Ce^3＋和Eu^2＋共激活氯硅酸锌钙的光谱和敏化特性

合成了Ｃｅ＾３＋和Ｅｕ＾２＋共激活的氯硅酸锌钙「Ｃａ８Ｚｎ（ＳｉＯ４）４Ｃｌ２：Ｃｅ＾３＋，Ｅｕ＾２＋」绿色荧光粉，并报道了它们的漫反射光谱，激光发光谱及发射光谱，观测到氯硅酸锌钙中Ｃｅ＾３＋对Ｅｕ＾２＋离子发光的显著敏化现象。阐述了氯硅酸锌钙中Ｃｅ＾３＋和Ｅｕ＾２＋发光作用缘于Ｃｅ＾３＋和Ｅｕ＾２＋之间的高效无辐一传递。     

铕对决明发根生长及有效成分生成的作用

以决明发根为材料,在培养基中附加０．００１～１０ｍｇ．Ｌ＾－１Ｅｕ＾３＋（ＥｕＣ１３）,测量发根的鲜重和干重,用高效液相色谱法测定游离蒽醌化合物含量。发有低剂量（０．００１,０．０１,１．０ｍｇ．Ｌ＾－１）Ｅｕ＾３＋抑制生长,０．００１ｍｇ．Ｌ＾－１Ｅｕ＾３＋抑制作用最强,干重比对照降低２２％;较低剂量（１０ｍｇ．Ｌ＾－１）Ｅｕ＾３＋处理的含量高于对照２６＾,高于Ｅｕ＾３＋１．０ｍｇ．Ｌ＾－１处理     

氟化镁锶中铕和铽的电荷迁移及其平衡解析

在氩气氛中，合成子ＳｒＭｇＦ４：ｘＥｕ，ｙＴｂ复合氟化物磷光体，该体系中Ｅｕ＾３＋和Ｅｕ＾２＋共存，随共掺入Ｔｂ浓度的增加，Ｅｕ＾３＋的荧光发射强度降低，Ｅｕ＾３＋的发光增强，并且Ｅｕ＾２＋的ＥＳＲ信号增强，认为Ｅｕ＾３＋和Ｔｂ３＋之间存在的电荷迁移，即Ｅｕ＾３＋Ｔｂ＾３＋→Ｅｕ＾２＋＋Ｔｂ＾４＋，通过半量手段研究了这一电荷迁移反应的平衡常数。     

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＿     

KZnF3中Ce^3＋→Eu^2＋的能量传递

研究了ＫＺｎＦ３中Ｃｅ＾２＋和Ｅｕ＾２＋的光谱特性,在共掺Ｃｅ＾３＋和Ｅｕ＾２＋的体系中,观察到了Ｃｅ＾３＋对Ｅｕ＾２＋的能量传递过程,计算了能量传递的量子效率,探讨了能量传递机理,研究发现,Ｃｅ＾３＋的存在有利于Ｅｕ＾２＋的ｆ－ｆ跃迁线状发射。     

Eu^2＋和Mn^2＋在Sr3MgSi2O8中的光致发光研究

研究了Ｅｕ＾２＋和Ｍｎ＾２＋共激活的Ｓｒ３ＭｇＳｉ２Ｏ８的荧光性质。Ｅｕ＾２＋和Ｍｎ＾２＋在４６０ｎｍ和６９０ｎｍ的发射峰分别由Ｅｕ＾２＋的５ｄ→４ｆ跃迁和Ｍｎ＾２＋的＾４Ｔ１（＾４Ｇ）→＾６Ａ１ｇ（＾６Ｓ）跃迁产生。未观察到单掺杂Ｍｎ＾２＋的Ｓｒ３ＭｇＳｉ２Ｏ８的荧光发射，而掺入Ｅｕ＾２＋后则出现了Ｍｎ＾２＋的６９０ｎｍ光致发光峰，表明Ｅｕ＾２＋对Ｍｎ＾２＋有敏化作用。Ｅｕ＾２＋的荧光寿命也受Ｍ     

Eu^2＋在BaF2—xYF3体系中的光谱性质及其对Tb3＋的能量传递

研究了钡钇复合氟化物体系中Ｅｕ＾２＋的光谱性质和变化规律，讨论了影响Ｅｕ＾２＋光谱的因素，特别是氧的存在对Ｅｕ＾２＋激发和发射能量的影响，发现在ＢａＹＦ５基质中Ｅｕ＾２＋对Ｔｂ＾３＋的有效参量传递。     

Eu^2＋和Mn^2＋在SrMgP2O7中的光致发光及其能量传递

研究了Ｅｕ＾２＋、Ｍｎ＾２＋共激活的ＳｒＭｇＰ２Ｏ７的发光性质、浓度与荧光性质的关系，Ｅｕ＾２＋和Ｍｎ＾２＋的发射光谱分别在４００ｎｍ及６７０ｎｍ附近，它们是Ｅｕ＾２＋的５ｄ－４ｆ跃迁和Ｍｎ＾２＋的＾４Ｔ１（＾４Ｇ）－＾６Ａ１ｇ（＾６Ｓ）跃迁发射，实验结果表明，Ｅｕ＾２＋对Ｍｎ＾２＋的荧光发射有较强的敏化作用，Ｍｎ＾２＋对Ｅｕ＾２＋的荧光寿命和强度也有显著影响。     

吡嗪—2,3—二羧酸体系导数荧光法同时测定铕,铽

研究了以吡嗪－２，３－二羧酸为荧光试剂应用导数荧光技术同时测定Ｅｕ＾３＋，Ｔｂ＾３＋的最佳条件，共存离子的影响和Ｅｕ＾３＋，Ｔｂ＾３＋－ＰＹＤＡ配合物的配合比，稳定常数及光机理，Ｅｕ＾３＋，Ｔｂ＾３＋的检测限分别达４．０和２．０ｎｇ／ｍＬ，利用本方法成功地测定了稀土试样中铕、铽的含量。     

Eu^3＋在CaYBO4中的取代和发光

用固相法制备化合物ＣａＹ１－ｘＢＯ４：ｘＥ７ｕ,研究Ｅｕ＾３＋在ＣａＹＢＯ４中的取代格位和发光特性。当Ｅｕ＾３＋掺杂浓度不大时,存在两具发光中心,认为是取代基质中有两个Ｙ格位的结果：通过对Ｅｕ－Ｏ的电荷迁移激发带位置的分析,表明Ｅｕ＾３＋所处八面体中心格位的对称性越低,Ｅｕ－Ｏ的电荷迁移带越偏向于短波;当Ｅｕ＾３＋的掺杂浓度较大（Ｘ〉０．１０）时,Ｅｕ＾３＋离子也可占据Ｃａ＾２＋格位,同时Ｅｕ＾２     

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.     

Enzymatic method for assaying calcium in serum with Ca++ -ATPase

A kinetic assay for total calcium in serum was developed which is based on the activation of Ca(++)-ATPase by free Ca(++) [Ca(++)](f) maintained by EGTA in the reaction mixture. The concentration of Ca(++)(f) was dependent on total reference calcium added or serum calcium. Ca(++)-ATPase activity was coupled to the reduction of NADH by pyruvate kinase (PK) and lactate dehydrogenase (LDH) and monitored by change in absorbance at 340 nm. The calcium in normal serum was 10.08 +/- 0.24 mg/dl (n = 35) by our method while with o-cresolphthalein complexone (CPC) method, the total calcium in the same 35 serum samples was 10.14 +/- 0.54 mg/dl. The range of within-run coefficient of variations (CVs) by this method was 0.9-2.87% at 8-12 mg/dl and day-to-day CVs were 0.72-3.17%. The presence of other ions and standard clinical interfering agents did not affect this assay system. The correlation between values obtained with our method (y) and CPC method (x) for normal serum was: y = 1.064x-0.580 mg/dl (r = 0.912, n = 59).     

稀土离子对钙调蛋白与单克隆抗体分子识别的影响

分别采用酶联免疫吸附(ELISA)法和荧光标记技术比较了Ca²⁺,La³⁺,Eu³⁺和Yb³⁺离子对钙调蛋白与单克隆抗体2C3之间分子识别的影响.结果表明,金属离子与钙调蛋白作用后会诱导其发生不同的构象变化,并进一步影响到钙调蛋白与单克隆抗体2C3分子之间的结合强度.当钙调蛋白分别与La³⁺,Eu³⁺,Yb³⁺作用后,它与单抗2C3分子之间的解离常数为(26.8±2.5),(21.8±3.4)和(64.8±5.1)nmol/L,而结合Ca²⁺前后的钙调蛋白与单抗分子的解离常数分别为(177.2±2.8)和(157±4.2)nmol/L.这一结果表明,稀土离子诱导钙调蛋白发生的构象变化明显不同于钙离子的作用,这种差异可能是稀土与钙离子对钙调蛋白调控作用表现出差别的原因.     

Association of (Ca + Mg)-ATPase activity with ATP-dependent Ca uptake in vesicles prepared from human erythrocytes.

Ghost membranes prepared from human erythrocytes exhibit 2 distinct (Ca + Mg)-ATPase1 activities (Quist and Roufogalis, Arch Biochem Biophys 168:240, 1975). (Ca + Mg)-ATPase activity dependent on a water soluble protein fraction is selectively lost from ghost membranes during preparation of vesicles under low ionic strength, slightly alkaline conditions. In this study, the Ca2+ dependence of the remaining membrane bound (Ca + Mg)-ATPase activity and ATP-dependent Ca uptake in vesicles were compared. The Ca2+ activation curves for (Ca + Mg)-ATPase activity and Ca uptake into vesicles were parallel over a Ca2+ range of 0.3-330 micrometer, and both curves have 2 apparent KA values for Ca2+ of 0.45 and 100 micrometer. Addition of a concentrated soluble protein fraction containing predominantly spectrin to the vesicles increased (Ca + Mg)-ATPase activity over twofold but did not affect the rate of Ca uptake. These findings suggest that the (Ca + Mg)-ATPase activity remaining in vesicles after extraction of the water soluble proteins is associated with the Ca pump whereas (Ca + Mg)-ATPase activity dependent on the soluble protein fraction is associated with some other function.     

Divalent cation dependent ATPase activities of red blood cell membranes: influence of the oxidation of membrane thiol groups close to each other

An Mg2+-dependent low ATPase activity can be detected in erythrocyte "white membranes," in addition to that of the well known (Ca2+ + Mg2+)-ATPase. The thiol oxidizing agent diamide affects both activities. The oxidation of neighboring thiols seems to leave the mechanism of the (Ca2+ + Mg2+)-ATPase amplification system evoked by Ca2+ largely unaffected. The perturbation caused by diamide in the membranes seems to affect primarily a step of the ATP hydrolysis mechanism that is common to both ATPase activities. The effectiveness of diamide seems to be the same when either Ca2+ and Mg2+, or Mg2+ alone are present during the reagent action. Reduction of disulfide bonds by DTE after diamide treatment restores the (Ca2+ + Mg2+)-ATPase activity but is unable to take the Mg2+-ATPase activity back to the original level. The hypothesis is discussed that the redox state of one (or more than one) couple of --SH close to each other and possibly connected to the active site, may be an important factor in optimizing the efficiency of Ca action on the (Ca2+ + Mg2+)-ATPase.     

Ca掺杂的Ba2Al2Si10N14O4∶Eu2+荧光粉发光性能

通过固相反应制备了系列Ca掺杂的Ba2Al2Si10N14O4∶Eu2+绿色荧光粉,发现当半径较大的Ba被Ca取代后导致了晶格的收缩,通过X射线衍射(XRD)测量和Unitcell软件计算发现Ca的最大掺杂量在20%。Ca掺入Eu0.4Ba1.6Al2Si10N14O4荧光粉后,可有效地提高光转换性能,并使激发光谱发生一定程度的红移和宽化,从而被近紫外宽波段光有效激发,与近紫外LED的发射光谱匹配。同时Ca的掺杂也使发射光谱发生了可控的红移,可以由520 nm的绿光红移至548 nm的黄光区域。进一步发现Eu2+的淬灭浓度随着20%Ca的掺入而降低,这是由于Ca掺入导致的晶格收缩使Eu2+离子间距离减小。最后在CIE色度图中对不同Ca,Eu浓度的荧光粉的色坐标位置进行比较,发现可通过Ca,Eu浓度的变化在很大范围内调制荧光粉的发光性能。     

Interpretation of 41Ca data using compartmental modeling in post-menopausal women

Calcium-41 (t(1/2) = 10(5) years) can be used after a single dose to follow calcium metabolism over a subject's lifetime. The aims of this study were to expand a (41)Ca kinetic model and estimate bone resorption in women with stable bone loss, compare the rates with those calculated with classical isotope studies, and to use the model to simulate dynamic changes in urinary (41)Ca:Ca ratios and bone balance for the design and interpretation of (41)Ca studies. Forty-two women >5 years post-menopause were given (41)Ca intravenously. Bone mineral content and bone mineral density of total body were measured by dual-energy X-ray absorptiometry at the beginning of the study. Urine collections were made periodically for up to ~5 years while subjects were free living. Urinary (41)Ca:Ca ratios were measured using accelerator mass spectrometry. The isotope data were analyzed by compartmental modeling. Four compartments were necessary to fit the urinary tracer data and total bone calcium. The final model included pathways for absorption, distribution, urinary excretion, and endogenous excretion and was used to calculate rates of bone turnover. Estimates of bone resorption in a subset of the women (n = 13), studied previously in a 3-week balance and full kinetic study with (45)Ca, agreed with those using (41)Ca methodology. Thus, rates of bone resorption can be estimated from (41)Ca urinary data in stable post-menopausal women. The model was used to simulate dynamic changes in urinary (41)Ca:Ca ratios and bone balance, as a result of interventions that perturb calcium metabolism to aid in study design and interpretation.     

Sarcoplasmic reticulum calcium ATPase is inhibited by organic vanadium coordination compounds: pyridine-2,6-dicarboxylatodioxovanadium(V), BMOV, and an amavadine analogue

The general affinity of the sarcoplasmic reticulum (SR) Ca (2+)-ATPase was examined for three different classes of vanadium coordination complexes including a vanadium(V) compound, pyridine-2,6-dicarboxylatodioxovanadium(V) (PDC-V(V)), and two vanadium(IV) compounds, bis(maltolato)oxovanadium(IV) (BMOV), and an analogue of amavadine, bis( N-hydroxylamidoiminodiacetato)vanadium(IV) (HAIDA-V(IV)). The ability of vanadate to act either as a phosphate analogue or as a transition-state analogue with enzymes' catalysis phosphoryl group transfer suggests that vanadium coordination compounds may reveal mechanistic preferences in these classes of enzymes. Two of these compounds investigated, PDC-V(V) and BMOV, were hydrolytically and oxidatively reactive at neutral pH, and one, HAIDA-V(IV), does not hydrolyze, oxidize, or otherwise decompose to a measurable extent during the enzyme assay. The SR Ca (2+)-ATPase was inhibited by all three of these complexes. The relative order of inhibition was PDC-V(V) > BMOV > vanadate > HAIDA-V(IV), and the IC 50 values were 25, 40, 80, and 325 microM, respectively. Because the observed inhibition is more potent for PDC-V(V) and BMOV than that of oxovanadates, the inhibition cannot be explained by oxovanadate formation during enzyme assays. Furthermore, the hydrolytically and redox stable amavadine analogue HAIDA-V(IV) inhibited the Ca (2+)-ATPase less than oxovanadates. To gauge the importance of the lipid environment, studies of oxidized BMOV in microemulsions were performed and showed that this system remained in the aqueous pool even though PDC-V(V) is able to penetrate lipid interfaces. These findings suggest that the hydrolytic properties of these complexes may be important in the inhibition of the calcium pump. Our results show that two simple coordination complexes with known insulin enhancing effects can invoke a response in calcium homeostasis and the regulation of muscle contraction through the SR Ca (2+)-ATPase.     

脑梗塞后血清常量元素钙镁含量的动态研究

为探讨急性脑梗塞后血清钙镁含量变化及其对预防和治疗的临床意义,随机选取３２例患者采用不同时期晨起空腹采血,应用ＭＴＢ法６４００－Ａ型临床电解质分析仪测定血清中Ｃａ＾２＋和Ｍｇ＾２＋的含量。结果表明,病例组发病１周时血清Ｃａ＾２＋和Ｍｇ＾２＋含量均低于对照组（Ｐ〈０．０１）,发病后２４ｈ血清Ｃａ＾２＋,Ｍｇ＾２＋含量逐渐降低,到发病１周后血清Ｃａ＾２＋、Ｍｇ＾２＋含量降低最明显,２周后血清Ｃａ＾２＋     

Ca2+ selectivity of the sarcoplasmic reticulum Ca2+-ATPase at the enzyme-water interface and in the Ca2+ entrance channel

The sarcoplasmic reticulum (SR) Ca(2+)-ATPase, a P-type transmembrane protein, can transport Ca(2+) from the cytoplasmic to the luminal side over other cations specifically. The proposed Ca(2+) entrance channel, composed of the main-chain carbonyl oxygen and side-chain carboxyl oxygen atoms of the amino acids, opens on the enzyme surface, just above the biphospholipid layer membrane-water interface, where Trp residues are frequently found. In this work, the physicochemical nature of Ca(2+) selectivity over Mg(2+) on the surface of the SR Ca(2+)-ATPase has been investigated using the density functional theory (DFT) method. The selection process can be regarded as the first step of the specificity of the enzyme to transport Ca(2+). Subsequently, the specificity of the entrance channel to conduct Ca(2+) over other cations has also been explored. As revealed by thermodynamic analyses, either the aromatic or the aliphatic amino acid residues distributed on the surface of Ca(2+)-ATPase have a bigger affinity to Mg(2+) than to Ca(2+), resulting in a concentration decrease of free Mg(2+) in the local region. Thus, Ca(2+) can transport into the Ca(2+)-entrance channel more easily. Whereafter, for a small quantity of Mg(2+) entering this channel accompanying the Ca(2+) current, the strong electrostatic interactions between Mg(2+) and the ligands will limit the activity of this metal ion, which facilitates the weakly bonded Ca(2+) passing through the channel at a relatively high rate, as suggested by the "sticky-pore" hypothesis. Furthermore, the corresponding theoretical investigations have demonstrated that the increase of the ligand electronegativity can enhance their discrimination between these two cations effectively.