Tyrosine resolution

Although some applications for preparative-scale separations have already been reported [132] and the first commercial systems are being developed [137, 138], examples in the field of the resolution of enantiomers are still rare. The first preparative chiral separation published was performed with a CSP derived from (S -N-(3,5-dinitrobenzoyl)tyrosine covalently bonded to y-mercaptopropyl silica gel [21]. A productivity of 510 mg/h with an enantiomeric excess higher than 95% was achieved for 6 (Fig. 1-3). 

This led to the conclusion that these amino acids were essential for the resolution capability and only 6 new libraries of 18 compounds had to be synthesized with these amino acid residues to define the position 3. Surprisingly, the separation abilities of all six libraries were very similar. Therefore, tyrosine was chosen for continuing deconvolution, since it is convenient as its aromatic ring can easily be detected by UV spectrometry. The last step, defining position 5, required the synthesis and testing of 6 individual hexapeptides. 

The improvements in resolution achieved in each deconvolution step are shown in Figure 3-3. While the initial library could only afford a modest separation of DNB-glutamic acid, the library with proline in position 4 also separated DNP derivatives of alanine and aspartic acid, and further improvement in both resolution and the number of separable racemates was observed for peptides with hydrophobic amino acid residues in position 3. However, the most dramatic improvement and best selectivity were found for c(Arg-Lys-Tyr-Pro-Tyr-(3-Ala) (Scheme 3-2a) with the tyrosine residue at position 5 with a resolution factor as high as 28 observed for the separation of DNP-glutamic acid enantiomers. 

Owing to the fully reversible equilibrium nature of the aldol addition process, enzymes with low diastereoselectivity will typically lead to a thermodynamically controlled mixture of erythro/threo-isomers that are difficult to separate. The thermodynamic origin of poor threo/erythro selectivity has most recently been turned to an asset by the design of a diastereoselective dynamic kinetic resolution process by coupling of L-ThrA and a diastereoselective L-tyrosine decarboxylase (Figure 10.47)... 

Asakura, T., Ohgo, K., Ishida, T., Taddei, P., Monti, P., and Kishore, R. (2005). Possible implications of serine and tyrosine residues and intermolecular interactions on the appearance of silk I structure of Bombyx mod silk fibroin-derived synthetic peptides High-resolution 13C cross-polarization/magic-angle spinning NMR study. Biomacromolecules 6, 468-474. 

A catalytically inactive, (tyrosinato)Cu(II)-containing form of GO (pH 4.5 acetate buffer) has been characterized by X-ray crystallography (119, 120) at 1.7-A resolution. Fig. 6 shows the active site. The Cu(II) ion is in a distorted square-based pyramidal environment of a tyrosine (Tyr 495) ligand in the apical position where it is probably bound in its protonated phenol form, a second (modified) tyrosinate (Tyr 272) as well as two histidines (His 496, His 581) in equatorial positions. The fifth coordination site is occupied by a buffer derived acetate that in the active en-... 

Muller et al.understand better the role of tyrosine in the structure and biological function of MDH. Resolution of the protein absorption spectrum, using iV-acetylphenylalanine ethyl ester in dioxane and A-acetyltyrosine ethyl ester in dioxane or 0.1 M phosphate buffer to model the effect of the local environments of the chromophoric groups, indicated that both the pig and the... 

J. R. Lakowicz, G. Laczko, and I. Gryczynski, Picosecond resolution of tyrosine fluorescence and anisotropy decays by 2-GHz frequency-domain fluorometry, Biochemistry 26, 82-90 (1987). 

Among protein aromatic groups, histidyl residues are the most metal reactive, followed by tryptophan, tyrosine, and phenylalanine.1 Copper is the most reactive metal, followed in order by nickel, cobalt, and zinc. These interactions are typically strongest in the pH range of 7.5 to 8.5, coincident with the titration of histidine. Because histidine is essentially uncharged at alkaline pH, complex-ation makes affected proteins more electropositive. Because of the alkaline optima for these interactions, their effects are most often observed on anion exchangers, where complexed forms tend to be retained more weakly than native protein. The effect may be substantial or it may be small, but even small differences may erode resolution enough to limit the usefulness of an assay. 

Novozymes, a subtilisin produced by Bacillus licheniformis, was used by Chen et al ° to carry out a dynamic kinetic resolution of benzyl, butyl, or propyl esters of DL-phenylalanine, tyrosine, and leucine. The hydrolysis was performed at pH 8.5 in 2-methyl-2-propanol/water (19 1) and the freed L-amino acids precipitated. The key feature bringing about continual racemization of the remaining D-amino acid esters was the inclusion of 20 mmol 1 pyridoxal phosphate. 

For resolution of the racemate 12 two different procedures can be applied 124 the en-antioselective enzymatic deacylation of chloroacetyl-DL-a-aminosuberic acid at pH 7.2 with Taka-acylase or the enantioselective salt precipitation of Z-dl-Asu-OH with D-tyrosine hydrazide according to the method of Vogler et alJ25 Complete enzymatic digestion is achieved in about ten days at 37 °C, and the optically pure L-enantiomer is obtained in 80% yield but the overall efficiency is lower than that of the chemical method. Fractional crystallization affords in good yields the Z-l-Asu-OH derivative 13 which is then used directly as a suitably protected intermediate in subsequent derivatization steps (see Scheme 6). Moreover, the recovery of the D-enantiomer from the mother liquors is also easy in this case. 

Figure 2.6 By resolution of df-amino acid esters under conditions of dynamic resolution 100% of a single enantiomer may be produced. Using catalytic amounts of pyiidoxyl-5-phosphate, which forms a Schiff s base with the ester and not the acid, the unreacted D-ester may be racemised in situ and for instance L-tyrosin has been obtained in 97% ee and 95% yield.

The Z-protected derivative, again prepared by standard methods using benzyl chloroformate,t208 may serve in the case of racemic pipecolic acid for resolution into the pure enantiomers by fractional crystallization with L-tyrosine hydrazide/208 Acylation with N-protected pipecolic acid or of pipecolyl peptides is performed by standard procedures via the active ester methods, e.g. A-hydroxysuccinimide ester/121 by the mixed anhydride method, e.g. with isobutyl chloro-formate 95-114 or pivalic acid chloride/121 as well as by DCC/HOBt/118 In the synthesis on solid support, longer coupling times are required when compared to N-protected proline.1[235 ... 

The crystal structure of the complex formed between carboxypeptidase Aa (abbreviated CPA) and glycyltyrosine (Gly-Tyr) has been refined to 2.0 A by Lipscomb et at. (444, 445) and it reveals (Fig. 90) interactions between the amide carbonyl oxygen and the catalytically essential Zn, and between the amide nitrogen and the hydroxyl of tyrosine-248 (Tyr-248). Scott et al. (443) synthesized both the [13C]amido (90% enriched) and amido[l3C, 15N]amido (90% and 99% enriched, respectively) isotopomers of Gly-Tyr. They then proceeded to probe the hydrolysis by a series of l3C and l5N high-resolution solid-state NMR spectra. 

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