Polypeptides hydrodynamic properties

The values of these hydrodynamic properties are at the levels expected for randomly coiled, single polypeptide chains of molecular weight 20,000 and devoid of intrachain cross-link restraints (32, S3). 

Both the wide variations in hydrodynamic properties and in the NMR spectroscopic properties of polysaccharides having different chemical structures must depend on details of the composition and linkages. Unlike polypeptides, the stereochemical possibilities for saccharide linkages are highly varied. The bond between the glycosidic carbon and oxygen atoms of a pyranoside residue can be either axial or equatorial as can be... 

Before discussing details of their model and others, it is useful to review the two main techniques used to infer the characteristics of chain conformation in unordered polypeptides. One line of evidence came from hydrodynamic experiments—viscosity and sedimentation—from which a statistical end-to-end distance could be estimated and compared with values derived from calculations on polymer chain models (Flory, 1969). The second is based on spectroscopic experiments, in particular CD spectroscopy, from which information is obtained about the local chain conformation rather than global properties such as those derived from hydrodynamics. It is entirely possible for a polypeptide chain to adopt some particular local structure while retaining characteristics of random coils derived from hydrodynamic measurements this was pointed out by Krimm and Tiffany (1974). In support of their proposal, Tiffany and Krimm noted the following points ... 

Nuclease behaves like a typical globular protein in aqueous solution when examined by classic hydrodynamic methods (40) or by measurements of rotational relaxation times for the dimethylaminonaphth-alene sulfonyl derivative (48)- Its intrinsic viscosity, approximately 0.025 dl/g is also consistent with such a conformation. Measurements of its optical rotatory properties, either by estimation of the Moffitt parameter b , or the mean residue rotation at 233 nin, indicate that approximately 15-18% of the polypeptide backbone is in the -helical conformation (47, 48). A similar value is calculated from circular dichroism measurements (48). These estimations agree very closely with the amount of helix actually observed in the electron density map of nuclease, which is discussed in Chapter 7 by Cotton and Hazen, this volume, and Arnone et al. (49). One can state with some assurance, therefore, that the structure of the average molecule of nuclease in neutral, aqueous solution is at least grossly similar to that in the crystalline state. As will be discussed below, this similarity extends to the unique sensitivity to tryptic digestion of a region of the sequence in the presence of ligands (47, 48), which can easily be seen in the solid state as a rather anomalous protrusion from the body of the molecule (19, 49). 

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