NANOSECOND LASER PHOTOLYSIS OF RHODOPSIN AND ISORHODOPSIN

Kinetic and spectral measurements have been carried out on the primary intermediate in the photolysis of rhodopsin and isorhodopsin, initiated by a 457 nm, 6 ns (FWHM) laser pulse. In rhodopsin the kinetic decay of bathorhodopsin was found to be 140 ± 15 ns at 20°C. The decay of bathorhodopsin to lumirhodopsin has an activation energy of 51 ± 4 kJ/mol (12.2 ± 1 kcal/mol). The decay kinetics of bathorhodopsin were found to be the same for rhodopsin in membrane and detergent solubilized suspensions. The kinetic decay of the batho product in the photolysis of isorhodopsin was found to be the same as rhodopsin.
The corrected transient spectrum 50 ns following excitation in rhodopsin has two peaks near 560 and 440 nm. A peak was also observed in isorhodopsin near 550 nm at 50 ns following excitation but no transient was observed in the blue. The 550 nm peak in isorhodopsin has an intensity similar to that in rhodopsin indicating that the quantum yields for the formation of batho products of rhodopsin and isorhodopsin are similar under the irradiation conditions used here. Transient spectra for rhodopsin and isorhodopsin 1 μs following excitation are also different. In isorhodopsin the corrected transient spectrum has a peak at 500 nm, similar to low temperature steady state irradiation spectra. The 1 μs transient spectrum in rhodopsin is more intense than in isorhodopsin and shows a peak at 475 nm.     

Lumi I --> Lumi II: the last detergent independent process in rhodopsin photoexcitationt

Time-resolved absorbance difference spectra were collected at delays from 1 to 128 micros after photolysis of membrane and detergent suspensions of rhodopsin at 20 degrees C. Fitting both sets of data with two exponential decays plus a constant showed a similar fast process (lifetime 11 micros in membrane, 12 micros in 5% dodecyl maltoside) with a small but similar spectral change. This demonstrates that the Lumi I - Lumi II process, previously characterized in detergent suspensions, has similar properties in membrane without significant effect of detergent. The slower exponential process detected in the data is quite different in membrane compared to detergent solubilized samples, showing that the pronounced effect of detergent on the later rhodopsin photointermediates begins fairly abruptly near 20 micros. Besides affecting the late processes, the data collected here shows that detergent induces a small blue shift in the 1 micros difference spectrum (the Lumi I minus rhodopsin difference spectrum). The blue shift is similar to one induced by chloride ion in the E181Q rhodopsin mutant and may indicate that the ionization state of Glu181 in rhodopsin is affected by detergent.     

“Three-in-one” Complexes Formed by Anionic Guests and Monosubstituted Cationic Alkyldiamino β-Cyclodextrin Derivatives

The effect of electrostatic interactions on the complexation of ionic guests by charged β-cyclodextrin (βCD) derivatives is reviewed. Special attention is paid to the numerous studies concerning the effect of electrostatic interactions on (i) the complexation of fluorescent and UV probes; (ii) the catalytic and chiral recognition properties of βCD derivatives; and (iii) the complexation of two bile salts (sodium cholate, NaC, and sodium deoxycholate, NaDC). The formation of three-in-one complexes between NaC and alkyldiamino βCD derivatives is also presented.     

Rhodopsin: its molecular substructure and phospholipid interactions.

Abstract—Rhodopsin in retinal rod outer segment disc membranes, was proteolyzed by treatment with papain. This treatment left three fragments of apparent mol wt of 26,000, 19,000 and 10,000 in the membrane. The circular dichroism (CD) of solubilized, proteolyzed rhodopsin, in both the UV and visible spectral regions, was essentially identical to that of native rhodopsin. This indicates that the retinal binding site configuration is essentially unchanged by proteolysis and that the proteolyzed form of rhodopsin retained the helical content of native rhodopsin. Far UV CD measurements on the fragments indicate that the secondary structural features of the proteolyzed complex were largely maintained when the complex was dissociated. This finding suggests that the proteolytic fragments represent independently stabilized domains within rhodopsin. Measurements of the dependence of the activation free energy of the unfolding of opsin (as determined by the rate of loss of regenerability of opsin) and the meta I to meta II transition on the level of phospholipid associated with opsin and rhodopsin. respectively, have allowed for a determination of the mode of stabilization of these proteins by phospholipid. This dependence has been shown to have a linear form for opsin and rhodopsin. Hence, it appears that the stabilization of the tertiary structure of both solubilized opsin and rhodopsin is attributable to the sum of their interactions with individual phospholipid molecules, interacting with the protein in a non-cooperative manner.     

Reconstitution of neutral amino acid transport from partially purified membrane components from Ehrlich ascites tumor cells

Solubilized protein fractions have been obtained from plasma membranes of Ehrlich ascites cells either by extraction with 0.5% Triton X-100 or by extraction with 2% cholate. Partial purification of the solubilized protein fraction has been obtained by utilizing a combination of ammonium sulfate precipitation and column chromatography. Leucine-binding activity has been detected in the Triton X-100 solubilized membrane fraction. The leucine-binding activity was measured by equilibrium dialysis and was saturable with high levels of leucine or phenylalanine and is not strongly effected by alanine. These properties are similar to those previously identified as System L. In addition, the cholate extracted protein fraction was partially purified and reconstituted into liposomes. Sodium dependent uptake of alanine and leucine could be demonstrated in the reconstituted vesicles. Concentrative uptake was dependent upon a sodium gradient. A membrane potential produced by valinomycin mediated potassium diffusion in the presence of sodium also stimulated amino acid transport in reconstituted liposomes.     

FUNCTIONAL PROPERTIES OF CATTLE RHODOPSIN IN SOLUBLE COMPLEX WITH PHOSPHOLIPIDS and DEOXYCHOLATE

Abstract— The necessary conditions of bleached rhodopsin to activate GTPase and to regenerate α-band were studied by changing the number of bound phospholipids to rhodopsin using gel filtration procedure. The number of bound phospholipids per mole of rhodopsin (bPL/rho) in the eluants was reproducibly controlled by the concentration of sodium deoxycholate (DOC) in the elution buffer. The eluants were soluble complexes composed of rhodopsin with original a-band, disk phospholipids and DOC. The regenerability of α-band depended on bPL/rho but neither on the concentration of DOC nor on state of aggregation of rhodopsin. The lowest number of bPL/rho for this activity under our experimental conditions was estimated to be30–50 in bPL/rho. GTPase was activated only by such complexes that had a nearly original quantity of bPL/rho in disk membranes. Other complexes with less bPL/rho showed aggregation upon bleaching and did not activate GTPase. The amount of phospholipids present in the disk membranes is sufficient to prevent aggregation of rhodopsin upon bleaching.     

Supramolecular ssDNA Templated Porphyrin and Metalloporphyrin Nanoassemblies with Tunable Helicity

Free‐base and nickel porphyrin–diaminopurine conjugates were formed by hydrogen‐bond directed assembly on single‐stranded oligothymidine templates of different lengths into helical multiporphyrin nanoassemblies with highly modular structural and chiroptical properties. Large red‐shifts of the Soret band in the UV/Vis spectroscopy confirmed strong electronic coupling among assembled porphyrin–diaminopurine units. Slow annealing rates yielded preferentially right‐handed nanostructures, whereas fast annealing yielded left‐handed nanostructures. Time‐dependent DFT simulations of UV/Vis and CD spectra for model porphyrin clusters templated on the canonical B‐DNA and its enantiomeric form, were employed to confirm the origin of observed chiroptical properties and to assign the helicity of porphyrin nanoassemblies. Molar CD and CD anisotropy g factors of dialyzed templated porphyrin nanoassemblies showed very high chiroptical anisotropy. The DNA‐templated porphyrin nanoassemblies displayed high thermal and pH stability. The structure and handedness of all assemblies was preserved at temperatures up to +85 °C and pH between 3 and 12. High‐resolution transition electron microscopy confirmed formation of DNA‐templated nickel(II) porphyrin nanoassemblies and their self‐assembly into helical fibrils with micrometer lengths.     

RHODOPSIN-PHOSPHOLIPID INTERACTION IN DETERGENT AND IN THE DISK

Abstract— Solubilization of cattle disk membrane in deoxycholate shifted the fluorescence emission maximum from 324 to 331 nm without changing the intensity. Tryptophyl residues are probably located at the hydrophobic interface between rhodopsin and phospholipid. Depletion of deoxycholate concentration from the solubilized disk by Sephacryl 200 column chromatography produced rhodopsin-phospholipid complexes with different characteristics that are the intermediate stages of membrane formation from homogeneous molecular solution. Association of rhodopsin takes place in a two-dimensional way even in the appreciably low content of phospholipid.
Sedimentation velocity studies showed that reassociation of lipid and rhodopsin occurs in 0.2% deoxycholate as well as in 0.05% sodium dodecylsulfate.
By using Sephacryl column we can now prepare, within 60 min, the rhodopsin-lipid complex that can form large vesicles in response to the addition of MgCl₂ without dialysis. This type of lipoprotein complex will be useful to the study of the mechanism of the two dimensional membrane formation.     

SPECTROSCOPIC STUDIES ON A RETINYLIDENE-IMINE-TETRAFLUOROBORATE

Abstract— N -retinylidene-butyl-l-aminium tetrafluoroborate (NRBH+BF₄^-) was used to determine the frequencies of the free (non-hydrogen-bonded) v (N+-H) and v (C=NH+) vibrations and their anharmon-icity constants. For this purpose the Fourier-transform IR and near-IR (overtone) spectra were recorded. The visible-UV spectra were also taken. The results locate the free v (N+-H) band at about 3250 ± 50 cm^-1; the vibration has normal anharmonicity while v (C=NH+) is very nearly harmonic. The UV and IR spectra show that the Schiff base is protonated, but that the proton is only very weakly hydrogen-bonded to the anion. Therefore, in this respect, NRBH+BF₄^- is a good model for the hydrogen-bonding environment of the region around the nitrogen of rhodopsin chromophores.     

POLARIZED UV-ABSORPTION SPECTRA OF RETINAL ISOMERS-I. MEASUREMENTS IN EXTREMELY THIN MONOCRYSTAL PLATELETS

Abstract Crystals of all- trans retinal and both different forms of 11- cis , 12-s- cis retinal were grown on quartz slides with faces (101), (001) and (101), respectively, forming thin platelets of less than 0.2 μm thickness. Polarized UV absorption spectra at room temperature were measured in the range from 20 to 43 × 10³ cm⁻¹ with a microscope-spectrophotometer. In this spectral range three diffuse absorption bands were observed for all crystal types at similar wave numbers. A main absorption band was found at 25–28 × 10³ cm⁻¹, and two further bands at 32–34 and 38–40 × 10³ cm⁻¹. In case of all- trans retinal the latter band is by far the weakest in this spectral range. Additionally, the crystal spectrum of all- trans retinal shows a shoulder at the low wavenumber side of the main band which cannot be resolved in the corresponding solution spectrum. In the crystal spectra of 11- cis , 12-s- cis retinal, however, only a strong dissymmetry is observed at this side of the main band.     

Spectra properties of rat liver mitochondrial choline dehydrogenase

Choline dehydrogenase contains the prosthetic group FAD, non-haem iron and acid labile sulfur. However, the absorption spectra of the purified enzyme do not change after adding substrate. The reduced absorption spectra of choline dehydrogenase can only be determined after the addition of dithionite. Those choline dehydrogenases situated in the mitochondrial inner membrane can be reduced by substrate and exist in the reduced state. When cholate was used to solubilize the substrate-reduced choline dehydrogenase, the reduced spectra will gradually disappear. However, if solubilization is carried out under anaerobic conditions, the reduced spectra can be retained, suggesting that the solubilized choline dehydrogenase can use oxygen as an acceptor.     

Chiroptical spectra of bicyclic selenolactams. Optical activity of the singlet–triplet transition

Two selenolactams with rigid 2-azabicyclo[2.2.1]heptane skeletons were prepared by reaction of the corresponding lactams with P₄Se₁₀. A comparison of their UV–vis and CD spectra with those of the carbonyl and thiocarbonyl analogues showed a similar character of the lowest-energy electronic transitions and the same signs of the corresponding Cotton effects. The MCD spectra of selenolactams revealed that their n–π* absorption band is dominated by the singlet–triplet component. A very weak CD corresponding to this component has an opposite sign to its much stronger singlet–singlet counterpart observed at the blue edge of the n–π* band.     

SPECTRA PROPERTIES OF RAT LIVER MITOCHONDRIAL CHOLINE DEHYDROGENASE

Choline dehydrogenase contains the prosthetic group FAD, non-haem iron and acid labile sulfur. However, the absorption spectra of the purified enzyme do not change after adding substrate. The reduced absorption spectra of choline dehydrogenase can only be determined after the addition of dithionite. Those choline dehydrogenases situated in the mitochondrial inner membrane can be reduced by substrate and exist in the reduced state. When cholate was used to solubilize the substrate-reduced choline dehydrogenase, the reduced spectra will gradually disappear. However, if solubilization is carried out under anaerobic conditions, the reduced spectra can be retained, suggesting that the solubilized choline dehydrogenase can use oxygen as an acceptor.     

Photocrosslinking of thin films of temperature‐sensitive polymers

The use of polymeric materials with temperature‐dependent degrees of swelling (especially polymers that exhibit lower critical solution temperature (LCST) behaviour in aqueous solutions) in microsystems requires the preparation and patterning of layers in the µm range. Copolymers based on N‐isopropylacrylamide were modi‐fied with a stilbazolium salt chromophore to yield photocrosslinkable temperature‐sensitive polymers. The chromophore and the polymers were characterized by UV, IR, 1H‐NMR (nuclear magnetic resonance) and 13C‐NMR spectra. The resulting polymers showed LCST behaviour, which was measured by differential scanning calorimetry. The photocrosslinking properties were studied by UV irradiation of the thin films and measurement of the changes in the UV absorption spectra. By irradiation of thin films through a mask it was possible to obtain patterned networks in the µm range (20 µm space width and ≥50 µm line width). The resulting patterned networks showed temperature‐dependent swelling properties in aqueous media. Copyright © 1999 John Wiley & Sons, Ltd.     

CONFORMATIONAL ANALYSIS OF THE RHODOPSIN CHROMOPHORE USING BICYCLIC RETINAL ANALOGUES

Abstract— For investigation of the chromophore conformation around the trimethyl cyclohexene ring and of the origin of the induced β-circular dichroism band in rhodopsin, two C₆-C₇ single bond-fixed retinal analogues, 6s-cb- and 6s-trans-locked bicyclic retinals (6 and 7, respectively) were synthesized and incorporated into bovine opsin in CHAPS-PC mixture. 6s-cb- and 6s-tram-Locked rhodopsin analogues (8 and 9 ) with A max at 539 and 545 nm, respectively, were formed. Interestingly, both 8 and 9 displayed α- and β-circular dichroism bands. The ellipticity of α-bands are similar in each other, while the β-band of 8 was about three times stronger than that of 9. Irradiation of 6s-trans-locked rhodopsin, 9, in the presence of hyroxylamine, resulted in the formation of only one of the enantiomers of 6s-rrans-locked retinal oxime showing a positive circular dichroism signal at around 390 nm. This fact strongly suggests that the retinal binding site of rhodopsin shows a chiral discrimination. From these experimental results, the interactions between the trimethyl cyclohexene ring portion in the chromophore and the neighbouring protein moiety in the rhodopsin molecule are discussed.     

ABSORBANCE and CIRCULAR DICHROISM SPECTRA OF 1-C1S PHOTOPRODUCT FORMED BY IRRADIATING FROG RHODOPSIN

Abstract— We showed by spectrophotometry and HPLC that a photoproduct having 7-cis retinal (1-cis photoproduct) can be derived from the photoisomerization of frog lumirhodopsin (L) and metarhodopsin I (M I). The efficiency of the isomerization was higher in M I than in L. The absorption maximum of the 1-cis photoproduct at -20°C is at 455 nm, and its maximum absorbance 1.1 times as large as that of rhodopsin. The photoproduct exhibited two positive CD bands at 450 nm α-band) and 320 nm (β-band); the molecular ellipticity at a-band ([θ] = 73000) being larger than that of rhodopsin ([θ] = 61000). Re-examination of the absorption spectra of rhodopsin intermediates gave the absorption maxima of L. M 1 and M 111 to be 522, 482 and 475 nm, respectively.     

Structure,optical and magnetic properties of LaFeO3 nanoparticles prepared by polymerized complex method

This work reports the study the structure, optical and magnetic properties of LaFeO₃ nanoparticles synthesized by the polymerized complex method. The LaFeO₃ nanoparticles were successfully obtained from calcination of the precursor at different temperatures from 750 to 1,050 °C in air for 2 h. The calcined LaFeO₃ nanoparticles were characterized by X-ray diffraction (XRD), transmission electron microscopy (TEM), UV–Visible spectroscopy, X-ray photoelectron spectroscopy (XPS), X-ray absorption near edge spectroscopy (XANES) and vibrating sample magnetometry. The XRD and TEM results showed that all LaFeO₃ samples had a single phase nature with the orthorhombic structure. The estimated crystallite sizes were in the range of 44.5 ± 2.4–74.1 ± 4.9 nm. UV–Vis spectra showed strong UV and Vis absorption with small band gap energy. The valence states of Fe ions were in the Fe³⁺ and Fe⁴⁺ state, as confirmed by XPS and XANES results. The weak ferromagnetic behavior with specific saturation magnetization of 0.1 emu/g at 10 kOe was obtained for the small particle of 44.5 ± 2.4 nm. The uncompensated spins at the surface was proposed as playing a part in the magnetic properties of small sized LaFeO₃.     

SPECTRAL PROPERTIES OF THE RHODOPSIN-SYSTEM OF THE CRAYFISH Astacus leptodactylus

Abstract— The absorption spectra of the membrane-bound and of the digitonin-solubilized visual pigment of crayfish Astacus leptodactylus were investigated by conventional spectrophotometry. A method was developed to isolate purified rhabdoms almost entirely free from screening pigments from a single retina. The quantity of isolated and purified rhabdoms from a single retina was sufficient to measure the absorption spectra of the visual pigment.
The absorption spectra of the chromoprotein system (R and M) show that both the membrane-bound and the digitonin-solubilized visual pigment isomers are stable at 0°C and pH 7.0. Rhodopsin and metarhodopsin are photoreversible under these conditions without any light-induced denaturation. The difference spectra for the chromoprotein isomers and those of different photostationary states yield maximal values for ΔE at 570 and 485 nm.
At neutral pH, 0°C, Λ_max of rhodopsin is 530 nm. Irradiation with light of Λ= 630 to 640 nm isomerizes rhodopsin nearly quantitatively to metarhodopsin with Λ_max, of 500 nm. The molar extinction coefficient of metarhodopsin is greater than that of rhodopsin by a factor of ˜ 1.41. each measured at its respective Λ_max Metarhodopsin can be isomerized to rhodopsin by irradiating at Λ > 630 nm. As the absorption spectra of the two chromoprotein isomers overlap, only part of the metarhodopsin can be reversed to rhodopsin. The maximal photoreversion can be achieved by irradiating at 460 nm. The stability of the digitonin-solubilized chromoprotein is remarkably dependent on temperature. Warming the digitonin extract of rhabdoms from 0 to 20 or 30°C caused a shift of the rhodopsin spectrum to shorter wavelengths (Λ_max= 485 nm) accompanied by a decrease of E_Λmax by about 30%.     

2,6-二取代苯并二噁唑的研究(Ⅲ)——2,6-二苯乙烯基苯并二噁唑和它们的衍生物

通过2,6-二甲基苯并[1,2d;4,5d′]二噁唑和2,6-二甲基苯并[1,2d;5,4d′]二噁唑分别与苯甲醛和取代苯甲醛缩合备制取七种相应的2,6-二苯乙烯基苯并[1,2d;4,5d′]二噁唑和2,6-二苯乙烯基苯并(1,2d;5,4d′]二噁唑。测定了全部化合物的熔点、红外光谱、紫外光谱、荧光光谱、激光转换效率。     

The absorption and circular dichroism spectra of chiral olefins

Absorption and CD spectra over the quartz and vacuum UV region down to 165 nm are reported for a range of chiral alkenes in the vapour phase and in solution from +70° to ?185°C. A major couplet of oppositely-signed CD bands with comparable band areas, near 48 and 55 kK, is observed in a number of dissymmetric olefins and in some cases a weaker Rydberg CD absorption is found at lower frequency. The Rydberg CD band is characterised by its sharp vibronic structure in the vapour phase and by large blue-shifts produced on passing to the condensed phase and by a reduction in temperature. The olefin couplet of major CD bands with opposite sign is assigned to a near-complete mixing of the electric-dipole π_x→π_x^* and the magnetic-dipole π_x→π_y^* excitations, producing a pair of isotiopic absorption bands with the same polarisation and comparable dipole strengths associated with the CD couplet. Three mixing mechanisms are discussed; sterically-induced π-bond torsion, a first-order static field model, and a second-order dynamic-coupling model dependent, respectively, upon the effective charge and upon the mean polarisability of dissymmetrically-located substituent. The latter two models give the octant rule previously proposed empirically connecting the sign of the rotational strength of the lower- and higher-frequency member of the olefin CD couplet with the position of the substituent in the chromophore coordinate frame.