鳖油的制备及其理化性质研究

利用传统炮制方法制备了鳖油 ,其得率为 5 8.31% ,并测定了其含量、酸价及皂化值等理化数据。其中多不饱和脂肪酸质量分数为 42 .47% ,GC分析结果二十碳五烯酸及二十二碳六烯酸烯质量分数分别为 14.82 %、19.10 %。     

三种鳖线粒体DNA细胞色素b基因序列的比较分析

对中华鳖、砂鳖和山瑞鳖线粒体DNA细胞色素b基因进行了引物设计、PCR扩增、序列测定和PCR-PFLP(Polymerase chain reaction-restriction fragment length polymorphism)分析。研究结果表明中华鳖、砂鳖与山瑞鳖线粒体DNACytb基因的序列全长相同,均为1140bp,其A、C、G、T含量相似,分别为378个(33.2%)、322个(28.2%)1、22个(10.7%)、318个(27.9%)、373个(32.7%)、324个(28.4%)、124个(10.9%)、319个(28.0%)、380个(33.3%)3、30个(28.9%)、127个(11.1%)、303个(26.7%)。同源性及序列差异率分析表明:中华鳖与砂鳖b基因序列的同源性为92.3%,中华鳖、山瑞鳖的为85.0%,砂鳖、山瑞鳖的为84.1%;中华鳖与砂鳖b基因核苷酸序列间的差异率为7.7%,中华鳖、山瑞鳖间的序列差异率为15.0%,砂鳖、山瑞鳖间的序列差异率为15.9%,而中华鳖、砂鳖、山瑞鳖各自个体间的序列差异率分别为2.37%、0.88%和0.18%,种间差异显著。用内切酶酶切分析其扩增产物,结果表明:用内切酶NdeⅠ可准确鉴别砂鳖,而用内切酶BamHⅠ则可准确鉴别山瑞鳖。内切酶NdeⅠ和BamHⅠ的联用分析,可使这三种鳖在分子水平都得到明确的鉴定。从三种鳖线粒体DNACytb基因核苷酸序列的显著差异和酶切位点的变化,可以进一步证明砂鳖是不同于中华鳖的鳖属一新种。     

松茸多糖提取方法的研究

利用不同温度 ,不同酸碱盐介质以及微波提取松茸多糖。结果表明 :用乙醚、甲醇将松茸子实体粉末进行回流提取后 ,再用质量浓度为 2 0g·L- 1 的Na2 CO3 溶液微波浸提 3次 ,可将松茸中的多糖及其它有效成分充分提取出来 ;其中松茸菌盖中提取的多糖质量分数为 3.6 5 %,菌柄中提取的多糖质量分数为 3.0 2 %。     

超声波辅助提取褐藻糖胶活性成分优化研究

研究了超声波辅助提取褐藻糖胶的新工艺,以“硫酸根+多糖”质量分数作为产品的主要理化指标,得到优化的提取工艺。硫酸根和多糖质量分数分别达到22.49%和36.97%。     

响应面法优化松茸发酵产多糖的培养条件

运用响应面法对松茸产多糖的发酵培养条件进行优化研究。首先根据C、N源实验结果,利用Plackett-Bur-man设计,对影响多糖产量的相关因素进行评估,筛选出具有显著效应的3个因素:玉米粉、豆粕和KH2PO4。在此基础上,利用最陡爬坡试验逼近以上3个因素的最大响应区域,采用Box-Behnken设计法对各因素的水平组合进行优化,获得松茸产多糖优化发酵的培养条件:玉米粉质量分数4.54%,豆粕质量分数4.96%,KH2PO4质量分数0.15%,MgSO4.7H2O质量分数0.05%,VB1质量分数0.001%,初始pH5.5,摇床转速180 r/min,发酵时间10 d。在此优化培养条件下松茸总多糖产量可达5.97 g/L。     

酶法脱蛋白提取大枣多糖工艺的研究

讨论了从提取环磷酸腺苷后的枣汁中提取枣多糖的最佳工艺条件,包括枣汁浓缩4倍,加无水乙醇调枣汁中乙醇体积分数为60%,醇沉5 h;木瓜蛋白酶脱蛋白效果最佳,木瓜蛋白酶液与枣汁的体积比为0.4∶ 1,温度60℃、pH5.0,酶解90 min,蛋白脱除率可达91.8%;AB-8树脂脱色,脱色率为73.64%,多糖得率为94.4%.红外光谱显示,提取的多糖与常规方法提取的多糖成分相同.     

响应面法优化酶法提取枸杞多糖的研究

选用响应面法优化及正交实验法进行淀粉酶提取枸杞多糖实验设计及分析。通过单因素实验后,正交实验确定淀粉酶酶解提取枸杞多糖的最佳条件为:pH=5.0,温度50℃,时间80 min,加酶量为0.5%,枸杞多糖提取率12.1%;响应面分析确定淀粉酶酶解提取枸杞多糖的最佳条件为酶解温度49.56℃、酶解时间140 min、酶浓度0.3%,枸杞多糖提取率为13.25%。酶法提取枸杞多糖比传统热水浸提提高了枸杞多糖的提取率,反应条件温和,而且通过响应面法进行实验设计和优化比正交实验法能得到更高的枸杞多糖提取率。     

低糖褐色乳酸菌饮品的稳定性研究

为提高低糖褐色乳酸菌饮品的稳定性,通过单因素实验研究可溶性大豆多糖和高脂果胶配比、H+浓度指数(pH值)以及蛋白质质量分数对其稳定性的影响;在此基础上使用Box-Behnken方法进行实验方案设计,对实验结果进行二次回归分析,优化得到最佳工艺参数:pH 3.71、蛋白质质量分数1.02%、可溶性大豆多糖和高脂果胶复配质量比例1.93∶1、总添加量0.4%,该条件下,沉淀率为2.51%。     

蛹虫草液体发酵产多糖的条件优化

多糖是蛹虫草Cordyceps militaris产生的重要活性成分。为提高其液体发酵胞外多糖的产量,通过单因素轮换法、方差分析、正交试验对蛹虫草菌株YCC-H产胞外多糖的发酵条件进行了优化。单因素结果表明液体发酵最适初始pH为5,最适葡萄糖浓度(质量分数)为6%,最适氮源为酵母膏,最适装液量为80 mL/250 mL,最适接种量(体积分数)为12%;在不同培养条件下菌体生物量变化较大;通过方差分析及正交试验进一步优化,结果显示：装液量(A)、氮源(B)、接种量(C)对蛹虫草产胞外多糖影响程度为B>A>C,最佳条件组合为A₂B₃C₂,即装液量80 mL/250 mL、酵母膏为唯一氮源、接种量(体积分数)为12%,其余因素选择单因素中最佳水平。经验证,该菌株合成胞外多糖的质量浓度达247.06 mg/L,较未优化前胞外多糖的产量23.67 mg/L提高了9.43倍。     

甜杏仁有效成份分析及多糖的体外抗氧化性研究

对甜杏仁的有效成份进行了分析并对其多糖的抗氧化性进行了研究,结果表明甜杏仁中脂肪、黄酮、多糖、蛋白质量分数分别为:46.53%、0.04%、1.73%、31%;抗氧化性研究表明0.2 g.L-1多糖液与同质量浓度Vc对羟自由基的清除相当,且对羟自由基.OH的抑制率随着质量浓度的增加而增强,质量浓度达到1.5 g.L-1时,清除率可达到88.8%。多糖液对超氧阴离子O2-.有很强的清除作用。     

宁夏不同地区灵武长枣果实多糖的单糖成分分析

以宁夏4个不同地区(灵武、中宁、青铜峡、银川)成熟期的灵武长枣果实为研究对象,经水提醇沉法提取,采用DEAE-cellulose52和HW-55S分离纯化,并利用GC-MS法进行多糖的单糖组成分析。结果表明:多糖提取率最高的是灵武地区,达到1.795%;分离纯化后,4个地区的长枣多糖各得到1个中性(Ju-0)和3个酸性组分(Ju-1、Ju-2、Ju-3),其中Ju-2含量最高;GC-MS分析可知灵武长枣多糖含有阿拉伯糖、鼠李糖、核糖、岩藻糖、木糖、甘露糖、半乳糖、葡萄糖、葡萄糖醛酸、半乳糖醛酸10种单糖,不含果糖,以阿拉伯糖、核糖、半乳糖和2种糖醛酸为主,木糖含量最低。各地区多糖的单糖组成、含量各不相同,从各组分来看,四个地区多糖的Ju-0和Ju-1组分组成均以阿拉伯糖、核糖、半乳糖为主,四个地区多糖的组成差异主要在于Ju-2和Ju-3组分。从各地区单糖总量来看,灵武地区是阿拉伯糖含量最高,中宁、青铜峡、银川地区以葡萄糖醛酸含量为最高。     

The extracellular polysaccharides of Rhizobium japonicum: Compositional studies

The extracellular polysaccharides of seven strains of Rhizobium japonicum were investigated by using a gas-chromatographic scheme developed for determination of the various sugars present. These polysaccharides were more heterogeneous in their composition than those of any other species of Rhizobium yet examined. Five strains (1809, 110, 123, 127, and 709) produced polysaccharides containing the same constituents, although in varying relative amounts: glucose (36–44%), galactose (7–25%), mannose (18–20%), 4-O-methylgalactose (5–13%), galacturonic acid (12–16%), and acetyl groups (4–8%). The sugars of the polysaccharide of strain 1809 were all of the d series. These are the first bacterial polysaccharides reported to contain 4-O-methylgalactose and the first Rhizobium polysaccharides in which galacturonic acid has been found. In contrast to this, the polysaccharide of strain 129 consisted of glucose (7%), galactose (51%), mannose (5%), xylose (5%), glucuronic acid (5%), and pyruvic acid (2%). The polysaccharide of strain 711 contained glucose (34%), galactose (13%), mannose (27%), and pyruvic acid (6%).     

Occurrence of pyruvic acid in capsular polysaccharides (K antigens) of klebsiellas

The capsular polysaccharides of 77 Klebsiella K-types were analysed for the presence of pyruvic acid. One half of the polysaccharides investigated were found to contain between 1.3 and 12% of the keto acid. A comparison between the analyses performed and the calculated values from some pyruvic acid containing polysaccharides of known structure showed that there is only in 5 out of 10 cases a good correlation with a regular substitution of the oligosaccharide repeating units.     

聚酰胺树脂分离纯化芦荟多糖的研究

文章采用聚酰胺吸附树脂,采用水、0．2M／LNaCl溶液、5％NaOH水溶液为洗脱剂梯度洗脱分离纯化,得到了三个芦荟多糖组分,通过IR、UV、GC等手段对其进行了分析。以甘露糖为标准,采用硫酸．苯酚法,测得水洗和NaOH水溶液洗脱所得多糖含量分别为90．10％和93．28％;以木糖、甘露糖、葡萄糖、半乳糖为单糖标准的GC分析结果显示：水洗所得多糖主要以甘露糖为主,同时含有少量的葡萄糖。     

Fractionation and characterization of polysaccharides from abaca fibre

Abaca fibre polysaccharides were fractionated into water soluble, pectic, 1% NaOH soluble, hemicellulosic and cellulose fractions by extraction with hot water, dilute hydrochloric acid (pH 1.6), aqueous 1% NaOH and 17.5% NaOH, respectively. Cellulose (60.4–63.6%) and hemicelluloses (20.8%) were the major polysaccharides in abaca fibres. The hot water soluble polysaccharides contained noticeable amounts of pectic substances and a large proportion of neutral polysaccharides. The pectic polysaccharide preparation was enriched in both galacturonic acid and neutral sugars, including xylose, glucose, galactose, arabinose, and rhamnose. Extraction of the fibre with aqueous 1% NaOH produced the hemicellulose–lignin complex, which was enriched in xylose and, to a lesser extent, glucose-, arabinose- and galactose-containing polysaccharides, together with 7.6% associated lignin. Further extraction of the delignified fibre residue with aqueous 17.5%. NaOH removed the hemicellulose fractions, which were strongly enriched in xylose-containing polysaccharides. Besides ferulic and p-coumaric acids, six other phenolic monomers were also detected in the mixtures of alkaline nitrobenzene oxidation of associated lignin in all the polysaccharide fractions. The content of bound lignin in water soluble, pectic, and 1% NaOH soluble polysaccharides (Fractions 1, 2, and 3), isolated directly from the lignified fibres, was 12 times that of the hemicellulosic preparations (Fractions 4 and 5) isolated from the delignified fibre residues.     

The quantitative immunochemical determination of pneumococcal and meningococcal capsular polysaccharides by light scattering rate nephelometry

A quantitative nephelometric method was used for the measurement of the individual pneumococcal, as well as meningococcal, polysaccharides in the polyvalent vaccine final containers. This method is simple, rapid, inexpensive, and provides both qualitative and quantitative analyses of the polyvalent polysaccharide vaccines. By this method the individual pneumococcal types, 1, 2, 3, 4, 6A, 7F, 8, 9N, 12F, 14, 18C, 19F, 23F and 25 polysaccharides, were found to be present at 90-114% of the manufacturer's indicated concentrations; meningococcal group A, C, Y and W135 polysaccharides were at 90-108% of the manufacturer's listed concentrations. This nephelometric method coupled with gel filtration can also be used for measurement of the molecular sizes or stability of individual polysaccharides in the final container. Pneumococcal polysaccharide types 3, 6A, 9N and 19F, used as representative types, were treated with 0.5 N hydrochloric acid. The molecular sizes for types 3 and 9 N polysaccharides were stable to acid treatment. In contrast, types 6A and 19F polysaccharides were degraded. Heating meningococcal groups A, C, Y and W135 polysaccharides at 37 degrees C for 48 h did not affect their molecular size in the polyvalent vaccine.     

Extraction of polysaccharides and the antioxidant activity from the seeds of Plantago asiatica L

The extraction conditions of polysaccharides from Plantago asiatica L. seeds were investigated. Four parameters affecting the polysaccharides extraction, extraction times, water to sample, extraction temperature and single extraction time, were determined by orthogonal experiments. Under the optimized conditions, the polysaccharides yield of P. asiatica L. seeds was 2.467%. The antioxidant activities of the polysaccharides were investigated. The reducing power of the polysaccharides was dose dependent, and the reducing capacity of the polysaccharides was inferior to butylated hydroxytoluene, which is known to be a strong reducing agent. The scavenging rates of the polysaccharides on superoxide and 1,1-diphenyl-2-picrylhydrazyl radicals were79.7% and 81.4%, at polysaccharides concentration of 0.75 mg/mL, respectively, a scavenging rates approximately similar to that of 0.75 mg/mL ascorbic acid (83.5% and 85.1%, respectively). Furthermore, it exhibited a moderate concentration-dependent ABTS radical scavenging activity, ferrous ion chelating potency and H₂O₂ scavenging activity. The data obtained in the in vitro models clearly establish the antioxidant potency of the polysaccharides extracted from Semen Plantaginis.     

Composition and properties of pectin polysaccharides of St. John’s wort Hypericum Perforatum L.

Three fractions of acidic water-soluble polysaccharides (concentration of glucuronic acid 10?C65%) were obtained from the above-ground part of St. Johns wort Hypericum perforatum L. by serial extraction with water and 0.7% aqueous solution of ammonium oxalate. Enzymatic hydrolysis of these polysaccharides using endo-polygalacturonase indicates that their carbohydrate chains contain the units of galacturone formed by 1,4-??-linked residues of non-substituted D-galacturonic acid. The extracted polysaccharides have been purified by means of gel filtration. It has been shown that water-soluble polysaccharides obtained by extraction with water manly contain the residues of galactose, mannose, glucose, and arabinose (the concentration of glucuronic acid being 10?C27%) while the polysaccharide fraction extracted using 0.7% aqueous solution of ammonium oxalate is presented by pectin polysaccharides. Only the residues of galacturonic acid (55?C72%) have been identified among glucuronic acids in its composition using chromatography/mass spectrometry of trimethylsilyl derivatives. In addition, this fraction contains the residues of the neutral monosaccharides which are typical for pectins: arabinoses, galactoses, rhamnoses, and glucose; there are also minor concentrations of residues of xylose and mannose. IR spectra of pectin polysaccharides of St. John??s wort have absorption bands in the ranges 1740, 1640?C1620, 1236?C1200, and 1200?C1000 cm^?1 which are typical for pectins. It has been demonstrated that aqueous solutions of pectin polysaccharides of St. John??s wort (2 mg/mL) have pronounced antioxidant activity (44% of the activity of trolox taken for 100%).     

乌梅丸水提液中多糖理化性质分析及预防结肠炎的作用

目的:考察乌梅丸水提液中多糖含量,建立HPLC法分析乌梅丸多糖分子量及单糖组成方法,观察其对右旋葡聚糖硫酸钠(DSS)所致小鼠溃疡性结肠炎(UC)的预防作用,为乌梅丸临床用药及药理活性成分的研究提供依据。方法:采用水提醇沉法提取多糖;硫酸-苯酚法测定乌梅丸多糖含量;凝胶色谱法-龙智达分子量工作站测定多糖分子量;PMP柱前衍生化法HPLC分析单糖组成;DSS(3%)法建立UC小鼠模型。ICR小鼠50只随机分为5组:正常组,模型组,乌梅丸多糖2.5%,5%,10%剂量组,每组10只。造模前7天,在乌梅丸多糖治疗各组的小鼠饮水中添加乌梅丸多糖,一直给药维持至实验结束(第14天)。结果:葡萄糖在0~0.08 mg·m L-1浓度范围内呈良好的线性关系(r=0.998);右旋葡聚糖酐标准品分子量在2500~2000000 Da范围内呈良好线性关系(r=0.998);乌梅丸水提液中多糖含量为40.3%,纯化的乌梅丸多糖糖含量为91.6%;分子量范围在171343~525009 Da之间,分布系数D=1.18;其多糖的单糖组成主要为甘露糖、葡萄糖醛酸、葡萄糖、半乳糖和木糖组成,其相对含量比为1.8:1.0:19.3:32.8:4.2;乌梅丸多糖能降低结肠组织损伤程度。结论:多糖可能是乌梅丸汤剂中有效的活性成分,对小鼠UC有一定的防治作用,其理化性质分析方法简便快速,结果准确,重复性好,可作为乌梅丸多糖的质量控制方法。     

Sulfated polysaccharides from marine green algae Ulva conglobata and their anticoagulant activity

Sulfated polysaccharides from the green algae Ulva conglobata were isolated and prepared by extraction in hot water, precipitation with ethanol and purification by ion-exchange and size-exclusion column chromatography. The characterizations of the sulfated polysaccharides were defined, and containing 23.04–35.20% sulfate ester groups, 10.82–14.91% uronic acid and 3.82–4.51% protein. Gas chromatography analysis shows that the sulfated polysaccharides from Ulva conglobata are mainly consisted of rhamnose with variable contents of glucose and fucose, trace amounts of xylose, glactose and mannose. The anticoagulant properties of the sulfated polysaccharides were compared with those of heparin by studying the activated partial thromboplastin time using normal human plasma. The sulfated polysaccharide from Ulva conglobata collected in Qingdao, China is the most potent among the sulfated polysaccharides tested. The mechanism of anticoagulant activity mediated by the sulfated polysaccharides is due to the direct inhibition of thrombin and the potentiation of heparin cofactor II.