Interaction of ferricytochrome c with zwitterionic phospholipid bilayers: a Raman spectroscopic study.

The vibrational Raman spectra of both pure L-alpha-dipalmitoylphosphatidylcholine (DPPC) liposomes and DPPC multilayers reconstituted with ferricytochrome c under varying conditions of pH and ionic strength are reported as a function of temperature. Total integrated band intensities and relative peak height intensity ratios, two spectral scattering parameters used to determine bilayer disorder, are invariant to changes in pH and ionic strength but exhibit a sensitivity to the bilayer concentration of the ferricytochrome c. Protein concentrations were estimated by comparing the 1636 cm-1 resonance Raman line of known ferricytochrome c solutions to intensity values for the reconstituted multilayer samples. Temperature-dependent profiles of the 3100-2800 cm-1 C-H stretching, 1150-1000 cm-1 C-C stretching, 1440 cm-1 CH2 deformation, and 1295 cm-1 CH2 twisting mode regions characteristic of acyl chain vibrations reflect bilayer perturbations due to the weak interactions of ferricytochrome c. The DPPC multilamellar gel to liquid-crystalline phase transition temperature, TM, defined by either the C-H stretching mode I2935/I2880 or the C-C stretching mode I1061/I1090 peak height intensity ratios, is decreased by approximately 4 degrees C for the approximately 10(-4) M ferricytochrome c reconstituted DPPC liposomes. Other spectral features, such as the increase in the 2935 cm-1 C-H stretching mode region and the enhancement of higher frequency CH2 twisting modes, which arise in bilayers containing approximately 10(-4) M protein, are interpreted in terms of protein penetration into the hydrophobic region of the bilayer.

Raman spectroscopic studies of dimyristoylphosphatidic acid and its interactions with ferricytochrome c in cationic binary and ternary lipid-protein complexes.

The vibrational Raman spectra of both pure 1-alpha-dimyristoylphosphatidic acid (DMPA) liposomes and DMPA multilayers reconstituted with ferricytochrome c at pH 7 and pH 4, with either sodium or calcium as the cation, are reported as a function of temperature. Multilayers composed of a 1:1 mol ratio DMPA and dimyristoylphosphatidylcholine with perdeuterated acyl chains (DMPC-d54) have also been reconstituted with approximately 10(-4) M ferricytochrome c for Raman spectroscopic observation. Total integrated band intensities and relative peak height intensity ratios, two spectral Raman scattering parameters used to characterize bilayer properties, are sensitive to the presence of both ferricytochrome c and the cation in the reconstituted liposomes. Temperature profiles, derived from the various Raman intensity parameters for the 3,100-2,800 cm-1 lipid acyl chain C-H stretching mode region specifically reflect bilayer perturbations due to the interactions of ferricytochrome c. At pH 4 the calcium DMPA multilamellar gel to liquid crystalline phase transition temperatures Tm, defined by either the C-H stretching mode I2850/I2880 and I2935/I2880 peak height intensity ratios, are 58.5 +/- 0.5 degrees C and 60.0 +/- 0.3 degrees C, respectively. This difference in Tm's resolves the phase transition process into first an expansion of the lipid lattice and then a melting of the lipid acyl chains. At pH 7 the calcium DMPA liposomes show no distinct phase transition characteristics below 75 degrees C. For sodium DMPA liposomes reconstituted with ferricytochrome c at either pH 4.0 or pH 7.0, spontaneous Raman spectra show altered lipid structures at temperatures above 40 degrees C. Resonance Raman spectra indicate that ferricytochrome c reconstituted in either calcium or sodium DMPA liposomes changes irreversibly above Tm. For either the binary lipid or ternary lipid-protein systems reconstituted with DMPC-d54, linewidth parameters of the DMPC-d54 acyl chain CD2 symmetric stretching modes at 2,103 cm-1 provide a sensitive measure of the conformational and dynamic properties of the perdeuterated lipid component, while the 3,000 cm-1 C-H spectral region reflects the bilayer characteristics of the DMPA species in the complex. Although calcium clearly induces a lateral phase separation in the DMPA/DMPC-d54 system at pH 7.5 (Kouaouci, R., J.R. Silvius, I. Grah, and M. Pezolet. 1985. Biochemistry. 24:7132-7140), no distinct lateral segregation of the lipid components is observed in the mixed DMPA/DMPC-d54 lipid system in the presence of either ferricytochrome c or the sodium and calcium cations at pH 4.0. However, domain formation, consisting of regions rich in DMPA and DMPC-d54, respectively, is suggested for the calcium binary lipid mixture at pH 4.0 by the different values for Tm and AT characterizing the DMPA and DMPC-d54 species.Spectral evidence strongly suggests that ferricytochrome c also induces domain formation in the ternary lipid-protein mixtures at pH 7.0, but only for the sodium cation.

Low-temperature electron paramagnetic resonance study of the ferricytochrome c-cardiolipin complex.

The electron paramagnetic resonance spectrum of the ferricytochrome c complex with cardiolipin was observed at temperatures below 20 K. For the low-spin iron(III) heme system complexed with the negatively charged lipid, the tetragonal and rhombic ligand field parameters (delta/lambda = 3.58, V/lambda = 1.82) differ significantly from those (delta/lambda = 2.53, V/lambda = 1.49) of the free ferricytochrome c sample. The g values of the complex (gx = 1.54 +/- 0.02, gy = 2.26 +/- 0.01, gz = 3.02 +/- 0.01) are compared to the values for free ferricytochrome c (gx = 1.25 +/- 0.02, gy = 2.25 +/- 0.01, gz = 3.04 +/- 0.01). Spectral alterations are interpreted in terms of the ligand field changes induced within the heme group by association with the negatively charged phosphoglyceride.

Membrane lipid response to clathrin coat protein determined by infrared spectroscopy. Possible involvement in coated vesicle formation.

Clathrin, the major structural protein associated with both coated pits and coated vesicles, has been implicated in the dynamics of various endocytotic processes. In an attempt to define the mechanisms involved in the transition from uncoated membranes to clathrin-coated pits and then to coated vesicles, we investigated by infrared spectroscopy the lipid perturbations arising from the interactions of the clathrin coat with the bilayers of intact membrane assemblies. A comparison of the lipid acyl chain symmetric methylene stretching modes at approximately 2850 cm-1 for isolated clathrin-coated vesicles, uncoated vesicles, and synaptic membranes at 21, 38, and 50 degrees C indicated that clathrin significantly increases the number of gauche chain conformers in the bilayer matrix of the coated vesicle system. The increase in lipid disorder at 21 degrees C, accompanying the observed 0.44-cm-1 frequency increase for coated vesicles compared to uncoated vesicles, is approximately equivalent to the intrachain disorder incurred in heating liquid crystalline dimyristoylphosphatidylcholine multilayers by approximately 10 degrees C. The implications of these results on coated vesicle formation are discussed.

A cyclotron target for the production of radioxenons.

A liquid cesium target has been developed which allows the production and separate identification of the neutron deficient isotopes of xenon. The present report describes irradiations utilizing 34--41 MeV protons to produce millicurie quantities of 127Xe and 129Xem. At higher energies, however, the target could be used without modification to produce xenon isotopes as light as 119.

Raman spectroscopic studies of model human pulmonary surfactant systems: phospholipid interactions with peptide paradigms for the surfactant protein SP-B.

The temperature dependence of dipalmitoylphosphatidylcholine (DPPC)/phosphatidylglycerol (PG) multilayers, reconstituted with various synthetic peptides for modeling human lung surfactant, was monitored by vibrational Raman spectroscopy. The synthetic peptides consisted, respectively, of residues 59-81 of the human surfactant protein SP-B and 21 amino acid residue peptides containing repeating units of arginine separated by either four or eight leucines (RL4 or RL8). Each peptide demonstrated the ability to reduce significantly the surface tension of analogues of the phospholipid mixture used in the Raman studies. Raman spectroscopic integrated band intensities and relative peak height intensity ratios, two spectral parameters used to determine bilayer disorder, provided sensitive probes for characterizing multilayer perturbations in the reconstituted liposomes. Temperature profiles derived from the various Raman intensity parameters for the 3100-2800-cm-1 carbon-hydrogen (C-H) stretching mode region, a spectral interval representative of acyl chain vibrations, reflected lipid reorganizations due to the bilayer interactions of these peptides. For the three reconstituted multilamellar surfactant systems, the gel-to-liquid-crystalline phase-transition temperatures Tm, defined by acyl chain C-H stretching mode order/disorder parameters, increased from 35 degrees C in the peptide free system to 37-38 degrees C, indicating increased lipid headgroup constraints for the model liposomes. Although the values of Tm were similar for the three recombinant lipid/peptide assemblies, individual phase-transition cooperativities varied significantly between systems and between spectroscopically derived order/disorder parameters.

Interactions of model human pulmonary surfactants with a mixed phospholipid bilayer assembly: Raman spectroscopic studies.

The temperature dependence and acyl chain packing properties of the binary lipid mixtures of dipalmitoylphosphatidylcholine-d62 (DPPC-d62)/dipalmitoylphosphatidylglycerol (DPPG) multilayers, reconstituted with two synthetic peptides for modeling the membrane behavior of the SP-B protein associated with human pulmonary surfactant, were investigated by vibrational Raman spectroscopy. The synthetic peptides consisted of 21 amino acid residues representing repeating charged units of either lysine or aspartic acid separated by hydrophobic domains consisting of four leucines (KL4 or DL4, respectively). These peptides were designed to mimic the alternating hydrophobic and hydrophilic sequences defining the low molecular weight SP-B protein. Raman spectroscopic parameters consisting of integrated band intensities, line widths, and relative peak height intensity ratios were used to probe the bilayer order/disorder characteristics of the liposomal perturbations reflected by the reconstituted membrane assemblies. Temperature profiles derived from the various Raman intensity parameters for the 3100-2800-cm-1 carbon-hydrogen (C-H) and the 2000-2300-cm-1 carbon-deuterium (C-D) stretching mode regions, spectral intervals representative of acyl chain vibrations, reflected lipid reorganizations specific to peptide interactions with either the DPPC-d62 or DPPG component of the liposome. For the multilamellar surfactant systems composed of either KL4 or DL4 reconstituted with the binary DPPG/DPPC-d62 lipid mixture, the breadth of the gel to liquid crystalline phase transition temperatures TM, defined by acyl chain C-H and C-D stretching mode order/disorder parameters, increased from about 1 degree C in the peptide-free systems to over 10 degrees C. This breadth in TM indicates an increased lipid disorder and a distinct noncooperative chain melting process for the model liposomes. In comparing the interactions of the synthetic peptides with DPPG/DPPC mixtures and with DPPC liposomes alone, the negatively charged DL4 peptide perturbs the DPPG component of the lipid mixture more strongly than the DPPC-d62 component; moreover, the DL4 peptide disrupts the structure of the DPPG lipid domains in the binary mixture to a greater extent than the KL4 peptide. The microdomain heterogeneity of the binary lipid mixture arising from lipid-peptide interactions is discussed in terms of the Raman spectral properties of the multilayers. The Raman data in conjunction with previous bubble surfactometer and animal studies (Cochrane & Revak, 1991) suggest that lipid domain structures are present in functional surfactants and that the dynamic bilayer microheterogeneity induced by the surfactant peptide or protein is essential for pulmonary mechanics.

Semi-preparative isolation of plant sulfoquinovosyldiacylglycerols by solid phase extraction and HPLC procedures.

Techniques are described for the semi-preparative isolation of sulfoquinovosyldiacylglycerol from plant leaf tissue lipid extracts and the resolution and analysis of component molecular species. Sulfoquinovosyldiacylglycerol was resolved from phospholipids in a polar lipid fraction by isocratic normal phase HPLC with detection at 208 nm. The mobile phase was composed of heptane-isopropanol-0.001 M KCl 40:52:8 (v/v/v). Yields from spinach leaf lipid extracts were 1.8 mg.10 g-1 fresh wt leaf tissue. Molecular species components of purified sulfoquinovosyldiacylglycerol were separated by reversed-phase C18 HPLC, and fatty acid positional distribution was defined.