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Column Systems, Dilution, and Splitting

the column diameters chosen for the two dimensions are determined by the amount of sample available and will dictate the flow rate ranges available to use. In split-flow systems, where only a portion of the first-dimension effluent is injected into the second dimension, the choice of column size is unlimited and the two methods can be developed independently. In comprehensive systems where the entire sample from the first dimension is injected into the second dimension, the flow rates are generally lower in the first dimension to accommodate the lower injection volumes into the second dimension. For example, for a 1-mm ID column in the first dimension with a flow rate of 50 (tL/min and a sampling rate of 1 min, 50 pL could be injected onto the second dimension. A 50-(lL injection onto a4.6-mm ID column flowing at 1 mL/min should be accommodated fairly well based upon its composition. In Chapter 6, the first dimension column diameters are estimated based upon the injection volume and sampling rate into the second dimension. [Pg.109]

Detection in 2DLC is the same as encountered in one-dimensional HPLC. A variety of detectors are presented in Table 5.2. The choice of detector is dependent on the molecule being detected, the problem being solved, and the separation mode used for the second dimension. If MS detection is utilized, then volatile buffers are typically used in the second-dimension separation. Ultraviolet detection is used for peptides, proteins, and any molecules that contain an appropriate chromophore. Evaporative light scattering detection has become popular for the analysis of polymers and surfactants that do not contain UV chromophores. Refractive index (RI) detection is generally used with size exclusion chromatography for the analysis of polymers. [Pg.109]


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Splitting system

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