Reversed phase mode

Nonpolar organic mobile phases, such as hexane with ethanol or 2-propanol as typical polar modifiers, are most commonly used with these types of phases. Under these conditions, retention seems to foUow normal phase-type behavior (eg, increased mobile phase polarity produces decreased retention). The normal mobile-phase components only weakly interact with the stationary phase and are easily displaced by the chiral analytes thereby promoting enantiospecific interactions. Some of the Pirkle-types of phases have also been used, to a lesser extent, in the reversed phase mode. 

Sugar analysis by hplc has advanced greatly as a result of the development of columns specifically designed for carbohydrate separation. These columns fall into several categories. (/) Aminopropyl-bonded siHca used in reverse-phase mode with acetonitrile—water as the eluent. (2) Ion-moderated cation-exchange resins using water as the eluent. Efficiency of these columns is enhanced at elevated temperature, ca 80—90°C. Calcium is the usual counterion for carbohydrate analysis, but lead, silver, hydrogen, sodium, and potassium are used to confer specific selectivities for mono-, di-, and... 

Cyclodextrin stationary phases utilize cyclodextrins bound to a soHd support in such a way that the cyclodextrin is free to interact with solutes in solution. These bonded phases consist of cyclodextrin molecules linked to siUca gel by specific nonhydrolytic silane linkages (5,6). This stable cyclodextrin bonded phase is sold commercially under the trade name Cyclobond (Advanced Separation Technologies, Whippany, New Jersey). The vast majority of all reported hplc separations on CD-bonded phases utilize this media which was also the first chiral stationary phase (csp) developed for use in the reversed-phase mode. 

Except for the high molecular weight range, nearly all substances can be separated by reversed-phase (RP) HPLC. The many different separation mechanisms in RP HPLC, based on hydi ophobic, hydi ophilic and ion-pairing interactions, and size exclusion effects together with the availability of a lai ge number of high quality stationary phases, explain its great populai ity. At present approximately 90% of all HPLC separations are carried out by reversed-phase mode of HPLC, and an estimated 800 different stationai y phases for RP HPLC are manufactured worldwide. 

Statistically, of the compounds enantioresolved by macrocyclic glycopeptide CSPs, new polar organic mode accounts for more than 40 %, balanced by reversed-phase mode, while typical normal-phase operation resulted in approximately 5 % of separations. Some categories of racemic compounds that are resolved on the glycopeptide CSPs at different operating modes are listed in Table 2-4. 

When analytes lack the selectivity in the new polar organic mode or reversed-phase mode, typical normal phase (hexane with ethanol or isopropanol) can also be tested. Normally, 20 % ethanol will give a reasonable retention time for most analytes on vancomycin and teicoplanin, while 40 % ethanol is more appropriate for ristocetin A CSP. The hexane/alcohol composition is favored on many occasions (preparative scale, for example) and offers better selectivity for some less polar compounds. Those compounds with a carbonyl group in the a or (3 position to the chiral center have an excellent chance to be resolved in this mode. The simplified method development protocols are illustrated in Fig. 2-6. The optimization will be discussed in detail later in this chapter. 

A general phenomenon observed with chiral stationary phases having hydrophobic pockets is that a decrease of flow rate results in an increase in resolution. This change has significant impact mostly in reversed-phase mode (see Fig. 2-10). 

For most free amino acids and small peptides, a mixture of alcohol with water is a typical mobile phase composition in the reversed-phase mode for glycopeptide CSPs. For some bifunctional amino acids and most other compounds, however, aqueous buffer is usually necessary to enhance resolution. The types of buffers dictate the retention, efficiency and - to a lesser effect - selectivity of analytes. Tri-ethylammonium acetate and ammonium nitrate are the most effective buffer systems, while sodium citrate is also effective for the separation of profens on vancomycin CSP, and ammonium acetate is the most appropriate for LC/MS applications. 

Another example of the use of small particle silica is in the analysis of theophylline in plasma, as shown in Figure 5 (40). The clean-up procedure is simply a single extraction of the plasma with an organic solvent. This analysis has also been achieved by reverse phase chromatography (41), and this points out the fact that in some separations (e.g. with components of moderate polarity) either the adsorption or reverse phase mode can be used. 

The PRISMA model was developed by Nyiredy for solvent optimization in TLC and HPLC [142,168-171]. The PRISMA model consists of three parts the selection of the chromatographic system, optimization of the selected mobile phases, and the selection of the development method. Since silica is the most widely used stationary phase in TLC, the optimization procedure always starts with this phase, although the method is equally applicable to all chemically bonded phases in the normal or reversed-phase mode. For the selection of suitable solvents the first experiments are carried out on TLC plates in unsaturated... 

Ionic solutes can be separated by ion-exchange chromatography using microparticulate resins or bonded ion-exchangers based on microparticulate silica. Such separations are often achieved more easily by ion-suppression or ion-pairing techniques, which use bonded phase columns in the reverse phase mode. 

Distilled or deionised water contains small amounts of organic impurities which can cause problems in long term use with bonded phase columns in the reverse phase mode. The non-polar stationary phase will collect these organics, which can alter the nature of the stationary phase or sometimes produce spurious peaks (Fig. 4.3c is an example of this). Water purification can be done by distillation from permanganate, by passage of the water through bonded phase columns, or by means of commercial systems, eg the Milli-... 

Simple and comprehensive 2D HPLC was reported in a reversed-phase mode using monolithic silica columns for the 2nd-D separation (Tanaka et al., 2004). Every fraction from the lst-D column, 15cm long (4.6 mm i.d.), packed with fluoroalkylsilyl-bonded (FR) silica particles (5 pm), was subjected to the separation in the 2nd-D using one or two octadecylsilylated (Cig) monolithic silica columns (4.6 mm i.d., 3 cm). Monolithic silica columns in the 2nd-D were eluted at a flow rate of up to lOmL/min with separation time of 30 s that provides fractionation every 15-30s for the lst-D, which is operated near the optimum flow rate of 0.4-0.8 mL/min. The 2D-HPLC systems were assembled, as shown in Fig. 7.6, so that the sample loops of the 2nd-D injectors were back flushed to minimize band broadening. 

Additionally, the inj ected matrix must also be miscible with the solvents used in the separations. For normal phase mode separations, all water must be removed from the injected matrix. Since many of the complex matrixes, such as plasma, urine, and other biological fluids contain a large amount of water, this requires more time consuming sample preparation. However, water can be injected into a polar organic or reverse phase mode separation. Even within the same mode, mobile phases that are very different can cause large disturbances in the baseline. Oda et al., (1991) solved this problem by inserting a dilution tube followed by a trap column in order to dilute the mobile phase used on the achiral column. Following the dilution tube, a trap column was used to reconcentrate the analyte of interest before the enantiomeric separation. 

Because plasma and urine are both aqueous matrixes, reverse-phase or polar organic mode enantiomeric separations are usually preferred as these approaches usually requires less elaborate sample preparation. Protein-, cyclodextrin-, and macrocyclic glycopeptide-based chiral stationary phases are the most commonly employed CSPs in the reverse phase mode. Also reverse phase and polar organic mode are more compatible mobile phases for mass spectrometers using electrospray ionization. Normal phase enantiomeric separations require more sample preparation (usually with at least one evaporation-to-dryness step). Therefore, normal phase CSPs are only used when a satisfactory enantiomeric separation cannot be obtained in reverse phase or polar organic mode. 

Ekgorg-Ott et al. (1997). An interesting trend was discovered when considering the relative amount of D-theanine present in the samples. The teas of the highest grades consistently contained the lowest amounts of D-theanine. The theanine achiral-chiral system configuration included a C18 column operated in the reverse-phase mode and a y-cyclodextrin CSP in the polar organic mode. 

Like plasma and urine, matrixes from plant or environmental sources contain a vast diversity of components. Thus, achiral-chiral LC-LC is also useful for analysis involving samples from these sources. Stalcup et al. (1991) studied the enantiomeric purity of scopolamine extracted from Datura sanguinea in both homogenized plant leaves and commercial extracts. A reverse-phase separation on a C j g column separated the scopolamine from other alkaloid and matrix components while the enantiomeric separation (also in the reverse-phase mode) was carried out on two coupled [3-cyclodextrin columns or a single acetylated (3-cyclodextrin column. The single... 

Ferretti et al. (1988) used an amino column coupled to a derivatized amylose column (Chiralpak AS) operated in the reverse-phase mode to separate the enantiomers of the antifungal agent voriconazole from several chiral impurities and one achiral impurity. Three of the chiral impurities are the other enantiomer and corresponding diastereomers of voriconazole. More chiral impurities result from a chlorinated voriconazole. Additionally, this multidimensional method could baseline separate all but two of the chiral impurities into their respective enantiomers. These separations are shown in Figure 14.5. 

Various chiral lumazines produced from the parent pterins by an enzymatic reaction were separated using achiral-chiral multidimensional LC-LC by Klein et al. (1994). A Ci 8 column and a flavoprotein column were used in the reverse-phase mode to achieve the separation of the threo forms of the lumazines. The flavoprotein column was unable to resolve the erythro forms. 

Thick-layer silica gel chromatography can also be employed [7], although most separations are now accomplished by high-performance liquid chromatography. Resolution of complex mixtures often requires both normal and reverse phase modes [19]. A further dimension is added, when bioactivity is correlated with spectroscopically-monitored chromatographic profiles. 

Identification and quantification of natural dyes need high performance analytical techniques, appropriate for the analysis of materials of complicated matrices containing a small amount of coloured substances. This requirement perfectly fits coupling of modern separation modules (usually high performance liquid chromatography in reversed phase mode, RPLC, but also capillary electrophoresis, CE) with selective detection units (mainly mass spectrometer). 

It is estimated that over 65% (possibly up to 90%) of all HPLC separations are carried out in the reversed-phase mode. The reasons for this include the simplicity, versatility, and scope of the reversed-phase method [23]. The hydrocarbon-like stationary phases equilibrate rapidly with changes in mobile-phase composition and are therefore eminently suitable for use with gradient elution. 

There are two commonly used ways to elute a given compound in HPLC the normal-phase mode (t)s><5m) and the reversed-phase mode (<5m><5s). Reversed-phase systems offer superior general selectivity. Solutes are eluted in ascending order of polarity in normal-phase systems and in descending order of polarity in reversed-phase systems. 

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