Proteins protein preparation

Silver nitrate is astringent and a protein precipitant, which is not medically desirable. Other forms of silver have been used to avoid this problem, including coUoidal silver, silver-protein preparations, and finely divided silver metal called Katadyn silver. [Pg.136]

Gel filtration is very suitable for the purity check of protein preparations, especially if these have been purified by adsorptive techniques. It can be expected that high-resolution gel filtration columns will easily separate dimeric forms from monomeric forms to reveal heterogeneities of the preparations. However, a size difference of less than 20% will not result in total resolution of the peaks (although the chromatogram may be used for a qualitative judgment of the... [Pg.70]

The simplest way to prepare a biocatalyst for use in organic solvents and, at the same time, to adjust key parameters, such as pH, is its lyophilization or precipitation from aqueous solutions. These preparations, however, can undergo substrate diffusion limitations or prevent enzyme-substrate interaction because of protein-protein stacking. Enzyme lyophilization in the presence of lyoprotectants (polyethylene glycol, various sugars), ligands, and salts have often yielded preparations that are markedly more active than those obtained in the absence of additives [19]. Besides that, the addition of these ligands can also affect enzyme selectivity as follows. [Pg.9]

The other method of monolayer transfer from the air/water interface onto solid substrates is illustrated in Figure 2. This method is called the Langmuir-Schaefer technique, or horizontal lift. It was developed in 1938 by I. Langmuir and V. Schaefer for deposition of protein layers. Prepared substrate horizontally touches the monolayer, and the layer transfers itself onto the substrate surface. The method is often used for the deposition of rigid monolayers and for protein monolayers, hi both cases the apphcation of the Lang-muir-Blodgett method produces defective films. [Pg.142]

Anionic poly(amidoamine) (PAMAM) dendrimer was selected as a model of the soluble acidic-rich proteins to prepare CaC03 film on a poly(ethylenimine) film [49]. The CaCOj/polylethylenimine) composite film was obtained in the... [Pg.155]

Ka5, J., Rauch, P. Labeled Proteins, Their Preparation and Application. 112,163-230(1983). [Pg.183]

White, J. W. (1992). Internal standard stable carbon isotope ratio method for determination of C-4 plant sugars in honey Collaborative trial study, and evaluation of improved protein preparation procedure. J. Assoc. Ojfic. Anal. Chem. 75,543-548. [Pg.136]

Another means of moving beyond pure protein preparations to high-throughput characterization of proteomes is to enrich for phosphopeptides from complex mixtures by metal affinity chromatography (Andersson and Porath, 1986). Using this method, protein mixtures are proteolyzed to create peptides and phosphorylated peptides are enriched by metal affinity chromatography and subsequently identified by mass spectrometry. This method is limited, however, because in many cases phosphopeptides absorb poorly or nonphosphorylated peptides absorb nonspecifically to the metal affinity resins (Ahn and Resing, 2001). [Pg.19]

FIGURE 15.1 One-dimensional capillary electrophoresis separation of a protein homogenate prepared from the hTERT cell line. Both separations were preformed in 30 pm ID, 145 pm OD, 20 cm long capillaries at 20,000 V. (a) Micellar electrokinetic chromatography performed with a 100 mM CHES, 100 mM Tris, and 15 mM SDS buffer at pH 8.7. Sample is electro-kinetically injected with 0.25 kV for 1 s (b) Capillary sieving electrophoresis performed in 5% Dextran (513 kDa), 100 mM CHES, 100 mM Tris, 3.5 mM SDS, pH 8.7. [Pg.352]

FIGURE 15.4 Computer record of a two-dimensional capillary electrophoresis analysis of a protein homogenate prepared from ahiopsy obtained from the fundus of a Barrett s esophagus patient. The data were generated hy performing 1 s transfers between capillaries and a 9 s second-dimension separation. The first-dimension separation employed the same buffer as the CSE separation in Fig. 15.1 and the second-dimension separation employed the same buffer as the MECC separation in Fig. 15.1. [Pg.355]

Umelo-Njaka, E., Nomellini, J.F., Bingle, W.H. et al. (2001) Expression and testing of Pseudomonas aeruginosa vaccine candidate proteins prepared with the Caulobacter crescentus S-layer protein expression system. Vaccine, 19 (11-12), 1406-1415. [Pg.54]

Big Chemical Encyclopedia

Chemical substances, components, reactions, process design ...