Some physical and chemical properties of trypsin-digested nucleoprotein

Author:

Marks Dawn B.1,Schumaker Verne N.1

Affiliation:

1. Department of Biochemistry, School of Medicine, University of Pennsylvania, Philadelphia, Pa. 19104, and Department of Chemistry and Molecular Biology Institute, University of California, Los Angeles, Calif. 90024, U.S.A.

Abstract

A DNA–peptide complex that is soluble in 0·2m-sodium chloride can be prepared by trypsin digestion of calf thymus nucleoprotein. The trypsin-digested nucleoprotein molecule contains about 70% of DNA and 30% of peptides by weight, and consists of one DNA molecule associated with arginine-rich peptides. A series of trypsin-digested nucleoprotein preparations differing only in molecular weight were prepared by blending. The intrinsic viscosity and average sedimentation coefficient were determined for each of these preparations. Then the DNA was isolated from each preparation and the hydrodynamic measurements were repeated on the DNA. From a comparison of these results it was concluded that the presence of the complex-forming peptides causes a large decrease in intrinsic viscosity of the DNA and an increase in sedimentation coefficient. In addition, the hydrodynamic data indicate that the DNA–peptide complex behaves like a coil in solution but is more compact than the same length of DNA. The ‘melting’ profiles, streptomycin precipitation curves and maximum viscosities obtained with ethidium bromide binding for the trypsin-digested nucleoprotein are similar to those of purified DNA, and markedly different from those of undigested nucleoprotein. These findings suggest that the peptides are not strongly associated with the DNA, and that secondary valency forces are involved in the binding.

Publisher

Portland Press Ltd.

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