Pulse-polarographic analysis of nucleic acids and proteins

Nucleic acids and proteins were studied by means of derivative and normal pulse polarography, and d.c. and a.c. polarography in connection with the dropping mercury electrode. It was shown that natural ribonucleic acids, as transfer, ribosomal and viral RNAs yield derivative pulse-polarographic peaks; from their heights and potentials conclusions can be made about their content of ordered structure in solution, similarly as in the case of deoxyribonucleic acids studied earlier. Synthetic single-stranded polyribo-cytidylic acid yields a well developed peak, whereas in the double-helical complex with polyriboguanylie acid it is inactive when using either derivative pulse polarography or d.c. polarography. Well developed peaks were obtained also with albumin (a protein containing reducible?S?S? groups), while only an inflex was observed on the d.c. polarogram. Proteins were also studied in media containing cobalt (Brdi?ka's solution) or nickel and it was shown that derivative pulse polarography due to its high sensitivity and accuracy enables us to carry out the measurements even in less common media than Brdi?ka's solution. This fact could be exploited in clinical chemistry as well as in the investigation of the nature of catalytic currents of proteins. The currents of double-helical polynucleotides obtained by means of normal pulse polarography exhibit a marked dependence on the initial potential and cannot represent a reliable indicator of structural changes of biopolymers in solution. They can however, be used in studies of the influence of the polynucleotide adsorption at different potentials on the subsequent reduction.