微波间歇萃取-分光光度法测定三七中总皂苷

本文建立了采用微波辅助间歇提取三七样品中的总皂苷,并以分光光度法测定其含量的实验方法。分别通过单因素实验和正交实验设计,优化了萃取溶剂浓度、溶剂用量、微波功率和微波辐射时间等提取条件,确定了微波辅助萃取法提取三七中皂苷类化合物的最佳条件为:使用浓度为60%的乙醇,在液固比100∶1的条件下,以255 W的微波功率,微波间歇萃取10×20 s。在上述最优条件下进行了精密度和回收率实验,加入回收率在97.7%~101.8%之间,RSD为1.54%(n=5)。与传统的索氏提取法和超声波提取法比较,微波辅助萃取法具有操作简便,宽速,重现性好等特点,实验结果表明此方法可推广应用于各类中草药中总皂苷的含量测定。     

硫氰酸钾-OP光度法测定有机相中微量铁

用二元或三元有机磷类萃取剂萃取铀时,铁也部分被萃取,工艺过程中需加以控制。有机相中微量铁可用邻菲咯啉比色法直接测定,此法以无水乙醇作稀释剂,三烷基氧膦(TRPO)作乙醇和煤油(试样)的混溶剂,但取样量不能超过1毫升,否则引起TRPO无法抑制的混浊。我用曾用萃取原子吸收分光光度法或用盐酸反萃后测定有机相中微量铁。随表面活性剂在胶束增溶分光光度法中的广泛应用,我们研究了Fe-SCN-OP的显色反应,并应用于二元或三元磷类萃取体系的有机相中微量铁的测定。本法操作简便,选择性良好,表观摩尔吸光系数为     

8-羟基喹啉-浊点萃取-流动分析光度法测定果蔬中铬价态

1 引言 浊点萃取法是一种新兴的液-液萃取技术,具有很高的富集倍数和提取率.流动分析光度法通常一次进样只需0.5～1.0 mL,可节省试样,减少二次污染.浊点萃取法与流动分析光度法结合可优势互补,更快速、简便.Cr(Ⅲ)是人体维持生命的必需元素,而Cr(Ⅵ)在生物体系内有很强的流动性和氧化性.因此,分析不同价态铬十分重要.铬价态的分析方法主要有共沉淀、萃取、离子交换、色谱等方法.基于Triton X-100的浊点现象,选择8-羟基喹啉为螯合萃取剂,在优化的实验条件下,使Cr(Ⅲ)-8-羟基喹啉 "原位"进入其富胶束相,Cr(Ⅵ)留在水相而彼此得以分离,提出了浊点萃取-流动分析光度法测定不同价态铬的新方法.     

流动注射-分光光度法测定天然产物对酪氨酸酶活性的影响

建立了一种快速、灵敏且高精度的流动注射-分光光度法用于研究天然产物对酪氨酸酶活性的影响。此方法基于一定介质条件下L-3,4-二羟基苯丙氨酸(L-DOPA)在酪氨酸酶的作用下,发生氧化生成棕褐色多巴醌,其最大吸收峰位于475 nm处,而酪氨酸酶抑制剂能降低酶促反应速度,减少多巴醌形成的量,从而降低475 nm下的吸光度值,形成倒峰。在优化实验条件下,半抑制浓度的曲酸抑制酪氨酸酶活性测定相对标准偏差(n=10)为0.036%,与分光光度法和酶标仪微量法相比,精密度提高了10倍以上。咖啡酸对酪氨酸酶有较强的激活作用,对二酚酶相对激活率达到50%时的浓度(IC50)为0.170 mmol/L;薰衣草花水相提取物具有较强的抑制活性,其IC50值为0.96 mg/m L。与分光光度法及酶标仪微量法相比,流动注射-分光光度法精密度高,重复性好,适用于天然产物对酪氨酸酶活性影响的测定。     

活性染料的溶剂浮选动力学研究及其直接有机相光度法测定

以活性艳红X-3B作为研究实样,对活性染料的溶剂浮选动力学进行了初步,研究.试验表明:在较低的流速下,速率常数的增加与气体流速成正比,溶剂浮选过程中-ln(At/Ao)与时间的关系符合一级动力学方程.所选3种活性染料同时进行气浮溶剂浮选,其萃取率均大于96%;与常用的溶剂萃取法相比较,溶剂浮选法具有富集倍数大,回收率高,溶剂用量少等优点.将浮选后有机相直接用于光度法分析.将此方法应用于测定某印染厂废水中活性艳红X-3B的含量,测得其浮选率为98.1%,回收率为93.6%.     

紫外分光光度法测定辣椒素在提取过程中的改进

国外曾采用紫外分光光度法测定辣椒素,是用异丙醇抽滤萃取,加炭吸附,经异丙醇、石油醚等溶剂提纯,从中反复蒸干溶剂。操作繁琐复杂,成本高,且出现误差机率大。本文采用异丙醇静置萃取,然后经活性氧化铝层析柱提纯。提纯和测定半天可以出结果。 (一)操作步骤取1.000g样品于25ml容量瓶中用异丙醇避光萃取24h,过滤。吸清液10ml于50ml层析柱(柱装置:下     

紫外分光光度法表征Lipozyme TL IM脂肪酶转酯化活性

建立了一种新的有机相脂肪酶转酯化活性测定方法. 以正己烷为溶剂,脂肪酶催化棕榈酸对硝基苯酯和正丁醇的转酯化反应为模型反应,通过测定反应液中310 nm下吸光值的变化计算反应转化率. 以气相色谱法对新建的紫外分光光度法进行验证,分别采用这两种方法测定了七种商品化脂肪酶的转酯化活性,两种方法所得实验结果基本一致. 利用紫外分光光度检测法考察了Lipozyme TL IM脂肪酶催化转酯化的时间进程及合成活性与酶量的关系,并对Lipozyme TL IM催化转酯化的性质（最适溶剂、酰基受体特异性、醇耐受性、最优反应温度和热力学稳定性）进行了表征.     

96孔板法用于高通量血管紧张素转化酶抑制剂体外检测

为在体外迅速检测血管紧张素转化酶抑制剂( ACEI)的抑制活性,选用96孔板,以呋喃丙烯酰三肽(FAPGG)为模拟底物,通过检测血管紧张素转化酶(ACE)酶解FAPGG生成N-[3-(呋喃)丙稀醇酰-2-苯丙氨酸( FAP)和双甘氨肽(GG)后340 nm处吸光值的下降衡量ACE的活性,采用加入ACEI前后ACE的活性变化衡量ACEI的活性.考察了不同缓冲体系、Cl-浓度、ACE酶活性(ACE酶浓度)、缓冲体系的pH值等对上述检测模型反应体系的影响,建立了高通量降血压肽活性体外检测方法,本方法最多可同时检测96个样品的ACE抑制活性,上机分析时间仅需10 s.不同批次活性平行测定的相对标准偏差均小于0.001％,p=0.667＞0.05,各测定结果无显著差异,重现性好,精密度较高.采用本方法测定了商品血管紧张素转化酶抑制剂Captopril的IC50值为16.19 nmol/L,与文献报道的测定结果一致.     

超声辅助液液萃取法提取烟用香精成分的研究

采用超声辅助液液萃取法(ULLE)提取某品牌烟用香精成分,GC-MS对其进行分析,研究了不同萃取剂、萃取时间和萃取温度对分析结果的影响,初步确定了最佳条件为:以二氯甲烷为萃取剂,饱和NaCl溶液作水相,室温下超声萃取5 min.又分别与同时蒸馏萃取法(SDE)和传统的液液萃取法(LLE)作以比较,对ULLE法和SDE法鉴定出的化学成分、重现性和定量值进行了对比.结果表明:超声辅助液液萃取具有操作简便、快速、节能、萃取效率高、重现性好等特点,适合于烟用香精成分的提取.     

溶剂诱导相变萃取法用于高效液相色谱-质谱分析的血浆样品前处理

在匀相的乙腈-水体系中添加一种疏水但与乙腈互溶的有机溶剂(如氯仿), 能诱导乙腈-水体系分相, 基于此现象建立了一种血浆样品处理方法溶剂诱导相变萃取(SIPTE). 与传统的液-液萃取法相比, 该法最大的优势为新形成的有机相为乙腈(仅含少量氯仿), 与常用的反相C₁₈柱兼容, 能直接进行高效液相色谱-质谱分析. 此外, 通过减少乙腈及氯仿的用量还可实现样品的自动浓缩. 本文通过测定血浆中尼群地平, 验证了该方法的有效性. 使用反相C₁₈柱, 以V(乙腈)∶V(水)=70∶30(含20 mmol/L甲酸铵)为流动相, 尼莫地平为内标, ESI正离子模式下选择离子监测(SIM)测定了血浆中尼群地平的浓度. 实验所得的线性、精密度和准确度结果良好, 表明所建立的方法灵敏、准确、简单、快速, 可用于药物代谢动力学研究.     

Improved method for direct high-performance liquid chromatography assay of angiotensin-converting enzyme-catalyzed reactions

A rapid and sensitive assay was developed for determination of the activity of angiotensin-converting enzyme (ACE) in the presence of inhibitory peptides present in soybean protein hydrolysates. The method utilizes reversed-phase high-performance liquid chromatography (HPLC) to separate and quantify hippuryl-histidyl-leucine (HHL) and hippuric acid (HA). HHL and HA were separated on a Symmetry C₁₈ column by gradient elution that used mixtures of trifluoroacetic acid (TFA)–acetonitrile and TFA–water as solvents. Analytical time and baseline separation of HA from HHL were improved over previous HPLC methods. In comparison to the standard spectrophotometric method, the new HPLC method obviates the need for ethyl acetate extraction of HA but requires direct injection of the ACE reaction mixture onto the HPLC column.     

On-line solid phase extraction of humic acid from environmental water and monitoring with flow-through chemiluminescence

An on-line solid phase extraction device combined with flow-through chemiluminescence monitoring was presented for the enrichment and determination of humic acid (HA) in water samples. The chemiluminescence principle was based on the enhancement effect of HA on the Ce(IV)/H(2)SO(4)-rhodamine 6G chemiluminescence system. For sample pretreatment, the on-line solid-phase extraction (SPE) material was packed into a cartridge which was then installed in the manifold. Experimental parameters including reagent concentration, flow rate and extraction time, were optimized. Under the optimized conditions, the relative standard deviation was 3.6% for determining 2 mg L(-1) HA standard solution and the detection limit was 3 μg L(-1). The proposed method was successfully applied to the determination of HA in the range of 0.1-35 mg L(-1). The results were validated by spike recovery experiments. The recovery was from 74.0% to 121%, which was good enough for the determination of HA in environmental waters.     

Trace humic and fulvic acid determination in natural water by cloud point extraction/preconcentration using non-ionic and cationic surfactants with FI-UV detection

A preconcentration and determination method for humic and fulvic acids at trace levels in natural water samples was developed. Cloud point extraction was successfully employed for the preconcentration of humic acid (HA) and fulvic acid (FA) prior to the determination by using a flow injection (FI) system coupled to a spectrophotometric UV-Vis detector. The quantitative extraction of HA and FA within the pH range 1-12 was obtained by neutralization of the anionic charge on the humic substances with a cationic surfactant, hexadecyltrimethylammonium bromide (CTAB). This generated a hydrophobic species that was subsequently incorporated (solubilized) into the micelles of a non-ionic surfactant polyethylene glycol, tert-octylphenyl ether (Triton X-114). The FI method for HA and FA determination was developed by injection of 100 microl of the extracted surfactant-rich phase using an HPLC pump with spectrophotometric detection at 350 nm. A 50 ml sample solution preconcentration allowed an enrichment factor of 167. The limit of detection (LOD) obtained under the optimal conditions was 5 microg l(-1). The precision for ten replicate determinations at 0.2 mg l(-1) HA was 3.1% relative standard deviation (RSD), calculated from the peak heights. The calibration using the preconcentration system for HA and FA was linear with a correlation coefficient (r2) of 0.9997 at levels near the detection limits up to at least 1 mg l(-1). The method was successfully applied to the determination of HA and FA in natural water samples (river water).     

A UPLC-DAD-Based Bio-Screening Assay for the Evaluation of the Angiotensin Converting Enzyme Inhibitory Potential of Plant Extracts and Compounds: Pyrroquinazoline Alkaloids from Adhatoda vasica as a Case Study

Angiotensin converting enzyme (ACE) plays a crucial role in regulating blood pressure in the human body. Identification of potential ACE inhibitors from medicinal plants supported the idea of repurposing these medicinal plants against hypertension. A method based on ultra-performance liquid chromatography (UPLC) coupled with a diode array detector (DAD) was used for the rapid screening of plant extracts and purified compounds to determine their ACE inhibitory activity. Hippuryl-histidiyl-leucine (HHL) was used as a substrate, which is converted into hippuric acid (HA) by the action of ACE. A calibration curve of the substrate HHL was developed with the linear regression 0.999. The limits of detection and quantification of this method were found to be 0.134 and 0.4061 mM, respectively. Different parameters of ACE inhibitory assay were optimized, including concentration, incubation time and temperature. The ACE inhibition potential of Adhatoda vasica (methanolic-aqueous extract) and its isolated pyrroquinazoline alkaloids, vasicinol (1), vasicine (2) and vasicinone (3) was evaluated. Compounds 1–3 were characterized by various spectroscopic techniques. The IC₅₀ values of vasicinol (1), vasicine (2) and vasicinone (3) were found to be 6.45, 2.60 and 13.49 mM, respectively. Molecular docking studies of compounds 1–3 were also performed. Among these compounds, vasicinol (1) binds as effectively as captopril, a standard drug of ACE inhibition.     

Rapid determination of the angiotensin I-converting enzyme inhibitory activity of peptide by HPLC method: A simulated gastrointestinal digestion study

Angiotensin I-converting enzyme (ACE) plays a vital role in blood pressure regulation. In vitro ACE inhibitory activity assays are commonly used for evaluating the activity of inhibitors in many researches. In the present study, a rapid, sensitive, simple, and accurate HPLC method for ACE inhibitory activity determination using chicken meat as a model was developed. Specific attention was paid to assess the ACE inhibitory activity of peptides released during simulated gastrointestinal digestion. Using hippuryl–histidyl–leucine as the substrate, ACE can catalyze it into hippuric acid, which is rapidly and sensitively detected by the HPLC at the retention time of 8–10?min. The ACE inhibitory activity of each digestion solution can be rapidly determined every 15?min or less. The model protein displayed a high ACE inhibitory activity during simulated gastrointestinal digestion, but the digestion solution in the stomach showed stronger activity than in the intestine.     

Determination of Molybdenum in Steels, Soil, and Sea Water by Spectroscopic Methods and Adsorption Voltammetry

Procedures were developed for the determination of molybdenum in steels, soil, and sea water using o,o"-dihydroxyazo compounds [Lumogallion IREA (LG) and Magneson IREA (MG)] and heterocyclic azo compounds [4-(2-pyridylazo)resorcinol (PAR) and 2-(5-bromo-2-pyridylazo)-5-diethylaminophenol (5-Br-PAAP)], including their determination in the presence of the third component, hydoxylamine (HA). The addition of the third component improved the selectivity of determination. The advantage of the developed procedures is that they do not involved extraction and, thus,shorten the analysis. Molybdenum can be determined in sea water in the presence of LG or LG + HA by diffuse reflectance spectroscopy or adsorption voltammetry using the added–found method or using visual tests. In the presence of MG, PAR, and 5-Br-PAAP, the standard addition method was used to eliminate the matrix effect.     

研究螯合萃取和协同萃取机理的两相滳定法

本文用严格而简洁的方法导出用两相滴定法研究螯合萃取和协同萃取机理的理论公式。用两相滴定法研究了1-苯基-3-甲基-4-苯甲酰基吡唑啉酮-5(HPZL)的苯溶液对锌离子的萃取机理以及HPZL和TBP(磷酸三丁酯)的苯溶液对锌离子的协同萃取机理,证明这个方法得到的结果是可靠的。对两相滴定法的优缺点和适用范围进行了讨论。     

反相液相色谱-串联质谱法鉴定油菜蜂花粉中的蛋白质及活性肽

基于鸟枪法蛋白质组学分析方法,使用反相液相色谱-串联质谱（RPLC-MS/MS）系统分析油菜蜂花粉蛋白质的胰蛋白酶酶解产物,结合数据库检索,共鉴定到353条肽段。鉴定到的肽段所归属的蛋白质中有239个蛋白质可检索到其分子生物学功能,主要功能为结合活性、酶活性、运输活性、抑制活性等。根据血管紧张素转化酶（ACE）抑制肽活性与多肽构效之间的关系,从鉴定到的肽段中筛选并适当修饰后得到5条可能具有ACE抑制活性的肽段,化学合成肽段后进行了活性验证。结果表明5条肽段均具有良好的活性,其中肽段AELDIVLALF和LAVNLIPFP表现出较高的ACE抑制活性,半数抑制浓度（IC₅₀）分别为（10.65±0.50）μmol/L和（23.66±1.08）μmol/L。该方法速度快,成本低,大大缩短了鉴定周期,达到了高通量筛选生物活性肽的目的。     

HPLC法同时测定尿样中芳香族化合物的6种代谢产物

建立了同时测定尿样中反,反-粘康酸、马尿酸、苯乙醇酸、苯乙醛酸、对氨基酚和对硝基酚的高效液相色谱法(HPLC).优化了色谱分离及检测条件,并采用时间程序波长检测.确定了最佳样品预处理条件:以5 mL二氯甲烷-异丙醇(7∶3)为萃取溶剂;样品用量5 mL;NaCI加入量0.75 g;萃取时间2 min,分别在酸性和中性条...