromatography on 10-p.m LiChrosorb RP-2 at ambient temperature with 2.0 mL/min of 20%(v/v) 2,2,4-trimethylpentane, 79.20% chloroform, and 0.80 % methanol with uv detection at 292 nm. 

Chemical assay is preferably performed by gas—hquid chromatography (glc) or by the conventional methods for determination of unsaturation such as bromination or addition of mercaptan, sodium bisulfite, or mercuric acetate. 

Gas—hquid chromatography is widely used both for a direct deterrnination of monomer quality and for identification and deterrnination of minor components. 

Until separation techniques such as chromatography (28,29) and counter-current extraction had advanced sufficientiy to be of widespread use, the principal alkaloids were isolated from plant extracts and the minor constituents were either discarded or remained uninvestigated. With the advent of, first, column, then preparative thin layer, and now high pressure Hquid chromatography, even very low concentrations of materials of physiological significance can be obtained in commercial quantities. The alkaloid leurocristine (vincristine, 22, R = CHO), one of the more than 90 alkaloids found in Catharanthus roseus G. Don, from which it is isolated and then used in chemotherapy, occurs in concentrations of about 2 mg/100 kg of plant material. 

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 concentration of aqueous solutions of the acid can be deterrnined by titration with sodium hydroxide, and the concentration of formate ion by oxidation with permanganate and back titration. Volatile impurities can be estimated by gas—Hquid chromatography. Standard analytical methods are detailed in References 37 and 38. 

Ref. 277 unless otherwise noted gc = gas chromatography hplc = high pressure Hquid chromatography ir = infrared spectroscopy uv = ultraviolet spectroscopy glc = ga sliquid chromatography eia = enzyme immunoassay vis = visible spectroscopy. 

High pressure Hquid chromatography (qv) (138) and coulometry can be used to detect and quantify anthraquinones and thek derivatives in a hydrogen peroxide process working solution. 

The fermentation-derived food-grade product is sold in 50, 80, and 88% concentrations the other grades are available in 50 and 88% concentrations. The food-grade product meets the Vood Chemicals Codex III and the pharmaceutical grade meets the FCC and the United States Pharmacopoeia XK specifications (7). Other lactic acid derivatives such as salts and esters are also available in weU-estabhshed product specifications. Standard analytical methods such as titration and Hquid chromatography can be used to determine lactic acid, and other gravimetric and specific tests are used to detect impurities for the product specifications. A standard titration method neutralizes the acid with sodium hydroxide and then back-titrates the acid. An older standard quantitative method for determination of lactic acid was based on oxidation by potassium permanganate to acetaldehyde, which is absorbed in sodium bisulfite and titrated iodometricaHy. 

Both vapor-phase chromatography and high performance Hquid chromatography, along with nuclear magnetic resonance spectroscopy, have been used for isomer and composition analysis. 

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. 

To determine the phosphoHpid and fatty acid compositions chromatographic methods (28) like gas chromatography (gc), thin-layer chromatography (tic), and high performance Hquid chromatography (hlpc) are used. Newer methods for quantitative deterrnination of different phosphoHpid classes include P-nmr (29). 

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. 

Solution Polymers. Methacryhc solution polymers are usually characterized by thek composition, soHds content, viscosity, molecular weight, glass-transition temperature, and solvent type. The compositions of methacryhc polymers are most readily determined by physicochemical methods such as spectroscopy, pyrolytic gas—Hquid chromatography, and refractive index measurements. The soHds content is determined by dilution followed by solvent evaporation to constant weight. Solution viscosities are most conveniendy determined with a Brookfield viscometer. Methods for estimating molecular weights by intrinsic viscosity are available (103). 

Gas—hquid chromatography is used extensively to determine the naphthalene content of mixtures. Naphthalene can be separated easily from thionaphthene, the methyl- and dimethylnaphthalenes, and other aromatics. Analysis of the various other impurities may require the use of high resolution capillary columns. 

Analytical and Test Methods. o-Nitrotoluene can be analyzed for purity and isomer content by infrared spectroscopy with an accuracy of about 1%. -Nitrotoluene content can be estimated by the decomposition of the isomeric toluene diazonium chlorides because the ortho and meta isomers decompose more readily than the para isomer. A colorimetric method for determining the content of the various isomers is based on the color which forms when the mononitrotoluenes are dissolved in sulfuric acid (45). From the absorption of the sulfuric acid solution at 436 and 305 nm, the ortho and para isomer content can be deterrnined, and the meta isomer can be obtained by difference. However, this and other colorimetric methods are subject to possible interferences from other aromatic nitro compounds. A titrimetric method, based on the reduction of the nitro group with titanium(III) sulfate or chloride, can be used to determine mononitrotoluenes (32). Chromatographic methods, eg, gas chromatography or high pressure Hquid chromatography, are well suited for the deterrnination of mononitrotoluenes as well as its individual isomers. Freezing points are used commonly as indicators of purity of the various isomers. 

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. 

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