Structure of human parathyroid hormone(1-34) in the presence of solvents and micelles.

The structure of the N-terminal 34-residue fragment of human parathyroid hormone was determined in 40% trifluoroethanol employing two-dimensional 1H nuclear magnetic resonance spectroscopy. The proton chemical shifts were assigned from magnitude and phase-sensitive COSY, relayed COSY, and NOESY spectra. Distance constraints, estimated from NOESY spectra, were used to create a set of structures by distance geometry (DGEOM) which were subsequently refined by restrained energy minimization and restrained molecular dynamics (CHARMm). The resulting structures contained two helices spanning residues 3-12 and residues 17-26. The NOE constraints for residues 13-16 did not provide a single structural solution; however, their conformations were not disordered. The structures prepared by DGEOM and refined with CHARMm contained either an irregular turn or a helical structure at residues 13-16. The secondary structure of human parathyroid hormone(1-34) was also assessed by circular dichroism in the presence of methanol, trifluoroethanol, and dodecylphosphocholine micelles. Under all three conditions, the peptide formed structures containing various amounts of helical content. The formation of helical secondary structure in the presence of micelles supports the proposal that the trifluoroethanol-induced structure of human parathyroid(1-34) was not an artifact of its environment but perhaps was an indication of the conformation that the molecule adopts when in close proximity to a membrane surface and possibly when bound to the parathyroid receptor.

The effect of recombinant human (1-84) or synthetic human (1-34) parathyroid hormone on the skeleton of adult osteopenic ovariectomized rats.

The purpose of this study was to evaluate the dose-effect relationship of recombinant human PTH [hPTH-(1-84)] and synthetic human PTH [sPTH-(1-34)] for the skeleton of estrogen-deplete osteopenic rats. Ex vivo densitometry of regionalized whole femurs and histomorphometry of proximal tibial cancellous bone were the end points. Retired breeder female rats, aged 6-7 months, were used. Ten were killed at baseline, and the rest were ovariectomized (OVX). On day 42, a pre-PTH treatment OVX group was killed. The rest were then treated by daily sc injection with hPTH (0, 1.55, 15.5, or 155 micrograms/kg BW.day) or sPTH (0.55, 5.5, or 55 micrograms/kg BW.day) and killed on day 70. The level of cancellous bone mineral was lower in pretreatment OVX rats than at baseline. It was higher in rats treated with 15.5-155 micrograms/kg.day hPTH and 5.5-55 micrograms/kg.day sPTH than in pretreatment and vehicle-treated OVX rats. Cancellous bone volume was also lower both 42 and 70 days after OVX. Although hPTH did not affect cancellous bone volume, treatment with 5.5-55 micrograms/kg.day sPTH caused higher bone volume than in either pretreatment or vehicle-treated OVX rats. Trabecular number declined after OVX and did not change with PTH treatment. In contrast, trabecular thickness declined after OVX, but was higher after 15.5-155 micrograms/kg.day hPTH and 5.5-55 micrograms/kg.day sPTH treatment. In OVX rats, the amount of mineralizing surface was greater by day 42 and fell toward control levels by day 70. It was greater in rats treated with 15.5-155 micrograms/kg.day hPTH or 5.5-55 micrograms/kg.day sPTH than in vehicle-treated OVX rats. On a molar basis, sPTH was modestly more potent than hPTH. Osteoclast surface was not affected by PTH treatment. Treating estrogen-deplete osteopenic adult rats for 28 days with 15.5-155 micrograms/kg.day hPTH or 5.5-55 micrograms/kg.day sPTH increases trabecular thickness, but not trabecular number, to cause a rise in bone mass. The extent of mineralizing surface rises without a change in resorption surface. The marked rise in mineralizing surfaces suggests that extended in vivo treatment with PTH activates osteogenic precursor cells near once quiescent surfaces to become osteoblasts.

Structure-function studies on bacteriorhodopsin. V. Effects of amino acid substitutions in the putative helix F.

To test structural and mechanistic proposals about bacteriorhodopsin, a series of analogues with single amino acid substitutions has been studied. Mutants in the proposed helix F of bacteriorhodopsin were chosen for investigation because of the probable interaction of this part of the protein with the retinal chromophore. Seven mutants of the bacteriorhodopsin gene were constructed by site-directed mutagenesis, and the gene products were expressed in Escherichia coli. The resulting mutant proteins were purified and assayed for their ability to interact with retinal in phospholipid/detergent micelles to form a bacteriorhodopsin-like chromophore. Four mutants, Ser-183----Ala, Tyr-185----Phe, Ser-193----Ala, and Glu-194----Gln, bound retinal to give pigments with absorption maxima approximately the same as the wild type. Three mutant opsins bound retinal to give chromophores that were blue-shifted relative to the wild type. Two Trp----Phe substitutions at positions 182 and 189 gave absorption maxima of 480 and 524 nm, respectively, and the mutant Pro-186----Leu gave a pigment with an absorption maximum of 470 nm. However, none of the amino acid substitutions eliminated the ability of the mutant bacteriorhodopsin to pump protons in response to illumination.

Wheat germ agglutinin dimers bind sialyloligosaccharides at four sites in solution: proton nuclear magnetic resonance temperature studies at 360 MHz.

Equilibrium binding studies have been performed over a range of temperatures from 25.4 to 47.3 degrees C between wheat germ agglutinin isolectin I (WGA I) and the alpha 2-3 isomer of (N-acetylneuraminyl)lactose (NeuNAc alpha 2-3Gal beta 1-4G1c). Proton nuclear magnetic resonance spectroscopy at 360 MHz has been used to monitor titrations in this system under conditions where the fraction of total ligand which is bound is small, yet the fractional occupation of sites covers a wide range. Several of the ligand resonances, including the N-acetyl methyl and the axial and equatorial hydrogens at carbon 3 of the NeuNAc residue, are shifted and broadened in the presence of WGA due to chemical exchange between the free and bound environments. The lifetime broadening of the N-acetyl resonance at room temperature of a series of related sialyloligosaccharides has been previously used by us to measure binding affinities to two WGA isolectins [Kronis, K.A., & Carver, J.P. (1982) Biochemistry 21, 3050-3057]. In this paper we report the temperature dependence of the apparent bound shifts and the apparent bound line widths of the N-acetyl, H3a, and H3e peaks. The true bound shifts for the three resonances have been obtained from these data by using the equations derived by Swift and Connick [Swift, T.J., & Connick, R.E. (1962) J. Chem. Phys. 37, 307-320]. The total bound shifts, per monomer, were found to be -1.98, -4.0, and -0.8 ppm for the N-acetyl, the H3a, and the H3e resonances, respectively.(ABSTRACT TRUNCATED AT 250 WORDS)

Thermodynamics of wheat germ agglutinin-sialyloligosaccharide interactions by proton nuclear magnetic resonance.

The thermodynamic parameters that characterize the binding of wheat germ agglutinin isolectin I (WGA I) to the alpha 2-3 isomer of (N-acetylneuraminyl)lactose have been determined by 360-MHz proton nuclear magnetic resonance spectroscopy. The chemical exchange of the ligand between the free and bound sites resulted in a broadening and upfield shifting of the N-acetyl methyl resonance [Kronis, K.A., & Carver, J.P. (1985) Biochemistry (preceding paper in this issue)] which has allowed the determination of the equilibrium constant, KD, and the dissociation rate constant, kD. In this paper, the analysis of the temperature dependence of the KD values between 25.4 and 51.6 degrees C yielded equilibrium parameters indicative of a large entropy barrier to binding: delta H degree = -13.3 +/- 1.0 kcal mol-1 and delta S degree = -31.9 +/- 2.4 cal mol-1 K-1. The Arrhenius plot of the effect of temperature on the dissociation rate (kD) and the plot of 1n (kD/T) vs. 1/T indicated that the transition complex represented an unfavorable energy state compared to the dissociated molecules with an activation energy (EA) of +18.0 kcal mol-1 and enthalpy and entropy of dissociation (delta HD not equal to and delta SD not equal to) values of +17.4 +/- 0.3 kcal mol-1 and +13.4 +/- 1.2 cal mol-1 K-1, respectively. The driving force for this binding reaction is the large negative delta H degree with a small enthalpic barrier to association (delta HA = +4.1 kcal mol-1).(ABSTRACT TRUNCATED AT 250 WORDS)

Specificity of isolectins of wheat germ agglutinin for sialyloligosaccharides: a 360-MHz proton nuclear magnetic resonance binding study.

The binding of three purified sialic acid containing oligosaccharides to two isolectins of wheat germ agglutinin (WGA I and WGA II) has been quantitated by measuring the broadening of a ligand resonance in the proton nuclear magnetic resonance (1H NMR) spectrum at 360 MHz. The ligands, isolated from bovine colostrum by using the procedure of Schneir and Rafelson [Schneir, M. L., & Rafelson, M. E., Jr. (1966) Biochim. Biophys, Acta 130, 1--11], were identified by 1H NMR as the alpha (2,3) and alpha (2,6) isomers of N-acetylneuraminyllactose, as well as the alpha (2,6) form of N,N'-diacetylneuraminyllactosamine. The dissociation constants, KD's, ranged from 0.7 to 10 mM (24 +/- 1 degree C). Two noteworthy features of WGA specificity emerge from an examination of the observed affinities: (1) both isolectins bind the alpha (2,3) isomer of N-acetylneuraminyllactose with higher affinity than the alpha (2,6) form and (2) WGA I binds two of the sialyloligosaccharides more tightly than does WGA II.