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Methodologies HPLC

Challenge methodology Screen degradation samples using suitable methodology (HPLC) 8-Document Prepare reports and share degradation structures and mechanisms... [Pg.66]

These methodologies have been reviewed (22). In both methods, synthesis involves assembly of protected peptide chains, deprotection, purification, and characterization. However, the soHd-phase method, pioneered by Merrifield, dominates the field of peptide chemistry (23). In SPPS, the C-terminal amino acid of the desired peptide is attached to a polymeric soHd support. The addition of amino acids (qv) requires a number of relatively simple steps that are easily automated. Therefore, SPPS contains a number of advantages compared to the solution approach, including fewer solubiUty problems, use of less specialized chemistry, potential for automation, and requirement of relatively less skilled operators (22). Additionally, intermediates are not isolated and purified, and therefore the steps can be carried out more rapidly. Moreover, the SPPS method has been shown to proceed without racemization, whereas in fragment synthesis there is always a potential for racemization. Solution synthesis provides peptides of relatively higher purity however, the addition of hplc methodologies allows for pure peptide products from SPPS as well. [Pg.200]

Luminol-based chemiluminescence methods have also been employed for detection of analytes in flowing stream analytical techniques such capillary electrophoresis (282), flow injection analyses, and hplc (267). AppHcations of the enhanced luminol methodology to replace radioassay methods have been developed for a number of immunological labeling techniques (121,283). [Pg.275]

On considering the solvent consumption and waste generation, it is clear that NIR measurements reduce drastically the amount of CH CN consumed compared with the HPLC procedure. On the other hand, the sample frequency obtained by the NIR methodology was higher than those obtained by HPLC. [Pg.141]

The most widely used HPLC detector methodology is, arguably, UV absorption, and this has capabilities as both a specific or general detector, depending upon the way it is used. [Pg.33]

Arguably the ultimate LC-MS interface would be one that provides El spectra, i.e. a spectrum from which structural information can be extracted by using famihar methodology, and this was one of the great advantages of the moving-belt interface. There is, however, an incompatibility between the types of compound separated by HPLC and the way in which electron ionization is achieved and therefore such an interface has restricted capability, as previously discussed with respect to the moving-belt interface (see Section 4.2 above). [Pg.147]

The particle-beam interface has been developed primarily to provide El spectra from HPLC eluates but may be combined with other ionization techniques such as CL If quantitative studies are being undertaken, a detailed study of experimental conditions should be undertaken. Isotope-dilution methodology is advocated for the most accurate results. [Pg.151]

If a buffer is present in the HPLC mobile phase, and this is essential for true thermospray ionization, it should ideally be volatile and this may necessitate modifying existing HPLC methodology. [Pg.156]

Procedures used vary from trial-and-error methods to more sophisticated approaches including the window diagram, the simplex method, the PRISMA method, chemometric method, or computer-assisted methods. Many of these procedures were originally developed for HPLC and were apphed to TLC with appropriate changes in methodology. In the majority of the procedures, a set of solvents is selected as components of the mobile phase and one of the mentioned procedures is then used to optimize their relative proportions. Chemometric methods make possible to choose the minimum number of chromatographic systems needed to perform the best separation. [Pg.95]

HPLC and LC/MS. HPLC methodology coupled with ultraviolet (UV), fluorescence (FL), photodiode-array (PDA) and/or a mass spectrometry (MS) detection has been developed. In general, neonicotinoids can be determined by HPLC/UV. Typical HPLC operating conditions are given in Table 2. [Pg.1133]

For these reasons we have developed a different approach that measures differential expression of intact proteins.21 In this approach the proteins are extracted from the cell, separated on an HPLC column, ionized via electrospray, and automatically deconvoluted into their respective uncharged nominal masses. By this methodology it is then possible to obtain accurate, intact protein profiles of the individual strains of bacteria. Because the masses of the detected proteins are accurate to +2 Da from run to run, it is possible to subtract protein profiles from known strains to quickly identify differences in protein expression among newly mutated strains. [Pg.205]

A wide variety of methodologies have been employed for the analysis of antioxidants in polymers and some standard methods are available. For high-density polyethylene ASTM method D5524 (ASTM International) — Determination of phenolic antioxidants in high-density polyethylene, describes a method whereby the sample is ground to a small particle size and then extracted by refluxing with cyclohexane. The cyclohexane extract is then examined by reverse-phase HPLC with UV detection. [Pg.574]

Parallel to the development of mass spectrometric instrumentation and methodologies, the improvements of separation techniques, such as gas chromatography (GC), high performance liquid chromatography (HPLC) and capillary electrophoresis (CE), and of their coupling with MS allowed the study of complex mixtures, that are generally encountered in most studies. [Pg.38]

The determination of F2-isoprostanes, oxidation products of arachidonic acid, has been proposed as a more reliable index of oxidative stress in vivo, overcoming many of the methodological problems associated with other markers. The isoprostanes have emerged as a most effective method of quantifying the potential of antioxidants to inhibit lipid peroxidation. However, one drawback of this method is that quantification of F2-iP requires sophisticated techniques, in particular GC/MS and HPLC/MS... [Pg.277]

With the advancing automatization and computerization of CE instruments, the application of micromachining techniques, and the improvement of the devices for coupling CE with CL detection, it is hoped that both techniques may be incorporated in the future as suitable methodology in routine laboratories, being complementary to classical techniques such as HPLC and offering new alternatives to the analytical chemist. [Pg.469]


See other pages where Methodologies HPLC is mentioned: [Pg.228]    [Pg.1093]    [Pg.331]    [Pg.228]    [Pg.1093]    [Pg.331]    [Pg.72]    [Pg.17]    [Pg.96]    [Pg.502]    [Pg.264]    [Pg.73]    [Pg.191]    [Pg.203]    [Pg.243]    [Pg.133]    [Pg.148]    [Pg.534]    [Pg.7]    [Pg.74]    [Pg.346]    [Pg.784]    [Pg.49]    [Pg.299]    [Pg.176]    [Pg.212]    [Pg.732]    [Pg.204]    [Pg.107]    [Pg.87]    [Pg.423]    [Pg.526]    [Pg.94]    [Pg.251]    [Pg.377]    [Pg.73]    [Pg.177]    [Pg.307]    [Pg.339]   
See also in sourсe #XX -- [ Pg.12 ]




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