Determination of sedimentation coefficients for small peptides.

Direct fitting of sedimentation velocity data with numerical solutions of the Lamm equations has been exploited to obtain sedimentation coefficients for single solutes under conditions where solvent and solution plateaus are either not available or are transient. The calculated evolution was initialized with the first experimental scan and nonlinear regression was employed to obtain best-fit values for the sedimentation and diffusion coefficients. General properties of the Lamm equations as data analysis tools were examined. This method was applied to study a set of small peptides containing amphipathic heptad repeats with the general structure Ac-YS-(AKEAAKE)nGAR-NH2, n = 2, 3, or 4. Sedimentation velocity analysis indicated single sedimenting species with sedimentation coefficients (s(20,w) values) of 0.37, 0.45, and 0.52 S, respectively, in good agreement with sedimentation coefficients predicted by hydrodynamic theory. The described approach can be applied to synthetic boundary and conventional loading experiments, and can be extended to analyze sedimentation data for both large and small macromolecules in order to define shape, heterogeneity, and state of association.     

Ultracentrifugal studies in capillary cells. I. Determination of sedimentation coefficients

A technique has been developed which is based on transport method equations and allows determination of sedimentation coefficients using less than 5 ng of a biological active principle. Glass capillaries of 0.30 mm inside diameter and 3.0 mm length are used as sedimentation cells. About 200 nl of pure or impure solutions with concentration as low as 0.05 mg/ml are ultracentrifuged in a swinging-bucket rotor with a conventional preparative ultracentrifuge. The capillary microcells are easily sectioned after centrifugation through a plane previously marked on the glass surface. The technique was successfully extended to the use of larger glass capillaries, up to 1.25 mm inside diameter, and plastic centrifuge tubes of 5.0 mm diameter and 0.40 ml capacity. The method has been experimentally verified with proteins and protein-polysaccharides of known sedimentation constants.     

Application of phase partition method for the fractionation of hydrophobic membrane proteins]

Phase partition method in a two-phase polyethylene glycol-dextrane system has been applied to fractionation in Triton X-100 of hydrophobic membrane proteins from Micrococcus lysodeikticus. This method allowed to separate the cytochrome b556 from other cytochromes. Spectral and gel electrophoretic patterns of isolated cytochrome are given.     

Frictional coefficients of multisubunit structures. II. Application to proteins and viruses

The theory of Kirkwood for the translational frictional coefficients of structures composed of identical subunits has been extended in the previous paper to the case where nonidentical subunits are involved. In this paper, the theory is applied to particular proteins and viruses. It is found that the calculated sedimentation coefficients of various states of aggregation of the reversibly associating proteins hemocyanin and phycocyanin are in excellent agreement with experiment. The dimensions of the fibrinogen molecule obtained from electron micrographs do not give good agreement between calculated and experimental frictional coefficients. The frictional coefficient of tobacco mosaic virus calculated without explicit consideration of end effects is in good agreement with experiment if a hydrodynamic diameter of 18O A., corresponding to the maximum diameter from x-ray studies, is used. Agreement is also good for the fast sedimenting form of bacteriophage T2 and the protein ghosts of bacteriophage λ but the slow form of T2 and whole λ have frictional coefficients considerably in excess of those calculated. Tail fiber configuration or head porosity are unable to account for the difference in sedimentation coefficients between the fast and slow forms of T2.     

Extension of the fragment method to calculate amino acid zwitterion and side chain partition coefficients

The fragment method of calculating partition coefficients (P) has been extended to include the common amino acids (AAs). The results indicate that polar and charged side chains influence the hydrophobicity of atoms in the side chain in a predictable manner. Field effects, as evidenced through polar proximity factors and bond factors, need to be considered for accurate estimation of transfer phenomena. The calculated log P and delta G degree ' values of the 20 AAs agree well with the observed values. Pro calculates to be more hydrophilic than the observed log P. Hydrophobicity scales for peptide side chain residues are compared and evaluated in terms of suitability. Calculated pi values for nonpolar side chain residues agree well with the observed values; calculated values for uncharged polar side chain residues deviate by about 0.6 log units except for Gln and Cys; and polar side chain residues with charged side chains calculate as too hydrophilic. Reasons for the differences are explored. We also suggest that tightly bound water to polar moieties in amino acids and peptides may be transferred into the octanol phase during partitioning experiments. A quantitative methodology is presented which characterizes the thermodynamic partitioning of groups and individual atoms in amino acids and proteins.     

Anomalies in sedimentation. IV. Decrease in sedimentation coefficients of chains at high fields

A theory is presented for the decrease of sedimentation coefficient at high centrifugal fields recently reported for samples of DNA by Rubenstein and Leighton and others. The theory uses the model of a chain of beads and springs to represent the molecule. Kirkwood's approximation is used for the sedimentation coefficient. The decrease in sedimentation coefficient with field comes about as a result of the uneven frictional forces in the chain, which on the average are less on segments near the center of the chain than on those near the ends. As a result the ends of the chain tend to drag behind the center, and the average intersegment distances are increased; consequently the hydrodynamic shielding of one segment by another is reduced, and the average friction is increased. The effect is thus characteristic of single molecules; intermolecular interaction is not involved. The sedimentation coefficient, S, varies as a power series in a parameter y that measures the distortion produced by the uneven friction: S = S⁰(1?D₂y² + D₄y⁴ ? ·). where S⁰ is the limiting value of S at zero centrifugal field and D₂ and D₄ are constants; y is proportional to the cen speed squared tunes the molecular weight squared divided by S⁰. It has been observed that the effects of centrifuge speed on S are negligible below certain critical values of the speed and molecular weight, but increase dramatically immediately above these values; this follows naturally from the high powers of the speed and molecular weight that appear in the above equation.     

An in vitro gas equilibration method for determination of chemical partition coefficients in fish.

1. A gas equilibration method for the determination of in vitro chemical partition coefficients in mammals was adapted for use with fish. 2. In vitro blood: water and tissue: blood partition coefficients were determined for three chlorinated ethanes in rainbow trout (Oncorhynchus mykiss). 3. In vitro partition coefficients accurately predicted chemical concentrations in tissues of exposed trout.     

Determination of diffusion coefficients of proteins in stationary phases by frontal chromatography

A strategy to determine effective diffusion coefficients of proteins in chromatographic gels is presented in this article. An experimental methodology based on frontal liquid chromatography was combined with a numerical methodology based on a mathematical model describing the chromatographic process including the extra-column dispersion, the dispersion due to the packed bed, the external mass transfer from the bulk phase to the stationary phase, and the diffusive transport within the stationary phase. The methodology has several advantages compared to previously reported methods to determine diffusion coefficients in that no other equipment than an HPLC is required, any class of stationary phases can be investigated as long as the experiments are performed under non-binding conditions, and no modification, e.g., moulding of slabs or membranes, to the stationary phase is required. To show the applicability of the methodology, the effective diffusion coefficients of lysozyme, bovine serum albumin, and immunoglobulin gamma in Sepharose CL-4B were determined and shown to be comparable with those determined with other methods.     

A genomics method to identify pathogenicity-related proteins. Application to aminoacyl-tRNA synthetase-like proteins

During their extended evolution genes coding for aminoacyl-tRNA synthetases (ARS) have experienced numerous instances of duplication, insertion and deletion of domains. The ARS-related proteins that have resulted from these genetic events are generally known as aminoacyl-tRNA synthetase-like proteins (ARS-like). This heterogeneous group of polypeptides carries out an equally varied number of functions that need not be related to gene translation. Several of these proteins remain uncharacterized. At least 16 different ARS-like proteins have been identified to date, but their functions remain incompletely understood. Here we review the individual phylogenetic distribution of these proteins in bacteria, and apply a new genomics method to determine their potential implication in pathogenicity.     

The use of sedimentation coefficients to distinguish between models for protein oligomers.

The sedimentation coefficients of proteins are dependent on their sizes, shapes and densities and on the density and viscosity of the solvent. However, when the sedimentation coefficients of an oligomeric protein and its protomer are measured under the same experimental conditions, the ratio of the two coefficients depends only on the protomer shape and the mode of aggregation. This property, which we shall call the sedimentation ratio, therefore provides a way of distinguishing between models for oligomeric proteins. To allow examination of the behaviour of the sedimentation ratio, sedimentation coefficients are calculated for a comprehensive range of protomer shapes and modes of aggregation in hexameric systems using equations derived by Kirkwood. As illustrations of the method the resulting sedimentation ratios are compared with experimental values for insulin and arthroped hemocyanin, which eliminates many of the possible structures for these proteins. When experimental estimates of degree of hydration and molecular dimensions are also considered, all but a group of virtually identical structures are eliminated for the insulin hexamer and a single most likely structure remains for arthropod hemocyanin. The insulin structure is in good agreement with that determined by X-ray crystallography while the hemocyanin hexameric structure is a hexagonal prism formed by the cyclic aggregation of prolate ellipsoids of axial ratio about 2.5 : 1.     

Determination of sedimentation coefficients of subcellular particles of rat liver homogenates. A theoretical and experimental approach

A simple and convenient method is described for the determination of the average sedimentation coefficients ($\overline{S}?values$) of subcellular particles in a homogenous solution by velocity sedimentation in the preparative ultracentrifuge (swinging-bucket rotor). Theoretically the method is based on the distribution of intact organelles between sediment and supernatant and the convergence of their sedimentation at high centrifugal effects. The data have been treated according to the rate equation of parallel sedimentation in horizontal cylindrical tubes which has been converted to a linear function. By measuring activities of marker enzymes in the sediments, the theory has been confirmed experimentally in the determination of $\overline{S}?values$ and the distribution between supernatant and sediment of intact mitochondria, lysosomes and peroxisomes of rat liver homogenates. The effect of particle concentration on the $\overline{S}?values$ of mitochondria has been determined.     

Determination of trace elements in standard reference materials by the ko-standardization method

Biological Trace Element Research - The ko-standardization method is suitable for routine multielement determinations by reactor neutron activation analysis (NAA). Investigation of NIST standard...