荧光分析法测定细胞内金属离子

综述了荧光分析法测定细胞内游离金属离子的原理、方法和进展。简要介绍了Ｆｕｒａ－２、Ｍａｇ－Ｆｕｒａ－２,ＳＢＦＩ和ＰＢＦＩ等荧光剂在生命科学研究中分别应用于细胞内Ｃａ＾２＋、Ｍｇ＾２＋、Ｎａ＾＋和Ｋ＾＋等离子的测定。     

铽离子荧光探针对酶与金属离子间能量转移和结合位的研究

应用荧光光度法研究了Ｔｂ＾３＋与牛胰脱氧核糖核酸酶（ＢＰＤ），枯草杆菌α－淀粉酶（ＢＳα－Ａ）的络合发光现象，实验表明，ＢＰＤ和ＢＳα－Ａ分别在ＰＨ＝７－８和５－６范围内与Ｔｂ＾３＋络合，并发射Ｔｂ＾３＋的特征荧光，Ｔｂ＾３＋与ＢＰＤ和ＢＳα－Ａ的络合比分别为２：１和４：１。并应用Ｆｏｒｓｔｅｒ理论测定了Ｔｂ＾３＋与ＢＰＤ和ＢＳα－Ａ之间能量传递的距离Ｒ分别为１．３９ｎｍ和１．４８ｎｍ，其临界距离     

KZnF3：Eu的水热合成及其光谱性质

采用中温水热法合马了立方钙钛矿单相ＫＺｎＦ３及ＫＺｎＦ３：Ｅｕ，通过ＳＥＭ观察了产物形态．ＸＰＳ测定结果表明，产物含氧量不高。荧光光谱及ＥＳＲ谱表明，ＫＺｎＦ３：Ｅｕ体系中Ｅｕ＾２＋与Ｅｕ＾３＋共存，进一步讨论了不等价取代中的电荷补偿途径。     

长白山白眉蝮蛇蛇毒磷脂酶A2的荧光光谱

利用荧光光谱系统研究了长白山白眉蝮蛇蛇毒磷脂酶Ａ２的荧光特性。研究结果表明：当发射波长与激发波长差为２０ｎｍ和７５ｎｍ时,ＰＬＡ２的同步荧光分别主要由酷氨酸（Ｔｙｒ）残基和色氨酸（Ｔｒｐ）残基所贡献。缓冲溶液的酸度变化能够明显影响ＰＬＡ２氨基酸侧链的电荷分布,从而改变ＰＬＡ２的荧光发射强度。了子Ｃａ＾２＋一方面能增强ＰＬＡ２的荧光强度,另一方面也能够加快ＰＬＡ２与底物二棕樟酰磷脂酰胆碱（ＤＰＰＣ）     

超价化合物NLi4^n＋和OLi4^n＋电子结构和性质

以６－３１Ｇ＾＊基组利用ＨＦ、ＭＰ２和ＤＦＴ方法优化了超价化合物ＮＬｉ４＾ｎ＋和ＯＬｉ４＾ｎ－的几何构型。研究结果表明，ＭＰ２和ＤＦＴ法计算出的ＯＬｉ４分子解离出Ｌｉ和Ｌｉ２的反应能与已有的实验值吻合，对于ＮＬｉ４分子，得到其解离出Ｌｉ和Ｌｉ２的反应能分别为１９１．７８和５１５．３７ｋＪ／ｍｏｌ（ＭＰ２值）。并预测了ＯＬｉ４＾ｎ＋和ＮＬｉ４＾ｎ＋分子的基振动频率。     

PtCl^2^—6接着PVP修饰电极及其对Fe^2^＋的催化氧化

研究了ＰｔＣｌ＾２＾－６接着ＰＶＰ修饰电极及其催化动力学，用循环伏安法考察了电极的电化学性质，结果表明在酸性溶液中对Ｆｅ＾２＾＋的氧化有显著的催化作用。采用旋转圆盘电极法，极化曲线法等就电极对Ｆｅ＾２＾＋氧化催化过程的控制步骤及有关动力学参数进行了测定。     

PAN—聚氨酯泡沫塑料富集ICP—AES同时测定天然水中铜锌镉锰…

研究了１－（２－吡啶偶氮）－２－萘酚（ＰＡＮ）在聚氨酯泡沫塑料上的吸附特征，对Ｃｕ＾２＾＋，Ｚｎ＾２＾＋，Ｃｄ＾２＾＋，Ｍｎ＾２＾＋，Ｆｅ＾２＾＋，Ｃｏ＾２＾＋和Ｐｂ＾２＾＋７种离子的吸附性能，以及富集体积，流速，基体元素的影响。建立了ＰＡＮ－聚氨酯泡塑料富集ＩＣＰ－ＡＥＳ同时测定天然水样中上述７种元素的分析方法，获得满意结果。     

卟啉化合物电化学性质研究 Ⅰ.5,10,15,20-四-(4-乙酰氧基苯)卟吩及其Cu、Zn、Fe、Co、Ni配合物的合成及循环伏安研究

本文报道了５，１０，１５，２０－四（４－乙酰氧基苯）卟吩（Ｔ（４ＡＯＰ）Ｐ）及其Ｃｕ，Ｚｎ，Ｆｅ，Ｃｏ，Ｎｉ配合物的合成及其在ＣＨ２Ｃｌ２－０．１ｍｏｌ／ＩＴＢＡＰ体系中的循环伏安（ＣＶ）。研究结果。ＣＶ实验表明：Ｃｕ＾２＾＋，Ｚｎ＾２＾＝，Ｎｉ＾２＾＋离子以稳定的＋２价存在于Ｔ（４ＡＯＰ）Ｐ中，电子转移反应在卟啉环上进行，而Ｆｅ＾３＾＋，Ｃｏ＾２＾＋离子在氧化还原过程中发生价态变化。实验发现...     

Eu^3＋,Bi^3＋Me2Y8（SiO4）6O2中的发光特性与取代格位

在紫外光激发下，Ｅｕ＾３＋和Ｂｉ＾３＋在Ｍｅ２Ｙ８（ＳｉＯ４）６Ｏ２基质（Ｍｅ＝Ｍｇ，Ｚｎ，Ｃａ，Ｓｒ）中分别发射红光（＾５Ｄ０－＾７Ｆ２）和蓝光（＾３Ｐ１－＾１Ｓ０）．Ｅｕ＾３＋发光的红橙比随着激发波长和Ｍｅ＾２＋的不同而变化。荧光拉曼光谱表明，Ｅｕ＾３＋在四种基质中同时占据了４ｆ格位和６ｈ格位。依据Ｂｉ＾３＋发光的Ｓｔｏｋｅｓ位移推断，当Ｍｅ＝Ｃａ，Ｚｎ时，Ｂｉ＾３＋主要占据４ｆ格位，而当Ｍｅ     

单基双掺稀土三基色荧光体系的发光特性

利用Ｅｕ＾３＋和Ｔｆｂ＾３＋对一对三价稀土离子之间电子组态具有共轭性的特征,双掺到同一基质中,由于电子转移,部分Ｅｕ＾３＋转换成Ｅｕ＾２＋,使发红光的Ｅｕ＾３＋、发绿光的Ｔｂ＾３＋和发蓝光的Ｅｕ＾２＋共存于同一体系。在空气气氛中合成了单基双掺稀土三基色荧光粉ＣａＢＰＯ５：Ｅｕ,Ｔｂ,研究了２５４和３６５ｎｍ激发下荧光体的发射特性。在双掺体系中引入Ｃｅ＾３＋,由于Ｃｅ＾３＋的敏化作用增强了Ｅｕ＾２＿     

Fluorescent studies on the binding-Ca2 + in fibrinolytic principle separated from snake venom

By using equilibrium dialysis, atomic absorption spectrometry, fluorescence titration and determination of fluorescence lifetime, it can be determined that each fibrinolytic principle (FP) molecule contains one Ca2+-binding site and one Ca2+ ion, which can be substituted by a Tb3+ ion completely. The intramolecular energy transfer between Tb3+ and the tryptophan (Trp) residue in FP has been investigated through fluorescence spectroscopy. In the FP molecule, the excited energy can transfer from the Trp residue as an energy donor to the Tb3+ ion substituted as an acceptor. The distance between Tb3+ and the Trp residue, approximately 0.38 nm, has been calculated with the experimental data and Forster theory.     

温度对铽（III）-转铁蛋白溶液构象的影响

在pH 7.4,0.01 mol/L N-2-羟乙基哌嗪-N’-2-乙磺酸（Hepes）条件下,铽 （III）与N,N’-二（2-羟苄基）乙二胺-N,N’-二乙酸（HBED）结合并发生交换 相互作用使铽（III）荧光增强10~4倍,通过监测铽（III）545 nm荧光强度的变化 测定了Tb-HBED配合物的条件稳定常数是lgK = 14.30 ± 0.49;Tb-HBED配合物中 配体、铽（III）荧光强度均随着温度的升高而降低。在pH 7.4,0.01 mol/L Hepes条件下,Tb_N-apoTf-Tb_C配合物中蛋白质的荧光强度随着温度的升高而降 低,而能量受体铽（III）的荧光强度随着温度的升高而增强,主要源于铽（III） 与螺旋5色氨酸残基间的无辐射能量转移;当温度由0 ℃上升到55 ℃时,平均能量 转移效率AE值增加了29%,给体、受体间距离R有约4.2%的减小,温度变化引起 Tb_N-apoTf-Tb_C配合物大的构象变化;铽（III）与人血清脱铁转铁蛋白的结合使 蛋白质的变性温度降低。同样条件下,Tb_N-apoOTf-Tb_C配合物与Tb_N-apoTf- Tb_C配合物有所不同,虽然能量给体的荧光强度随着温度的增加而减小,但铽（ III）荧光强度没有明显的增强;铽（III）对蛋白质的变性温度几乎没有影响。     

A tryptophan-containing open-chain framework for tuning a high selectivity for Ca2+ and 13C NMR observation of a Ca2+-indole interaction in aqueous solution

Two molecular architectures featuring the cation-responsive tryptophan indole were designed and investigated for the development of a novel fluorescent chemosensor for Ca2+. We observed that the Trp-based open-framework chemosensor EW2 exhibits remarkable selectivity for Ca2+ over Mg2+, Ba2+, K+, Na+, and Li+ in water between pH 4.6 and 7.0 on the basis of Ca2+-induced high fluorescence enhancement of the Trp residue. A combined 13C NMR and CD spectroscopic study has demonstrated a dynamic reorientation of the indole ring due to the cation-indole interaction accompanying the Ca2+-induced dramatic fluorescence enhancement. The results suggest that the highly sensitive, metal-ion-dependent Trp indolyl C(3) chemical shifts may serve as a promising indicator for monitoring metal ion-indole noncovalent interaction in solution.     

The study of terbium regenerated bacterirhodopsin

Bacteriorhodopsin (bR) is the only retinal-contain- ing protein in the purple membrane of Halobacterium halobium[1]. Upon illumination, the protein undergoes a photocycle and pumps protons across the cell mem-brane[2,3]. It has been found that well-washed…     

Sensitization of lanthanides by nonnatural amino acids

The sensitization of Eu(III) and Tb(III) by ethylenediaminetetraaceticacid (EDTA)-derivatized tryptophan (Trp), 7-azatryptophan (7AW) and 5-hydroxytryptophan (5HW) has been examined. These Trp analogs were utilized in the present study because they can be incorporated into proteins in place of native Trp residues and because they absorb strongly beyond 305 nm (where Trp absorbance goes to zero), allowing selective excitation of such species in the presence of other Trp-containing proteins. All three indole derivatives were able to sensitize Tb(III) luminescence, with the relative sensitization being in the order Trp > 5HW > 7AW. On the other hand, only the 7AW-EDTA complex was able to sensitize Eu(III) luminescence, likely owing to a better spectral overlap between 7AW emission and Eu(III) absorbance. The sensitized emission of Tb(III) and Eu(II) displayed the expected long emission lifetimes at 545 nm [for Tb(III)] and 617 nm [for Eu(III)], indicating that long-lifetime lanthanide emission could be produced using nonnatural amino-acid donors. Thus, 7AW- and 5HW-sensitized lanthanide emissions should prove to be useful in biophysical studies, such as the use of fluorescence energy transfer to probe biomolecular interactions in vivo.     

The characterization for the binding of calcium and terbium to Euplotes octocarinatus centrin

Centrin is a member of the EF-hand superfamily that plays critical role in the centrosome duplication and separation. In the present paper, we characterized properties of metal ions binding to Euplotes octocarinatus centrin (EoCen) by fluorescence spectra and circular dichroism (CD) spectra. Changes of fluorescence spectra and alpha-helix contents of EoCen proved that Tb(3+) and Ca(2+) induced great conformational changes of EoCen resulting in exposing hydrophobic surfaces. At pH 7.4, Ca(2+) (and Tb(3+)) bond with EoCen at the ratio of 4:1. Equilibrium experiment indicated that Ca(2+) and Tb(3+) exhibited different binding capabilities for C- and N-terminal domains of protein. C-terminal domain bond with Ca(2+) or Tb(3+) approximately 100-fold more strongly than N-terminal. Aromatic residue-sensitized Tb(3+) energy transfer suggested that site IV bond to Tb(3+) or Ca(2+) more strongly than site III. Based on fluorescence titration curves, we reckoned the conditional binding constants of EoCen site IV quantitatively to be K(IV)=(1.23+/-0.51)x10(8)M(-1) and K(IV)=(6.82+/-0.33)x10(5)M(-1) with Tb(3+) and Ca(2+), respectively. Metal ions bond to EoCen in the order of IV>III>II, I.     

Two-dimensional fluorescence correlation spectroscopy IV: resolution of fluorescence of tryptophan residues in alcohol dehydrogenase and lysozyme

Generalized two-dimensional (2D) fluorescence correlation spectroscopy has been used to resolve the fluorescence spectra of two tryptophan (Trp) residues in alcohol dehydrogenase and lysozyme. In each protein, one Trp residue is buried in a hydrophobic domain of the protein matrix and the other Trp residue is located at a hydrophilic domain close to the protein-water interface. Fluorescence quenching by iodide ion, a hydrophilic quencher, was employed as a perturbation to induce the intensity change in the spectra. The Trp residue which is located at the hydrophilic domain is effectively quenched by the quencher, while the Trp residue located at the hydrophobic domain is protected from the quenching. Therefore, the fluorescence of these two Trp residues have a different sensitivity to the quenching, showing a different response to the concentration of the quencher. Fluorescence spectra of the two Trp residues in alcohol dehydrogenase, which are heavily overlapped in conventional one-dimensional spectra, have been successfully resolved by the 2D correlation technique. From the asynchronous correlation map, it was revealed that the quenching of Trp located at the hydrophobic part was brought about after that of Trp located at the hydrophilic part. In contrast, the fluorescence spectra of the two Trp residues could not be resolved after the alcohol dehydrogenase was denatured with guanidine hydrochloride. These results are consistent with the well-known structure of alcohol dehydrogenase. Furthermore, it was elucidated that the present 2D analysis is not interfered by Raman bands of the solvent, which sometimes bring difficulty into the conventional fluorescence analysis. Fluorescence spectra of the Trp residues in lysozyme could not be resolved by the 2D correlation technique. The differences between the two proteins are attributed to the fact that the Trp residue in the hydrophobic site of lysozyme is not sufficiently protected from the quenching.     

Tb3+离子与植物辣根过氧化物酶的作用方式探讨

利用紫外可见吸收光谱、红外光谱、荧光光谱、原子吸收及酶分离方法,首次研究了稀土离子Tb^3 与植物辣根过氧化物酶(HRP)的相互作用方式．结果表明,Tb^3 与HRP作用方式包括：(1)Tb^3 与肽链上的氨基酸残基作用,影响酶活性中心的微结构;(2)Tb^3 能部分取代酶中的Ca^2 ;(3)Tb^3 能部分剪切肽链上的氨基酸残基,改变酶的结构。因此,Tb^3 与HRP的相互作用可能以一种方式为主,或几种作用方式同时存在。     

尖吻蝮蛇毒抗凝血因子Ⅱ的稀土离子荧光探针研究

尖吻蝮蛇毒抗凝血因子(ACF)分子中有两个钙离子结合位点,钙离子对ACF的内源荧光有增强作用,稀土离子(Nd³⁺,Sm³⁺,Eu³⁺,Gd³⁺和Tb³⁺)能取代ACF分子中的钙离子,并对ACF的内源荧光有不同程度的猝灭作用,其中Tb³⁺接受ACF分子中Trp残基传递的能量后,特征荧光增强.稀土离子与ACF荧光滴定表明,ACF分子中有两个稀土离子结合位点,稀土离子和钙离子在ACF分子中两个结合部位是共同的竞争结合部位.ACF与不同稀土离子之间有相近的表观结合常数K₁或K₂.Tb³⁺与RE³⁺(RE=Nd,Sm,Eu或Gd)间线性自由能关系表明,稀土离子与ACF结合时,没有明显的空间效应.ACF分子中的两个结合位点在结构上都有较大的柔性,这种结构柔性为钙离子在ACF与活化凝血因子X的结合反应中起到的促进作用提供了结构基础.     

The quantum cutting of Tb(3+) in Ca(6)Ln(2)Na(2)(PO(4))(6)F(2) (Ln = Gd, La) under VUV-UV excitation: with and without Gd(3+)

The VUV-vis spectroscopic properties of Tb(3+) activated fluoro-apatite phosphors Ca(6)Ln(2-x)Tb(x)Na(2)(PO(4))(6)F(2) (Ln = Gd, La) were studied. The results show that phosphors Ca(6)Gd(2-x)Tb(x)Na(2)(PO(4))(6)F(2) with Gd(3+) ions as sensitizers have intense absorption in the VUV range. The emission color of both phosphors can be tuned from blue to green by changing the doping concentration of Tb(3+) under 172 nm excitation. The visible quantum cutting (QC) via cross relaxation between Tb(3+) ions was observed in cases with and without Gd(3+). Though QC can be realized in phosphors Ca(6)La(2-x)Tb(x)Na(2)(PO(4))(6)F(2), we found that Gd(3+)-containg phosphors have a higher QC efficiency, confirming that the Gd(3+) ion indeed plays an important role during the quantum cutting process. In addition, the energy transfer process from Gd(3+) to Tb(3+) as well as (5)D(3)-(5)D(4) cross relaxation was investigated and discussed in terms of luminescence spectra and decay curves.