两种红树林植物海漆和海桑化学成分研究

本论文对两种红树林植物海漆 (Excoecaria agallocha L.) 和海桑（Sonneratia caseolaris L.）的化学成分进行了系统研究。 采用常规的硅胶柱层析、制备薄层层析、凝胶 Sephadex LH-20 柱层析、MCI柱层析、反相硅胶柱层析、半制备型 HPLC 以及重结晶等手段，从海漆 (Excoecaria agalloch L. ) 中分离得到 40 个化合物，从海桑（Sonneratia caseolaris L.）中分离得到 30 个化合物。利用各种现代波谱技术 (IR、UV、ESI-MS、EI-MS、1D-NMR、2D-NMR等) 及其化学物理性质，确定了海漆中 32 个化合物的结构，其中包括 1 个新的三萜天然产物以及 15 个首次从海漆中报道的化合物；确定了海桑中 27 个化合物的结构，其中包括 1 个新化合物和一个首次报道其碳谱数据的化合物。本文为首次报道海桑的化学成分研究。 对海漆和海桑粗提物及分离得到的部分化合物进行了抗肝癌细胞毒活性筛选，化合物S22表现出较强活性，其IC50为2.8 μg/mL；海漆和海桑粗提物及其它部分单体化合物只表现出微弱活性；阳性对照丝裂霉素C的IC50为1.1 μg/mL。 对分离得到的部分样品还进行了抗菌活性测试，各样品在测试浓度下对测试菌均未表现出明显的抗菌活性。 首次研究了海漆挥发性成分及其季节性变化。利用水蒸汽法提取了不同季节海漆的挥发性成分，通过GC-MS鉴定其化学组成，发现脂肪酸、二萜和倍半萜是海漆挥发性成分的主要组成，不同季节的挥发性成分差异较大。

两株海藻内生真菌次生代谢产物及其生物活性研究

海洋微生物拥有丰富多样的次生代谢途径，其中海洋生物内生真菌次生代谢产物研究日益受到天然产物化学界的重视。本论文以菌丝体生物量、发酵产物重量、抗菌与细胞毒活性、薄层色谱分析结果以及高效液相色谱分析结果等为评价依据对采自青岛沿海的13株海藻内生真菌在四种液体培养基上的静置发酵产物进行了综合评价，并从中选择了黑曲霉Aspergillus niger EN-13（分离自褐藻囊藻Colpomenia sinuosa）和杂色曲霉A. versicolor EN-7（分离自褐藻鼠尾藻Sargassum thunbergii）两株真菌进行了30升规模发酵（分别采用GPYM培养基和PDB培养）和化学成分的研究，对分离得到的大部分化合物进行了初步的生物活性筛选。 发酵提取物采用常规的硅胶柱层析、反相硅胶柱层析，凝胶Sephadex LH-20柱层析、制备薄层层析、半制备高效液相色谱以及重结晶等分离手段，得到单体化合物。利用各种现代波谱技术(IR、UV、EI-MS、FAB-MS、HR-ESI-MS、1H-NMR、13C-NMR、DEPT、1H-1H COSY、HSQC、HMBC等)并结合化学方法从两种菌株发酵提取物中鉴定了55个化合物的结构。其中从菌株A. niger EN-13分离鉴定了31个化合物，发现9个新化合物，包括2个鞘酯类化合物（AN-1~2）、3个萘并-γ-吡喃酮类化合物（AN-3~5）、3个苯乙基取代的α-吡喃酮类化合物（AN-17, AN-19~20）和1个甾体Diels-Alder加成产物（AN-21），另有1个新的天然环二肽（AN-27）被分离鉴定；从菌株A. versicolor EN-7分离鉴定了24个化合物，发现2个新化合物，为蒽醌AV-12与AV-17，另外，从前一菌株（A. niger EN-13）中鉴定的2个新鞘酯类化合物（AN-1~2）在A. versicolor EN-7中也被再次分离到。 对大部分单体化合物进行了抗菌活性、DPPH自由基清除活性和细胞毒活性测试。结果显示新化合物AN-1、AN-5和AN-20具有弱或中等强度的抑制白色念珠菌生长的活性，AN-4、AN-5、AN-21显示了弱或中等强度的抑制黑曲霉生长的活性，AV-12、AV-17显示了弱的抑制大肠杆菌生长的活性。在DPPH自由基清除活性筛选中，AN-5显示了中等强度的活性，其EC50为109.3 mM，与阳性对照BHT相近（EC50为81.8 mM）。其它部分已知化合物在抗菌和DPPH自由基清除活性的筛选中也显示了弱或中等强度的活性。在针对人肝癌细胞株SMMC-7721和人肺腺癌细胞株A549的体外细胞毒活性筛选中，所测样品均未显示显著活性。

A modified HPLC method for analysis of PSP toxins in algae and shellfish from China

Improvements to an established HPLC method are introduced. The modified method is more efficient for separation and detection of the toxins responsible for paralytic shellfish poisoning (PSP). The PSP toxin content of two strains of Alexandrium tamarense and approximately forty shellfish samples collected from different locations in China have been analyzed with this HPLC method. Only one shellfish sample, collected from Lianyungang, China, contained PSP toxins.

An efficient combination of supercritical fluid extraction and high-speed counter-current chromatography to extract and purify homoisoflavonoids from Ophiopogon japonicus (Thunb.) Ker-Gawler

Supercritical fluid extraction (SFE) was used to extract homoisoflavonoids from Ophiopogon japonicus (Thunb.) Ker-Gawler. The optimization of parameters was carried out using an orthogonal test L-9 (3)(4) including pressure, temperature, dynamic extraction time and the amount of modifier. The process was then scaled up by 100 times with a preparative SFE system under the optimized conditions of 25 MPa, 55 degrees C, 4.0 h and 25% methanol as a modifier. Then crude extracts were separated and purified by high-speed counter-current chromatography (HSCCC) with a two-phase solvent system composed of n-hexane/ethyl acetate/methanol/ACN/water (1.8:1.0:1.0:1.2:1.0 v/v). There three homoisoflavonoidal compounds including methylophiopogonanone A 6-aldehydo-isoophiopogonone A, and 6-formyl-isoophiopogonanone A, were successfully isolated and purified in one step. The collected fractions were analyzed by HPLC. In each operation, 140 mg crude extracts was separated and yielded 15.3 mg of methylophiopogonanone A (96.9% purity), 4.1 mg of 6-aldehydo-isoophiopogonone A (98.3% purity) and 13.5 mg of 6-formyl-isoophiopogonanone A (97.3% purity) respectively. The chemical structure of the three homoisoflavonoids are identified by means of ESI-MS and NMR analysis.

Analysis of the monosaccharide composition of fucoidan by precolumn derivation HPLC

We developed an HPLC method for analysis of the monosaccharide composition of fucoidans. The fucoidan was hydrolyzed into monosaccharides with 2 mol/L trifluoroacetic acid. Using ribose as the internal standard, the monosaccharide derivatives, obtained with 1-Phenyl-3-methyl-5-pyrazolone (PMP), were separated by reverse-phase HPLC using a gradient elution process, and monitored by ultraviolet detection at 245 nm. In the concentration range of 0.1-2.0 mmol/L, the peak area of each monosaccharide had a good linear relationship with its concentration (r(2)> 0.998). The average recoveries of mannose, rhamnose, glucuronic acid, glucose, galactose, xylose, and fucose were 86.2%, 95.1%, 62.5%, 102.0%, 94.8%, 66.6%, and 105.1%, respectively. This method was accurate and had good reproducibility and could be used to determine the monosaccharide contents of fucoidans.

Crystallographic and NMR studies on sterols from green alga Chaetomorpha basiretorsa Setchell

Chemical investigation of the ethanol extract of the marine green alga Chaetomorpha basiretorsa Setchell led to the isolation of a new sterol stigmast-4,28-dien-3 alpha 6 beta-diol 1 in addition to the five known sterols of beta-lawsaritol 2, saringosterol 3, 24-hydroperoxy-24-vinyl - cholesterol 4, beta-stigmasterol 5, 29-hydroxystigmasta-5, 24(28) -dien-3 beta-ol 6. Compounds were isolated by normal phase silica gel and Sephadex LH - 20 gel colum chromatography, reverse phase HPLC and recrystalization. Their structures were elucidated by spectroscopic methods including MS, IR 1D/2D NMR and X-ray analysis. Cytotoxicity of compounds was screened by using the standard WIT method. All these compounds were isolated from the green alga Chaetomorpha basiretorsa Setchell for the first time and they were inactive (50% inhibitory concentration was greater than 10 mu g /cm(3)) against KB, Bel -7402, PC - 3M, Ketr 3 and MCF - 7 cell lines.

The chemical constituents from red alga Gymnogongrus flabelliformis Harv.

Eight compounds were isolated from red alga Gymnogongrus flabelliformis Harv. In normal phase silica gel, Sephadex LH-20 gel column chromatography, reverse phase HPLC, and recrystallization. Based on MS and 1D NMR spectroscopic data, their structures were determined as: stigmast-4-en-3-one (I), cholest-4-en-3-one (II), cholesterol (III), uracil (IV), uridine (V), adenosine (VI), succinic acid (VII), and 5-hydroxy-4-methyl-5-pentyl-2,5-dihydro-furan-2-on (VIII). All of them were obtained from this species for the first time. Cytotoxicity of these compounds was screened using standard MTT method, but all the compounds were inactive (IC50 > 10 mu g/ml).

Residues of enrofloxacin, furazolidone and their metabolites in Nile tilapia (Oreochromis niloticus)

The residues of enrofloxacin and its metabolite in Nile tilapia (Oreochromis niloticus) were studied after oral dose of 50 mg/kg for 7 days. To find the differences between Nile tilapia and Chinese shrimp (Penaeus chinensis), the residues of enrofloxacin in P chinensis were also studied under the same conditions. The results showed that enrofloxacin metabolized into ciprofloxacin in both Nile tilapia and P chinensis, the maximal concentration of enrofloxacin in muscle, liver and plasma of Nile tilapia were 3.61 mu g/g, 5.96 mu g/g, 1.25 mu g/ml respectively, and ciprofloxacin in muscle was 0.22 mu g/g. The maximal concentration of enrofloxacin and ciprofloxacin in P chinensis were 1.68 mu g/g and 0.07 mu g/g respectively. The predicted withdrawal time for Nile tilapia was 22 days, and P. chinensis was 12 days under our experiment conditions. The residues of fitrazolidone [3-(5-nitrofurfurylidenamino)-2-oxazolidinone] and its main metabolite 3-amina-2-oxazolidinone (AOZ) in Nile tilapia were first determined by HPLC/MS. Results showed that after oral dose of 30 mg/kg for 7 days, the maximum concentration of farazolidone in Nile tilapia was 413 mu g/kg after 6 h, whereas AOZ residue reached its maximum (31 mu g/kg) right after stopping treatment. In contrast to the high metabolic rate of furazolidone, AOZ was very difficult to eliminate in vivo, thus the withdrawal time of furazolidone in Nile tilapia was 22 days at least. (c) 2005 Elsevier B.V. All rights reserved.

GC-MS法测定藏木香栽培品种挥发油的化学成分

[目的]基于气相色谱-质谱（GC-MS）法测定藏木香栽培品种挥发油的化学成分。[方法]采用水蒸气蒸馏法从藏木香栽培品种中提取挥发油,并用GC-MS联用仪对其挥发油的化学成分进行研究。[结果]分离并确认了37种成分,其主要成分是桉叶油二烯5,11（13）-内酯-8,12,异-榄香烯,异-喇叭烯,桉叶油二烯4,11（13）-内酯-8,12。[结论]分析获得的主要化学成分及其功效为藏木香这一天然药用植物资源的人工规范化栽培和进一步综合开发利用提供了科学依据。

RP-HPLC测定几种花类药材黄酮含量

目的：为充分利用花类药材，建立马蔺花、桃花、月季等15种花类药材中黄酮含量测定的RP—HPLC方法，并比较它们的含量。方法：花类药材用甲醇提取，反相高效液相色谱法分析药材中槲皮素、山柰酚、异鼠李素3种黄酮苷元。结果：采用KromasilC_18柱（4．6mm×250／mm，5μm），以甲醇-0．1％磷酸（50：50）为流动相，可使3种黄酮苷元达到基线分离，其中马蔺花含槲皮素1．536％，桃花含山柰酚0．572％，茶花含异鼠李素0．029％，皆为听测样品中最高。结论：本实验首次采用RP—HPLC法测定这15种花类药材的总黄酮含量，本方法操作简便，快速，准确，可作为黄酮的定量分析方法。

青海栽培和野生唐古特大黄蒽醌类成分的HPLC对比分析

采用HPLC法测定青海栽培唐古特大黄中的5种蒽醌含量,并和野生唐古特大黄药材进行了比较.结果表明,二、三、四年龄栽培唐古特大黄中芦荟大黄素、大黄酸、大黄素、大黄酚、大黄素甲醚5种蒽醌总量分别为1.21%,2.01%,1.62%,其中三、四年龄栽培唐古特大黄已达到<药典>规定的药用标准;野生大黄的总蒽醌含量远高于栽培大黄为3.64%.

藏药提宗龙胆和线叶龙胆花中四种苦苷类成分的HPLC测定

应用HPLC分析方法同时测定藏药提宗龙胆和线叶龙胆两种植物花中落干酸、獐牙菜苦苷、龙胆苦苷、獐牙菜苷4种苦苷类成分的含量.采用Econosphere C_(18)色谱柱(250×4.6 mm,5 μm),以甲醇-0.5%乙酸为流动相进行梯度洗脱,流速为1.0 mL/min;检测波长为245 nm.结果表明,除提宗龙胆中未检出獐牙菜苦苷外,其它成分均在两种植物中存在,但含量存在一定的差异.

藏药短管兔耳草中松果菊苷和麦角甾苷的RP-HPLC分析

建立了藏药短管兔耳草中松果菊苷和麦角甾苷含量的高效液相色谱分析法.采用Waters XTerra RP18色谱柱(150mm×4.6 mm,5μm),以甲醇-1%冰醋酸溶液(28:72,V:V)为流动相,流速1.0 mL/min,检测波长330 nm,柱温30℃,在20 min内分离检测了该两种化合物.松果菊苷和麦角甾苷进样量分别在0.077～4.950μg(r=0.999 9)和0.085～5.450μg(r=0.999 9)内呈良好线性,平均加样回收率分别为98.35%和92.50%,RSD分别为2.35%和2.86%.所建立的方法简便、快捷、结果准确可靠,重现性好,可用于藏药短管兔耳草的质量控制,并为兔耳草属植物中苯丙素苷类化合物的分离分析提供一定的参考.

抱茎獐牙菜中当药黄素的HPLC测定研究

[目的]采用反相高效液相色谱法对抱茎獐牙菜中当药黄素的含量进行测定。[方法]色谱柱为Kromasil C18（250min×4．60mm，5μm），流动相为甲醇-浓度0．02％磷酸水溶液，梯度洗脱，流速为1ml／min，检测渡长为260nm。[结果]当药黄素在0．92-4．60μg范围内线性关系良好，r=0．99950平均加样回收率为98．73％，RSD为0.31％。[结论]抱茎獐牙菜中当药黄素在花的部位含量最高。该测定方法适应性广，可用于测定抱茎獐牙菜中的当药黄素。

HPLC测定藏药帕朱胶囊中胡椒碱

帕朱胶囊是藏医最常用的治疗胃寒性疾病药物之一。收载于《中华人民共和国卫生部药用标准•藏药》（第一册），主要由寒水石、河子、石榴子、胡椒和荜茇等药物组成；功能主治健胃散寒，除痰、破痞瘤，养荣强壮。现代临床试验表明，帕朱胶囊对中晚期肿瘤患者有改善细胞免疫及体液免疫功能的作用，同时还可以减轻患者疼痛症状。尽管帕朱胶囊长期以来被广泛使用，但是却没有很好的质量控制标准。我们采用超临界CO2萃取方法提取帕朱胶囊的可溶性成分，并用GC—MS法对提取部位进行化学成分分析，发现其主要成分为胡椒碱，含量占提取物的44，2％。因此，本实验用HPLC法对帕朱胶囊中所含胡椒碱进行测定，以期建立胡椒碱的科学检测方法，提高产品质量控制标准。