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Open column cellulose

Because plants present chlorophylls and carotenoids simultaneously, it may be useful to separate both groups from each other in a laboratory or preparative scale in order to avoid contamination in further purification steps, mainly when they are prepared in large amounts. Clean-up procedures using an open column packed with absorbents such as alumina, magnesia, polyethylene powder, powdered sucrose, DEAE-Sepharose, starch, cellulose, or MgO HyfloSupercel are good approaches. MgO HyfloSupercel in a proportion of 1 1 or 1 2 is the usual adsorbent. Sucrose and cellulose are interesting as they do not alter the chlorophylls, but they are tedious to work with. [Pg.432]

The hydrophilic silica-based diol packings have been modified by derivation through some of the diol groups with carboxymethyl and diethy-laminoethyl functions to make weak anionic and cationic protein size-separation columns. These provide the HPLC equivalent of the CM- and DEAE-cellulose columns used in protein purification on open columns and are used with the same type of buffers to provide ion exchange purifications of proteins. [Pg.101]

Classical separations by open column chromatography with different stationary phases (silica gel, reversed-phase C-18 or C-8, polyamide, cellulose) and elution with appropriate solvent mixtures are also useful for flavonoid fractionation and purification. Different column systems can be used. The classical open column chromatography uses relatively large particle sizes (0.2-6 mm), with limited resolution, and solvent filtration through the column proceeds by the pressure of the solvent column placed on top of the stationary phase. In other cases, smaller... [Pg.213]


See other pages where Open column cellulose is mentioned: [Pg.4]    [Pg.126]    [Pg.514]    [Pg.61]    [Pg.156]    [Pg.2]    [Pg.198]    [Pg.198]    [Pg.30]    [Pg.216]    [Pg.6]    [Pg.77]    [Pg.23]    [Pg.192]    [Pg.21]    [Pg.282]   
See also in sourсe #XX -- [ Pg.125 ]




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