新的植物毒素蒜头果蛋白的荧光光谱研究

蒜头果蛋白(Malanin)是从我国稀有植物蒜头果中分离纯化出的一种具有高细胞毒性的蛋白质。用荧光光谱法研究在温度、酸度、有机溶剂、表面活性剂、变性剂及荧光猝灭剂等不同条件对蒜头果蛋白溶液构象的变化。实验表明,Malanin在天然状态下荧光发射峰位于340 nm处,色氨酸(Trp)残基较大程度位于Malanin分子的疏水区。十二烷基硫酸钠、异硫氰酸胍、丙烯酰胺和碘化钾的加入均可使Malanin的分子构象发生变化,导致分子内Trp残基的荧光猝灭。异硫氰酸胍的加入使Trp残基的荧光发射峰位明显红移,表明位于Malanin分子较疏水环境内的Trp残基相对外露。     

色氨酸的非线性分频荧光研究

色氨酸 (Trp)在 350nm处产生一个荧光峰 ,在 70 0nm处产生一个 (分频 )荧光峰 ,此两峰荧光强度F3 50nm 和F70 0nm 均与Trp浓度 ( 0～ 1× 10 -5mol·L-1 )成线性关系 ,随着Trp浓度增大 ,350和 70 0nm半峰宽(Δλ) 3 50 ,(Δλ) 70 0 缓慢减小 ,而F70 0nm/F3 50nm 值和半峰宽比 (Δλ) 70 0 /(Δλ) 3 50 为一常数 ,此两峰具有相似的荧光特性。根据建立的分频荧光能级原理和非线性共振分频荧光原理探讨了色氨酸分频荧光峰产生的原因     

细菌视紫红质能化态时表面电位的非线性光学机制

用荧光标记物1，8-ANS与细菌视紫红质结合，测得紫膜细菌视紫红质在能化态时的表面电位远大于非能化态时的对应值。在细菌视紫红质分子的激光四波混频实验中，应用激子表象理论，获得了紫膜能化态时的激子饱和密度和激子长度，说明在bR—ANS络合物中，细菌视紫红质中色氨酸残基对ANS的激发能量转移效率提高，能化态时表面电荷密度增加，从而使非辐射共振转移变为激子转移，也证明了紫膜能化态时表面电位的非线性光学机制。     

表面荧光机制的理论研究

本文研究了 Rh B分子的 539.0 nm和 572 .5nm两荧光峰在表面增强活性银胶颗粒表面上的增强和淬灭效应 :在同一分子体系中同时观察到 530 .0 nm荧光峰的增强和 572 .5nm荧光峰的淬灭 ,并对其进行了理论计算。结果表明这两个荧光峰的增强或淬灭主要取决于局域电磁场增强和分子到金属表面无辐射能量转移衰减过程的竞争效应。当满足吸收共振增强和辐射共振增强时 ,荧光被增强 ;反之 ,荧光被淬灭。计算表明 ,荧光增强因子最高为 1     

牛α-乳白蛋白-亚油酸复合物的结构及抗肿瘤活性

利用内源性荧光光谱、荧光探针(ANS)结合荧光光谱及圆二色谱,以乳白蛋白-油酸为参照,研究了乳白蛋白结合亚油酸后,疏水性氨基酸、疏水性区域、三级结构及二级结构的变化,并利用亚甲基蓝的方法评价了该复合物的抗肿瘤活性。荧光光谱结果显示,与乳白蛋白-油酸复合物类似,乳白蛋白结合亚油酸后,其内源性荧光光谱显著红移,从331.07 nm移至337.60 nm;外源性ANS结合光谱蓝移,从516.20 nm移至508.50 nm;且荧光强度增加,表明乳白蛋白结合亚油酸后同样出现了疏水性氨基酸及疏水性区域暴露的现象。圆二色谱结果表明,与乳白蛋白-油酸复合物类似,乳白蛋白结合亚油酸后,三级结构部分丧失,二级结构中β-转角及无规卷曲的含量显著降低,β-折叠含量增加。细胞实验证实了乳白蛋白-亚油酸复合物具有良好的抗肿瘤效果。该研究从复合物结构和功能的两方面,为新型抗肿瘤乳白蛋白-亚油酸复合物的开发提供了依据。     

谷胱甘肽比率荧光探针分子的设计合成及其光谱性能

将喹啉和丹磺酰胺两种荧光基团同时引入配体L1,利用L1与锌离子自组装构筑三核锌有机-金属大环化合物H-1(比率荧光探针),实现了对生物分子谷胱甘肽(GSH)的有效识别。利用紫外光谱、荧光光谱、~1H NMR、ESI-MS等表征方法研究了H-1对生物分子谷胱甘肽(GSH)的光谱识别作用。紫外滴定光谱表明,当向H-1中加入谷胱甘肽分子后,425 nm处的吸收峰强度降低,320 nm处的吸收峰强度增大,等吸收点为355 nm。利用320 nm处的吸光度值模拟计算平衡常数,lg K为4.03±0.11,说明H-1与GSH形成了1∶1的包合物。荧光光谱分析表明,当向H-1中加入GSH后,以340 nm光激发,波长为513 nm处丹磺酰胺的荧光强度下降,并且发生红移,而396 nm处喹啉基团的荧光强度增大。利用喹啉基团与丹磺酰胺基团荧光发射峰强度变化的比值可以精准检测谷胱甘肽分子,检测限可达到2.5×10~(-6)mol·L~(-1)。     

1-苯胺基萘-8-磺酸盐在各种固体基质中发光特性的研究

1-苯胺基萘 - 8-磺酸盐 (ANS)在不同的固体基质中发光特性的研究发现 :(1 ) ANS分子发射峰位置与在甲醇溶液中相比 ,发生明显的蓝移 ,可能是由于约束在固体基质中的荧光分子的运动受到一定的限制而接近单分子发光的行为。与纯粉末 ANS荧光相比 ,发生红移。ANS在极性的滑石基质中 ,发射峰移向更短的波长 ,在非极性的石蜡基质中移向更长的波长 ,反映固体基质微观环境的变化。 (2 ) ANS分子荧光寿命明显缩短 ,主要原因是在固体基质中 ,荧光发射速率常数 kf 增大。 (3) ANS分子相对量子产率明显增大 ,荧光分子运动受限 ,减弱分子之间的相互作用 ,减小了由于碰撞引起的猝灭 ,分子结构刚性增强。该结果对于研究固体基质的物化性质、探讨光化学反应中能量转移现象具有重要意义。     

同步荧光光谱法研究肿瘤芳香族氨基酸残基含量的变化

用同步荧光光谱法评估原发性肝细胞癌患者血浆、肝癌荷瘤小鼠以及培养细胞(HepG2和HL-7702)中酪氨酸(Tyr)和色氨酸(Trp)残基水平变化。固定发射波长λ_em和激发波长λ_ex之间的波长差Δλ分别为20和60 nm,激发和发射单色器同时进行扫描,确定350 nm为Trp的同步特征发射峰位置,318 nm为Tyr的同步特征发射峰位置。结果表明,肝癌患者及荷瘤小鼠血浆蛋白质所含Tyr和Trp残基的荧光强度明显增加。相反,肝癌细胞或荷瘤小鼠肿瘤组织中Tyr和Trp残基荧光强度却随生长时间增长而减少。进一步实验表明,具有抗癌活性的苦参碱处理癌细胞后,细胞Tyr和Trp残基的荧光强度升高。这些结果表明,Tyr和Trp残基的变化可能参与了肿瘤的发生发展。     

内周天线CP43、CP47中β-Car到Chla分子间的能量传递

采用超快荧光光谱动力学对从菠菜中分离纯化的内周天线CP43、CP47进行研究,获取了它们的动力学三维荧光谱,CP43的荧光光谱范围为640～780nm,最大峰位于680nm处,在该峰值处的荧光寿命约为3.54ns;CP47的荧光光谱范围为630～775nm,最大峰位于691nm处,在该峰值处的荧光寿命约为3.22ns,在CP43和CP47中,Chla分子发射荧光的效率分别约为38.3%和40.6%.依据分子的退激发途径,我们分析认为在CP43、CP47中β-Car→Chla分子的能量传递速率常量分别为9.06×10¹¹s^-1,1.3×10¹²s^-1;能量传递效率分别为47.5%、66.5%;并估计β-Car分子与Chla分子外周之间的距离分别为0.110nm、0.085nm.     

胆红素与血红蛋白分子作用的发光光谱分析

利用荧光光谱技术研究了胆红素对血红蛋白分子中发光基团结构变化的影响及其与血红蛋白结合方式。结果表明,不同浓度的胆红素可以不同程度地猝灭血红蛋白荧光,导致330nm处色氨酸残基荧光峰下降,410nm处荧光峰消失;pH值94时血红蛋白与胆红素以非静电引力如疏水作用、范德华力的协同作用结合,且随着作用时间的延长,荧光强度下降。血红蛋白中氨基酸残基上的-NH₂与胆红素分子中两个-COOH结合,形成复杂的卷曲结构。血红蛋白的紫外光谱受胆红素分子中二吡咯发色团的影响,导致光吸收劈裂,在350,406nm处形成肩峰。另外,体系受温度影响也较大。     

Concentration quenching effect of organic light‐emitting devices using DCM1‐doped tetraphenylgermole

We examine the concentration quenching of a 4‐(dicyanomethylene)2‐methyl‐6‐(p‐dimethylaminostyryl)‐4H‐pyran (DCM1)‐doped 1,1‐bis(2‐phenylethynyl)‐2,3,4,5‐tetraphenylgermole (HPAG)‐based light‐emitting diode. Originally, HPAG emits in the ~500‐nm (green) region, which can be converted to a red‐emission material by using DCM1 doping. As the DCM1 concentration increased from 1 to 10 wt%, the electroluminescence peak positions are red‐shifted from 604 to 644 nm, respectively. Increasing doping density not only shows the red‐shift but also shows decreasing luminance efficiency. Förster energy transfer between the HPAG host material and the DCM1 guest material is responsible for the strong red‐emission behavior. The calculated Förster radius (4.0 nm) for excellent Förster energy transfer characteristics with increasing doping concentration of DCM1 is consistent with experimental results. The maximum luminance efficiency was 6.64 cd/A at 11.0 mA/cm². The HPAG germole compound shows excellent red‐emission host–guest system properties for red organic light‐emitting device applications. Copyright © 2011 John Wiley & Sons, Ltd.     

The Paths of Excitation Energy Deactivation in LH1 Reduced Mutant and Wild-Type Strains of Rhodobacter sphaeroides

The P3 mutant of Rhodobacter sphaeroides had an altered ratio of reaction center to core (LH1) and peripheral (LH2) antenna complexes compared to the wild-type strain. Intracytoplasmic membranes from these two strains were purified and then resuspended in buffer or immobilized in isotropic and stretched polymer film. The absorption, photoacoustic, and delayed luminescence spectra were measured. The ratios of infrared absorption and photoacoustic bands (located at about 880 nm for LH1 and at 850 and about 800 nm for LH2) as well as the half-width of these bands are different for the LH2 and LH1 mutants and wild-type strain. The whole yields of thermal deactivation of the two strains were comparable, but in the absorption region of LH2 it was slightly lower in the case of the mutant than for the wild-type strain. The delayed luminescence main maxima were observed at about 860 and 700 nm. The first one could be due to emission of bacteriochlorophyll a of LH2 complexes. The emission at about 700 nm is probably due to dihydromesochlorophyll, which is usually, to some extent, produced from bacteriochlorophyll a in bacterial complexes. The delayed luminescence emission is competing with excitation energy transfer to the reaction center. The intensity of the delayed luminescence of the mutant strain was higher than that of the wild-type strain when both samples were excited in a region of carotenoid absorption. The mutant contains less carotenoids than the wild-type strain. Carotenoids work as efficient antenna. When they at a lower concentration the excitation can be trapped more easily by some chlorophyll-like pigment isolated from the excitation energy chain. The dependences of delayed luminescence spectra on the light polarization and excitation wavelengths for the wild-type strain and for the mutant were different. The anisotropy of delayed luminescence showed that bacteriochlorophyll a molecules of different orientations were contributing to the mutant and the wild-type strain emission. All the results suggest that the excitation energy transfer from the antenna to the reaction center in the mutant and the wild-type strain is similar.     

Energy transfer dynamics in B-phycoerythrin from the red alga Porphyridium purpureum

The B-phycoerythrin hexamer (αβ)₆γ of Porphyridium purpureum was isolated and purified. The absorption, circular dichroism, fluorescence and ultrafast time-resolved spectra were obtained. The results showed a double absorption peak at 545 nm and 565 nm and a shoulder peak at 498 nm, and fluorescence emission maxima at 580 nm and 620 nm were observed. The circular dichroism spectra in the near-ultraviolet region were obtained and resolved for the first time, which showed that the two peaks at 260 nm and 305 nm were considered to be correlated to phenylalanine (Phe) and tryptophan (Trp) in a conservative hydrophobic microenvironment, respectively. The circular dichroism spectra in the visible region showed that PEB139α/PEB158β and PEB82α/PEB82β existed as two exciton-coupled bilin pairs. Energy transfer within the exciton-coupled pairs was by exciton splitting, while between the exciton-coupled pairs was by Förster resonance. From the studies of the energy transfer dynamics by ultrafast time-resolved fluorescence spectroscopy, it was confirmed that the energy transfer of the B-PE hexamer had three time components of 8 ps, 60 ps, and 1200 ps. In addition, the internal energy transfer pathways of B-phycoerythrin hexamer were identified by deconvoluting the fluorescence decay curve at different detection wavelengths.     

Two distinguishable fluorescent modes of 1-anilino-8-naphthalenesulfonate bound to human albumin

We study the interaction of 1-anilino-8-naphthalenesulfonate (ANS) with human (HSA) and bovine serum albumin (BSA) by phase and modulation fluorescence spectroscopy. We determined that both HSA and BSA show one or two distinguishable fluorescent sites, depending of the ANS/serum albumin ratio. At above a 11 ANS/HSA molar ratio, the steady-state emission spectra for ANS can be resolved in two components: component 1, emitting with a lifetime (₁) of 16 ns and a _1max of 478 nm, with a quantum yield (_f1) of 0.67, and component 2, with a lifetime (₂) of 2–4 ns and a _2max of 483 nm, with an average quantum yield (_f2) of about 0.11. Considering these findings, the binding analysis is fitted with a model of two independent sites. Site 1 has an association constantK _as1=0.87×10⁶M^–1 and a capacity of 1.04 mol of ANS/mol of HSA, and site 2 aK _as2=0.079×10⁶M^–1 and a capacity of 2.34 mol of ANS/mol of HSA. Analysis of fluorescence lifetime distributions shows that the rigidity of the fluorophore environment at site 1 changes when site 2 is occupied. These findings suggest an interconnection between the two sites and that ligands can stabilize the protein's globular structure. To assess the identity of the ANS binding sites we used diazepam as a marker of the site located at the IIIA HSA subdomain and aspirin as a marker of sites located at the IIIA and IIA HSA subdomains. Both ligands displace ANS only from site 1, suggesting that it corresponds to the binding site located at the IIIA sub-domain of the protein. We determined that theK _as values for diazepam and aspirin are 0.113× 10⁶ and 0.021×10⁶ M ^–1 respectively.     

Spectroscopic Determination of Heparin Sodium Using Europium (III) as a Probe Ion

Abstract

A sensitive, rapid, accurate and precise procedure for the microdetermination of heparin sodium in bulk, in injection and in blood serum. The procedure was built around the fact that heparin possesses many active binding sites; carboxylic, hydroxylic, amino and sulphonated groups, which are strongly bound to Eu³⁺ ions. Such binding enhances the europium emission at 616 nm which is a forbidden transition. The emission of europium at 592 nm comes from a non hypersensitive transition and is not affected by the ligand which is bound to europium ions. The intensity ratio R, defined as I₅₉₂/I₆₁₆ was used to determine the amount of free and bound europium ions. There is a linear relationship between bound europium ions and heparin sodium within the concentration range 1–12 ug. mL^?1 (0.07–0.84 USP. IN). Reaction conditions were studied and percentage recoveries was 99.77 ± 1.68. The relative stability of the complex was 1.2E⁵ and the correlation coefficient was 0.99923. Heparin was isolated from serum using ECTEOLA-cellulose and Sephadex G25 columns. The method shows good agreement with an anilinonaphthalene-1-sulfonate (ANS) and protamine fluorometric method.     

BeAl2O4:Cr3+紫外光谱的研究

在强场理论的基础上,本文考虑了组态相互作用,拟合了各能级位置,并对其紫外光谱进行了讨论.     

DEDO: A specific,fluorescent inhibitor for spectroscopic investigations of Na,K-ATPase

The interaction between the fluorescent ouabain derivative DEDO and purified renal Na,K-ATPase (isolated from different animal species) is investigated. Equilibrium binding studies provide a pK value of about 7.5 and a stoichoimetric coefficient of 1. Nonmodified ouabain exhibits the same affinity to the rabbit enzyme; the enzyme originating from the other sources binds DEDO 10 times less strongly than ouabain. Kinetic studies indicate that this is the consequence of a 10 times higher dissociation rate constant of the complexes formed with DEDO. The fluorescence emission intensity of DEDO is enhanced, being dependent on the enzyme source. The single decay time of DEDO is 3 ns in the absence and 21 ns in the presence of the rabbit enzyme and 14 ns in the presence of the pig renal enzyme. This result suggests that the fluorophore of DEDO is bound to a very hydrophobic environment of the enzyme. Further characterization of the static fluorescence spectra provides evidence for energy transfer between Trp residues of the enzyme and DEDO. Distance estimations suggest that one or two Trp residues are likely to be located in the proximity of the fluorophore.     

Dynamics ofLens culinaris agglutinin studied by red-edge excitation spectra and anisotropy measurements of 2-p-toluidinylnaphthalene-6-sulfonate (TNS) and of tryptophan residues

The fluorescence of 2-p-toluidinylnaphthalene-6-sulfonate bound toLens culinaris agglutinin and of the Trp residues of the protein was investigated. Red-edge excitation spectra and steady-state anisotropy as a function of temperature indicate that the TNS is bound rigidly. Red-edge excitation spectra, steady-state anisotropy as a function of sucrose and anisotropy decay experiments performed on Trp residues fluorescence prove that the internal fluorophore presents residual motion independent of the global rotation of the protein. Fluorescence anisotropy decay allows to calculate the rotational correlation time (351 ps) of this local motion. Quenching resolved emission anisotropy with iodide gives values equal to 0.257 and 0.112 for the anisotropies of the buried and the surface Trp residues, respectively. This result indicates that the Trp residues present at the surface of the protein have important local motions compared to those embedded in the protein matrix. The results obtained from TNS and Trp residues indicate that the agglutinin has different dynamic domains.     

n-Si(As):Yb1130nm四能级发光研究

在n-Si(As):Yb中首次观察到1130nm的尖锐发光.通过掺入Yb的剂量与发光强度的关系以及红外吸收、透射光谱的测量,讨论了敏化剂Yb与激活剂As之间能量传递过程.适当选取Yb与As的浓度比可提高发光效率.     

Absorption,excitation and fluorescence spectra of thallium activated cesium bromide

Absorption, excitation and fluorescence spectra of T1⁺ doped cesium bromide have been investigated at various thallium concentrations. At very low thallium concentration two absorption bands are obtained at 225 nm and 264 nm. With rise of thallium concentration additional absorption bands are obtained at 230, 244, 258, 270 and 285 nm. A single bell-shaped fluorescence band at 357 nm in the ultraviolet region is obtained at low thallium concentration. Two additional visible fluorescence bands appear at 440 and 540 nm with rise in thallium content. The excitation spectra for ultraviolet emission band and visible emission bands are found to be different. Accordingly the ultraviolet emission band is attributed to the characteristic A emission in T1⁺ ion and the visible bands are attributed to dimer centers havingD _4h site symmetry.