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Immunosorbent extraction

In the past two decades quite a few new techniques have emerged for the treatment of aqueous samples prior to organic analysis. Perhaps the most important development is that of solid-phase extraction (SPE), which has successfully replaced many off-line steps. This technique can be considered to have introduced a genuine new era in sample handling [1]. The many varieties in which the technique is available and can be applied have made it the key step in handling of aqueous samples. Among the successful varieties are solid-phase microextraction (SPME), matrix solid-phase dispersion, disk extraction and immunosorbent extraction. Several reviews covering these topics have appeared in the literature in the past decade (see e.g. Refs. [2,3] for nonylphenol... [Pg.422]

The low selectivity of the SPE columns currently in use can be increased with more selective sorbents such as the immunosorbents, which have been quite extensively used in SPE-LC (72). Immunoaffinity-based solid-phase extraction (lASPE) sorbents have also been used in coupled gas chromatography for determining... [Pg.367]

The need to understand the fate of pesticides in the environment has necessitated the development of analytical methods for the determination of residues in environmental media. Adoption of methods utilizing instrumentation such as gas chro-matography/mass spectrometry (GC/MS), liquid chromatography/mass spectrometry (LC/MS), liquid chromatography/tandem mass spectrometry (LC/MS/MS), or enzyme-linked immunosorbent assay (ELISA) has allowed the detection of minute amounts of pesticides and their degradation products in environmental samples. Sample preparation techniques such as solid-phase extraction (SPE), accelerated solvent extraction (ASE), or solid-phase microextraction (SPME) have also been important in the development of more reliable and sensitive analytical methods. [Pg.605]

V. Lopez-AvUa and J. Benedicto, Determination of veterinary drugs in dry milk powder by supercritical fluid extraction-enzyme hnked immunosorbent assay, in Veterinary Drug Residues Food Safety, ed. W.A. Moats and M.B. Medina, American Chemical Society, Washington, DC, Chapter 15, pp. 145-148 (1995). [Pg.712]

Enzyme-linked immunosorbent assay (ELISA). Li and Li developed an ELISA procedure for imidacloprid to determine its residues in coffee cherry and bean extracts. A 25-g amount of sample extracted with 300 mL of methanol and 1% sulfuric acid (3 1, v/v) for 3 min. An aliquot of the sample extract (0.5 mL) is mixed with 1 mL of water and a gentle stream of nitrogen is used to evaporate methanol. The solution is then extracted with 1 mL of ethyl acetate, the extract is reconstituted in 1 mL of PBST (phosphate-buffered saline containing 0.05% Tween 20) and competitive ELISA is performed to quantify imidacloprid in the extract. Eor methanol extracts of coffee cherries and beans fortified with imidacloprid at 0.5 mgL recoveries of imidacloprid by the ELISA method were 108 and 94, respectively. [Pg.1133]

Rosengren S, Firestein GS, Boyle DL. Measurement of inflammatory biomarkers in synovial tissue extracts by enzyme-linked immunosorbent assay. Clin Diagn Lab Immunol 2003 10(6) 1002-1010. [Pg.197]

V. Lopez-Avila, C. Charan, and J. van Emon, Supercritical fluid extraction-enzyme-linked immunosorbent assay applications for determination of pesticides in soil and food, in Immunoassays for Residue Analysis Food Safety (R.C. Beier and L.H. Stanker eds), ACS Symposium Series 621, American Chemical Society, Washington (1996). [Pg.76]

D.S. Aga, E.M. Thurman, and M.L. Pomes, Determination of alachlor and its sulfonic acid metabolite in water by solid-phase extraction and enzyme-linked immunosorbent assay. Anal. Chem. 66, 1495-1499 (1994). [Pg.79]

Immunoaffinity procedures have also been developed to selectively extract corticosteroids from different sample matrices. Thus, Seymour et al. demonstrated the higher efficiency of the immunoaffinity methods compared with the conventional extraction procedures using organic solvents [177]. Immunosorbents have also been used for online procedures followed by HLPC-UV [178, 179], HPLC-APCI-MS [179,180], GC-MS [176,181], or capillary electrophoresis [182]. Poly(hydroxyethyl methacrylate) (HEMA) was evaluated as a support material for the anti-dexamethasone antibodies used in IAC. The online IAC-HPLC-MS allowed determination of dexamethasone and flumethasone in equine urine with LODs in the range 3-4 ng mL-1 [180]. The cross-reactivity values obtained in the ELISA and the recoveries of an IAC-HPLC procedure are presented in Table 7. Bagnati et al. developed an immunoaffinity extraction... [Pg.230]

The method based on immunosorbents coupled on-line with liquid chromatography-atmospheric pressure chemical ionization mass spectrometry [109], discussed in section 9.4.2.1, has been applied to the determination of substituted urea type herbicides. Supercritical fluid extraction with methanol modified carbon dioxide has been applied to the determinants of sulfonyl urea herbicides in soil [261],... [Pg.250]

ECD = electron capture detector ELISA = enzyme-linked immunosorbent assay GC = gas chromatography HRGC = high resolution gaschromatography MS = mass spectrometry MTBE = methyl-tert-butyl ether ppb = parts per billion ppm = parts per million ppt = parts per trillion SPE = solid phase extraction... [Pg.147]

Zajicek, J.L. Tillitt, D.E. Huckins, J.N. Petty, J.D. Potts, M.E. Nardone, D.A. 1996, Application of Enzyme-Linked Immunosorbent Assay (ELISA) for Measurement of Polychlorinated Biphenyls (PCBs) from Hydrophobic Solutions Extracts of Fish and Dialysates of Semipermeable Membrane Devices (SPMDs). In Environmental Immunochemical Methods, ACS Symposium Series 646 American Chemical Society Washington, D.C. Chapter 26, pp 307-325. [Pg.138]

Enzyme-linked immunosorbent assay is a heterogenous immunoassay. Reactions involve a solid phase to which components are sequentially presented and successively bound. This method is very effective in the determination of the total alkaloid content. The positive characteristics of this method are the use of non-toxic reagents and basic equipment with low costs, a small sample volume and the ability to measure alkaloids in crude sample extracts. According to the literature, compared with results obtained from GLC, the precision of ELISA for quinolizidine alkaloids is not as high as that of the gas chromatography procedure, but is adequate for plant breeding purposes. The use of enzymes in developing the methods of quinolizidine alkaloids analysis looks likely to increase in the future. [Pg.136]

Immunoaffinity cleanup was first applied in drug residue analysis for the determination of chloramphenicol in swine muscle tissue by LC (113). The lAC column was prepared using monoclonal antibodies originally developed for an enzyme-linked immunosorbent assay (ELISA) method (171) specific for chloramphenicol. Meat samples were extracted with water, and a concentrated phosphate buffer was added to the filtered extracts before immunoaffinity cleanup. A phosphate buffer was used in the washing process, whereas chloramphenicol was eluted from the column with a glycine/sodium chloride solution of pH 2.8. For subsequent LC analysis, this eluate was extracted with ethyl acetate, evaporated, and reconstimted in the mobile phase. The same analytical scheme was later successfully applied for the determination of chloramphenicol in eggs and milk as well (170, 172). [Pg.620]

Apart from radioimmunoassays, various enzyme-linked immunosorbent assays have been described as well. Campbell et al. (42) first reported a sensitive and specific ELISA using polystyrene tubes and a polyclonal antibody. However, the performance of this method was not evaluated with real samples but only with standards and aqueous muscle tissue extracts. Sensitive ELISAs were also developed for the determination of chloramphenicol in milk (43) and eggs (44) the results drawn by the latter assay correlated well with those obtained by application of a radioimmunoassay. [Pg.842]

T. K. Nevanen, H. Simolin, T. Suortti, A. Koivula, and H. Soderlund, Development of a High-Throughput Format for Solid-Phase Extraction of Enantiomers Using an Immunosorbent in 384-Well Plates, Anal. Chem. 2005, 77, 3038. [Pg.682]

Fig. 8 Chromatograms obtained after the injection of a soil extract containing 20 ng g-1 of triazines (a) without and (b) with a clean-up on the terbutylazine MIP and (c) on the anti-triazines immunosorbent. (1) atrazine (2) simazine (3) terbutylazine. UV detection at 220 nm [48]... Fig. 8 Chromatograms obtained after the injection of a soil extract containing 20 ng g-1 of triazines (a) without and (b) with a clean-up on the terbutylazine MIP and (c) on the anti-triazines immunosorbent. (1) atrazine (2) simazine (3) terbutylazine. UV detection at 220 nm [48]...
J.L. Zajicek, D.E. Tillitt, T.R. Schwartz, C.J. Schmitt and R.O. Harrison, Comparison of an enzyme-linked immunosorbent assay (ELISA) to gas chromatography (GC) measurement of polychlorinated biphenyls (PCBs) in selected US fish extracts, Chemosphere, 40 (2000) 539-548. [Pg.600]

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See also in sourсe #XX -- [ Pg.393 ]



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