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Fixation isolated proteins

Since the Schiff base formation is reversible, it should be reduced by sodium borohydride for the fixation of the label. The rate of the reduction of the Schiff base becomes slow as the number of the phosphate groups of the label increases. However, except for adenylate kinase, the NP -PL bound to the proteins were easily fixed by borohydride reduction. After reductive fixation, labeled proteins are cleaved by appropriate methods. The labeled lysine is cleaved by neither trypsin nor lysyl endopeptidase. There are at least three ways to detect the labeled peptide during isolation 1) use of radioactive reagent, 2) use of radioactive sodium borohydride for reduction of the Schiff base, and 3) use of fluorescence derived from the pyridoxyl moiety of the reagent (excitation at 295 nm and emission at 390 nm at acidic pH). The labeled lysyl residue is not positively identified in the amino acid sequence analysis. However, the presence of the label in the peptide isolated can be confirmed by the presence of pyridoxyl lysine in the amino acid analysis. [Pg.76]

Plant Cells and Tissues Structure-Function Relationships. Methods for the Cytochemical/Histochemical Localization of Plant Cell/Tissue Chemicals. Methods in Light Microscope Radioautography. Some Fluorescence Microscopical Methods for Use with Algal, Fungal, and Plant Cells. Fluorescence Microscopy of Aniline Blue Stained Pistils. A Short Introduction to Immunocytochemistry and a Protocol for Immunovi-sualization of Proteins with Alkaline Phosphatase. The Fixation of Chemical Forms on Nitrocellulose Membranes. Dark-Field Microscopy and Its Application to Pollen Tube Culture. Computer-Assisted Microphotometry. Isolation and Characterization of... [Pg.313]

The studies discussed so far deal - for good reasons - with the isolated FeMoco. However, qualitative molecular modeling has also been used to identify possible proton transfer routes from the surface of the nitrogenase protein to the FeMoco (40) and mechanistic aspects of biological nitrogen fixation are discussed in the light of such data (10-12). [Pg.60]

Bazhenova, T.A., Bazhenova, M.A., Petrova, G.N., and Shilov, A.E. (2000) Catalytic behavior of isolated FeMo-cofactor of nitrogenase in non-protein surroundings, Current Plant Science and Biotechnology in Agriculture 38 (Nitrogen Fixation From Molecules to Crop Productivity), 49-50. [Pg.191]

Since protein complex formation and Ca2+ are critical to cell fixation within a tissue, dissociation media usually contain some type of proteolytic enzyme and the Ca2+ chelator, EDTA. The proteolytic enzyme can be of general specificity, such as trypsin, or can be a more targeted enzyme, such as a collagenase selective for the collagen-type characteristic of the tissue of interest. Hyaluronidase has been also used with matrix rich in hyaluronic acid, such as for isolation of duodenal entero-cytes. In all cases, the appropriate incubation times and concentrations to achieve cell dispersal, but retain high viability, need to be determined empirically. One factor... [Pg.132]

See other pages where Fixation isolated proteins is mentioned: [Pg.190]    [Pg.254]    [Pg.525]    [Pg.525]    [Pg.254]    [Pg.153]    [Pg.174]    [Pg.87]    [Pg.327]    [Pg.192]    [Pg.300]    [Pg.18]    [Pg.112]    [Pg.657]    [Pg.45]    [Pg.378]    [Pg.111]    [Pg.479]    [Pg.857]    [Pg.1360]    [Pg.718]    [Pg.39]    [Pg.54]    [Pg.290]    [Pg.374]    [Pg.395]    [Pg.309]    [Pg.3100]    [Pg.288]    [Pg.479]    [Pg.246]    [Pg.55]    [Pg.56]    [Pg.857]    [Pg.2416]    [Pg.718]    [Pg.266]    [Pg.82]    [Pg.468]    [Pg.733]    [Pg.2085]    [Pg.52]    [Pg.55]    [Pg.268]   
See also in sourсe #XX -- [ Pg.2 , Pg.196 ]



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Protein isolate

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