313 resultados para HPLC-fluorescence
Resumo:
The three-dimensional fluorescence spectrum was used to detect the changes in dissolved organic substances from the cultured Skeletonema costatum, Alexandrium tamarense, Alexandrium mimutum, Scrippsiella trochodea, Prorocentrum donghaiense and Prorocentrum micans. The result indicates that all of the microalgaes can produce FDOM in the growth courses. Diatom such as Skeletonema costatum can produce humic-like FDOM. However dinoflagellate can produce protein-like FDOM at exponential growth phase. When the algae grows into decadency phase, the intensity of humic-like and protein-like fluorescence augments rapidly, which may be due to a mass of FDOM realeased by the old or dead cell fragmentation and the degradation of bacteria by using non-FDOM. The fluorescent intensity of Alexandrium tamarense, Alexandrium mimutum, Prorocentrum donghaiense and Prorocentrum micans can reduce at anaphase of decadency phase because of the degradation of bacteria and light. The same genus of algae can produce similar FDOM, for example: Alexandrium tamarense, and Alexandrium mimutum, Prorocentrum donghaiense and Prorocentrum micans, but the positions of the fluorescence peaks are different.
Resumo:
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.
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A method of hydride generation-atomic fluorescence spectrometry was proposed in the present paper for the determination of trace arsenic and selenium in jellyfish. The samples were treated by the combination of microwave digestion and lyophilization. The optimal conditions for treating and analyzing samples were established. The problem of the effect of the superfluous acid in the digesting solution on the results was solved, and the influence of coexisting foreign ions on the determination of arsenic and selenium was investigated. The accuracy of the method was confirmed by the method of standard additions. This method proved to be simple, rapid and repeatable, and is suitable for the analysis of biologic samples containing water.
Resumo:
Chromosome identification is an essential step in genomic research, which so far has not been possible in oysters. We tested bacteriophage P1 clones for chromosomal identification in the eastern oyster Crassostrea virginica, using fluorescence in situ hybridization (FISH). P1 clones were labeled with digoxigenin-11-dUTP using nick translation. Hybridization was detected with fluorescein-isothiocyanate-labeled anti-digoxigenin antibodies and amplified with 2 layers of antibodies. Nine of the 21 P1 clones tested produced clear and consistent FISH signals when Cot-1 DNA was used as a blocking agent against repetitive sequences. Karyotypic analysis and cohybridization positively assigned the 9 P1 clones to 7 chromosomes. The remaining 3 chromosomes can be separated by size and arm ratio. Five of the 9 P1 clones were sequenced at both ends, providing sequence-tagged sites that can be used to integrate linkage and cytogenetic maps. One sequence is part of the bone morphogenetic protein type 1b receptor, a member of the transforming growth factor superfamily, and mapped to the telomeric region of the long arm of chromosome 2. This study shows that large-insert clones such as P1 are useful as chromosome-specific FISH probes and for gene mapping in oysters.
Resumo:
Chromosomal location of the 5S ribosomal RNA gene was studied in the eastern oyster, Crassostrea virginica Gmelin. using fluorescence in situ hybridization (FISH). Metaphase chromosomes were obtained from early embryos, and the FISH probe was made by PCR (polymerase chain reaction) amplification of the 5S rRNA gene and labeled by incorporation of digoxigenin-1 1-dUTP during PCR. Hybridization was detected with fluorescein-labeled antidigoxigenin antibodies. Two pairs of FISH signals were observed on metaphase chromosomes. Karyotypic analysis showed that the 5S rRNA gene cluster is interstitially located on short arms of chromosomes 5 and 6. On chromosome 5, the 5S rRNA genes were located immediately next to the centromere, whereas on chromosome 6, they were located approximately half way between the telomere and the centromere. Chromosomes of C. virginica are difficult to identify because of their similarities in size and arm ratio, and the chromosomal location of 5S rRNA genes provides unambiguous identification of chromosomes 5 and 6. Previous studies have mapped the major rRNA gene cluster (18S-5.8S-28S) to chromosome 2. and this study shows that the 5S rRNA gene cluster is not linked to the major rRNA genes and duplicated during evolution.
Resumo:
Karyotype and chromosomal location of the major ribosomal RNA genes were studied in the hard clam (Mercenaria mercenaria Linnaeus) using fluorescence in situ hybridization (FISH). Metaphase chromosomes were obtained from early embryos. Internal transcribed spacers (ITS) between major RNA genes were amplified and used as FISH probes. The probes were labeled with digoxigenin-11-dUTP by polymerase chain reaction and detected with fluorescein-labeled anti-digoxigenin antibodies. FISH with the ITS probes produced two to four signals per nucleus or metaphase. M. mercenaria had a haploid number of 19 chromosomes with a karyotype of seven metacentric, four metacentric or submetacentric, seven submetacentric, and one submetacentric or subtelocentric chromosomes (7M + 4M/SM + 7SM + 1SM/ST). Two ITS loci were observed: one located near the centromere on the long arm of Chromosome 10 and the other at the telomere of the short arm of Chromosome 12. FISH signals on Chromosome 10 are strong and consistent, while signals on Chromosome 12 are variable. This study provides the first karyotype and chromosomal assignment of the major RNA genes in M. mercenaria. Similar studies in a wide range of species are needed to understand the role of chromosomal changes in bivalve evolution.
Resumo:
采用HPLC法同时测定了藏药达乌里秦艽中龙胆苦苷(gentiopicroside)、獐牙菜苦苷(swertiamarin)、獐牙菜苷(sweroside)和落干酸(loganic acid)4种主要环烯醚萜苷类成分,利用在线质谱(MS)进行了定性分析,并与同属藏药麻花艽进行了比较。色谱柱为Eclipse XDB-C_8(4.6 mm×150 mmi.d.,5μm),流动相A:体积分数5%乙腈(含10 mmol甲酸)水溶液,流动相B:体积分数95%乙腈水溶液,以流动相A在0~15 min内由100%线性减至90%,15~20 min内保持90%不变线性梯度洗脱。流速1.0 mL/min,检测波长240 nm,柱温30℃。结果表明,4种成分均达到了基线分离,具有较好的线性关系和回收率。本法可作为达乌里秦艽药材有效成分的测定方法,为其有效成分的进一步开发利用提供依据。
Resumo:
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。
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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%.
Resumo:
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.
Resumo:
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.
Resumo:
[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。
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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。
Resumo:
[目的]建立独一味药材HPLC指纹图谱,研究不同地区独一味药材的质量,为其质量控制提供有效的方法。[方法]采用RP-HPLC方法梯度洗脱,测定10批不同地区的独一味样品。[色谱备件]Kromasil C18柱(250mm×4.60mm,5μm),流动相为甲醇-0.4%的磷酸水溶液(55:45),梯度洗脱程序为0~70min,甲醇的体积分数由1%线性增加至15%;70~100min内,甲醇由15%线性增加至17%;100~130min内,甲醇由17%线性增加至20%;130~150min,甲醇由20%线性增加至100%;流速为1ml/min,检测波长为254n/n,柱温为30℃。[结果]确定了独一味药材中的7个共有峰。根据聚类分析结果,将独一味药材分为3类。[结论]该研究建立的方法重复性好,可用于不同地区独一味药材的质量评价,结合含量测定可用于独一味药材的质量的全面控制。
Resumo:
利用荧光衍生试剂1,2-苯并-3,4-二氢咔唑-9-乙基对甲苯磺酸酯(BDETS)作为脂肪酸柱前衍生化试剂,采用梯度洗脱在Eclipse XDB-C_8色谱柱上对游离脂肪酸(FFA)(油酸、亚油酸、软脂酸和硬脂酸)衍生物进行分离.利用柱后在线的串联质谱以大气压化学电离源(APCI)正离子模式实现了各组分的质谱定性.荧光检测的激发和发射波长分别为λ_(ex)=333 nm,λ_(em)=390 nm.脂肪酸的线性回归系数大于0.9990,检出限为3.38~6.59 nmol/L.建立的方法具有良好的重现性.利用此方法对超临界CO_2提取的唐古特白刺籽油中几种游离脂肪酸进行了分析.结果表明白刺籽油中含有大量的游离不饱和脂肪酸.
