Stationary phases Pirkle type

The separation of bi-naphthol enantiomers can be performed using a Pirkle-type stationary phase, the 3,5-dinitrobenzoyl phenylglycine covalently bonded to silica gel. Eight columns (105 mm length) were packed with particle diameter of 25 0 fiva. The solvent is a 72 28 (v/v) heptane isopropanol mixture. The feed concentration is 2.9 g for each enantiomer. The adsorption equilibrium isotherms were determined by the Separex group and already reported in Equation (28) [33]. 

Mobile phases are usually binary or ternary mixtures of solvents. Selectivity is affected mostly by mobile phase composition rather than strength, and peak shape and retention are both influenced by the addition of organic modifiers.101 Some compounds naturally have 77-donor or 77-acceptor groups and can be resolved directly. In many cases, however, introduction of 77-donating groups by derivatization steps is necessary. Figure 2.20 shows the proposed three-point interaction of 3-aminobenzo[a]pyrene, a polycyclic aromatic hydrocarbon (PAH), with a Pirkle-type stationary phase.111 Two possible interactions are illustrated, showing the best orientations for maximum interaction. 

Recently, optically active polythiophenes, incorporating as ring substituents chiral selectors such as (R)-(-)- and CS )-(+)-/V-(3,5-dinitrobcnzoyl)-a-phcnylglycinc used in Pirkle-type stationary phases, have been synthesized.167 These may have potential in enantioselective analysis of chiral chemicals using high performance liquid chromatography (HPLC). 

Figure 6.39 Pirkle -type stationary phase—ionically bound (/ )-7Y-(dinitrobenzoyl)-phenyl-...

Two of the more common Pirkle type stationary phases in use today are the a-Burke 1 and the Whelk-01. The structure of a-Burke 1 is given below. 

Protein Based Stationary Phases The Pirkle Type Stationary Phases Coated Cellulose and Amylose Derivatives Macrocyclic Glycopeptide Stationary Phases Cyclodextrin Based Chiral Stationary Phases Synopsis References Chapter 9... 

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. 

There is a wide variety of commercially available chiral stationary phases and mobile phase additives.32 34 Preparative scale separations have been performed on the gram scale.32 Many stationary phases are based on chiral polymers such as cellulose or methacrylate, proteins such as human serum albumin or acid glycoprotein, Pirkle-type phases (often based on amino acids), or cyclodextrins. A typical application of a Pirkle phase column was the use of a N-(3,5-dinitrobenzyl)-a-amino phosphonate to synthesize several functionalized chiral stationary phases to separate enantiomers of... 

Chiral stationary phases for the separation of enantiomers (optically active isomers) are becoming increasingly important. Among the first types to be synthesized were chiral amino acids ionically or covalently bound to amino-propyl silica and named Pirkle phases after their originator. The ionic form is susceptable to hydrolysis and can be used only in normal phase HPLC whereas the more stable covalent type can be used in reverse phase separations but is less stereoselective. Polymeric phases based on chiral peptides such as bovine serum albumin or a -acid glycoproteins bonded to... 

Chiral separations result from the formation of transient diastereomeric complexes between stationary phases, analytes, and mobile phases. Therefore, a column is the heart of chiral chromatography as in other forms of chromatography. Most chiral stationary phases designed for normal phase HPLC are also suitable for packed column SFC with the exception of protein-based chiral stationary phases. It was estimated that over 200 chiral stationary phases are commercially available [72]. Typical chiral stationary phases used in SFC include Pirkle-type, polysaccharide-based, inclusion-type, and cross-linked polymer-based phases. 

New brush-type phases (donor-acceptor interactions) are appearing all the time. " Examples are stationary phases comprising quinine derivatives and trichloro-dicyanophenyl-L-a-amino acids as chiral selectors. Quinine carbamates, which are suitable for the separation of acidic molecules through an ionic interaction with the basic quinine group, are also commonly used but in general they are classified with the anion-exchange type of chiral selectors (see further) because of their interaction mechanism, even though r-donor, r-acceptor properties occur. (Some separations on Pirkle-type CSPs are shown in Table 2.)... 

There are numerous chiral stationary phases available commercially, which is a reflection of how difficult chiral separations can be and there is no universal phase which will separate all types of enantiomeric pair. Perhaps the most versatile phases are the Pirkle phases, which are based on an amino acid linked to aminopropyl silica gel via its carboxyl group and via its amino group to (a-naphthyl)ethylamine in the process of the condensation a substituted urea is generated. There is a range of these type of phases. As can be seen in Figure 12.23, the interactions with phase are complex but are essentially related to the three points of contact model. Figure 12.24 shows the separation of the two pairs of enantiomers (RR, SS, and RS, S,R) present in labetalol (see Ch. 2 p. 36) on Chirex 3020. 

Many types of chiral stationary phase are available. Pirkle columns contain a silica support with bonded aminopropyl groups used to bind a derivative of D-phenyl-glycine. These phases are relatively unstable and the selectivity coefficient is close to one. More recently, chiral separations have been performed on optically active resins or cyclodextrins (oligosaccharides) bonded to silica gel through a small hydrocarbon chain linker (Fig. 3.11). These cyclodextrins possess an internal cavity that is hydro-phobic while the external part is hydrophilic. These molecules allow the selective inclusion of a great variety of compounds that can form diastereoisomers at the surface of the chiral phase leading to reversible complexes. 

High-performance LC is also a suitable method for separating BHA isomers. Commercially available BHA is a mixture of two positional isomers, an approximately 85 15 ratio of 3-BHA and 2-BHA. The former is approximately 2.4 times more effective as a food antioxidant than is 2-BHA, and half as effective as an inhibitor of benzo(a)pyrene-induced for stomach neoplasia in mice. For the separation, Ansari (116) used isocratic elution with 7% of 2-propanol in hexane on a Pirkle Type I-A column packed with 5- 01 y-aminopropyl packing, modified with lV-3,5-dinitrobenzoyl derivative of D-phenylglycine. Column eluent was monitored at 288 nm, with a detection limit between 1 and 2 ng. Under these conditions, isomers were separated without derivatization, where the phenolic group of 3-BHA was sterically hindered by an o-rm-butyl group and therefore could not interact with stationary phase that resulted in its rapid elution. 

Pirkle-Type and Related Chiral Stationary Phases... 

In view of the importance of chiral resolution and the efficiency of liquid chromatographic methods, attempts are made to explain the art of chiral resolution by means of liquid chromatography. This book consists of an introduction followed by Chapters 2 to 8, which discuss resolution chiral stationary phases based on polysaccharides, cyclodextrins, macrocyclic glyco-peptide antibiotics, Pirkle types, proteins, ligand exchangers, and crown ethers. The applications of other miscellaneous types of CSP are covered in Chapter 9. However, the use of chiral mobile phase additives in the separation of enantiomers is discussed in Chapter 10. 

The Pirkle-type chiral stationary phases are quite stable and exhibit good chiral selectivities to a wide range of solute types. These CSPs are also popular for the separation of many drug enantiomers and for amino acid analysis. Primarily, direct chiral resolution of racemic compounds were achieved on these CSPs. However, in some cases, prederivatization of racemic compounds with achiral reagents is required. The applications of these phases are discussed considering re-acidic, re-basic, and re-acidic-basic types of CSP. These CSPs have also been found effective for the chiral resolution on a preparative scale. Generally, the normal phase mode was used for the chiral resolution on these phases. However, with the development of new and more stable phases, the reversed phase mode became popular. 

Finn JM, Rational design of Pirkle type chiral stationary phases, in Chromatographic Chiral Separations, Zief M, Crane LJ (Eds.), Chromatographic Science Series Vol. 40, Marcel Dekker, New York (1988). 

---