KINETICS OF STACKING INTERACTIONS IN FLAVIN ADENINE DINUCLEOTIDE FROM TIME-RESOLVED FLAVIN FLUORESCENCE

The time dependence of the fluorescence of flavin adenine dinucleotide (FAD) was measured with a subnanosecond-resolving fluorometer. In contrast to the fluorescence decay of FMN, the decay of FAD was proved to be nonexponential. The time-dependent fluorescence of FAD can be interpreted by assuming an equilibrium between closed and open conformers in the ground state. The rate constant for folding in the excited state and the fluorescence lifetime of the intramolecular complex could be evaluated from analysis of the observed fluorescence decay. The results on FAD were compared to those on NADH obtained earlier.     

A BLUE LIGHT-SENSITIVE CYTOCHROME-FLAVIN COMPLEX FROM CORN COLEOPTILES. FURTHER CHARACTERIZATION*

Abstract— The partially purified blue light-sensitive membrane-associated flavin-cytochrome complex from etiolated corn coleoptiles shows a unique sharp α-band at 555 nm in its light-minus-dark difference spectrum at liquid nitrogen temperature. This band is clearly distinguishable from the α-bands found in fractions enriched for mitochondria and endoplasmic reticulum respectively. The photoactive membrane fraction is shown to have ATPase activity that is not stimulated by K⁺ and that is not inhibited by oligomycin. Other than flavin fluorescence at 525 nm obtained upon excitation at 450 nm, there is a second fluorescent component with emission at 430 nm on excitation at 350 nm. The mid-point potential of the Triton X-100 solubilized b-cytochrome, measured by simultaneously monitoring the reduction of the pyocyanine 600-800 nm peak and the appearance of the 427 nm Soret peak of the b-cytochrome upon titration with dithionite in the presence of ferricyanide, is estimated to be ?65 mV. The kinetics of the blue light-induced reduction and dark rcoxidation of the 6-cytochrome suggest that the mid-point potential of the b-cytochrome is not affected by Triton X-100 solubilization.     

RED/FAR-RED PHOTOREVERSIBILITY: NOT AN APPROPRIATE PHYTOCHROME ASSAY FOR RED-LIGHT PREIRRADIATED CORN COLEOPTILES

Abstract— Based on measurements with a single beam spectrophotometer, it has been found that subsequent red/far red irradiation cycles, which are usually given to monitor phytochrome content by dual wavelength spectroscopy, induce chlorophyll-related absorption changes in maize coleoptiles. Therefore, the difference signal, usually measured between 730 and 800 nm or 660 and 730 nm after saturating red and far red irradiations, does not represent solely the phytochrome content of preirradiated samples.     

FLUORESCENCE LIFETIME STUDY OF THE DENATURATION OF RIBONUCLEASE-A

Abstract. Fluorescence quantum yield and lifetime measurements of the tyrosine residues in ribonuclease-A (RNase) were used to study the conformational changes involved in the denaturation of the enzyme. Measurements were done on RNase and on selectively acetylated RNase in the native, the partly denatured (reductive cleavage of S-S bridges or treatment with 8 M urea) and in the fully denatured state. The data were interpreted to mean that the opening of the S-S bridges causes large parts of the enzyme chain to unfold while leaving a hydrophobic region; including one of the tyrosine residues, intact. The biological activity of RNase is destroyed by this unfolding. Urea apparently does penetrate the protein coil but does not greatly affect the RNase structure since some of its biological activity is still retained. The opening of the S-S bridges in the presence of urea destroys the native conformation (and biological activity) completely leaving the protein in the form of an uncoiled polypeptide chain. It is suggested which parts of the protein structure might be affected by partial denaturation.     

三元若丹明激光染料荧光寿命研究

利用单光子计数技术测试了新型三元若丹明激光染料在不同溶剂中的荧光寿命、荧光光谱及其寿命的实验数据.实验表明,所研究的三元若丹明染料存在着有效的分子内能量传递过程,这些过程使得激光染料的荧光量子效率及光稳定性明显改善.     

胭脂红酸的荧光发射寿命及荧光猝灭

以蒸馏水中的糖原悬浮液为参照物，测定了胭脂红酸的荧光发射寿命，τ＝０．０９３±０．０１０ｎｓ．研究了ＯＨ－和Ｉ－对胭脂红酸荧光的猝灭，后者遵守Ｓｔｅｒｎ－Ｖｏｌｍｅｒ方程，其猝灭常数ＫＱ＝１．２７±０．０９Ｌ·ｍｏｌ￣（－１），前者则不是遵守此方程的简单荧光猝灭，这可能是由于胭脂红酸中酚基的存在降低了最低激发态能量的原因。     

锌酞菁类染料荧光寿命的非瞬态实验估算

合成了一系列的锌酞菁染料。用循环伏安法测定了它们的氧化还原电位, 并测定了用典型的电子受体猝灭它们的荧光动力学数据。按电子转移模式确定了各染料-电子受体对的荧光猝灭速率常数κ_q对电子从染料向受体转移的自由能变化⊿G函数关系。根据测得的氧化还原电位和光谱数据计算出⊿G, 根据函数关系计算出κ_q, 代入到猝灭动力学数据κ_qτ。这样,就用非瞬态的实验估算出染料的荧光寿命r。与已知的实测文献值进行比较, r的大致范围是可信的。     

新型双发色团染料荧光光谱及其寿命的研究

有效的染料激光操作需要较高的荧光量子效率,若丹明是在500~700 nm光谱区中一类最重要的激光染料.然而,染料的基态分子和三线态对辐射能量的吸收将会大大降低激光输出效率,再者,由于若丹明类染料在紫外区的吸收系数较小,为了有效吸收泵浦能量(如用XeCI准分子激光,308 nm),就必须使用高浓度染料溶液,在这种情况下,若丹明类染料较小的Stokes位移就势必造成基态分子更大的重复吸收,即造成更大的谐振腔损耗^[1].     

RESOLUTION OF SPECTRAL AND LIFETIME HETEROGENEITY OF TRYPTOPHAN FLUORESCENCE IN BACTERIORHODOPSIN

Abstract— The picosecond time-resolved fluorescence decay of bacteriorhodopsin (BR) was analyzed by the maximum entropy method. Results showed five distributions of lifetimes indicating at least five decay components. A wavelength-dependent study of emission decay of BR was carried out in the wavelength region from 310 to 390 nm. The decay at each wavelength was resolvable into four decay components by the discrete exponential analysis. The three short lifetime components (100 ± 20 ps, 400 ± 50 ps and 1.0 ± 0.1 ns) were independent of wavelength, whereas the longest lifetime component was wavelength dependent (varying from 4.1 ns at 310 nm to 5.7 ns at 390 nm). These results are inconsistent with the existing model of associating the fluorescence of bacteriorhodopsin with two or four lifetime components. An attempt is made to associate the five decay components with the emitting tryptophans of BR.     

BLUE LIGHT INDUCED, REVERSIBLE IN ACTIVATION OF THE TONOPLAST-TYPE H+-ATPase FROM CORN COLEOPTILES IN THE PRESENCE OF FLAVINS

Abstract— Irradiation (λ_max 447 nm; 58.5 W m^-2) of a microsomal membrane fraction of corn coleoptiles for 5 min in the presence of the in vivo concentration of riboflavin inactivates the tonoplast-type H⁺-ATPase. This inhibition is O₂-dependent, is enhanced in D₂O and suppressed by NaN₃, indicating participation of singlet molecular oxygen in the inactivating mechanism. Besides singlet oxygen, the superoxide anion (O₂^-) is generated during irradiation, which obviously has no effect on the H⁺-pumping activity. However, in the presence of superoxide dismutase (SOD), O₂^- is transformed into H₂O₂ which causes an additional strong inhibition of H⁺. ATPase activity. This inhibition can be increased by ethylenediaminetetraacetic acid (EDTA), which is known to be an electron donor of the excited flavin molecule. In contrast, catalase prevents the H₂O₂-mediated photoinactivation of the H⁺ -ATPase. The light dependent inactivation of H⁺-transport does not occur if reduced glutathion (GSH) is added prior to or after irradiation. These results indicate that the blue light mediated inhibition of the H⁺-ATPase is mediated by singlet oxygen and H₂O₂ which oxidize essential SH-groups of the enzyme into disulfides. Reduction of the formed disulfides by GSH restores the activity of the enzyme.     

A FLAVOPROTEIN IN Phycomyces blakesleeanus WITH SHORT FLUORESCENCE LIFETIME

Abstract— The photoreceptor system for the blue-light-induced phototropism in the fungus Phycomyces blakesleeanus includes one or more flavin chromophores, probably located in the plasma membrane of the sporangiophore. From a plasma-membrane fraction of short synchronous sporangiophores, we have enriched, by column chromatography, specific proteins with covalently bound flavins. These flavoproteins were analyzed by a fluorescence lifetime assay. Flavoproteins with fluorescence lifetimes significantly less than 5 ns have been predicted to be involved in blue-light reception. We studied samples from a wild type strain and from the night-blind mutant LI. (genotype madC). For the enriched flavoprotein samples, we found predominant fluorescent components with lifetimes of 1.5 ns (74%) for wild type and 1.8 ns (83%) for LI. According to this assay, one or both of these flavoproteins are likely components of the blue-light photoreceptor system in P. blakesleeanus.     

STATIC and TIME-RESOLVED FLUORESCENCE OF AN AMPHIPHILIC FLAVIN IN AEROSOL OT REVERSED MICELLES

Spectral and time-resolved fluorescence studies have been carried out on N(3)-undecyllumi-flavin dispersed in reversed micelles composed of the surfactant sodium di(2-ethylhexyl) sulfosuccinate (Aerosol OT, AOT), various amounts of water and n -heptane as continuous phase. The fluorescence spectral properties (spectral distribution, quantum efficiencies and lifetimes) as function of the water to AOT molar ratio suggest that the flavin occupies a position within the surfactant boundary layer in close contact with water. The fluorescence anisotropy exhibits biexponential decay with a short (0.3 ns) and a longer (1.6–2.4 ns) correlation time. The contribution of the short component increases with the growth of the droplet providing evidence for enhanced flexibility of the flavin in the interfacial layer.     

FLUORESCENCE LIFETIME OF ACRIDINE ORANGE IN SODIUM DODECYL SULFATE PREMICELLAR SOLUTIONS

Abstract— The absorption and fluorescence spectra, and the fluorescence lifetime of acridine orange (AO) were measured in a wide range of the sodium dodecyl sulfate (SDS) concentration below and above the critical micelle concentration (cmc). The fluorescence consisted of two components with different lifetimes; short (<3 ns) and long (>3 ns). The short and long lifetime components are attributed to the AO monomer and dimer associated with detergent, respectively. The lifetime of the dimer increased with increasing the SDS concentration just below the cmc. It decreased suddenly to a constant value just above the cmc. The lifetime of the monomer showed only a slight increase in the concentration range of SDS employed.     

FLUORESCENCE PROPERTIES OF C-PHYCOCYANIN ISOLATED FROM A THERMOPHILIC CYANOBACTERIUM

Abstract The fluorescence lifetime of purified C-phycocyanin from the thermophilic cyanobacterium, Phormidium laminosum (strain OH-1-p. Cl 1), was measured as 1.48 ± 0.06 ns using the technique of time-correlated single-photon counting under very weak excitation pulses. The natural radiative lifetime (∼6.1 ns) of the pigment was calculated by integrating the absorption spectrum using the Strickler–Berg equation. From these two lifetimes we calculate a fluorescence quantum yield of ∼0.24 which is very close to the value ∼0.22 which we measure relative to the known value of cresyl violet in methanol. Both the fluorescence lifetime and the quantum yield of the pigment from this organism are lower than most previous values reported in the literature. We conclude that our lower values are not due to high light intensity, pH, buffer, concentration, instrumentation artifacts, aggregation effects or the thermophilic nature of the organism. Instead, we suggest that the photophysical properties of C-phycocyanin are species dependent, perhaps due to the specific molecular environment of the tetrapyrrole.     

LIGHT QUENCHING OF FLUORESCENCE: A NEW METHOD TO CONTROL THE EXCITED STATE LIFETIME AND ORIENTATION OF FLUOROPHORES

Abstract Experimental studies have recently demonstrated that fluorescence emission can be quenched by laser light pulses from modem high-repetition rate lasers, a phenomenon we call “light quenching.” In this overview article, we describe the possible effects of light quenching on the steady-state and time-resolved intensity and anisotropy of fluorophores. One can imagine two classes of experiments. Light quenching can occur within the single excitation pulse, or light quenching can be accomplished with a second time-delayed quenching pulse. The extent of light quenching depends on the amplitude of the emission spectrum at the quenching wavelength. Different effects are expected for light quenching by a single laser beam (within a single laser pulse) or for a time-delayed quenching pulse. Depending upon the polarization of the light quenching beam, light quenching can decrease or increase the anisotropy. Remarkably, the light quenching can break the usual z-axis symmetry of the excited state population, and the measured anisotropy (or polarization) depends upon whether the observation axis is parallel or perpendicular to the propagation direction of the light quenching beam. The polarization can increase to unity under selected conditions. Quenching with time-delayed light pulses can result in step changes in the intensity or anisotropy, which is predicted to result in oscillations in the frequency-domain intensity and anisotropy decays. These predicted effects of light quenching, including oscillations in the frequency-domain data, were demonstrated to occur using selected fluorophores. The increasing availability and use of pulsed laser sources requires consideration of the possible effects of light quenching and offers the opportunity for a new class of two-pulse or multiple-pulse time-resolved experiments where the sample is prepared by the excitation pulse and subsequent quenching pulses to modify the excited state population, followed by time- or frequency-domain measurement of the optically prepared excited fluorophores.     

FLUORESCENCE PROPERTIES OF PORPHYRIN-GLOBIN FROM HUMAN HEMOGLOBIN

Fluorescence excitation and emission spectra, decays, and quantum yields are reported for the porphyrin-globin of hemoglobin (Hb^desFe) in aqueous solution of pH 8, at 4°C. A very weak fluorescence was observed in the UV (maximum at 334 nm), due to tryptophan and tyrosine residues, in addition to the strong porphyrin emission in the visible (maxima at 624 and 692 nm) reported previously. The absorption and fluorescence properties of the porphyrins of Hb^desFe were compared to those for free porphyrin in organic solvents and in aqueous solution. The close similarity of the fluorescence decays and quantum yields in Hb^desFe and in solution indicate the absence of stronger, specific porphyrin-protein interactions; however, slight spectral shifts point to the existence of water molecules in the Hb^desFe porphyrin environment. The fluorescence study also demonstrates the existence of efficient Trp-porphyrin energy transfer of Förster type. The extent of transfer is in satisfactory agreement with the value expected from crystallographic data for hemoglobin. The results are discussed and compared to previous fluorescence studies of hemoglobin and apohemoglobin. An improved method for the preparation of Hb^desFe is reported.     

FLUORESCENCE LIFETIME AND QUANTUM YIELD OF PHENYLALANINE AQUEOUS SOLUTIONS. TEMPERATURE AND CONCENTRATION EFFECTS

Abstract— –The influence of concentration and temperature on the fluorescence quantum yield and lifetime (measured by a monophoton technique) of phenylalanine is studied in neutral aqueous solutions (8 × 10^-4-10^-1 M ) over the temperature range 0–70°C. The rate constants for emission, internal conversion and intersystem crossing are evaluated and show that both non radiative processes contribute efficiently to the deactivation of the singlet state. Evidence for excited dimer formation at high concentration is presented. The binding energy of excimers was found to be 0.19 e V.