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Descriptions of assays

Analytical Samples In the description of assays and tests, the approximate quantity of the analytical sample to be used is usually indicated. The quantity actually used, however, should not deviate by more than 10% from that stated. [Pg.4]

C = CONSTRUCT R RELAX 0 = WEAK 4 = STRONG. SEE REFERENCE 51 FOR DESCRIPTION OF ASSAY AND EXPLANATION OF RESULTS. [Pg.355]

The General Tests and Assays. This section of the USP gives methods for tests that are general in nature and apply to a number of the substances. Procedures are iacluded for such tests as heavy metals, melting point, chloride, sulfate, sterility, bacterial endotoxins, and pyrogens. Also iacluded are descriptions of various analytical techniques, such as spectrophotometry, chromatography, and nmr, and descriptions of tests to be used on glass or plastic containers, mbber closures, etc. [Pg.445]

A total material balance assay is a Fischer assay in which the retort gases are collected. A complete material balance closure and yields in excess of those expected from Fischer assay results are achieved. More complete descriptions of both the Fischer assay and the Tosco material balance assay methods have been reported (9). [Pg.346]

Ethylene oxide is sold as a high purity chemical, with typical specifications shown ia Table 14. This purity is so high that only impurities are specified. There is normally no assay specification. Proper sampling techniques are critical to avoid personal exposure and prevent contamination of the sample with trace levels of water. A complete review and description of analytical methods for pure ethylene oxide is given ia Reference 228. [Pg.463]

Free drug concentration description of, 36-37 measurement of, in receptor compartment, 39 Frovatriptan, 163f Full agonism, 200-202 Full agonists affinity of, 261 description of, 27—30 dose-response curves for, 90, 200-202 Furchgott method for affinity measurements, 261 potency ratios for, 202—204, 219—220 Functional assays... [Pg.295]

A number of handbooks and monographs are available with detailed descriptions of a variety of plant products and their use (Shahidi and Naczk, 1995). From a more practical point of view, an interlaboratory comparison between six university and industry laboratories of 17 extracts of spices, teas, coffees, and grape skin and of tomato peel slurry established within the framework of an EU sponsored programme, would be of interest (Schwarz et al, 2001). In this collaboration, detailed chemical analysis of the content of different phenolic compounds is compared with six antioxidant assays for the 17 extracts including different extraction procedures. [Pg.340]

Kansy, M., Senner, F., Gubemator, K. Physicochemical high throughput screening parallel artificial membrane permeation assay in the description of passive absorption processes. /. Med. Chem. 1998, 43, 1007-1010. [Pg.49]

Description of an assay in which the plate type (96-well, 384-well, etc.) and assay type (fluorescence, luminescence, etc.) are defined. [Pg.74]

The processes of both seed formation and fibril extension are dependent on temperature and on peptide concentration, with 37°C being required for establishing equilibrium within 24 h with 30 pM Pi 4o- A full description of the assay system may be found elsewhere [97,117], A 4 h reaction time is typically within the linear portion of the time course. This nucleus-dependent assay detects mainly inhibitors that are substoichiometric with the monomeric peptide, which is present at high concentration. It is relatively insensitive to inhibitors that target the monomeric peptide. Whether the inhibitors interact with the growing end of a seed or with a low abundance conformational form of the p peptide that is competent to add to the seed is difficult to determine at this time. Similar dose-response curves are obtained for Congo Red as an inhibitor with either thioflavin T (ThT) fluorescence or filtration of radioiodinated peptide readouts (Fig. 4) Caveats in the interpretation of both the ThT and radiometric filtration assays for the evaluation of putative inhibitors are discussed elsewhere [97]. [Pg.263]

These three areas will be discussed as they relate to aqueous solubility. This will be followed by a general discussion of experimental approaches to measuring aqueous solubility in a discovery setting. Detailed descriptions of varied discovery solubility assays can be found in the excellent review by Kerns [1],... [Pg.216]

The major enzymes used in ELISA technology include horseradish peroxidase (HRP), alkaline phosphatase (AP), (3-galactosidase (P-gal), and glucose oxidase (GO). See Chapter 26 for a detailed description of enzyme properties and activities. HRP is by far the most popular enzyme used in antibody-enzyme conjugates. One survey of enzyme use stated that HRP is incorporated in about 80 percent of all antibody conjugates, most of them utilized in diagnostic assay systems. [Pg.787]

See other pages where Descriptions of assays is mentioned: [Pg.158]    [Pg.364]    [Pg.173]    [Pg.294]    [Pg.518]    [Pg.159]    [Pg.373]    [Pg.210]    [Pg.158]    [Pg.364]    [Pg.173]    [Pg.294]    [Pg.518]    [Pg.159]    [Pg.373]    [Pg.210]    [Pg.445]    [Pg.221]    [Pg.341]    [Pg.820]    [Pg.296]    [Pg.297]    [Pg.298]    [Pg.523]    [Pg.585]    [Pg.411]    [Pg.714]    [Pg.301]    [Pg.100]    [Pg.401]    [Pg.410]    [Pg.178]    [Pg.133]    [Pg.114]    [Pg.118]    [Pg.5]   
See also in sourсe #XX -- [ Pg.12 , Pg.44 , Pg.153 , Pg.231 ]



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