毛萼香茶菜二萜化合物的高效液相色谱定量分析

本文报道用HPLC分离测定毛萼香茶菜(Rabdosia eriocalyx)中的二萜化合物。总二萜提取物在zorbax ODS柱上,用甲醇-水(70:30)作流动相,毛萼晶乙、毛萼晶丙等五个化合物在18分钟内能很好分离。以odonicin为内标,用峰面积比测定各组份的含量。结果符合一般含量测定的要求,此法可作为香茶菜二萜化合物一类生物活性物质的分析及发现新二萜化合物的前导性有效筛选手段。     

滇重楼种子中的甾体皂甙

我们在研究重楼属植物甾体皂甙的过程中寻找到一个活性甙Ⅶ,为了进一步开发利用资源,对栽培的滇重楼种子中的甾体皂甙进行了研究。 2 kg新鲜的滇重楼种子经甲醇热回流提取4次,合并回收甲醇得108 g,用石油醚脱脂后经D-101大孔树脂柱层析,从85％EtOH洗脱部分得粗甙12.5 g。粗甙经硅胶     

高效液相色谱-柱后光化学衍生法测定变性淀粉中黄曲霉毒素含量的研究

本文采用高效液相色谱-柱后衍生法对变性淀粉中的黄曲霉毒素G2、G1、B2和B1含量进行测定.样品采用乙腈-水(84:16,v/v)提取,经免疫亲和柱净化,C18色谱柱分离,以乙腈-甲醇-水(10:30:60,v/v)为流动相进行洗脱,用HPLC光化学衍生-荧光检测器检测样品含量.结果表明,4种黄曲霉毒素的标准曲线线性均...     

大孔吸附树脂分离富集苜蓿皂甙的研究

本项工作以对苜蓿皂甙的吸附量和解吸率为指标筛选大孔吸附树脂。研究结果表明,X-5吸附树脂具有较好的吸附性能和解吸效果。研究应用正交试验方法进一步对大孔吸附树脂分离纯化苜蓿皂甙的工艺条件进行试验分析,确定苜蓿皂甙分离富集的最佳操作条件为:上样浓度8mg/mL,色谱柱的径高比1∶7,药材-树脂比例1∶3;吸附完全后,先以水洗脱,除去杂质,再以50%乙醇洗脱,可以得到纯度较好的苜蓿皂甙。     

重楼属植物的化学数量分类学研究

重楼属植物是重要的药用植物。从1938年起,国内外科学家对它们的化学成分和药用价值已经进行了40多年的研究。我所从重楼属植物中分离鉴定了16个不同的甾体皂甙。本文利用高压液相色谱对重楼属植物甾体皂甙的定性和定量分析结果,根据L. B. Thien, W. H. Heimermann, R. T. Holman植物化学成分间的数量关系计算公式,对14种重楼的三组甾体皂甙含量进行计算,得出这14种重楼化学成分之间的数量关系,并画出数量关系图。     

南瓜籽抗前列腺增生化学成分研究

本文研究了南瓜籽抗前列腺增生活性及功效成分。南瓜籽乙醇回流提取,经石油醚萃取,硅胶柱、ODS反向柱层析柱分离,用核磁共振方法鉴定结构。结果表明:南瓜籽醇提石油醚萃取相经硅胶柱层析氯仿∶甲醇(8∶2、7∶3)梯度洗脱物对小鼠前列腺增生活性的抑制效果最明显,再经ODS柱分离,得到了三个单体化合物,分别为3-甲酸-1,4-环己二烯-2-十一烷酸甲酯(1),3-甲酸-1,4-环己二烯-2-十一烯酸甲酯(2),2-十一烯酸甲酯-3-十一烷酸-环己-1,4-二烯酯(3)。化合物1~3为首次从南瓜籽中分离得到的酯类物质。     

红花化学成分的分离与鉴定

目的:对菊科植物红花(carthmus tinctorius L.)的干燥花的化学成分进行研究。方法:运用硅胶柱色谱﹑Sephadex LH-20柱色谱﹑ODS柱色谱、制备HPLC等分离手段进行化学成分的分离纯化,根据理化性质及波谱数据鉴定其结构。结果:从红花体积分数70%乙醇水溶液的提取物中分离得到3个化合物,分别鉴定为(+)-松脂酚((+)-pinoresinol)(1)(+)-表松脂酚((+)-epipinoresinol)(2)槲皮素(3)结论:化合物1、2为首次从红花属植物中分离得到。     

山楂核(乙酸乙酯层)的化学成分Ⅱ

目的: 对蔷薇科山楂属植物山楂(Crataegus pinnatifida Bge.)核乙酸乙酯层化学成分进行研究。方法: 运用硅胶柱色谱﹑Sephadex LH-20柱色谱﹑ODS柱色谱、制备HPLC等分离手段进行化学成分的分离纯化,根据理化性质及波谱数据鉴定其结构。结果: 从山楂核体积分数70%乙醇水溶液的提取物中分离得到4个化合物,分别鉴定为香草酸(vanillic acid)(1)、香草醛(vanillan)(2)、异香草醛(isovanillan)(3)、丁香醛(syringaldehyde)(4)。结论: 化合物1-4均为首次从山楂属植物中分离得到。     

用高效液相色谱法(HPLC)测定肌苷中有关物质和降解产物

用HPLC测定肌苷中有关物质和降解产物 ,与主药有良好的分离效果。色谱柱为HypersilC1 8(2 5 0mm× 4 .6mm ,5 μm) ,流动相甲醇 -水 (甲醇与水体积比为 10∶90 ) ,流速 1mL·min- 1 ,检测波长 2 4 8nm。     

SPE-HPLC法快速检测发酵液中紫杉醇的含量

针对红豆杉内生真菌发酵液中紫杉醇的含量测定进行探讨,以建立快速高效低耗的检测方法.采用C_(18)固相萃取柱对紫杉醇进行吸附,用不同浓度的甲醇-乙酸铵和甲醇分别作为洗脱剂对其进行洗脱,比较两者的洗脱效果,洗脱液用HPLC进行检测;色谱条件为:流动相甲醇(v):水(v):乙腈(v)=20: 45: 35,流速:0.70 ml/min,检测波长:227 nm.结果表明,浓度为80%的甲醇溶液洗脱效果较好,紫杉醇的回收率为87.6%.     

Isolation and identification of the probing stimulants in the rice plant for the white-back planthopper, Sogatella furcifera (homoptera: delphacidae)

Adult females of the white-back planthopper, Sogatella furcifera, showed characteristic behavior of stylet sheath deposit on a parafilm membrane when fed on a 2% aqueous crude rice leaf and stem extract containing 15% sucrose. Subsequent bioassays revealed that the butanol-soluble fraction of the extract was highly active against the insects. When the butanol fraction was chromatographed on an ODS open column and eluted in sequence with a mixture of an increasing concentration of methanol in water, the 40 % methanol fraction was separated as the most active. A further bioassay of the HPLC components in the active fraction revealed that two major components (1 and 3) stimulated the high probing activity of the white-back planthopper only when they were combined. Of the active components, one component (3) was identified to be tricin 5-O-glucoside by spectroscopic analyses.     

Evidence for a DNA inversion system in Bordetella pertussis

An isolation procedure was developed to provide within one day microcystin-LR, a cyclic heptapeptide toxin from Microcystis aeruginosa PCC 7806. After ODS (octadecylsilyl) solid phase extraction, the crude toxin fraction was chromatographed using a strong anion exchange column. The toxin was eluted with 0.02 M ammonium bicarbonate. An at least 95% purity was revealed on HPLC separation by monitoring at 214 nm. Application of the procedure to the cyclic pentapeptide toxin nodularin from Nodularia spumigena AV2 was examined.     

法夫酵母 JMU-MVP14菌体中类胡萝卜素成分分析

结合薄层色谱、柱色谱、以及高效液相色谱对虾青素高产菌株-法夫酵母JMU-MVP14中的类胡萝卜素成分进行初步研究。研究结果表明,硅胶柱层析和氧化镁柱层析相结合的方法对法夫酵母JMU-MVP14菌体中的类胡萝卜素成分有很好的分离效果。经过柱层析分离纯化后,各组分中类胡萝卜素的种类单一,有利于进一步通过各种波谱技术对其进行定性。此方法弥补了单纯依靠高效液相色谱（ODS 柱）对法夫酵母 JMU-MVP14菌体中类胡萝卜素分离效果不佳,可供选择的商业化类胡萝卜素标准品少,液相保留时间漂移等因素给法夫酵母JMU-MVP14菌体中类胡萝卜素定性带来的不足。     

Comparative structural study of N-linked oligosaccharides of urinary and recombinant erythropoietins

The structures of the N-linked oligosaccharides of the urinary erythropoietin (u-EPO) purified from urine of aplastic anemic patients were analyzed and compared with those for recombinant erythropoietin (r-EPO) prepared with baby hamster kidney (BHK) cells. Asparagine-linked neutral oligosaccharides were released from each EPO protein by N-oligosaccharide glycopeptidase (almond) digestion. The reducing ends of the oligosaccharide chains thus obtained were aminated with a fluorescent reagent, 2-aminopyridine, and the mixture of pyridylamino derivatives of the oligosaccharides was separated by high-performance liquid chromatography (HPLC) on an ODS silica column. More than 8 and 13 kinds of oligosaccharide fractions for u-EPO and r-EPO (BHK), respectively, were completely separated by the one-step HPLC procedure. The structure of each oligosaccharide thus isolated was analyzed by a combination of sequential exoglycosidase digestion and another kind of HPLC with an amide-silica column. Furthermore, high-resolution proton nuclear magnetic resonance (1H NMR) spectroscopy and methylation analyses were carried out in the case of r-EPO (BHK).(ABSTRACT TRUNCATED AT 250 WORDS)     

Isolation of kappa-carrageenan oligosaccharides using ion-pair liquid chromatography--characterisation by electrospray ionisation mass spectrometry in positive-ion mode

Oligo-kappa-carrageenans participate as elicitors in the cell-cell recognition process in marine plants. Analytical methods can be usefully applied to gain insight into the biochemistry of these biological processes. Therefore, enzymatically digested oligomers of kappa-carrageenans have been separated and isolated on a Spherisorb ODS1 (250 x 4 mm i.d., particle size 5 microm) column using ion-pair liquid chromatography coupled with an evaporative light scattering detector. Heptylamine (5 mM, pH4) has been selected as the ion-pairing agent and MeOH as the organic modifier in a gradient mode. Overloading the column with 1mg of the mixture, the chromatographic mechanism presented adequate stability. The mobile phase of each isolated oligomer was evaporated and the residue was infused into an electrospray ionisation mass spectrometry (ESIMS) in positive-ion mode with 4:1 MeCN-water as mobile phase. Each ESIMS spectrum presented ions consisting of the oligomer attached with a number of heptylammonium ions depending on the molecule size. In addition, the different m/z values permitted direct detection of the oligomers in ESIMS positive-ion mode. The analytical method developed separated the oligomers up to dotriacontasaccharide.     

Purification of glycomacropeptide from non-dialyzable fraction of sweet whey by hydrophobic interaction chromatography on phenyl-agarose

Non-dialyzable fraction of sweet whey was chromatographed on a column of phenyl-agarose equilibrated with 0.01 M sodium phosphate buffer, pH 6.8 containing 5 M NaCl. Most whey proteins were adsorbed on the column, while the glycomacropeptide (GMP) was not. Amino acid analysis of the GMP fraction showed presence of traces (each < 1 residue/peptide) of arginine, histidine and phenylalanine which are not found in GMP. The estimated yield of GMP fraction was approximately 1.6 g l^-1 of sweet whey.     

Simultaneous determination of N2-(3-aminopropyl)biopterin (oncopterin), biopterin and neopterin by high-performance liquid chromatography with fluorescence detection

A high-performance liquid chromatographic method is described for the simultaneous determination of N²-(3-aminopropyl)biopterin (oncopterin, a newly found natural pteridine in urine from cancer patients), biopterin, and neopterin in urine. For the detection and quantification of the compounds, fluorometry was used. Using Develosil ODS K-5 and Develosil ODS HG-5 reversed-phase columns and a Nucleosil 100-5SA strong cation-exchange column, oncopterin, biopterin, and neopterin in urine were completely separated and assayed simultaneously by fluorescence detection. Similar values of oncopterin were obtained using each of the three columns, and the Develosil ODS K-5 reversed-phase column gave the most satisfactory separation. The sensitivity was high enough to measure 1 pmol of each pteridine. The HPLC method was highly reproducible. Our preliminary results indicate that oncopterin could be a most sensitive marker for cancer.     

Red Mexican grapefruit: a novel source for bioactive limonoids and their antioxidant activity

Citrus limonoids have shown to inhibit the growth of cancer in colon, lung, mouth, stomach and breast in animal and cell culture studies. For the first time in the present study, an attempt has been made to isolate antioxidant fractions and five limonoids from red Mexican grapefruit seeds. Defatted seed powder was successively extracted with hexane, ethyl acetate (EtOAc), acetone, methanol (MeOH) and MeOH/water and the extracts were concentrated under vacuum. Radical scavenging activity of 1,1-diphenyl-2-picrylhydrazyl (DPPH) and total phenolic content were also measured for comparison with the antioxidant capacity in the phosphomolybdenum method for the above extracts. Acetone and MeOH extracts, respectively, showed the highest (85.7%) and lowest (53.3%) radical scavenging activity, at 500 ppm. The total phenolic contents were found to be highest in the acetone extract (15.94%) followed by the MeOH extract (5.92%), ethyl acetate extract (5.54%) and water extract (5.26%). Antioxidant capacity of the extracts as equivalents to ascorbic acid (micromol/g of the extract) was in the order, EtOAc extract > acetone extract > water extract > methanol extract. Furthermore, the EtOAC and acetone extracts were loaded onto silica gel columns to obtain four limonoid aglycons. MeOH fraction was loaded onto a dowex-50 and sepabeads resin column to obtain a limonoid glucoside. The purity of the isolated five compounds was analyzed by HPLC using a C18 column and UV detection at 210 nm. Finally, the structures of the compounds were identified as obacunone, nomilin, limonin, deacetylnomilin (DAN) and limonin-17-beta-D-glucopyranoside (LG) using 1H and 13C NMR studies.     

Slow transacylation of peptidyladenosine allows analysis of the 2'/3'-isomer specificity of peptidyltransferase

2'-O-(N-acetyl-L-phenylalanyl-L-phenylalanyl)adenosine and 3'-O-(N-acetyl-L-phenylalanyl-L-phenylalanyl)adenosine (Ac-Phe-Phe-Ado) were chemically synthesized, and these two isomers were clearly separated from each other by high-performance liquid chromatography (HPLC) on an ODS column. By this HPLC method, the abundance ratio of the 2'-isomer and 3'-isomer in equilibrium in aqueous solution at pH 7.0 and 0 degrees C was found to be 0.30:0.70, and the equilibration rate was determined as 0.59 +/- 0.04 min-1. Thus, the rate of transacylation between the 2'-isomer and 3'-isomer of peptidyl-tRNA was found to be much slower than that for the two isomers of aminoacyl-tRNA. The HPLC method was used for isomer analysis of the product of the Escherichia coli ribosomal peptidyltransferase reaction. By the use of an isomerizable analogue, 2'(3')-O-L-phenylalanyladenosine (Phe-Ado), as the acceptor of the N-acetyl-L-[3H]phenylalanine (Ac-[3H]Phe) group in the Ac-[3H]Phe-tRNAPhe.poly(U).70S ribosome system, the reaction product was found exclusively to be the 3'-isomer of Ac-[3H]Phe-Phe-Ado. Thus, the slow transacylation of peptidyladenosine allows the analysis of the 2'/3'-isomer specificity of peptidyltransferase.     

大孔吸附树脂分离纯化地黄中梓醇工艺的研究

利用大孔吸附树脂分离提取地黄中梓醇。以地黄粗提液中梓醇含量为指标,高效液相色谱(HPLC)为含量测定方法,考察九种不同极性大孔吸附树脂对梓醇的吸附和解吸附性能,筛选出最佳树脂D101进行分离实验。结果表明,D101大孔吸附树脂的静态吸附容量为69.2mg/g干树脂,其吸附等温线符合Langmuir和Freundlich吸附等温式。采用5%乙醇作为洗脱剂,洗脱液减压浓缩后进行硅胶柱层析分离,氯仿：甲醇（8：2）梯度洗脱得到梓醇单体,纯度达90%以上,梓醇得率为6%。