Preparative Chiral Stationary Phases

Table 6.1 Most used commercially available preparative chiral stationary phases.

Pirkle, W.H. Pochapsky. T.C. Mahler, G.S. Corey. D.E. Reno. D.S. Alessi. D.M. Useful and easily prepared chiral stationary phases for the direct chromatographic separation of the enantiomers of a ariety of deriv atised amines, ammo... 

Stationary phase In order to prepare chiral stationary phase, 10 g of -cyclodextrin (/3-CD) and 5 g of silica gel H were weighed and dried at 110 C in an oven under vacuum for 12 h. /3-CD was dissolved in approximately 120 ml of anhydrous dimethylformamide (DMF) with a small amount of sodium the mixture was stirred for 2-3 h at 90" C and filtered. Silica gel H and 2.5 g of KH-560 (3-glycidoxypropyltrimethoxysilane) were added to the filtrate and the mixture was stirred for 12-18 h at 90" C. The suspension was filtered and washed with DMF, toluene, methanol, water, again with methanol, and then dried in air. To 2 g of obtained /3-CD-bonded silica gel, 6 ml of 0.3% aqueous solution of carboxy-methyl cellulose (CMC) sodium were added, and the slurry obtained was spread as a layer 0.2-0.4 mm thickness on glass plates 2.5 x 7.5 cm in size. Plates were dried in air and activated before use in an oven at 80°C for 1 h. 

Chiral Hplc Columns. There are about 40 commercially available chiral columns which are suitable for analytical and preparative purposes (57). In spite of the large number of commercially available chiral stationary phases, it is difficult and time-consuming to obtain good chiral separation. In order to try a specific resolution meaninghilly, a battery of chiral hplc columns is necessary and this is quite expensive. 

Gas chromatography (gc) is inferior to hplc in separating abiUty. With gc, it is better to use capillary columns and the appHcation is then limited to analysis (67). Resolution by thin layer chromatography or dc is similar to Ic, and chiral stationary phases developed for Ic can be used. However, tic has not been studied as extensively as Ic and gc. Chiral plates for analysis and preparation of micro quantities have been developed (68). 

Synthetic chiral adsorbents are usually prepared by tethering a chiral molecule to a silica surface. The attachment to the silica is through alkylsiloxy bonds. A study which demonstrates the technique reports the resolution of a number of aromatic compoimds on a 1- to 8-g scale. The adsorbent is a silica that has been derivatized with a chiral reagent. Specifically, hydroxyl groups on the silica surface are covalently boimd to a derivative of f -phenylglycine. A medium-pressure chromatography apparatus is used. The racemic mixture is passed through the column, and, when resolution is successful, the separated enantiomers are isolated as completely resolved fiactions. Scheme 2.5 shows some other examples of chiral stationary phases. 

J. Dingenen and J. N. Kinkel, Preparative cliromatograpliic resolution of racemates on chiral stationary phases on laboratoiy and production scales by closed-loop recycling cliromatography , J. Chromatogr. 666 627-650 (1994). 

HPLC separations are one of the most important fields in the preparative resolution of enantiomers. The instrumentation improvements and the increasing choice of commercially available chiral stationary phases (CSPs) are some of the main reasons for the present significance of chromatographic resolutions at large-scale by HPLC. Proof of this interest can be seen in several reviews, and many chapters have in the past few years dealt with preparative applications of HPLC in the resolution of chiral compounds [19-23]. However, liquid chromatography has the attribute of being a batch technique and therefore is not totally convenient for production-scale, where continuous techniques are preferred by far. 

W. H. Pirkle and B. C. Hamper, The direct preparative resolution of enantiomers by liquid chromatography on chiral stationary phases in Preparative Liquid Chromatography, B. A. Bidling-meyer (Ed.), Journal Chromatography Library Vol. 38, 3 Edition, Elsevier Science Publishers B. V, Amsterdam (1991) Chapter 7. 

Enantiomeric separations have become increasingly important, especially in the pharmaceutical and agricultural industries as optical isomers often possess different biological properties. The analysis and preparation of a pure enantiomer usually involves its resolution from the antipode. Among all the chiral separation techniques, HPLC has proven to be the most convenient, reproducible and widely applicable method. Most of the HPLC methods employ a chiral selector as the chiral stationary phase (CSP). 

Proteins. A chiral stationary phase with immobilized a -acid glycoprotein on silica beads was introduced by Hermansson in 1983 [18, 19]. Several other proteins such as chicken egg albumin (ovalbumin), human serum albumin, and cellohy-drolase were also used later for the preparation of commercial CSPs. Their selectivity is believed to occur as a result of excess of dispersive forces acting on the more retained enantiomer [17]. These separation media often exhibit only modest loading capacity. 

In addition to the development of the powerful chiral additive, this study also demonstrated that the often tedious deconvolution process can be accelerated using HPLC separation. As a result, only 15 libraries had to be synthesized instead of 64 libraries that would be required for the full-scale deconvolution. A somewhat similar approach also involving HPLC fractionations has recently been demonstrated by Griffey for the deconvolution of libraries screened for biological activity [76]. Although demonstrated only for CE, the cyclic hexapeptides might also be useful selectors for the preparation of chiral stationary phases for HPLC. However, this would require the development of non-trivial additional chemistry to appropriately link the peptide to a porous solid support. 

Fig. 3-11. Concept of reciprocal combinatorial approach to the preparation of chiral stationary phase. (Reprinted with permission from ref. [55]. Copyright 1999, American Chemical Society.)...

In the next step, the best candidate from the series 2-oxo-4-(9-phenanthryl)-dihy-dropyrimidine 22 was prepared and isolated in enantiomerically pure form, then attached to a macroporous polymer support. To attach the isolated selector to the amino functionalized macroporous polymethacrylate support, a suitable reactive handle had to be introduced into the dihydropyrimidine. We chose to functionalize the methyl group at the C6 carbon atom by a simple bromination to afford (-)-22. Coupling of this compound to the amino functionalized support then gave the desired chiral stationary phase CSP 12 (Scheme 3-6) containing 0.20 mmol g of the selector. 

Despite the difficulties caused by the rapidly expanding literature, the use of chiral stationary phases (CSPs) as the method of choice for analysis or preparation of enantiomers is today well established and has become almost routine. It results from the development of chiral chromatographic methods that more than 1000 chiral stationary phases exemplified by several thousands of enantiomer separations have been described for high-performance liquid chromatography (HPLC). 

In 1996, Fu et al. reported the S3mthesis of the planar chiral heterocycles 64, formally DMAP fused with a ferrocene core [82]. While the original synthesis provided racemic 64a in only 2% overall yield requiring a subsequent resolution by preparative HPLC on a chiral stationary phase, a recently improved synthesis furnished the racemic complexes 64 in 32-40% yield over seven steps. A subsequent resolution with di-p-toluoyltartaric or dibenzoyltartaric acid gave access to the enantiomers with >99% ee (28 14% yield for each isomer in this step) [83]. 

The last several years have seen an enormous growth in the number and use of chiral stationary phases in liquid chromatography [742,780-791]. Some problems with the gas chromatographic approach are that the analyte must be volatile to be analyzed and larger-scale preparative separations are frequently difficult. For entropic reasons relatively high temperatures tend to minimize the stability differences between the diastereomeric complexes and racemization of the stationary phase over time may also occur. The upper temperature limit for phases such as Chirasil-Val is about 230 C and is established by the rate of racemization of the chiral centers and not by column bleed. Liquid chromatography should be s ior in the above... 

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... 

Miller, L., Orihuela, C., Fronek, R., and Murphy, J., Preparative chromatographic resolution of enantiomers using polar organic solvents with polysaccharide chiral stationary phases,. Chromatogr. A, 865, 211, 1999. 

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