荧光猝灭法研究山豆根碱与人血清白蛋白间的相互作用

利用荧光光谱法研究了中药有效成分山豆根碱与人血清白蛋白(HSA)间的非共价结合特性。在37℃和47℃两个作用温度下,山豆根碱与HSA间的结合常数K分别为1.5671×103L.mol-1和2.4923×103L.mol-1,结合位点数n分别为0.8309和0.8630,表明温度升高有利于两者的结合。计算了热力学参数,表明该药物与蛋白的相互作用是一个熵增加和吉布斯自由能降低的自发过程,并由此推断山豆根碱与HSA之间的作用力是以疏水相互作用为主,为研究山豆根碱的药理作用和生物学效应,以及山豆根碱对蛋白质构像的影响等提供了重要信息。     

石英芯片电泳分离检测尿中蛋白的研究

通过对缓冲体系、缓冲液浓度、酸度、乳酸钙浓度、乙胺浓度、电泳电压和进样时间的优化选择，用石英芯片电泳一紫外检测法分离了纯人白蛋白和人运铁蛋白；在75mmol／L硼酸盐（pH10．55）（含0．8mmol／L乳酸钙、1％（φ）乙胺）运行缓冲液中，上述两组分在3min内完全分离；纯人白蛋白和人运铁蛋白的线性范围分别为1．0～15．0g/L和1．0～10．0g／L；检出限（S／N=3）均为0．5g／L，应用于临床尿蛋白分离测定，并与Helena琼脂糖凝胶电泳仪电泳结果进行比较，获得一致结果。     

血清蛋白-荧光素复合物单扫极谱波与应用

在0．08mol／L的HAc中，荧光素与牛血清白蛋白(BSA)或人血清白蛋白(HSA)相互作用形成复合物。复合物使荧光素在-0．58V(vs．SCE)处的还原峰电流增大，峰电流的增大值与加入的BSA或HSA的浓度在一定的范围内呈线性关系。BSA在2—24μg／mL范围内呈线性关系，检出限为1μg／mL；HSA在2—22μg／mL范围里呈线性关系，检出限为0．8μg／mL。应用该法测定了人血清蛋白样品，结果令人满意。     

刚果红与血清白蛋白相互作用的极谱分析

在pH4．7HAc-NaAc缓冲溶液中，刚果红与蛋白质(BSA或HSA)作用形成络合物，使刚果红-0．35V(vs SCE)的还原峰电流下降，峰电流的降低值同所加的BSA或HSA质量浓度在一定范围内呈线性关系；BSA和HSA的线性范围分别为0．5～12mg／L和0．5～11mg／L，检出限分别为0．25和0．20mg／L；运用该法测定了人血清白蛋白样品，结果令人满意。     

少量人发中硫的测定

建立了测定一根长2～3cm人发中硫的间接分光光度法,表观吸光系数为5.1×10~4,络合物组成Ba:CPA-mA为1:2,比耳定律范围为0～20μg硫。硫的检测限为0.025μg/mL,变动系数为2.7%,回收率为91.2～97.2%,且不用掩蔽即可直接进行测定,测定211例人发的结果表明,含硫量范围为(28.5±3.2)×10~3μg/g。     

A comparison of double-focusing sector field ICP-MS, ICP-OES and octopole collision cell ICP-MS for the high-accuracy determination of calcium in human serum

Human serum is routinely measured for total calcium content in clinical studies. A definitive high-accuracy and low-uncertainty method is required for reference measurements to underpin medical diagnoses. This study presents a novel octopole collision cell ICP-MS, high-accuracy, methodology and comparison of that technique with double-focusing sector field ICP-MS and an ICP-OES method. Double-matched isotope dilution mass spectrometry (IDMS) was employed for ICP-MS techniques and an exact matching bracketing technique using scandium as an internal standard was used for ICP-OES analysis. Medium resolution mode was utilised for double-focusing sector field ICP-MS analysis to resolve the dominant interferences on the ⁴⁴Ca/⁴²Ca isotope pair. Hydrogen reaction gas was employed to chemically resolve a number of polyatomic interferences predominantly through charge transfer reactions in the octopole collision cell. Comparison data presented for NIST CRM 909b human serum analysis from all three techniques demonstrates highest accuracy (99.6%) and lowest uncertainty (1.1%) for octopole collision cell ICP-MS. Data from ICP-OES using a non-IDMS technique produces comparably accurate data and low-uncertainties. The much higher total expanded uncertainties for double-focusing sector field ICP-MS compared with octopole collision cell data are explained by lower precision on the measurement of the ⁴⁴Ca/⁴²Ca isotope ratio. Data for octopole collision cell ICP-MS submitted for an international blind trial comparison (CCQM K-14) demonstrated excellent agreement with the mean of all participants with a low expanded uncertainty.     

Inclusion of molybdenocene dichloride (Cp2MoCl2) in 2-hydroxypropyl- and trimethyl-β-cyclodextrin: Structural and biological properties

Organometallic-cyclodextrin inclusion compounds were obtained by the treatment of molybdenocene dichloride (Cp₂MoCl₂) with the modified cyclodextrins (CDs) heptakis-2,3,6-tri-O-methyl-β-CD (TRIMEB) and 2-hydroxypropyl-β-CD (HPβCD) in aqueous solution. The products were isolated by liophilisation and characterised in the solid-state by powder XRD, thermogravimetric analysis, Raman and FTIR spectroscopy, and ¹³C CP MAS NMR spectroscopy. The results are consistent with inclusion of Cp₂MoCl₂, rather than hydrolysis products such as [Cp₂Mo(H₂O)X]⁺ (X = Cl, OH) or [Cp₂Mo(H₂O)₂]²⁺. The pure non-included metallocene Cp₂MoCl₂ and its inclusion compounds with unmodified β-CD, TRIMEB and HPβCD were screened for their potential antiproliferative and cytotoxic activity, in both human cancer and healthy cell lines. Inclusion in CD was found to enhance the cytotoxic effect of Cp₂MoCl₂, with the TRIMEB adduct displaying the highest anti-tumour activity, along with the lowest toxicity towards non-neoplastic cells.     

Determination of doxorubicin in human plasma by excitation-emission matrix fluorescence and multi-way analysis

Direct determination of doxorubicin (DXR), a cytotoxic anthracycline antibiotic, in human plasma was accomplished based on excitation-emission matrix (EEM) fluorescence measurements and multi-way chemometric methods based on parallel factor analysis (PARAFAC) and N-PLS. Several different procedures, such as residual analysis, core consistency diagnostic (CONCORDIA) and split-half analysis were employed to determine the correct number of factors in PARAFAC. These procedures converged to a choice of two factors, attributed to DXR and to the sum of two fluorescence species present in the plasma. Sample PARAFAC loadings were employed to build a regression model against concentration, resulting in a RMSECV of 0.060 μg ml⁻¹. N-PLS using two factors produced a RMSECV of 0.045 μg ml⁻¹. Figures of merit (FOM), such as sensitivity (SEN), selectivity (SEL) and limit of detection (L_D) were determined for both PARAFAC and N-PLS.     

人血中10种常见毒品的GC-MS同时检测方法研究

建立了同时检测人血液中鸦片类、巴比妥类和苯二氮卓类10种常见毒品的气相色谱-质谱新方法。系统地对提取溶剂及其组成配比、体系pH值、超声振荡提取时间等样品预处理条件以及色谱柱等GC-MS分析条件进行考察和优化。运用选择离子模式(SIM)检测,每种成分选择4个特征离子。所选的离子分别为:摇头丸m/z44、77、136、207;异戊巴比妥m/z156、55、141、41;司可巴比妥m/z168、97、195、41;咖啡因m/z194、82、109、67;安眠酮m/z235、213、250、91;美沙酮m/z72、57、165、213;吗啡m/z271、150、201、81;安定m/z256、221、283、165;氯氮平m/z243、227、256、192;艾司唑仑m/z207、239、293、259,其中黑斜体为定量离子。在选定的条件下,异戊巴比妥等7种药物在0.10~25.0 mg/L范围内线性关系良好,安定等3种药物在0.50~25.0 mg/L范围内线性关系良好,方法回收率在96%~103%之间,RSD在1.64%~6.32%之间,检出限为0.01~0.05 mg/kg。本文同时研究了pH值对吗啡类药物的影响机理。与文献报道的检测方法比较,本法更加简便易行,灵敏度提高1个数量级以上,分析时间缩短,用色谱保留时间与质谱同时定性,消除血液中其他成分干扰,结果准确可靠,选择性和重复性好,可应用于中毒患者体液样品及毒物成分的分析检测。     

Development and Validation of a Liquid Chromatographic Method for Determination of Efavirenz in Human Plasma

A simple, rapid, and sensitive high-performance liquid chromatographic method for estimation of efavirenz in human plasma has been developed and validated. Chromatography was performed with C₁₈ analytical column and 50:50 acetonitrile–phosphate buffer (pH 3.5) as mobile phase. Compounds were monitored by UV detection at 247 nm. The retention time for efavirenz was 6.45 min and that for the internal standard, nelfinavir, was 2.042 min. Response was a linear over the concentration range of 0.1 μg–10 μg mL⁻¹ in human plasma. The method was simple, specific, precise and accurate and was useful for bioequivalence and pharmacokinetic studies of efavirenz.