胶束电动毛细管色谱法测定红丝线提取物中紫蓝素的含量

建立了胶束电动毛细管电泳色谱法(MECC)测定红丝线提取物中紫蓝素的含量的方法。毛细管柱内径75μm,长50.2cm;运行电压25kV,检测波长585nm,温度25℃;缓冲液为25mmol/L,β-CD10mmol/L,硼酸盐-20%乙腈(pH值8.0);进样方式:压力进样,进样时间5s。结果表明紫蓝素在10～100μmol/L浓度范围内具有良好的线性关系(r=0.9995),回收率为95.3%～103.2%。该方法快速、简便、并且较为准确,适用于测定红丝线提取物中紫蓝素的含量。     

稀释液中添加海藻糖对山羊精子功能和膜完整性的影响

选用5只年龄为3～4岁的波尔山羊公羊研究在稀释液中添加海藻糖对山羊精子功能和膜完整性的影响。山羊精子分别用含6.6 mmol/L、13.2 mmol/L、19.8 mmol/L、26.4 mmol/L、39.6 mmol/L、52.9 mmol/L、66.1mmol/L、79.3 mmol/L的不同海藻糖的Tris-柠檬酸-葡糖糖(TCG)稀释液(卵黄:18%;甘油:6%)稀释和冷冻。结果表明:39.6 mmol/L、52.9 mmol/L、66.1 mmol/L、79.3 mmol/L组降温后的精子活率显著(P<0.05)降低;52.9 mmol/L、66.1 mmol/L、79.3 mmol/L组降温后的精子畸形率和39.6 mmol/L组降温后的膨胀精子率显著(P<0.05)提高。26.4 mmol/L组和39.6 mmol/L组冻融后的精子活率显著(P<0.05)高于对照组;66.1mmol/L和79.3 mmol/L组冻融后的精子活率、畸形率分别显著(P<0.05)低于和高于对照组。19.8 mmol/L、26.4 mmol/L、39.6 mmol/L组冻融后精子获能率显著(P<0.05)低于对照组。39.6 mmol/L组冻融后顶体完整率和膨胀精子率显著(P<0.05)高于对照组,而66.1 mmol/L组和79.3 mmol/L组显著(P<0.05)低于对照组。39.6 mmol/L组的受胎率显著(P<0.05)高于对照组,而66.1mmol/L组和79.3 mmol/L组的受胎率显著(P<0.05)低于对照组。结果表明,在含18%的卵黄(v/v)、6%甘油(v/v)的TCG稀释液中,添加适宜浓度(26.4mmol/L和39.6 mmol/L)海藻糖,可显著提高山羊精子功能和膜的完整性。     

氯化三辛基甲胺/氯仿/正丁醇反胶束萃取地木耳多糖

采用阳离子表面活性剂氯化三辛基甲胺(TOMAC)/氯仿/正丁醇反胶束体系萃取地木耳中的多糖。分析有机溶剂氯仿与助表面活性剂正丁醇比例、TOMAC浓度、多糖粗提液浓度、促溶剂盐酸胍浓度、盐离子种类和浓度对前萃取率的影响。结果表明:向0.5 mg/m L多糖粗提液中加入10 mmol/L盐酸胍(Gu HCl)和0.06 mol/L Na Cl,与等体积25 mmol/L TOMAC/氯仿-正丁醇(V∶V=3∶1)的反胶束体系混合,地木耳多糖前萃取率为53.21%;反萃时水相中Na Cl浓度为0.14 mol/L,盐酸胍浓度浓度为0.6 mol/L,在此条件下地木耳多糖反萃取率为93.2%。     

十二烷基硫酸钠对高压静电场对酶作用的影响

研究了十二烷基硫酸钠(SDS)对高压静电场对酶作用的影响。结果表明:在强度为3×103V/cm的电场作用下,十二烷基硫酸钠使过氧化氢酶对高压静电场的作用变得更加敏感。低浓度的十二烷基硫酸钠中,过氧化氢酶在高压静电场的作用下活力升高;0.04mmol/L～0.12mmol/L的十二烷基硫酸钠中,酶活力在高压静电场作用下先升高后下降;高于0.40mmol/L,则酶活力单调下降。十二烷基硫酸钠对高压静电场中的过氧化氢酶具有一定的保护作用。     

分光光度法测水红花子中花旗松素含量

目的:检测水红花子中花旗松素的含量.方法:采用紫外分光先度法,在常温下(25℃)290nm处,对水红花子乙醇提取物进行吸光度测定.结果:此方法线性范围:0.002～0.01 g/L,花旗松素浓度与吸光度线性关系:y=0.0724x 0.007,r2=0.9986;平均回收率为99.37%,RSD=0.897%.结论:紫外分光光度法测定水红花子中花旗花素合量操作简便、快速和准确度高,具有一定实用价值.     

四种山蓝加工方法的比较

用高效液相色谱法和分光光度法测定了四种加工方法所得山蓝加工提取物中有效成分含量 ,结果表明 ,经阴干 ,晒干 ,乙醇浸泡几种传统加工方法加工的山蓝中紫蓝素含量分别为 31 1、4 5 6、4 72 mg/1 0 0 g(干重 ) ,而采用避氧热处理加工的山蓝中 ,紫蓝素含量达 1 .73g/1 0 0 g。用传统加工方法对山蓝进行加工 ,有效成分含量低 ,制约了山蓝的利用价值 ,而避氧热处理能大大提高有效成分含量 ,提升山蓝的品质。研究结果对山蓝的加工、炮制和开发利用有重大意义。     

对SDS稳定的V8(V125T)蛋白酶突变体的高效表达及性质研究

谷氨酰内切酶能特异性切割谷氨酸、天冬氨酸残基羧基端结合的肽键。将含有V8蛋白酶突变体(V125T)基因的表达质粒的重组大肠杆菌BL21(DE3),在50L发酵罐中发酵,融合蛋白为可溶性表达,可得菌湿重50g/L,相对蛋白表达量为33%。融合蛋白采用GST亲和纯化、肠激酶激活、DEAE-FF阴离子交换层析,得到纯的V8(V125T)突变体,经纯化后可获得0.998mg蛋白/g菌(湿重),比活为13.47 U/mg pro.纯化过程的酶活回收率达到了97.9%。对纯酶进行酶学性质分析,以Z-Phe-Leu-Glu-p NA作为底物测得V8(V125T)蛋白酶的Km为0.339mmol/L,Vmax为16.642μmol/min。其最适pH为8.0,在pH4.0~10.0之间较稳定;最适反应温度在45℃,12h内在4~35℃有很好的温度稳定性;25℃条件下1mmol/L的金属离子对酶具有不同程度的影响,其中Fe~(3+)的抑制作用最强;2mol/L尿素及1mmol/L EDTA对酶活性无影响,在0.1%SDS中保存12h、在0.5%SDS中4h和在1%SDS中1h,活性均能维持90%以上,在0.5%,0.1%SDS保存12h,仍能保持80%和64%的活性,与未突变的重组V8蛋白酶相比,该突变体对SDS的耐受性得到极大提高。     

CHO细胞无血清培养基的工艺优化

本文以表达人肿瘤坏死因子受体-人Ig G-Fc抗体融合蛋白的CHO细胞为研究对象,通过对影响其细胞密度、活力及蛋白表达量和聚体百分比的进行了3个大类因素的考察,即水解物:0.5%酵母提取物,0.5%谷类水解物,0.5%大豆蛋白水解物,0.5%植物蛋白胨;脂类物质:10 mmol/L磷脂酰胆碱,10 mg/L乙醇胺,0.05%脂肪乳剂;激素类物质:10μmol/L氢化可的松(肾上腺皮质激素),10 mg/L胰岛素,20 n M孕酮(类固醇激素)。结果表明,水解物中0.5%酵母水解物,脂类物质中10 mg/L乙醇胺,激素类物质中10 mg/L胰岛素对提高CHO细胞密度、活力和蛋白表达量和降低聚体含量具有重要促进作用。     

兰州地区健康体检者血脂水平分析

目的:通过检测兰州地区健康体检者空腹血脂水平了解本地区人群血脂水平现状及血脂异常情况,建立本地区血脂参考值。方法:采用全自动生化分析仪检测兰州市2328名健康体检者,血清胆固醇(TC)、甘油三酯(TG)、高密度脂蛋白胆固醇(HDL-C)、低密度脂蛋白胆固醇(LDL-C)。比较不同年龄、性别血脂水平差异。结果:本地区2328名被检者,女性TC平均(4.54±0.94)mmol/L,TG中位数1.24mmol/L、HDL-C平均(1.34±0.26)mmol/L、LDL-C平均(2.61±0.76)mmol/L;男性TC平均(4.52±0.84)mmol/L、TG中位数1.56mmol/L mmol/L、HDL-C平均(1.20±0.23)mmol/L LDL-C平均(2.76±0.72)mmol/L,血脂水平随年龄增加逐渐升高(P<0.05)。血脂参考范围为女性TC:2.70~6.38 mmol/L、TG:0.52~3.66 mmol/L、HDL-C:0.83~1.85 mmol/L、LDL-C:1.12~4.10 mmol/L男性:TG:2.87~6.17 mmol/L、0.65~4.00 mmol/L、0.75~1.65 mmol/L、1.35~4.17 mmol/L。男性高TC、高TG、低HDL-C和高LDL-C患病率为18.2%、42.8%、19.6%和28%,女性高TC、高TG、低HDL和高LDL的患病率分别为22.1%、25.5%、2.7%和23.5%。结论:兰州地区血脂水平随年龄、性别、地区不同存在较大差异,临床上不能采用统一标准衡量,而应根据本地区建立的参考值诊断高脂血症。积极控制血脂水平、降低高脂血症患病率预防心脑血管疾病发生。     

高原鼠兔血清中N-isopropyl oxamate的RP-HPLC检测方法的建立

目的:探索N-isopropyl oxamate和血清蛋白结合水平,建立高原鼠兔血液中精子型乳酸脱氢酶(LDH-C4)特异性抑制剂N-isopropyl oxamate的高效液相色谱(HPLC)检测方法。方法:取体重150~200 g高原鼠兔20只,随机分为对照组和抑制剂组(n=10)。通过外源性加入不同浓度的N-isopropyl oxamate,检测其与血清蛋白的结合水平。采用将血清先用胰蛋白酶酶解,再加入三氯乙酸的前处理法进行HPLC检测。结果:当空白高原鼠兔血清加入抑制剂标准品达到血清中浓度为0.05 mmol/L、0.1 mmol/L、1 mmol/L、10 mmol/L、16.7 mmol/L、33.3 mmol/L、100 mmol/L时,抑制剂与血清蛋白的结合率分别为100%、100%、100%、86.84%、54.11%、40.10%、20.18%。在本文建立的方法下,回收率、精密度、稳定性均良好。N-isopropyl oxamate在0.0125~0.25 mmol/L内浓度与峰面积线性关系好。空白血清加入标准品达到终浓度为0.15 mmol/L、0.3 mmol/L和1 mmol/L时,平均回收率分别为98.05%、98.98%、98.12%;精密度相对标准偏差(RSD)分别为1.17%、0.92%、0.83%;稳定性RSD分别为1.38%、1.40%、0.88%。方法的重复性RSD为1.76%,最低定量限为0.0125 mmol/L。结论:N-isopropyl oxamate与高原鼠兔血清具有很强的亲和力,直接用三氯乙酸沉淀蛋白的前处理方法无法准确检测其浓度,而先用胰蛋白酶消化血清,再用三氯乙酸沉淀蛋白的方法可实现血液中HPLC的精确检测。     

RP-HPLC测定红丝线中香豆素的含量

采用反相高效液相色谱法,测定红丝线中香豆素的含量。色谱柱为ZORBAXXDB-C18(4.6mm×150mm,5μm);流动相:V(甲醇)∶V(0.01mol/L磷酸二氢钠溶液(pH5.4))=45∶55;流速:1mL/min;检测波长278nm。香豆素的线性范围为2.5~30mg/L(r=0.9998),回收率97.5%~101%。该法简便、准确,重复性好,适用于测定红丝线中香豆素的含量。     

高效毛细管电泳法直接测定红豆杉悬浮培养细胞中游离芳香族氨基酸

建立了红豆杉悬浮培养细胞中游离芳香族氨基酸的高效毛细管电泳的分离直接紫外吸收测定方法。在优化的实验条件下 ,以间苯二酚为内标 ,未涂层融硅毛细管 (75 μmi.d .,总长 37cm ,有效分离长度 30cm)为分离通道 ,40mmol/L磷酸缓冲液 (pH10 .46 )为电泳介质 ,3sec(0 .5 psi)压力进样 ,15kV恒压电泳 ,2 0 0nm检测 ,在 9min内三种氨基酸得到分离测定。色氨酸、苯丙氨酸和酪氨酸的线性范围分别为 2 .5 0～ 2 5 0 μmol/L(r =0 .996 2 ,RSD =2 .5 2 % )、1.2 5～ 2 5 0 μmol/L(r =0 .996 6 ,RSD =2 .12 % )和 2 .5 0～ 2 5 0 μmol/L(r=0 .9940 ,RSD =2 .93% ) ,苯丙氨酸回收率为 96 .8%± 1.37% ,酪氨酸回收率为 99.2 %± 3.0 4%。     

甜樱桃品种SSR-PCR反应体系的优化

以甜樱桃品种那翁为试材,研究了樱桃SSR技术中PCR反应体系的主要成分对SSR扩增结果的影响,并比较了采用聚丙稀酰胺凝胶及琼脂糖电泳检测扩增产物多态性的差异.结果表明:在PCR反应体系中,DNA最适浓度30～45 ng;Mg2+的最适浓度范围为1.5～3.0 mmol/L;dNTP最适浓度为0.2～0.3 mmol/L;引物的最适浓度为0.3～0.4 μmol/L;Taq聚合酶在20 μl反应体系中宜加入0.5 U.利用此反应体系,对24份樱桃代表资源进行了SSR反应,用6%的非变性聚丙稀酰胺凝胶电泳检测,扩增产物在100～250 bp之间,不同品种间DNA谱带多态性丰富.琼脂糖电泳检测的DNA多态性不如聚丙稀酰胺凝胶丰富.     

Determination of erythromycin in rat plasma with capillary electrophoresis-electrochemiluminescence detection of tris(2,2'-bipyridyl) ruthenium(II)

A fast and sensitive approach for determination of erythromycin in rat plasma was described. The method used capillary electrophoresis coupled with end-column electrochemiluminescence (ECL) detection of Ru(bpy)(3)(2+). The separation column used had an inner diameter of 75 microm. The running buffer was 15 mmol/L sodium phosphate (pH=7.5). The solution in the detection cell was 50 mmol/L sodium phosphate (pH=8.0) and 5 mmol/L Ru(bpy)(3)(2+). ECL intensity varied linearly with erythromycin concentration from 1.0 ng/mL to 10 microg/mL. The detection limit (S/N=3) was 0.35 ng/mL. The relative standard deviations, of ECL intensity and migration time for eight consecutive injections of 1.0 microg/mL erythromycin (n=8), were 1.3% and 1.8%, respectively. The method was successfully applied to erythromycin determination in rat plasma. The recovery ranged from 92.5 to 97.5%.     

RP-HPLC内标法测定5种中草药的齐墩果酸含量

建立了反相高效液相色谱-内标法测定了齐墩果酸的含量。以苯甲酸为内标物,C18反相柱（250mm×4.6mmi.d.,5μm）为分析柱,甲醇-水-冰醋酸（95：5：0.1）为流动相,流速1.0mL/min;检测波长210nm,柱温35℃。齐墩果酸浓度10.0～500mg/L范围内,对照品与苯甲酸的色谱峰面积比呈良好的线性关系。该方法准确、快速、灵敏度高、重现性好。     

Determination of MDMA and MDA in rat urine by semi-micro column HPLC-fluorescence detection with DBD-F and their monitoring after MDMA administration to rat.

A simultaneous semi-micro column HPLC method with fluorescence detection of abused drugs, such as 3,4-methylenedioxymethamphetamine (MDMA), 3,4-methylenedioxyamphetamine (MDA), amphetamine (AP) and methamphetamine (MP) in rat urine was examined by using 4-(N,N-dimethylaminosulphonyl)-7-fluoro-1,2,3-benzoxadiazole (DBD-F) as a labelling reagent and alpha-phenylethylamine as an internal standard (IS). A sample (50 microL) of rat urine was added to 5 microL IS and 100 microL 100 mmol/L borate buffer (pH 12) and extracted with 1.5 mL n-hexane. After evaporation, 50 microL 75 mmol/L borate buffer (pH 8.5) and 50 microL 20 mmol/L DBD-F in CH3CN were added to the residue and mixed well. The resultant solution was heated for 20 min at 80 degrees C and then cooled in an ice bath. A good separation of DBD-derivatives could be achieved within 45 min using a semi-micro ODS column with an eluent of CH3CN/CH3OH/10 mmol/L imidazole-HNO3 buffer (pH 7.0) (= 45:5:50, v/v/v %). The DBD derivatives were monitored at 565 nm with an excitation at 470 nm. The calibration curves showed good linearity (r = 0.997) with 0.5-15 ng/mL detection limits at a S/N ratio of 3. MDMA and MDA in rat urine could be monitored for 15 h after a single administration of MDMA to rat (2.0 mg/kg, i.p.). The concentrations for MDMA and MDA (n = 3) were 0.13-160.1 and 0.17-10.9 microg/mL, respectively.     

Determination of ibuprofen in pharmaceutical formulations using time-resolved terbium-sensitized luminescence.

A sensitive and specific luminescence method for the determination of ibuprofen (IB) in pharmaceutical formulations in aqueous solution is described. The method is based on the luminescence sensitization of terbium (Tb(3+)) by formation of ternary complex with IB in the presence of tri-n-octylphosphine oxide (TOPO) and Tween-20 as surfactant. The luminescence signal for Tb-IB-TOPO is monitored at lambda(ex) = 229 nm and lambda(em) = 545 nm. Optimum conditions for the formation of the complex in aqueous system, were 16 mmol/L TRIS buffer, pH 5.7, TOPO 200 micromol/L and 15 micromol/L of Tb(3+), which allows for the determination of 9.7 x 10(-7) - 9.7 x 10(-6) mol/L IB with a detection limit of 1.2 x 10(-7) mol/L. The relative standard deviations of the method were <1.4%, indicating excellent reproducibility. The proposed method was successfully applied for the assays of IB in pharmaceutical formulations with average recoveries of 100.3-102.5%.     

Determination of deferiprone in urine and serum using a terbium‐sensitized luminescence method

Optimized conditions, validation and practical applications of a new, rapid and specific fluorometric method for the determination of deferiprone (DFP) in urine and serum samples are reported. The proposed method, which is based on the formation of a luminescent complex with Tb³⁺ ion, is evaluated in terms of linearity, accuracy, precision, stability, recovery and limits of detection (LOD) and quantification (LOQ). Under optimum conditions (pH 7.5, [Tb³⁺] = 3 × 10^–4 mol/L, temperature 0 °C and excitation wavelength 295 nm), the relative intensities at 545 nm are linear, with the concentration of DFP in the range 0.072–13 mmol/L for urine and serum samples. The LOD and LOQ, respectively, are calculated to be 0.014 and 0.045 mmol/L for urine and 0.022 and 0.072 mmol/L for serum samples. The intra‐day and inter‐day values for the precision and accuracy of the proposed method are all < 5%, and the recovery of the method is in the range 97.1–103.8%. The method was applied to human urine and serum samples collected from patients receiving DFP. The results indicated that the method can be successfully applied to the determination of DFP in human urine and serum samples collected for clinical or biopharmaceutical investigations in which simple, rapid, cheap and specific determination methods facilitate and speed up the analytical procedure. Copyright © 2011 John Wiley & Sons, Ltd.