Molecular dynamics study on the interaction of a mithramycin dimer with a decanucleotide duplex

The complex of a minor groove binding drug mithramycin (MTR) and the self-complementary d(TAGCTAGCTA) 10-mer duplex was investigated by molecular dynamics (MD) simulations using the AMBER 7.0 suite of programs. There is one disaccharide and trisaccharide segment projecting from opposite ends of an aglycone chromophore of MTR. A MTR dimer complex (MTR)2Mg2+ is formed in the presence of a coordinated ion Mg2+. A NMR solution structure of two (MTR)2Mg2+ complexes bound with one DNA duplex, namely, the 2:1 duplex complex, was taken as the starting structure for the MD simulation. The partial charge on each atom was calculated using the multiple-RESP fitting procedure, and all of the missing parameters in the Parm99 force field used were adapted comparably from the literature. The length of the MD simulation was 5 ns, and the binding free energy for the formation of a 1:1 or 2:1 duplex complex was determined from the last 4 ns of the simulation. The binding free energies were decomposed to components of the contributions from different energy types, and the changes in the helical parameters of the bound DNA duplex plus the glycosidic linkages between sugar residues of the bound MTR dimer were determined. It was found that binding of the first (MTR)2Mg2+ complex with the DNA duplex to form a 1:1 duplex complex does not cause stiffening of the duplex especially in the unoccupied site of the duplex. However, the overall flexibility of the DNA duplex is reduced substantially once the second (MTR)2Mg2+ complex is bound with the unoccupied site to form the 2:1 duplex complex. The van der Waals interactions were found to be dominant in the central part of the DNA duplex where sugar residues from each bound (MTR)2Mg2+ complex were inwardly pointing and the corresponding minor groove was widened.     

Direct observation of substrate-enzyme complexation by surface forces measurement

The substrate-enzyme complexation of heptaprenyl diphosphate synthase was directly investigated using colloidal probe atomic force microscopy (AFM) and a quartz crystal microbalance (QCM) in order to obtain new insights into the molecular mechanism of the enzyme reaction. This enzyme is composed of two dissociable subunits that exhibit a catalytic activity only when they are associated together in the presence of a cofactor, Mg2+, and a substrate, farnesyl diphosphate (FPP). The QCM measurement revealed that FPP was preferentially bound to subunit II in the presence of Mg2+, while the AFM measurement showed that the adhesive force between the subunits was observed only in the presence of both Mg2+ and FPP. This is the first direct demonstration of the specific interaction involved in the enzyme reaction. The dependence of the Mg2+ concentration on the specific interaction between subunits I and II well agreed with that on the enzyme activity of heptaprenyl diphosphate synthase. This indicated that the observed adhesive forces were indeed involved in the catalytic reaction of this enzyme. On the basis of these results, we discussed the processes involved in the substrate-enzyme complexation. The first, the substrate FPP bound to subunit II using Mg2+, followed by the formation of the subunit I-FPP-Mg2+-subunit II complex. Our study showed a very useful methodology for examining the elemental processes of biological reactions such as an enzyme reaction.     

OFF-OFF-ON switching of fluorescence and electron transfer depending on stepwise complex formation of a host ligand with guest metal ions

Stepwise complex formation is observed between 2,3,5,6-tetrakis(2-pyridyl)pyrazine (TPPZ) and a series of metal ions (M(n+) = Sc3+, Y3+, Ho3+, Eu3+, Lu3+, Nd3+, Zn2+, Mg2+, Ca2+, Ba2+, Sr2+, Li+), where TPPZ forms a 2:1 complex [(TPPZ)2-M(n+)] and a 1:1 complex [TPPZ-M(n+)] with Mn+ at low and high concentrations of metal ions, respectively. The fluorescence intensity of TPPZ begins to increase at high concentrations of metal ions, when the 2:1 (TPPZ)2-M(n+) complex is converted to the fluorescent 1:1 TPPZ-M(n+) complex. This is regarded as an "OFF-OFF-ON" fluorescence sensor for metal ions depending on the stepwise complex formation between TPPZ and metal ions. The fluorescence quantum yields of the TPPZ-M(n+) complex vary depending on the metal valence state, in which the fluorescence quantum yields of the divalent metal complexes (TPPZ-M2+) are much larger than those of the trivalent metal complexes (TPPZ-M3+). On the other hand, the binding constants of (TPPZ)2-M(n+) (K1) and TPPZ-M(n+) (K2) vary depending on the Lewis acidity of metal ions (i.e., both K1 and K2 values increase with increasing Lewis acidity of metal ions). Sc3+, which acts as the strongest Lewis acid, forms the (TPPZ)2-Sc3+ and TPPZ-Sc3+ complexes stoichiometrically with TPPZ. In such a case, "OFF-OFF-ON" switching of electron transfer from cobalt(II) tetraphenylporphyrin (CoTPP) to O2 is observed in the presence of Sc3+ and TPPZ depending on the ratio of Sc3+ to TPPZ. Electron transfer from CoTPP to O2 occurs at Sc3+ concentrations above the 1:2 ratio ([Sc3+]/[TPPZ]0 > 0.5), when the (TPPZ)2-Sc3+ complex is converted to the TPPZ-Sc3+ complex and TPPZ-(Sc3+)2, which act as promoters of electron transfer (ON) by the strong binding of O2*- with Sc3+. In sharp contrast, no electron transfer occurs without metal ion (OFF) or in the presence at Sc3+ concentrations below the 1:2 ratio (OFF), when the (TPPZ)2-Sc3+ complex has no binding site available for O2*-.     

Binding studies of nNOS-active amphibian peptides and Ca2+ calmodulin, using negative ion electrospray ionisation mass spectrometry

Amphibian peptides which inhibit the formation of nitric oxide by neuronal nitric oxide synthase (nNOS) do so by binding to the protein cofactor, Ca2+calmodulin (Ca2+CaM). Complex formation between active peptides and Ca2+CaM has been demonstrated by negative ion electrospray ionisation mass spectrometry using an aqueous ammonium acetate buffer system. In all cases studied, the assemblies are formed with a 1:1:4 calmodulin/peptide/Ca2+ stoichiometry. In contrast, the complex involving the 20-residue binding domain of the plasma Ca2+ pump C20W (LRRGQILWFRGLNRIQTQIK-OH) with CaM has been shown by previous two-dimensional nuclear magnetic resonance (2D NMR) studies to involve complexation of the C-terminal end of CaM. Under identical conditions to those used for the amphibian peptide study, the ESI complex between C20W and CaM shows specific 1:1:2 stoichiometry. Since complex formation with the studied amphibian peptides requires Ca2+CaM to contain its full complement of four Ca2+ ions, this indicates that the amphibian peptides require both ends of the CaM to effect complex formation. Charge-state analysis and an H/D exchange experiment (with caerin 1.8) suggest that complexation involves Ca2+CaM undergoing a conformational change to a more compact structure.     

A new model for magnesium chemistry in the upper atmosphere

This paper describes the kinetic study of a number of gas-phase reactions involving neutral Mg-containing species, which are important for the chemistry of meteor-ablated magnesium in the upper mesosphere/lower thermosphere region. The study is motivated by the very recent observation of the global atomic Mg layer around 90 km, using satellite-born UV-visible spectroscopy. In the laboratory, Mg atoms were produced thermally in the upstream section of a fast flow tube and then converted to the molecular species MgO, MgO(2), OMgO(2), and MgCO(3) by the addition of appropriate reagents. Atomic O was added further downstream, and Mg was detected at the downstream end of the flow tube by laser-induced fluorescence. The following rate coefficients were determined at 300 K: k(MgO + O → Mg + O(2)) = (6.2 ± 1.1) × 10(-10); k(MgO(2) + O → MgO + O(2)) = (8.4 ± 2.8) × 10(-11); k(MgCO(3) + O → MgO(2) + CO(2)) ≥ 4.9 × 10(-12); and k(MgO + CO → Mg + CO(2)) = (1.1 ± 0.3) × 10(-11) cm(3) molecule(-1) s(-1). Electronic structure calculations of the relevant potential energy surfaces combined with RRKM theory were performed to interpret the experimental results and also to explore the likely reaction pathways that convert MgCO(3) and OMgO(2) into long-lived reservoir species such as Mg(OH)(2). Although no reaction was observed in the laboratory between OMgO(2) and O, this is most likely due to the rapid recombination of O(2) with the product MgO(2) to form the relatively stable O(2)MgO(2). Indeed, one significant finding is the role of O(2) in the mesosphere, where it initiates holding cycles by recombining with radical species such as MgO(2) and MgOH. A new atmospheric model was then constructed which combines these results together with recent work on magnesium ion-molecule chemistry. The model is able to reproduce satisfactorily some of the key features of the Mg and Mg(+) layers, including the heights of the layers, the seasonal variations of their column abundances, and the unusually large Mg(+)/Mg ratio.     

Crystal and electronic structures of magnesium(II), copper(II), and mixed magnesium(II)-copper(II) complexes of the quinoline half of styrylquinoline-type HIV-1 integrase inhibitors

A new target in AIDS therapy development is HIV-1 integrase (IN). It was proven that HIV-1 IN required divalent metal cations to achieve phosphodiester bond cleavage of DNA. Accordingly, all newly investigated potent IN inhibitors contain chemical fragments possessing a high ability to chelate metal cations. One of the promising leads in the polyhydroxylated styrylquinolines (SQLs) series is (E)-8-hydroxy-2-[2-(4,5-dihydroxy-3-methoxyphenyl)-ethenyl]-7-quinoline carboxylic acid (1). The present study focuses on the quinoline-based progenitor (2), which is actually the most probable chelating part of SQLs. Conventional and synchrotron low-temperature X-ray crystallographic studies were used to investigate the chelating power of progenitor 2. Mg2+ and Cu2+ cations were selected for this purpose, and three types of metal complexes of 2 were obtained: Mg(II) complex (4), Cu(II) complex (5) and mixed Mg(II)-Cu(II) complexes (6 and 7). The analysis of the crystal structure of complex 4 indicates that two tridentate ligands coordinate two Mg2+ cations, both in octahedral geometry. The Mg-Mg distance was found equal to 3.221(1) A, in agreement with the metal-metal distance of 3.9 A encountered in the crystal structure of Escherichia coli DNA polymerase I. In 5, the complex is formed by two bidentate ligands coordinating one copper ion in tetrahedral geometry. Both mixed Mg(II)-Cu(II) complexes, 6 and 7 exhibit an original arrangement of four ligands linked to a central heterometallic cluster consisting of three octahedrally coordinated magnesium ions and one tetrahedrally coordinated copper ion. Quantum mechanics calculations were also carried out in order to display the electrostatic potential generated by the dianionic ligand 2 and complex 4 and to quantify the binding energy (BE) during the formation of the magnesium complex of progenitor 2. A comparison of the binding energies of two hypothetical monometallic Mg(II) complexes with that found in the bimetallic magnesium complex 4 was made.     

Study of beta-lactoglobulin/acacia gum complex coacervation by diffusing-wave spectroscopy and confocal scanning laser microscopy

Complex coacervation has been investigated on mixtures of beta-lactoglobulin (beta-lg) and acacia gum (AG) at pH 4.2 where these two macromolecules interact electrostatically. Changes in beta-lg/AG complex coacervation induced by the presence of beta-lg aggregates were considered. The nature and structure of particles resulting from complex coacervation were determined by using confocal scanning laser microscopy (CSLM). CSLM revealed fundamental differences in the structure of each of the studied dispersions (at 1 wt.% total concentration). Spherical vesicular coacervates and precipitates (based on beta-lg aggregates) were the hallmark of BLG/AG dispersions (beta-lg dispersion containing insoluble aggregates). Only coacervates were visible in AF-BLG/AG dispersions (beta-lg dispersion free of insoluble aggregates). The latter were characterised by the presence of large foam-like coacervates induced by partial coalescence of single coacervates, especially at the 2:1 protein to polysaccharide (Pr:Ps) ratio. Diffusing wave spectroscopy (DWS) was used to study the stability of dispersions as a function of time. Depending on the Pr:Ps ratio and the presence of beta-lg aggregates, the intensity correlation function (g(2)(t)) shifted to lower correlation times rapidly after mixing of both macromolecules. This revealed the formation of a large number of small particles, characterised by faster Brownian motion. At 1 and 5 wt.% total concentration, the 8:1 Pr:Ps ratio exhibited a rapid decrease of the backscattered intensity in time, both for BLG/AG and AF-BLG/AG mixtures, revealing rapid sedimentation/coalescence of particles. This precluded the achievement of a stable correlation function. For the 2:1 Pr:Ps ratio, mixtures exhibited both coalescence and sedimentation phenomena as confirmed by shifts in the g(2)(t) towards larger correlation times and the decrease of the initial value of g(2)(t) with time. Mixtures obtained for the 1:1 Pr:Ps ratio were characterised by small variations in the DWS signal, emphasising the stability of produced particles. The increase of the total biopolymer concentration reduced the effect of both Pr:Ps ratio and presence of protein aggregates. From CSLM and DWS observations, possible differences in the complex coacervation mechanism in both types of mixtures were highlighted. The use of protein aggregates to control complex coacervation was underlined.     

Fourier transform infrared study of low-temperature CO adsorption on CuMgAl-hydrotalcite

Single-phase CuMgAl ternary hydrotalcite with (Cu+Mg)/Al atomic ratio of 3.0 and Cu/Mg atomic ratio of 1.0 was synthesized by coprecipitation. Thermoanalytical studies of this sample showed transformations in three stages in the temperature range up to ca. 900 K yielding mainly CuO phase. In situ diffuse reflectance infrared Fourier transform (DRIFT) spectroscopic measurements showed the presence of carbonates even after calcination of the sample at 973 K. The genesis of Cu+ sites during thermal treatment in vacuo at different temperatures for this sample was followed by IR spectroscopy of CO adsorbed at low temperature. Essentially no Cu+ sites are present on a sample calcined at 723 K, consistent with X-ray photoelectron spectroscopic (XPS) data. However, sample subjected to activation (1 h of O2 treatment at 723 K followed by 1 h of evacuation at the same temperature) upon CO adsorption at 85 K unambiguously showed the presence of Cu+ sites. 12CO-13CO coadsorption studies confirmed the presence of dicarbonyls, which are converted to linear Cu+-CO species during evacuation at 85 K. Concentration of the accessible Cu+ sites increased with the increase in activation temperature up to 873 K and decreased with a further temperature rise. The copper sites on the sample are heterogeneously distributed and their distribution depends on the activation temperature. Two routes of reduction of Cu2+ to Cu+ are proposed: (i) autoreduction during evacuation and (ii) reduction by CO.     

Single molecular multianalyte (Ca2+, Mg2+) fluorescent probe and applications to bioimaging

Intracellular signal transduction relies on spatial and temporal signal transmitter dynamics. To clarify the correlations of these transmitter molecules, multicolor-imaging has been widely used. However, in the case of applying multiple indicators in a cell, spectral overlap of the indicators prevents accurate quantitative analysis. Moreover, the invasive (toxic) effect, the localization, the metabolism, as well as photobleaching of these indicators complicate the situation. Here, we show that single-molecular multifluorescent probes can overcome these problems. While intracellular calcium plays a critical role as a signal transmitter and magnesium acts as a cofactor in many situations, the correlations between the two cations are now the main issue. We designed and synthesized a Ca2+-Mg2+ responsive multifluorescent probe, KCM-1. KCM-1 shows a spectral blue shift upon complexation to Ca2+ and a red shift to the presence of Mg2+. With data analyzed at different excitation wavelengths, the concentrations of Ca2+ and Mg2+ are simultaneously quantified. Furthermore, by using the AM-ester method, intracellular Ca2+ and Mg2+ concentrations are simultaneously imaged. Such a type of intracellular multiple analyte imaging by a single-molecular multifluorescent probe is successfully demonstrated for the first time.     

用分子对接方法预测HIV-1整合酶与金精三羧酸抑制剂的相互作用

用分子对接方法(Docking)研究了HIV-1整合酶与其抑制剂金精三羧酸的结合过程.为弄清金属离子在结合中所起的作用,选择含有一个Mg+2或不含Mg+2的两种不同的整合酶受体分别与金精三羧酸对接.结果表明, Mg+2对稳定配体与受体的结合起了重要作用. 金精三羧酸配体与含有一个金属Mg+2的整合酶受体对接,最优结合自由能为-45.19 kJ/mol. 当Mg+2失去后,整合酶的活性中心构象将发生变化,使金精三羧酸抑制剂与整合酶的结合自由能(-24.35 kJ/mol)明显增加. 预测了未知的HIV-1整合酶与其抑制剂金精三羧酸的复合物结构, 并可对基于结构的抗HIV-1整合酶的药物设计提供重要信息.     

Comparative studies of the photoinduced reactions in the Mg+-SCNC2H5 and Mg+-NCSC2H5 complexes

The photoinduced reactions of the complexes Mg+-SCNC2H5 and Mg+-NCSC2H5 are studied comparatively in the spectral range of 230-440 nm. One-photon excitation of the complexes through the Mg+ chromophore (3 2P <-- 3 2S) gives rise to the evaporative fragment as well as the molecular activation and charge transfer products. The action spectra of the complexes consist of three broad peaks for Mg+-SCNC2H5 and two for Mg+-NCSC2H5, which accord with the structures obtained from quantum mechanics calculations. These calculations reveal two association isomers for Mg+-SCNC2H5: one is with Mg+ being linked to the S atom and the other to the N atom. The former is more stable than the latter by only 0.23 eV. Both of the isomers have been shown to exist in the complex source employed in our experiments. On the other hand, only one stable structure is found for the complex Mg+-NCSC2H5 characterized by the Mg+-N linkage. In general, the photofragments are dominated by Mg+ at lambda > 400 nm, which decreases with decreasing wavelength accompanied by the increase in other photoproducts. In addition, the branching ratios of Mg+ to other photoproducts are nearly constant in the short wavelength region but decrease with decreasing wavelength. The observed photoreactions have been reasonably explained.     

Properties of (Mg2 + Ca2+)-ATPase of erythrocyte membranes prepared by different procedures: influence of Mg2+, Ca2+, ATP, and protein activator.

Erythrocyte membranes prepared by three different procedures showed (Mg2+ + Ca2+)-ATPase activities differing in specific activity and in affinity for Ca2+. The (Mg2+ + Ca2+)-ATPase activity of the three preparations was stimulated to different extents by a Ca2+-dependent protein activator isolated from hemolysates. The Ca2+ affinity of the two most active preparations was decreased as the ATP concentration in the assay medium was increased. Lowering the ATP concentration from 2 mM to 2-200 microM or lowering the Mg:ATP ratio to less than one shifted the (Mg2+ + Ca2+)-ATPase activity in stepwise hemolysis membranes from mixed "high" and "low" affinity to a single high Ca2+ affinity. Membranes from which soluble proteins were extracted by EDTA (0.1 mM) in low ionic strength, or membranes prepared by the EDTA (1-10 mM) procedure, did not undergo the shift in the Ca2+ affinity with changes in ATP and MgCl2 concentrations. The EDTA-wash membranes were only weakly activated by the protein activator. It is suggested that the differences in properties of the (Mg2+ + Ca2+)-ATPase prepared by these three procedures reflect differences determined in part by the degree of association of the membrane with a soluble protein activator and changes in the state of the enzyme to a less activatable form.     

大环双核Zn(Ⅱ)配合物的合成与结构表征

在Zn²⁺的存在下,2,6-二甲酰基对氟苯酚和1,4-丁二胺通过环缩合反应,合成了一种对称的大环双核锌配合物：[Zn₂L¹(μ-OAc)]ClO₄·0.5CH₃OH。通过远红外、紫外、二维核磁、电喷雾质谱和荧光等研究了配合物的结构。并用X-射线晶体衍射测定了配合物的结构。晶体结构表明,在一个不对称的单元中含2个化学组成相同、分子结构基本相似的大环配合物阳离子A和B。每个大环中的锌离子都处于扭曲的四面体中,且由2个酚氧桥相连。配合物的三维结构由配合物中的非经典氢键构成。     

Photodissociation of Mg+-XCH3 (X=F, Cl, Br, and I) complexes. II. Fragment angular and energy distributions

Angular and energy distributions of photofragments from Mg+-XCH3 (X=F, Cl, Br, and I) were deduced from time-of-flight (TOF) profiles measured by rotating the polarization direction of the dissociation laser with respect to ion beam direction. The TOF profiles of ICH3+ and MgI+ fragment ions produced from Mg+-ICH3 complex with 266 and 355 nm photons showed clear but opposite recoil anisotropy to each other. In addition, BrCH3+ formed by a dissociation of the Mg+-BrCH3 complex at a photolysis wavelength of 266 nm also showed an anisotropic distribution in the TOF profile which had the same behavior as the profile of ICH3+. For Mg+-FCH3 complex, CH3+ and MgF+ formed with a 266 nm photon had also spatial anisotropy, in which the TOF profile of MgF+ was almost opposite to that of MgI+. These anisotropic distributions were explained by (1) local excitation on the Mg+ ion, (2) rapid dissociation compared with a rotational period of the parent complex, and (3) geometrical structures of the parent complexes. Anisotropy beta parameter values were determined to be +1.30(ICH3+), -0.50(MgI+), +0.74(BrCH3+), and +0.75(CH3+ and MgF+). This dependence on the halogen atom observed in beta values was qualitatively explained by both the geometrical parameters and classical rotational periods of parent complexes. In the product energy distribution, 46%, 40%, 21%, 16%, and 16% of available energies were found to be transferred into translational energies of ICH3+, MgI+, BrCH3 +, CH3+, and MgF+, respectively. These values were compared with energy distributions estimated by a statistical prior distribution and a nonstatistical impulsive model. For ICH3+ and MgI+, the translational energies determined from the measurement had values between those estimated from statistical and nonstatistical models. On the other hand, the energy partitioning for the product ions of BrCH3+, CH3+, and MgF+ was found to be almost statistical. From these considerations, we concluded that nonstatistical processes were more important in the dissociation of Mg+-ICH3 than in other systems.     

Speciation of cyclo(Pro-Gly)<Subscript>3</Subscript> and its divalent metal-ion complexes by electrospray ionization mass spectrometry

Electrospray ionization mass spectrometry (ESI-MS) was used to study the binding of selected group II and divalent transition-metal ions by cyclo(Pro-Gly)3 (CPG3), a model ion carrier peptide. Metal salts (CatXn) were combined with the peptide (M) at a molar ratio of 1:10 M/Cat in aqueous solvents containing 50% vol/vol acetonitrile or methanol and 1 or 10 mM ammonium acetate (NH4Ac). Species detected include [M+H]+, [M+Cat-H]+, [M2+Cat]2+, [M+Cat+Ac]+, and [M+Cat+X]+. The relative stabilities of complexes formed with different cations (Mg2+, Ca2+, Sr2+, Mn2+, Co2+, Ni2+, Cu2+, and Zn2+) were determined from the abundance of 1:1 and 2:1 M/Cat species relative to that of the unbound peptide. The largest metal ions (Ca2+, Sr2+, and Mn2+) formed the most stable complexes. Reducing the buffer concentration increased the overall extent of metal binding. Results show that the binding specificity of CPG3 depends upon the size of the metal ion and its propensity for electrostatic interaction with oxygen atoms. Product ion tandem mass spectrometry of [M+H]+ and [M+Cu-H]+ confirmed the cyclic structure of the peptide, although the initial site(s) of metal attachment could not be determined.     

Layered Double Hydroxides with Hydrotalcite—type Structure Containing Fe^3＋,Al^3＋ and Mg^2＋

IntroductionLayered double hydroxides( LDHs) with hy-drotalcite ( HT ) - type structure are composed oftrivalent and divalent metal ions and have the gen-eral formula[1] ,[M2 + 1-x M3 + x ( OH) 2 ]x+ An-x/ n· m H2 O,where M3 + is a trivalentmental ion,such as Al3 + ,Fe3 + ,La3 + ,Ni3 + ,Mn3 + etc.,M2 + is a divalentmetal ion,such as Mg2 + ,Zn2 + ,Ca2 + ,Cu2 + ,Co2 +etc.,An-is a charge compensating anion,such asOH-,Cl-,NO-3 ,CO2 -3 etc.,m is the number ofthe moles of co- intercalat…     

苝醌/富勒烯C60超分子与电子给体的电子转移作用

利用紫外-可见吸收光谱、瞬态吸收光谱及X射线衍射等方法研究了苝醌染料竹红菌素镁离子配合物(Mg2+-HA)与富勒烯C60的相互作用. 结果表明, Mg2+-HA与C60在溶液和固体状态下都能够形成稳定的超分子. Mg2+-HA存在条件下, C60能够溶于多种极性溶剂, 在二甲基亚砜(DMSO)中的溶解度能够达到1×10^-4 mol·L^-1. 作为超分子体系中的光捕获分子, Mg2+-HA能显著地提高C60与N,N-二甲基苯胺(DMA)的光诱导电子转移反应效率, 生成的C60负离子自由基的电子自旋共振光谱(ESR)信号强度比未加入Mg2+-HA时增强了9倍左右.     

两个异双核稀土席夫碱配合物的结构和荧光性质

采用模板法合成了2个异双核三价稀土席夫碱配合物: {[Ce_1.5Sm_0.5(clapi)]₂}·2CH₃CN(1)和{[La_1.5Sm_0.5(clapi)]₂}·2CH₃CN(2). 通过元素分析和红外光谱对这两个配合物进行了表征. 测定了配合物1的晶体结构, 结果表明配合物1属于三斜晶系, P1空间群. 晶胞参数: a=1.067056(2) nm, b=1.14700(3) nm, c=1.38734(3) nm, α=109.4240(10)°, β=98.0520(10)°, γ=105.8050(10)°, Z=1, D_c=1.650 Mg/m³, F(000)=740, R₁=0.0582, wR₂=0.1184[I>2σ(I)]. 研究了配合物1和2在CH₂Cl₂中的室温荧光性质, 2个配合物都显示了Sm³⁺较弱的红色荧光, 研究结果证明荧光惰性稀土离子能够影响稀土配合物的荧光性质.     

Effect of metal ions (Li+, Na+, K+, Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+) and water coordination on the structure of glycine and zwitterionic glycine

Interactions between metal ions and amino acids are common both in solution and in the gas phase. Here, the effect of metal ions and water on the structure of glycine is examined. The effect of metal ions (Li+, Na+, K+, Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+) and water on structures of Gly.Mn+(H2O)m and GlyZwitt.Mn+(H2O)m (m = 0, 2, 5) complexes have been determined theoretically by employing the hybrid B3LYP exchange-correlation functional and using extended basis sets. Selected calculations were carried out also by means of CBS-QB3 model chemistry. The interaction enthalpies, entropies, and Gibbs energies of eight complexes Gly.Mn+ (Mn+ = Li+, Na+, K+, Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+) were determined at the B3LYP density functional level of theory. The computed Gibbs energies DeltaG degrees are negative and span a rather broad energy interval (from -90 to -1100 kJ mol(-1)), meaning that the ions studied form strong complexes. The largest interaction Gibbs energy (-1076 kJ mol(-1)) was computed for the NiGly2+ complex. Calculations of the molecular structure and relative stability of the Gly.Mn+(H2O)m and GlyZwitt.Mn+(H2O)m (Mn+ = Li+, Na+, K+, Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+; m = 0, 2, and 5) systems indicate that in the complexes with monovalent metal cations the most stable species are the NO coordinated metal cations in non-zwitterionic glycine. Divalent cations Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+ prefer coordination via the OO bifurcated bonds of the zwitterionic glycine. Stepwise addition of two and five water molecules leads to considerable changes in the relative stability of the hydrated species. Addition of two water molecules at the metal ion in both Gly.Mn+ and GlyZwitt.Mn+ complexes reduces the relative stability of metallic complexes of glycine. For Mn+ = Li+ or Na+, the addition of five water molecules does not change the relative order of stability. In the Gly.K+ complex, the solvation shell of water molecules around K+ ion has, because of the larger size of the potassium cation, a different structure with a reduced number of hydrogen-bonded contacts. This results in a net preference (by 10.3 kJ mol(-1)) of the GlyZwitt.K+H2O5 system. Addition of five water molecules to the glycine complexes containing divalent cations Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+ results in a net preference for non-zwitterionic glycine species. The computed relative Gibbs energies are quite high (-10 to -38 kJ mol(-1)), and the NO coordination is preferred in the Gly.Mn+(H2O)5 (Mn+ = Mg2+, Ca2+, Ni2+, Cu2+, and Zn2+) complexes over the OO coordination.     

NMR evidence for Mg(II) binding to N1 of ATP

The conformation of the complex of [ATP-Mg]2+ is studied by 1H, 15N and 31P NMR on ATP in the absence and presence of MgCl2 in a wide pH range from 1 to 10. 1H-15N HMBC experiments show a large change in the 15N chemical shift of N1 up to 10 ppm around pH 3.7, suggesting that there is a strong interaction between Mg2+ and N1 of ATP at this pH. 31P NMR indicates that at pH 3.7 the phosphate chain also binds Mg2+. 1H diffusion measurements imply that the [ATP-Mg]2+ complex involves only one ligand and one metal ion.