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Albumin, absorption

Park CH, Maack T. Albumin absorption and catabolism by isolated perfused proximal convoluted tubules of the rabbit. J CUn Invest 1984 73 767-777. [Pg.818]

The absorption of metoprolol after po dosing is rapid and complete. The dmg undergoes extensive first-pass metabolism in the liver and only 50% of the po dose in bioavailable. About 12% of the plasma concentration is bound to albumin. The elimination half-life is 3—7 h and less than 5% of the po dose is excreted unchanged in the urine. The excretion of the dmg does not appear to be altered in patients having renal disease (98,99,108). [Pg.127]

Absorption kinetic studies on fasted rats dosed by lipid-emulsion gavage revealed rapid appearance of triehloroethylene in the blood (typieally peaking at 15 minutes post-exposure) followed by rapid disappearance (Templin et al. 1993). Rats similarly dosed with radiolabelled trichloroethylene showed rapid serum albumin adduction which peaked at 4-8 hours, then decayed with a half-life consistent with that of albumin itself (Stevens et al. 1992). However, some of the detected radioactivity may have been due to trichloroethylene metabolites rather than the parent compound. [Pg.112]

Around 99% of calcium is contained in the bones, whereas the other 1% resides in the extracellular fluid. Of this extracellular calcium, approximately 40% is bound to albumin, and the remainder is in the ionized, physiologically active form. Normal calcium levels are maintained by three primary factors parathyroid hormone, 1,25-dihydroxyvitamin D, and calcitonin. Parathyroid hormone increases renal tubular calcium resorption and promotes bone resorption. The active form of vitamin D, 1,25-dihydroxyvitamin D, regulates absorption of calcium from the GI tract. Calcitonin serves as an inhibitory factor by suppressing osteoclast activity and stimulating calcium deposition into the bones. [Pg.1482]

AC ADME ANS AUC BA/BE BBB BBM BBLM BCS BLM BSA CE CHO CMC CPC CPZ CTAB CV DA DOPC DPPC DPPH aminocoumarin absorption, distribution, metabolism, excretion anilinonaphthalenesulfonic acid area under the curve bioavailability-bioequivalence blood-brain barrier brush-border membrane brush-border lipid membrane biopharmaceutics classification system black lipid membrane bovine serum albumin capillary electrophoresis caroboxaldehyde critical micelle concentration centrifugal partition chromatography chlorpromazine cetyltrimethylammonium bromide cyclic votammetry dodecylcarboxylic acid dioleylphosphatidylcholine dipalmitoylphosphatidylcholine diphenylpicrylhydrazyl... [Pg.304]

The interaction between 4-(4-hydroxybut-2-ynyloxy)-3-(phenylsulfonyl)-l,2,5-oxadiazole-2-oxide 16 and bovine serum albumin (BSA) was studied by spectroscopic methods including fluorescence and UV-Vis absorption spectroscopy. The results indicate that molecules 16 bind with BSA forming 1 1 complex. Thermodynamic parameters, such as AH, AG, and A.Y, were calculated. The results indicate that the binding reaction is mainly entropy driven and hydrophobic forces play a major role in this reaction <2006CHJ1050>. [Pg.325]

In a normal human adult, about 2 g of zinc is filtered by the kidneys daily and about 0.3 to 0.6 mg is actually excreted each day (Goyer 1986). Zinc homeostasis in rats, unlike most mammals, is maintained by zinc secretion from the intestines rather than by regulation of zinc absorption (Elinder 1986). Initial uptake of zinc from the rat gastrointestinal tract involves binding to albumin and transport of the zinc-albumin complex from intestine to liver (Hoadley and Cousins 1988). [Pg.640]

For quantitative analysis of protein concentration the colorimetric Bradford-assay [147] is most commonly used. Here another Coomassie dye, Brilliant Blue G-250, binds in acidic solutions to basic and aromatic side chains of proteins. Binding is detected via a shift in the absorption maximum of the dye from 465 nm to 595 nm. Mostly calibration is performed with standard proteins like bovine serum albumin (BSA). Due to the varying contents of basic and aromatic side chains in proteins, systematic errors in the quantification of proteins may occur. [Pg.77]

Among the series of dyes, in which the effect of binding to human serum albumin (HSA) was studied [41], the dye 8 (Fig. 10) exhibited J-aggregate absorption and fluorescence bands, while these bands were not observed for the free dye. This led to the conclusion about the J-aggregation of the dye 8 in the HSA binding site. [Pg.152]

Figure 11.12 Absorption spectrum of the albumin-bromcresol green complex ... Figure 11.12 Absorption spectrum of the albumin-bromcresol green complex ...
Bromcresol purple has been suggested as showing improved specificity for albumin and less variation in colour intensity compared with bromcresol green. The dye-albumin complex shows an absorption maximum at 603 nm and the use of a reagent buffered at pH 5.2 appreciably reduces the tendency of the complex to precipitate. [Pg.396]

Figure 2.11. The dependence of the position of the fluorescence spectrum maximum on excitation wavelength for tryptophan in a model medium (glycerol) at different temperatures (a) and singletryptophan proteins (b). 1, Whiting parvalbumin, pH 6.S in the presence of Ca2+ ions 2, ribonuclease Th pH 6.5 3, ribonuclease C2, pH 6.5 4, human serum albumin, pH 7.0, +10"4 M sodium dodecyl sulfate 5, human serum albumin, pH 3.2 6, melittin, pH 7.5, +0.15 M NaCl 7, protease inhibitor IT-AJ from Actinomyces janthinus, pH 2.9 8, human serum albumin, pH 7.0 9, -casein, pH 7.5 10, protease inhibitor IT-AJ, pH 7.0 11, basic myelin protein, pH 7.0 12, melittin in water. The dashed line is the absorption spectrum of tryptophan. Figure 2.11. The dependence of the position of the fluorescence spectrum maximum on excitation wavelength for tryptophan in a model medium (glycerol) at different temperatures (a) and singletryptophan proteins (b). 1, Whiting parvalbumin, pH 6.S in the presence of Ca2+ ions 2, ribonuclease Th pH 6.5 3, ribonuclease C2, pH 6.5 4, human serum albumin, pH 7.0, +10"4 M sodium dodecyl sulfate 5, human serum albumin, pH 3.2 6, melittin, pH 7.5, +0.15 M NaCl 7, protease inhibitor IT-AJ from Actinomyces janthinus, pH 2.9 8, human serum albumin, pH 7.0 9, -casein, pH 7.5 10, protease inhibitor IT-AJ, pH 7.0 11, basic myelin protein, pH 7.0 12, melittin in water. The dashed line is the absorption spectrum of tryptophan.
B. Hicks, M. White, C. A. Ghiron, R. R. Kuntz, and W. A. Volker, Flash photolysis ofhuman serum albumin Characterization of the indole triplet absorption spectrum and decay at ambient temperature, Proc. Natl. Acad. Sci. U.S.A. 75, 1172-1175 (1978). [Pg.133]

Kim KJ, Matsukawa Y, Yamahara H, Kalra VK, Lee VH, Crandall ED (2003) Absorption of intact albumin across rat alveolar epithelial cell monolayers. Am J Physiol 284(3) L458-L465... [Pg.281]

This section will provide an overview on ADME models from our group to illustrate our approach for building predictive models on structurally diverse training sets. Datasets for intestinal human absorption and human serum albumin binding are discussed, while models for other relevant ADME properties have also been obtained. Those models, however, do not stand alone but are used in combination with those models tailored for affinity and selectivity in the frame of multidimensional lead optimization. [Pg.350]

See other pages where Albumin, absorption is mentioned: [Pg.223]    [Pg.195]    [Pg.173]    [Pg.223]    [Pg.195]    [Pg.173]    [Pg.468]    [Pg.212]    [Pg.424]    [Pg.63]    [Pg.280]    [Pg.268]    [Pg.281]    [Pg.279]    [Pg.75]    [Pg.508]    [Pg.520]    [Pg.135]    [Pg.448]    [Pg.538]    [Pg.566]    [Pg.1179]    [Pg.88]    [Pg.88]    [Pg.115]    [Pg.351]    [Pg.501]    [Pg.390]    [Pg.49]    [Pg.149]    [Pg.269]    [Pg.271]    [Pg.218]    [Pg.318]    [Pg.180]    [Pg.32]   
See also in sourсe #XX -- [ Pg.45 ]



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Serum albumin absorption spectra

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