膠過濾 的英文怎麼說
中文拼音 [jiāoguòlǜ]
膠過濾
英文
gel filtration-
The separation of the formica rufa linnaeus samples by pel filtration chromatography. in this part, the author has primarily separated the formica rufa linnaeus samples by glucosan gel g - 50 filtration chromatography. the principle is the difference of the molecular weight of different components
紅褐林蟻樣品的凝膠過濾層析分離本部分旨在通過葡聚糖凝膠g - 50過濾層析初步分離紅褐林蟻樣品,根據分子量大小不同而達到分離目的。Strain bl21, and gene expression was induced by iptg. the target proteins were directed into the periplasmic space by the staphylococcal protein a signal sequence preceding the rgd - hirudin gene. using ion exchange chromatography and gel filtration chromatography, the chimera proteins were purified, and both of them showed a single band in tricine - sds - page. the results of activity analysis suggested that these two chimera proteins not only have antithrombin activities, but gain platelet aggregation inhibitory activities as well
通過離子交換層析和凝膠過濾層分別對兩種嵌合體蛋白進行純化,純化產物在tricine - sds - page中都顯示為單一條帶。活性分析結果表明兩種嵌合體蛋白在保留水蛭素抗凝血酶活力的同時,還呈現抗血小板聚集活性。6 - phosphogluconate dehydrogenase ( 6 - pgadase, ec 1. 1. 1. 44 ) was isolated by homogenate, ammunium sulfate fractionation, deae - sepharose chromatography, blue - sepharose affinity chromatography and gel filtration with sephadex g - 200 from bacillus subtilis, and some properties of the enzyme had been studied. a 113. 8 - fold purification was obtained with a 8. 2 % yield. the purified enzyme moved as a single electrophoretic band in page
將枯草芽孢桿菌超聲波破壁后的粗提取物進行分段鹽析、 deae - sepharose陰離子交換柱層析, blue - sepharosecl - 6b特異結合柱層析和sephadexg - 200凝膠過濾等純化步驟,得到聚丙烯酰胺凝膠電泳為單一蛋白區帶,比活為1 . 46u mg的酶制劑。Based on the extensive studies of subtilisin - like protease ( prl ) of metarhizium anisopliae, extracellullar serine protease is suggested to be a key enzyme involved in the fimgal penetration to invertebrates. the investigation of serine protease in the nematode infected by owvtl may help to understand the mechanism of nematophagous fimgi as biological control agents. a 3l kda serine protease was isolated and purified from the liquid culture of h rhossiliensis owvtl challenged with nematode panagrellus redivivus
本研究利用線蟲誘導下owvt - 1菌株液體發酵,通過粗分級分離、離子交換層析和凝膠過濾層析分離提純了一個分子量為31kda的絲氨酸蛋白酶,生物學測定表明其對大豆胞囊線蟲二齡幼蟲具有致死作用,同時測定了該酶理化特性,酶活力在75附近酶活力最高,隨著ph的增加酶的穩定性升高,與膽堿酯酶具有相似的ph曲線,對特異性底物aape ( suc - ala - ala - pro - glu - pna )具有作用, ssi和ci - 2抑制該酶的活性。The xerocomus spadiceus lectin, xsl, was isolated from extracts of fruiting bodies of the mushroom xerocomus spadiceus using a procedure that involved ( nh4 ) 2so4 precipitation, anion exchange chromatography on deae - cellulose, affinity chromatography on affi - gel blue gel, cation exchange chromatography on cm - cellulose, and gel filtration by fast protein liquid chromatography on superdex 75
從磚紅絨蓋牛肝菌( xerocomusspadiceus )子實體粗提物中,經過deae -纖維素陰離子交換層析、 affi - gelbluegel親和層析、 cm -纖維素陽離子交換層析和superdex75fplc凝膠過濾,純化了磚紅絨蓋牛肝菌凝集素。Our company, which is located in chengguan, ruian city, is an enterprise specializing in developing and manufacturing various skip - type banbury series products with tremendous technical strength and advanced assembly equipments. our products has assimilated advanced technology at abroad and integrated the productive characteristics in the rubber and plastic industries
瑞日橡塑機械有限公司地處瑞安市城關,是一家專業研製和生產各種翻斗式密煉機開放式煉膠塑機橡膠過濾擠出機冷喂料擠出機tpr , eva造粒機等橡膠設備橡塑機械繫列產品的企業。Using i - dopa as a specific substrate, phenoloxidase ( po ) from penaeus chinensis hemolymph was purified by gel - filtration and ion - exchange chromatography, and characterized in terms of its molecular weight and enzymatic properties in this study
本文以中國對蝦( penaeuschinensis )的血淋巴為材料,利用凝膠過濾和離子交換等方法,對酚氧化酶( phenoloxidase )進行了分離純化和生物化學性質研究。Glycoproteins were detected from the elution of classified proteins by gel chromatography. glycoproteins from the leaves of camellia sinensis were respectively detected by preparatory quality of gel chromatography and glycoprotein staining in sds - gel
各分級蛋白進行sephadexg - 100凝膠過濾,使分級蛋白中的蛋白質按其分子量的大小先後洗脫,從每個分級蛋白凝膠過濾的收集液中,鑒定了茶樹葉糖蛋白。Under these conditions the fibrinolytic activity of the supernatant can reach 820 urokinase units per milliliter broth. ba - dfe was purified from the supernatant of b. amyloiquefaciens dc - 4 culture broth by ammonium sulfate precipitation, ion - exchange chromatography on cm - and deae - sepharose fast flow, hydrophobic interaction chromatography on phenyl sepharose 6 fast flow and gel filtration on sephadex g - 50. the purified enzyme displayed thermophilic, hydrophilic and strong fibrinolytic activity
通過硫酸銨分級沉澱、 cm - sepharosefastflow和deae - sepharosefastflow離子交換層析、 phenylsepharose6fastflow疏水層析和sephadexg - 50凝膠過濾等方法,從解澱粉芽孢桿菌dc - 4的發酵液中分離純化出電泳純的ba - dfe 。The enzyme activity in fermentation liquid could be inhibited by pmsf and dfp. the fermentation liquor also showed good dehairing activity. the alkaline protease ( named dhap, dehairing alkaline protease ) in the fermentation liquid was purified with hydrophobic interaction chromatography, ion exchange and gel filtration
通過cm - sepharosefastflow離子交換層析, deae - sepharosefastflow離子交換層析, sephacryls - 100 , sephacryls - 200凝膠過濾層析,疏水層析等純化步驟對短小芽孢桿菌發酵液中的堿性蛋白酶進行了純化。Gel filtration chromatography, gfc
凝膠過濾色譜法It was unadsorbed on cm - cellulose in 10mmol / l naac - hac ( ph 5. 4 )
Sephadexg - 75凝膠過濾得到電泳級純的凝集素。Gel filtration chromatography
凝膠過濾色譜法Sds - page and sephcryl s - 200 gel filtration detected the molecular weight of dnaase
利用sds page及sephacryl 200凝膠過濾測定分于量。At last, we got the pure protein with the determination of electrophoresis. the molecular weight of the enzyme is estimated at 30903 through gel filtration and sds - page electrophoresis. the isoelectric point is 8. 6 ?. 3
經sds凝膠電泳和凝膠過濾層析兩種方法測定該酶的分子量分別為33113dalton和28840dalton ;其等電點pi = 8 . 6 0 . 3 。In order to attain bioactive glycoprotein, glycoprotein of the leaves of camellia sinensis, was purified from coarse glycoproteins purified by sephadex g - 100 gel chromatography, by cona - sepharose 4b affinity chromatography
為了純化天然糖蛋白,進行了茶樹葉糖蛋白的cona - sepharose4b親和層析,從sephadexg - 100凝膠過濾收集的粗糖蛋白中,分離茶樹葉糖蛋白。The apparent molecular weight of g6pd, determined by gel filtration, was 220kd ; the subunit molecular weight was 50. 5kd as determined by sds - page, suggesting that the native enzyme was a tetramer consisting of four identical subunits
凝膠過濾法測定該酶表觀分子量約為220kd , sds - page測定亞基分子量約為50 . 5kd ,可見該酶是由四個相同亞基構成的四聚體。The purified lectin showed a single protein band on sds - page, and the subunit molecular weight was 12kd. the molecular weight was 45kd determined by gel filtration on sephacryl s - 100. the result implied that there are four same subunits per lra
經sds - page檢測為單一蛋白帶,亞基分子量為12kd , sephacryls - 100凝膠過濾測得其表觀分子量為45kd ,表明lra是由四個相同亞基組成的蛋白。An antifungal protein, named as b16, was purified from the supernatant of the fermentation broth of strain 041381 by 80 % saturation ammonium sulfate, desalt and gel filtration on sephadex g - 75, which with molecular weight at about 30 - 40 kd on the basis of sds - page
菌株041381發酵上清液經70飽和度硫酸銨沉澱,透析脫鹽, sephadexg - 75凝膠過濾層柱,得到活性物質b16 。以sds - page膠為基礎進行電泳分析, b16的分子量為30 - 40kd 。5mmol / l h2o2 can completely kill the three kinds of enzymes. so we can come to the conclusion that sod in aloe is fe - sod. determined by sephacryl s - 200 column, the molecular weight of sod - i is approximately 46 000d, that of sod - ii is 35 000d, that of sod - iiiis 40 000d
可以判定該酶是鐵超氧化物歧化酶凝膠過濾法測得sod i的分子量約為46000d , sod 11的分子量約為35000d子量為, sod ill分子量約為40000d 。分享友人