IV. an Improved Separation Method for Twenty Two Compounds Related

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The Quantitative Determination of Metabolites of 6-Mercaptopurine in Biological Materials IV. An Improved Separation Method for Twenty two Compounds Related to Purine and 6-Thiopurine Metabolism Using High-Pressure Liquid Cation-Exchange Chromatography Hans-Joachim Breter * Physiologisch-Chemisches Institut der Universität Mainz (Z. Naturforsch. 32 c, 905 — 907 [1977]; received August 17, 1977) 6-Mercaptopurine Metabolites, Separation of 6-Thiopurine Bases and Ribonucleosides, Separation of Common Purine Bases and Ribonucleosides, High-Pressure Liquid Cation-Exchange Chromatography An improved method is described for the separation of 22 compounds normally related to purine and 6-thiopurine metabolism in biological materials using high-pressure liquid cation-exchange chromatography on strongly acidic exchange resin. The column (0.18X100 cm) is eluted with 0.4 M ammonium formate, pH 4.6, at a linear flow velocity of 5.2 cm •min-1 at 50 °C. The elution volumes of sulphate anions, allopurinol, 6-thioxanthine, adenine, adenosine, and guanosine are demonstrated additionally to further 16 purine and 6-thiopurine compounds.

Introduction the sulphate fraction within the void volume and the elution volumes of adenine, 2-hydroxy-6-mer- Many attempts have been made to determine 6- captopurine (6-thioxanthine), allopurinol, adeno mercaptopurine (6MP) and its metabolites in bio sine, and guanosine have been determined among logical materials, particularly in blood samples of the compounds which are retained on the exchange patients as a measure of therapeutic efficacy or as a resin. The improved separation method for 20 com guide to more effective therapy. For this purpose pounds related to 6MP metabolism is reported in the separation from plasma constituents of 6MP this paper. and of some of its metabolites was carried out either by paper 1, thin-layer 2, or liquid 3 and gas 4 Materials and Methods column chromatography. The detection of 6MP and its metabolites was done by fluorimetry5, colori 6-Mercaptopurine (6MP), 6-mercaptopurine ribo- metry6, UV-detection3, radioactivity measure nucleoside (6MPR), 6-methylmercaptopurine ments 1, and mass spectrometry 7. (6MeMP), 6-methylmercaptopurine ribonucleoside Recently, we reported a separation method by (6MeMPR), 6-thioguanine (2A6MP), 6-thioguanine high-pressure liquid cation-exchange chromato ribonucleoside (2A6MPR), and 6-methylthioguanine graphy for 6-thiopurine bases and (deoxy-) ribo (2A6MeMP) were purchased from Papierwerke Waldhof-Aschaffenburg, Mannheim (West Ger nucleosides and for some common oxidized purines 8 many) , 6-mercaptopurine deoxyribonucleoside and presented the advantages of a variable-wave- (6MPdR) from P • L-Biochemicals, Milwaukee, Wi length HPLC detector for the identification and (USA), 6- (l-methyl-4-nitro-imidazolyl-) mercapto- quantitative determination of these compounds on purine (6MNIMP) from Deutsche Wellcome, Burg- the picomole level 9. These methods have frequently wedel (West Germany), 2-hydroxy-6-mercaptopurine been applicated in our laboratory to routine deter (20H6MP) from EGA-Chemie, Weinheim (West minations of 6-thiopurines in extracts from L5178Y Germany), 6-thiouric acid (6TUA) and allopurinol murine lymphoma cells grown with radioactively (Alp) from Calbiochem, San Diego, Ca (USA). labeled [8-14C] or [6-35S] 6MP 10- n . Uric acid (UA), xanthine (Xan), hypoxanthine Additionally to the 17 purine and 6-thiopurine (Hx), xanthine ribonucleoside (Xao), inosine (Ino), compounds 8 we have now confirmed the location of adenine (Ade), guanine (Gua), adenine ribonucleo side (rAdo), guanine ribonucleoside (rGuo), barium * Present Address: The University of Kentucky, Albert B. chloride, sulphuric acid, and further reagents were Chandler Medical Center, Department of Biochemistry, from E. Merck, Darmstadt (West Germany). All Lexington, Ky 40506 (USA). reagents used were of the highest available purity. 906 H.-J. Breter • HPLC-Separation of 6-Thiopurines

Strongly acidic cation-exchange resin, type M71, organic materials. Additionally the elution volumes particle diameter 10— 12/

0.02

0.01 i c inCM 0)o

ovt -O < 0 15 30 45 60 75 90 105 120 135 150 165 180 205 220 Elution time [min]

Fig. 1. Elution pattern of the separation of 20 compounds related to purine and 6-thiopurine metabolism. (The bars in dicate the elution volumes of tritiated water, adenine and guanine ribonucleoside; designates the pressure peak which represents initial changes in column pressure and flow; for abbreviations and separation conditions see Materials and Methods.) H.-J. Breter • HPLC-Separation of 6-Thiopurines 907

acetate, pH 8.7, at 71 °C. Since Hx and allopurinol In contrast to previous suggestions8 it seems hardly possess any charge within their molecules at realistic that 8-hydroxy-6-mercaptopurine, the oxi pH 4.6 they are retained by adsorption phenomena dation product of 6MP by xanthine oxidase, is not exclusively. This, however, gives no difference in eluted within the void volume but is retained on the elution volumes of Hx and allopurinol. exchange column, too, comparable to 2-hydroxy-6- The purine ring of 6MP after desulphurization mercaptopurine. Unfortunately, we still could not ob may be used for the synthesis of the common tain a sample of pure reference material of 8-hy- purines, adenine and guanine, and their (deoxy-) droxy-6-mercaptopurine. As to our knowledge, this ribonucleotides. Since the determinations of purine compound has not yet been reported as an intra and 6-thiopurine nucleotides in cell extracts are cellular metabolite of 6MP. carried out on the (deoxy-) ribonucleoside (and base) level after the incubation of the extracts with 6-Methylthioguanine and azathioprine which alkaline phosphatase (and, in addition, purine are most strongly retained on the exchange resin nucleoside phosphorylase), the elution volumes of were not contained in the radioactively labeled cell adenine- and guanine ribonucleoside and of adenine extracts. Therefore, the doubling of the linear flow and guanine must be known. The desulphurized velocity after 75 min 8 was omitted and the column purine residue of [8-14C]6MP which is used as the needed no regeneration interval after each chromato radioactively labeled precursor may appear as a graphic run. common purine derivative. The bases adenine and guanine do not interfere with 6-thiopurine compounds in the elution pattern, A cknowledgements their ribonucleosides, however, are not separated This work was supported by grants from the from 6MPR and 2A6MPR. Therefore, accurate Research Group of Programmed Synthesis at the quantitative determinations of rAdo and rGuo Institute for Physiological Chemistry (Director: should be carried out with 254 nm UV-detectors, Professor Dr. R. K. Zahn) and from the Fonds der whereas 6MPR and 2A6MPR are easily determined Deutschen Chemischen Industrie. The technical as using a variable-wavelength UV-detector at 322 sistance of Mrs. Gabriele Fenzl is gratefully and 342 nm, respectively 9. acknowledged.

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