葛根提取的外文文献(11页).doc
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1、-葛根提取的外文文献-第 16 页Chemical Engineering and Processing: Process IntensificationVolume 47, Issue 12, November 2008, Pages 22562261Extraction of isoflavonoids from Pueraria by combining ultrasound with microwave vacuum Yang Hua, Tao Wanga, MingxiaoWangb, Sufang Hana, Pingyu Wana, Maohong Fanc, a Beijing
2、 University of Chemical Technology, Beijing 100029, China b General Hospital of China National Coal Group Corp., Beijing 110013, China c School of Materials Science and Engineering, Georgia Institute of Technology, Atlanta, GA 30332-0245, USA Received 24 December 2006. Revised 30 September 2007. Acc
3、epted 12 December 2007. Available online 11 January 2008. , How to Cite or Link Using DOI Permissions & ReprintsAbstractThis study proposes a new method to quickly extract and dry isoflavonoids from Pueraria Lobata Ohwi (Pueraria) by combining ultrasound and microwave technologies. The time required
4、 to extract isoflavonoids at comparable levels of production by ultrasound disruption was 20 times shorter than by conventional reflux extraction. Moreover, test results for drying the extracted substance from Pueraria show that the microwave-vacuum method is 10 times faster than the conventional tw
5、o-step vacuum approach. Finally, different instrumental analyses of isoflavonoids obtained from Pueraria using the proposed new method show that extraction by ultrasound disruption and microwave-vacuum drying affects neither the structure nor the composition of the extracted substance.Keywords:Extra
6、ction; Isoflavonoids; Microwave drying; Ultrasound1. IntroductionUltrasound has been used to extract compounds from the various parts of plants for more than three decades 1. Due to the disruption of cell walls and enhanced mass transfer of cell contents, ultrasound is able to accelerate the extract
7、ion of organic compounds from the bodies of plants 2and3. Compared with conventional solvent extraction, the use of ultrasound makes the extraction of valuable compounds more efficient by means of shorter time frames and lower extraction temperatures. Ultrasound is currently employed to extract such
8、 pharmacologically active compounds as polysaccharides, cellulose, flavonoids, saturated hydrocarbons, fatty acid esters, and steroids from plant materials 4.Microwave drying is often used to evaporate water in wood, foodstuffs, drugs, and ores, among other commodities 5and6; it can also be used for
9、 distillation 7 and extraction 8, 9and10. Combining the application of microwaves with vacuum techniques for drying offers two major advantages, namely, rapid drying due to the ability of microwaves to heat solvents instantaneously and homogeneously, and enhanced rate and extent of mass transfer at
10、sub-atmospheric pressure and low temperatures, which is essential for thermo-labile products. Such drying technologies are therefore important for industries such as pharmaceuticals 11.The present study of the extraction of isoflavonoids from Pueraria by ultrasound disruption, together with their dr
11、ying by means of combined microwave and vacuum technologies, offers an alternative to conventional technologies for extracting and drying isoflavonoids from Pueraria.2. Experimental2.1. Plant materials and chemicalsPueraria collected in Chinas Henan province was washed, dried, and cut into 5mm segme
12、nts. The standard sample of Puerarin was supplied by Chinas National Institute for the Control of Pharmaceutical and Biological Products. Analytical reagent-grade ethanol and ethyl acetate were used in all experiments.2.2. ExtractionFig. 1 shows the combined microwave-ultrasound experimental setup u
13、sed for extraction. The apparatus consists mainly of an extraction component (a), a microwave drying component (b) and a solvent recycling component (c). Ultrasound extraction was carried out using a CF-1520 50kHz 1200W ultrasound disintegrator. A GALANZ WP700L17 microwave oven with a Teflon evapora
14、ting dish was used for drying.Fig. 1.Schematic drawing of the apparatus used for extraction (a: extracting part; b: microwave drying part; c: solvent recycling part; 1: bracket; 2: ultrasound transducer; 3: beaker; 4: sealing gasket; 5: teflon evaporating dish; 6: turning plate; 7: microwave oven; 8
15、: teflon tube; 9: latex tube; 10: inlet; 11: outlet; 12: vacuum sucker).View thumbnail imagesTwenty grams of Pueraria were put into a 1000ml beaker for ultrasound extraction. After 400ml of 70% ethanol added, the beaker was put on the ultrasound disintegrator, followed by extraction under the ultras
16、ound horn for 30min at room temperature. Samples taken periodically were analyzed using an UV-2102PC UltravioletVisible (UVVIS) spectrophotometer.A reflux extraction experiment was also performed for purposes of comparison. After 20g of Pueraria were transferred into a 1000ml three-neck flask, 400ml
17、 of 70% ethanol was added. The mixture was stirred at 600rpm and refluxed for 120min, during which samples were taken periodically for analysis by UV spectrophotometer.2.3. Drying of extracted productA GALANZ WP700L17 microwave oven with a Teflon evaporating dish was used for drying the extracted pr
18、oduct. For recycling the solvent and ensuring safety, the microwave oven was made airproof by drilling a hole through its roof and passing a Teflon tube through the hole. The tube was connected to a vacuum system to withdraw steam and volatile chemicals, allowing water and organic solvents to be eva
19、porated by the microwave-vacuum apparatus.To initiate drying, 200ml of ultrasound-extracted resultant was put in an evaporating dish and placed in the microwave oven. The extracted resultant became solid in about 10min. Another 200ml of extracted resultant was dried using a rotating evaporator until
20、 no distillate came out, followed by drying it into powders for about 80min in an oven.2.4. Analytical methodsThe extracted Pueraria isoflavonoids were analyzed by UV at 250nm wavelength 12. The standard curve of absorbance versus Puerarin concentration was obtained in the following manner: ten mill
21、igrams standard sample of Puerarin was first put into a 50ml volumetric flask; then 95% ethanol was added to the scale, followed by shaking the mixture until it was homogeneous. Aliquots of solutions (0.2, 0.4, 0.6, 0.8, and 1.0ml) were taken from the flask and placed into 10ml volumetric flasks. 1.
22、0ml of ethanol was then added to each flask and deionized water was added to the flask scales to complete the preparation of standard solutions. Blank samples were prepared using the same procedures previously mentioned but without the addition of extracted isoflavonoids. The UV absorbance of blank
23、and each standard sample was measured at a 250nm wavelength.The extract resultant was analyzed as follows; one milliliter of extract was transferred into a 50ml volumetric flask followed by the addition of 95% ethanol to the scale and mixing. The solution was left overnight. One milliliter of supern
24、atant was then transferred into a 25ml volumetric flask; deionized water was added to the scale, followed by measuring the absorbance at 250nm. The concentration of isoflavonoids in the solution was obtained from the standard curve. The level of isoflavonoids in the sample is calculated as (1)where
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