Packed Column Sizing

Column Packing Column Size Temperature Reference... 

It is clear that the separation ratio is simply the ratio of the distribution coefficients of the two solutes, which only depend on the operating temperature and the nature of the two phases. More importantly, they are independent of the mobile phase flow rate and the phase ratio of the column. This means, for example, that the same separation ratios will be obtained for two solutes chromatographed on either a packed column or a capillary column, providing the temperature is the same and the same phase system is employed. This does, however, assume that there are no exclusion effects from the support or stationary phase. If the support or stationary phase is porous, as, for example, silica gel or silica gel based materials, and a pair of solutes differ in size, then the stationary phase available to one solute may not be available to the other. In which case, unless both stationary phases have exactly the same pore distribution, if separated on another column, the separation ratios may not be the same, even if the same phase system and temperature are employed. This will become more evident when the measurement of dead volume is discussed and the importance of pore distribution is considered. 

A trend in chromatography has been to use monosized particles as supports for ion-exchange and size-exclusion chromatography and to minimize the column size, such as using a 15 X 4.6-mm column packed with 3-/rm polymer particles for size exclusion chromatography. The more efficient and lower back pressure of monosized particles is applied in the separation. 

With soft gels, column packing has often been plagued with such problems as inferior reproducibility and excessive time requirements. These problems are alleviated with physically stable Toyopearl HW media. However, an improperly packed column can have significantly reduced efficiency. The two key variables for the successful packing of Toyopearl HW media, packing velocity and column size, have been evaluated to determine the optimal packing conditions. 

The packed columns of Shodex OHpak SB-800HQ series are packed with polyhydroxymethacrylate gels and are designed for use with high-resolution, high-speed aqueous size exclusion chromatography. The packed columns are best suited for the analysis of water-soluble polymers and proteins (Table 6.8). 

All packing materials produced at PSS are tested for all relevant properties. This includes physical tests (e.g., pressure stability, temperature stability, permeability, particle size distribution, porosity) as well as chromatographic tests using packed columns (plate count, resolution, peak symmetry, calibration curves). PSS uses inverse SEC methodology (26,27) to determine chromatographic-active sorbent properties such as surface area, pore volume, average pore size, and pore size distribution. Table 9.10 shows details on inverse SEC tests on PSS SDV sorbent as an example. Pig. 9.10 shows the dependence... 

Styragel columns are compatible with most solvents commonly used in size exclusion chromatography. Exceptions are found on both sides of the polarity scale the use of standard general-purpose Styragel columns with aliphatic hydrocarbons or with alcohols (except hexafluoroisopropanol) and water is generally not recommended. However, it is possible to pack columns in special solvents for special-purpose applications. The interested user should contact Waters for additional information. 

Each of the PLgel individual pore sizes is produced hy suspension polymerization, which yields a fairly diverse range of particle sizes. For optimum performance in a chromatographic column the particle size distribution of the beads should be narrow this is achieved by air classification after the cross-linked beads have been washed and dried thoroughly. Similarly, for consistent column performance, the particle size distribution is critical and is another quality control aspect where both the median particle size and the width of the distribution are specified. The efficiency of the packed column is extremely sensitive to the median particle size, as predicted by the van Deemter equation (4), whereas the width of the particle size distribution can affect column operating pressure and packed bed stability. 

The instrumentation of HdC, including a pump, an injector, a column (set), a detector, and a recorder or computer, is very similar to size exclusion chromatography SEC). The essence of this technique is the column. There are two types of HdC columns open microcapillary tubes and a nonporous gel-packed column. This chapter emphasizes column technology and selection and the applications of this technique on the molecular weight analysis of macromolecules. 

Although the OTHdC has several unique applications in polymer analysis, this technique has several limitations. First, it requires the instrumentation of capillary HPLC, especially the injector and detector, which is not as popular as packed column chromatography at this time. Second, as discussed previously, the separation range of a uniform capillary column is rather narrow. Third, it is difficult to couple capillary columns with different sizes together as SEC columns. 

SEC, size exclusion chromatography OTHdC, open tubular hydrodynamic chromatography PCHdC, packed column hydrodynamic chromatography ThFFF, thermal field flow fractionation. 

Incoming water is sprayed through a packed column, which provides for an enlarged surface area, and aids the release of gases from the thin film of water produced in the packing. Depending on the DA size and design, the applied vacuum is maintained either by vacuum pumps or by stream-jet eductors. 

A number of analytical techniques such as FTIR spectroscopy,65-66 13C NMR,67,68 solid-state 13 C NMR,69 GPC or size exclusion chromatography (SEC),67-72 HPLC,73 mass spectrometric analysis,74 differential scanning calorimetry (DSC),67 75 76 and dynamic mechanical analysis (DMA)77 78 have been utilized to characterize resole syntheses and crosslinking reactions. Packed-column supercritical fluid chromatography with a negative-ion atmospheric pressure chemical ionization mass spectrometric detector has also been used to separate and characterize resoles resins.79 This section provides some examples of how these techniques are used in practical applications. 

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