A. Resonance Raman spectroscopy and optical spectroscopy were used to monitor the redox state of Heme A, having a and a3 centers, in cytochrome oxidase during potentiometric titrations. A novel approach was derived for obtaining simultaneous resonance Raman and optical absorption measurements of dilute protein solutions whose titrations curves are controlled potentiometrically. Quantitative Raman intensities, excited at 441.6 nm and measured as a function of solution voltage, yield the midpoint potential of the heme A centers. The techniques were first tested by deriving the well-known midpoint potential of cytochrome c. Cyanide- inhibited cytochrome oxidase was examined as a simplified model of the native enzyme in which the heme a3 is locked into the oxidized state. The spectroscopic analyses indicate that even when heme a3 cannot undergo oxidoreduction, the heme a centers show effective Em's near 260 and 350 mV. Measurements on native (unbound) cytochrome oxidase give two effective Em values near 260 and 350 mV for heme a and lower Em's near 260 and 350 mV for the heme a3 centers. These results argue against the Neoclassical model of cytochrome redox behavior in which the heme a and heme a3 centers are predicted to be equally reduced at all voltages. That is, these finding are consistent with recent reports of differential heme a and heme a3 redox behavior. B. A solid-state acousto-optic tunable filter (AOTF) was combined with krypton laser excitation, holographic filters and a photon-counting silicon avalanche photodiode detection to construct a miniaturized Raman spectrometer with no moving parts. The miniature AOTF spectrometer is used as an accessory to a Raman imaging microscope system in our laboratory. Although this spectrometer is optimized for the collection of Raman microspectra, it also functions as a microspectrometer for fluorescent studies.

Project Start
Project End
Budget Start
Budget End
Support Year
21
Fiscal Year
1993
Total Cost
Indirect Cost
City
State
Country
United States
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Bhargava, Rohit; Fernandez, Daniel C; Hewitt, Stephen M et al. (2006) High throughput assessment of cells and tissues: Bayesian classification of spectral metrics from infrared vibrational spectroscopic imaging data. Biochim Biophys Acta 1758:830-45
Schlucker, S; Liang, C; Strehle, K R et al. (2006) Conformational differences in protein disulfide linkages between normal hair and hair from subjects with trichothiodystrophy: a quantitative analysis by Raman microspectroscopy. Biopolymers 82:615-22
Levin, Ira W; Bhargava, Rohit (2005) Fourier transform infrared vibrational spectroscopic imaging: integrating microscopy and molecular recognition. Annu Rev Phys Chem 56:429-74
Fernandez, Daniel C; Bhargava, Rohit; Hewitt, Stephen M et al. (2005) Infrared spectroscopic imaging for histopathologic recognition. Nat Biotechnol 23:469-74
Huffman, Scott W; Schlucker, Sebastian; Levin, Ira W (2004) Reorganizational dynamics of multilamellar lipid bilayer assemblies using continuously scanning Fourier transform infrared spectroscopic imaging. Chem Phys Lipids 130:167-74
Bhargava, Rohit; Levin, Ira W (2004) Gram-Schmidt orthogonalization for rapid reconstructions of Fourier transform infrared spectroscopic imaging data. Appl Spectrosc 58:995-1000
Zuzak, Karel J; Gladwin, Mark T; Cannon 3rd, Richard O et al. (2003) Imaging hemoglobin oxygen saturation in sickle cell disease patients using noninvasive visible reflectance hyperspectral techniques: effects of nitric oxide. Am J Physiol Heart Circ Physiol 285:H1183-9
Schlucker, Sebastian; Schaeberle, Michael D; Huffman, Scott W et al. (2003) Raman microspectroscopy: a comparison of point, line, and wide-field imaging methodologies. Anal Chem 75:4312-8
Hendler, Richard W; Barnett, Steven M; Dracheva, Swetlana et al. (2003) Purple membrane lipid control of bacteriorhodopsin conformational flexibility and photocycle activity. Eur J Biochem 270:1920-5
Bhargava, Rohit; Levin, Ira W (2003) Time-resolved Fourier transform infrared spectroscopic imaging. Appl Spectrosc 57:357-66

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