Deoxyribonuclease chromatography

Cacia, J., Quan, C. P., Vasser, M., Sliwkowski, M. B., and Frenz, J., Protein sorting by high-performance liquid chromatography I. Biomimetic interaction chromatography of recombinant human deoxyribonuclease I on polyionic stationary phases, /. Chromatogr., 634, 229, 1993. 

Fig. 1. Chromatography of bovine pancreatic juice on DEAE-cellulose (anionic proteins) and Amberlite IRC-50 (cationic proteins) (1). RNAase, ribonuclease ChTg-a, chymotrypsinogen A Tg, trypsinogen ProCp-B and Cp-B, procarboxypeptidase B and carboxypeptidase B DNAase, deoxyribonuclease ProCp-A, procarboxypeptidase A.

Fig. 4. Chromatography of dog pancreatic juice on DEAE-cellulose (13, 14). The column is equilibrated with 0.005 M phosphate, pH 8.0 and eluted by a concentration gradient of phosphate indicated in the figure by a straight line. (1) Unfractionated cationic proteins (2) amylase (3) lipase (4) deoxyribonuclease (5) anionic chymotrypsinogen (6), (9), and (10) carboxypeptidase A and its precursor (7) and (8) carboxypeptidase B and its precursor. Ordinates on the left, optical density of the fractions at 280 m/ . Ordinates on the right, molarity of the phosphate. Abscissas, volume of eluate expressed in number of interstitial volumes of the column.

Keller and Cohen (36) also subjected to chromatography acidic extracts of cattle pancreatic microsomes and ribosomes. In microsomes they found the expected amounts of all enzymes which are known to be stable in acid, viz., chymotrypsinogen A, trypsinogen, deoxyribonuclease, and ribonuclease. The amounts of chymotrypsinogen B were abnormally low and ribonuclease B was perhaps not present. The results concerning ribosomes were made somewhat uncertain by the ability of these particles to incorporate proteins from the medium. Nevertheless, a series of characteristic enzymes could be isolated from what appears to be the very site of their biosynthesis. 

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