An efficient method for extraction of astaxanthin from green alga Haematococcus pluvialis

Haematococcus pluvialis is one of the potent organisms for production of astaxanthin, a high value ketocarotenoid. Astaxanthin is accumulated in thick-walled cyst cells of Haematococcus. The thick cell wall is made up of sporopollenin-like material, algaenan, which hinders solvent extraction of astaxanthin. In the present study, an improved method for extraction of astaxanthin without homogenization of cells is reported. Extractability of astaxanthin from cyst cells was evaluated by treating cells with various solvents and pretreating the cells with organic and mineral acids at 70 degrees C followed by acetone extraction. Hydrochloric acid treatment facilitated 86-94% extractability of astaxanthin. Treatment time, temperature, and concentration of the acid were found to be critical factors for maximum extractability. The treatment did not affect the astaxanthin ester profile and the treated cells can be preserved until further use.     

Identification and quantification of astaxanthin esters in shrimp (Pandalus borealis) and in a microalga (Haematococcus pluvialis) by liquid chromatography-mass spectrometry using negative ion atmospheric pressure chemical ionization

Negative ion liquid chromatography-atmospheric pressure chemical ionization mass spectrometry [negative ion LC-(APCI)MS] was used for the identification of astaxanthin esters in extracts of commercial shrimp (Pandalus borealis) and dried microalga (Haematococcus pluvialis) samples. A cleanup step using a normal phase solid phase extraction (SPE) cartridge was applied prior to analysis. Recovery experiments with astaxanthin oleate as model compound proved the applicability of this step (98.5 +/- 7.6%; n = 4). The assignment of astaxanthin esters in negative ion LC-(APCI)MS was based on the detection of the molecular ion (M*-) and the formation of characteristic fragment ions, resulting from the loss of one or two fatty acids. Quantification of individual astaxanthin esters was performed using an astaxanthin calibration curve, which was found to be linear over the required range (1-51 micromol/L; r2 = 0.9996). Detection limits, based on the intensity of M*-, a signal-to-noise ratio of 3:1, and an injection volume of 20 microL, were estimated to be 0.05 microg/mL (free astaxanthin), 0.28 microg/mL (astaxanthin-C16:0), and 0.78 microg/mL (astaxanthin-C16:0/C16:0), respectively. This LC-(APCI)MS method allows for the first time the characterization of native astaxanthin esters in P. borealis and H. pluvialis without using time-consuming isolation steps with subsequent gas chromatographic analyses of fatty acid methyl esters. The results suggest that the pattern of astaxanthin-bound polyunsaturated fatty acids of P. borealis does not reflect the respective fatty acid pattern found in triacylglycerides. Application of the presented LC-(APCI)MS technique in common astaxanthin ester analysis will forestall erroneous xanthophyll ester assignment in natural sources.     

雨生红球藻诱变后生长速率和超微结构的变化

为探讨亚硝基胍(N-methyl-N’-Nitro-N-Nitrosoguanidine,NTG)对雨生红球藻(Haematococcus pluvialis)生长速率及超微结构变化的影响,用不同浓度的NTG处理藻类,对藻类的生长速率、色素含量和超微结构的变化进行了研究.结果表明:即使低浓度(0.5 g·L-1)的NTG对雨生红球藻也是致死的,致死率与NTG浓度呈正相关.藻类经中等浓度(2.5g·L-1) NTG诱变后,存活藻类的增长速率K值和虾青素含量分别达到0.381 ±0.0289和2.9±0.29 mg·L-1.低浓度NTG处理藻类其叶绿素含量略有上升,但高浓度(3.5g·L-1)时叶绿素含量明显减少.低NTG浓度处理时藻类细胞结构变化不大,但高浓度处理时细胞膜、线粒体及叶绿体等均遭受不同程度的损伤.本研究可为深入理解NTG诱变藻类的生理生化机制提供借鉴.     

CO2和乙酸钠对雨生红球藻生长及其虾青素积累的影响

雨生红球藻(Haematococcus pluvialis)是强抗氧化剂虾青素的天然优质来源,碳源是影响雨生红球藻虾青素产量的重要因素之一.为探究CO2和乙酸钠在雨生红球藻生长和虾青素积累中的作用,本研究通过测定生化指标和荧光定量PCR的方法,比较了这2种碳源对雨生红球藻干重、虾青素含量、生长相关酶及基因转录水平等的影...     

Hydrolysis kinetics of secoisolariciresinol diglucoside oligomers from flaxseed

Flaxseed is the richest dietary source of the lignan secoisolariciresinol diglucoside (SDG) and contains the largest amount of SDG oligomers, which are often hydrolyzed to break the ester linkages for the release of SDG and the glycosidic bonds for the release of secoisolariciresinol (SECO). The alkaline hydrolysis reaction kinetics of SDG oligomers from flaxseed and the acid hydrolysis process of SDG and other glucosides were investigated. For the kinetic modeling, a pseudo-first-order reaction was assumed. The results showed that the alkaline hydrolysis of SDG oligomers followed first-order reaction kinetics under mild alkaline hydrolytic conditions and that the concentration of sodium hydroxide had a strong influence on the activation energy of the alkaline hydrolysis of SDG oligomers. The results also indicated that the main acid hydrolysates of SDG included secoisolariciresinol monoglucoside (SMG), SECO, and anhydrosecoisolariciresinol (anhydro-SECO) and that the extent and the main hydrolysates of the acid hydrolysis reaction depended on the acid concentration, hydrolysis temperature, and time. In addition, the production and change of p-coumaric acid glucoside, ferulic acid glucoside and their methyl esters and p-coumaric acid, ferulic acid, and their methyl esters during the process of hydrolysis was also investigated.     

Hydrolysis kinetics of fenthion and its metabolites in buffered aqueous media

This study investigates the hydrolysis kinetics of fenthion and its five oxidation metabolites in pH 7 and pH 9 buffered aqueous media at 25, 50, and 65 degrees C. Five metabolites and three hydrolysis products were synthesized and purified. The reactant and the corresponding hydrolysis products were determined by HPLC. Rate constant and half-life studies revealed that fenthion and its metabolites were relatively stable in neutral media, and their stability decreased as pH increased. The half-lives at 25 degrees C ranged from 59.0 days for fenthion to 16.5 days for fenoxon sulfone at pH 7, and from 55.5 days for fenthion to 9.50 days for fenoxon sulfone at pH 9; half-lives were greatly reduced at elevated temperatures. The activation energy (E(a)) was found to range from 16.7 to 22.1 kcal/mol for the compounds investigated. The phenol hydrolysis product of fenthion and fenoxon, 3-methyl-4-methylthiophenol was not stable in pH 7 and pH 9 buffered solutions at 50 degrees C, whereas 3-methyl-4-methylsulfonylphenol and 3-methyl-4-methylsulfinylphenol were relatively stable under the same conditions. At pH 9, the primary hydrolysis mechanisms of fenthion and its oxidation metabolites were combination of hydroxide ion and neutral water molecule attacking on the P atom to form corresponding phenol derivatives. Under neutral conditions, the primary hydrolysis mechanisms of fenthion and its oxidation metabolites were assumed to be the combination of water molecule attacking on the P atom to form phenol derivatives and on the C atom to yield dealkylation products.     

Antioxidant activities of astaxanthin and related carotenoids

The antioxidant activities of astaxanthin and related carotenoids have been measured by employing a newly developed fluorometric assay. This assay is based on 4,4-difluoro-3,5-bis(4-phenyl-1, 3-butadienyl)-4-bora-3a,4a-diaza-s-indacene (BODIPY 665/676) as an indicator; 2,2'-azobis-2,4-dimethylvaleronitrile (AMVN) as a peroxyl radical generator; and 6-hydroxy-2,5,7, 8-tetramethylchroman-2-carboxylic acid (Trolox) as a calibrator in an organic and liposomal media. By employing this assay, three categories of carotenoids were examined: namely, the hydrocarbon carotenoids lycopene, alpha-carotene, and beta-carotene; the hydroxy carotenoid lutein; and the alpha-hydroxy-ketocarotenoid astaxanthin. The relative peroxyl radical scavenging activities of Trolox, astaxanthin, alpha-tocopherol, lycopene, beta-carotene, lutein, and alpha-carotene in octane/butyronitrile (9:1, v/v) were determined to be 1.0, 1.0, 1.3, 0.5, 0.4, 0.3, and 0.2, respectively. In dioleoylphosphatidyl choline (DOPC) liposomal suspension in Tri-HCl buffer (pH 7.4 at 40 degrees C), the relative reactivities of astaxanthin, beta-carotene, alpha-tocopherol, and lutein were found to be 1.00, 0.9, 0.6, and 0.6, respectively. When BODIPY 665/676 was replaced by 4,4-difluoro-5-(4-phenyl-1,3-butadienyl)-4-bora-3a, 4a-diaza-s-indacene-3-undecanoic acid (BODIPY 581/591 C(11)) as an indicator, astaxanthin showed the highest antioxidant activity toward peroxyl radicals. The relative reactivities of Trolox, astaxanthin, alpha-tocopherol, alpha-carotene, lutein, beta-carotene, and lycopene were determined to be 1.0, 1.3, 0.9, 0.5, 0.4, 0.2, and 0.4, respectively.     

Effects of phenolic propyl esters on the oxidative stability of refined sunflower oil

The oxidative stability of refined sunflower oil in the presence and in the absence of propyl caffeate (PC), propyl hydrocaffeate (PHC), propyl ferulate (PF), and propyl isoferulate (PI) has been evaluated according to the Rancimat method. The antioxidant activity of the phenolic derivatives was compared with that obtained with native [alpha-tocopherol (alpha-TOH)] and synthetic [propyl gallate (PG)] antioxidants. The results allow the establishment of a decreasing order of antioxidant power: PG > PHC > PC > alpha-TOH > PI > PF. The oxidative stability was improved neither by the addition of PF nor by a supplement of alpha-TOH. Moreover, a positive antioxidant effect was obtained for PC that was placed between those of alpha-TOH and PG. The antioxidant activity of PHC was higher than that of its analogue (PC). A dose-dependent effect was observed for PG, PHC, and PC. A chain-breaking mechanism was proposed for the antioxidant activity of propyl phenolic esters because the same ranking order of efficacy was obtained for their antiradical activities evaluated by using the 2,2-diphenyl-1-picrylhydrazyl radical method.     

Effects of riboflavin and fatty acid methyl esters on cholesterol oxidation during illumination

The effect of riboflavin or fatty acid methyl esters on cholesterol photooxidation was studied. Samples containing cholesterol, either alone or in combination with riboflavin or fatty acid methyl esters, were illuminated at 25 degrees C in an incubator for 28 days. The various cholesterol oxidation products (COPs) and cholesterol were analyzed by gas chromatography-mass spectrometry (GC-MS), and riboflavin was determined by HPLC. Results showed that the presence of riboflavin or fatty acid methyl esters facilitated production of COPs and degradation of cholesterol, and the degradation fits a first-order model. The COPs formed during light storage included 7 alpha-OH, 7 beta-OH, 7-keto, 3,5-cholestadien-7-one, 5,6alpha-EP, and 5,6beta-EP. The addition of riboflavin caused formation of 3,5-cholestadien-7-one through dehydration of 7-keto, whereas in the presence of docosahexaenoic acid methyl ester, the formation of 5,6alpha-EP or 5,6beta-EP was favored. Riboflavin was more effective for generation of COPs than fatty acid methyl esters.     

Isolation and purification of lutein from the microalga Chlorella vulgaris by extraction after saponification

A simple and efficient method for the isolation and purification of lutein from the microalga Chlorella vulgaris was developed. Crude lutein was obtained by extraction with dichloromethane from the microalga after saponification. Partition values of lutein in the two-phase system of ethanol-water-dichloromethane at different ratios were measured by HPLC so as to assist the determination of an appropriate condition for washing water-soluble impurities in the crude lutein. Partition values of lutein in another two-phase system of ethanol-water-hexane at different ratios were also measured by HPLC for determining the condition for removing fat-soluble impurities. The water-soluble impurities in the crude lutein were removed by washing with 30% aqueous ethanol, and the fat-soluble impurities were removed by extraction with hexane. The final purity of lutein obtained was 90-98%, and the yield was 85-91%.     

Hydrolysis and transformation of grape glycosidically bound volatile compounds during fermentation with three Saccharomyces yeast strains

The ability of three Saccharomyces wine yeasts (S. cerevisiae AWRI 838, S. cerevisiae AWRI 1537, and S. bayanus AWRI 1375) to liberate volatile compounds from sugar-bound aroma precursors was investigated using synthetic and grape glycosides under different experimental conditions. In model systems involving the incubation of yeast cells with either synthetic or grape-derived glycosides under conditions more favorable for glycosidase activities and less favorable for acid-catalyzed hydrolysis (pH 5.0 and 30 degrees C), all yeast strains studied proved to be capable of hydrolyzing glycosides, with S. bayanus AWRI 1375 displaying greater hydrolytic activity than S. cerevisiae AWRI 838 and AWRI 1537. During the fermentation of a chemically defined grape juice-like medium containing glycosidic precursors extracted from Vitis vinifera cv. White Frontignac (synonym Muscat à Petit Grains Blanc), all yeasts promoted a significant hydrolysis of different precursors, which varied according to the chemical structures of both the sugar and the aglycon moieties, as determined by GC-MS analysis of trifluoroacetylated derivatives. Hydrolysis of the White Frontignac derived glycosidic precursors during fermentation resulted in the release of monoterepene alcohols, terpene oxides, terpene diols, and 3-oxo-alpha-ionol, demonstrating the significant potential of these yeast strains to contribute to wine varietal volatile composition during alcoholic fermentation.     

Formation pathways of ethyl esters of branched short-chain fatty acids during wine aging

The particular behavior during wine aging of fermentative branched fatty acid ethyl esters, related to yeast nitrogen metabolism, compared that of their straight-chain analogues, related to yeast lipid metabolism, was first checked in 1-5 year aged Muscadet wines. Quantitative SIDA measurements showed that the levels of the former increased, whereas those of the latter decreased. Then, three hypothetical pathways suggested in the literature to explain these variations of branched esters were investigated. Two Muscadet and Sylvaner wines were spiked with levels of deuterated isobutanoic acid and its ethyl ester, similar to those of their natural analogues, then they were submitted to model aging. Quantitative SIDA measurements on the formation of these natural and labeled ethyl esters from the corresponding acids revealed that the behavior of the natural and labeled compounds were similar. The acid levels were much higher than the ester levels in the initial young wine, and a significant upward trend of their esterification ratios to those of the acid-ester equilibrium was observed with aging. Thus, this equilibrium proved to be the most effective in generating the branched fatty acid ethyl esters during wine aging. In contrast, the formation of these acids by Strecker-type degradation of wine amino acids in the conditions of the model aging or by hydrolysis of their glycoconjugates proved to be ineffective.     

青花菜贮藏期间颜色变化动力学模型的建立

该试验利用CIE-L^*a^*b^*(Commission International de I'Eclairage,国际照明委员会制定的色彩空间坐标表色系统)中的a^*、b^*、H°、TCD(Total Color Difference,总色差)以及叶绿素含量和黄化级数来衡量青花菜色泽的变化情况, 旨在建立贮藏期间多种颜色指标的动力学模型。试验组分为0℃、5℃、10℃条件下分别在HDPE(high-density polyethylene高密度聚乙烯)薄膜单球包装与不包装两种情况下进行。试验结果显示，包装提升了青花菜贮藏期间的活化能，延迟了呼吸跃变的启动。非线性回归分析的结果表明，色泽参数b^*和TCD的速率常数符合Arrhenius模型，模型符合一级动力学反应；而a^*和H°的变化则可用多项式表示。贮藏青花菜的黄化级数与色泽参数b^*之间具有良好的相关性，为利用计算机视觉系统进行颜色分级提供了理论依据。     

小黄鱼边角料的酶解工艺及酶解液性能研究

为开发利用小黄鱼边角料制备浓缩鱼汤,本研究采用酶解工艺对小黄鱼边角料进行酶解并对其酶解液的功能活性进行研究。以氨基酸态氮含量为指标,通过单因素及响应面试验探究酶制剂种类及添加量、pH值和酶解时间对酶解效率的影响;采用DEAE层析柱对酶解液进行分离纯化,SDS-PAGE凝胶电泳测定酶解多肽的分子量;通过测定酶解多肽对·OH和DPPH自由基的清除率、对细菌生长曲线的影响判断酶解多肽的抗氧化性和抗菌性。结果表明,以碱性蛋白酶为酶制剂,当酶与底物蛋白比为322 U·g^-1、固液比(m∶v)为1∶2、pH值为11.0、温度为55℃、酶解时间为2 h时,小黄鱼酶解液中氨基酸态氮含量为0.545 2 g·100g^-1;酶解液经DEAE柱分离得到了Ⅰ、Ⅱ、Ⅲ、Ⅳ四组多肽,其中组分Ⅲ多肽的分子量小于3.3 kDa;当酶解液中氨基酸态氮含量分别为8.62和25.59 mg·mL^-1时,对·OH和DPPH自由基的清除率分别约为80%和61%;组分Ⅲ多肽对枯草芽孢杆菌、酵母菌、金黄色葡萄球菌、大肠杆菌均有不同程度的生长抑制作用。本研究为小黄鱼边...     

Evolution and stability of anthocyanin-derived pigments during Port wine aging.

For three years, the evolution of the three major anthocyanidin monoglucosides (malvidin 3-glucoside, malvidin 3-acetylglucoside, and malvidin 3-coumaroylglucoside) and their anthocyanin-pyruvic acid adducts was monitored in Port wines stored in oak barrels. The degradation reactions of all pigments followed first-order kinetics in all the wines studied. The degradation rate constants of the anthocyanin-pyruvic acid adducts were much lower than those of the anthocyanidin monoglucosides. The results of both anthocyanins and pyruvic acid adducts show that acylation on the sugar moiety of all the pigments decreased their stability in wine. The levels of malvidin 3-glucoside-pyruvic acid adduct and its acylated forms increased right after wine fortification with wine spirit before starting to decrease around 100 days. The initial formation of anthocyanin-pyruvic acid adducts was concurrent with the degradation of anthocyanidin monoglucosides.     

高透光率青梅浓缩汁贮藏过程颜色的动力学研究

该文研究了高透光率青梅浓缩汁在贮藏过程中吸光度与贮藏温度、贮藏时间的关系,建立了颜色变化动力学模型,为高透光率青梅浓缩汁贮藏条件的优化控制及保质期预测提供了科学依据。结果表明：高透光率青梅浓缩汁的吸光度变化(A₀-A)符合Arrhenius模型,且为零级反应,其反应常数K₀为1.13×10⁷,活化能Ea为59.89 kJ/mol。经验证,该模型预测值与试验实测值的相关系数达0.999,表明该模型是合适有效的。     

Pretreatment and Enzymatic Hydrolysis of Sorghum Bran

Sorghum bran has potential to serve as a low‐cost feedstock for production of fuel ethanol. Sorghum bran from a decortication process (10%) was used for this study. The approximate chemical composition of sorghum bran was 30% starch, 18% hemicellulose, 11% cellulose, 11% protein, 10% crude fat, and 3% ash. The objective of this research was to evaluate the effectiveness of selected pretreatment methods such as hot water, starch degradation, dilute acid hydrolysis, and combination of those methods on enzymatic hydrolysis of sorghum bran. Methods for pretreatment and enzymatic hydrolysis of sorghum bran involved hot water treatment (10% solid, w/v) at 130°C for 20 min, acid hydrolysis (H₂SO₄), starch degradation, and enzymatic hydrolysis (60 hr, 50°C, 0.9%, v/v) with commercial cellulase and hemicellulose enzymes. Total sugar yield by using enzymatic hydrolysis alone was 9%, obtained from 60 hr of enzyme hydrolysis. Hot water treatment facilitated and increased access of the enzymes to hemicellulose and cellulose, improving total sugar yield up to 34%. Using a combination of starch degradation, optimum hot water treatment, and optimum enzymatic hydrolysis resulted in maximum total sugar yield of up to 75%.     

2,4-D丁酯的水解与光解特性研究

通过室内模拟试验,研究2,4-D丁酯在不同pH值和温度下的水解动态和在有机溶剂中的光解特性。结果表明,2,4-D丁酯的水解与光解均符合一级动力学方程。在pH7以下的缓冲溶液中,2,4-D丁酯的水解反应十分缓慢,但在碱性溶液中其水解速率加快。25℃下2,4-D丁酯在pH5、7和9的缓冲溶液中的水解半衰期分别为23.5、5.8d和10.7min。2,4-D丁酯的水解速率随温度升高而增加,在温度为15、25℃和35℃的pH7缓冲溶液中的水解半衰期分别为21.5、5.8、3.9d,平均温度效应系数为2.57。2,4-D丁酯水解反应的活化能与温度之间无明显相关性,而活化熵与温度呈显著相关性。2,4-D丁酯的水解主要由活化熵所驱动。采用GC-MS技术对2,4-D丁酯水解产物进行鉴定,确定水解产物主要是2,4-二氯苯氧乙酸和2,4-二氯苯酚。2,4-D丁酯在正己烷中光解速率比在甲醇中快,在丙酮中几乎不发生光解,其光解速率随浓度的升高而减慢。