硫酸化酶 的英文怎麼說

中文拼音 [liúsuānhuà]
硫酸化酶 英文
sulfurylase
  • : 名詞[化學] sulphur; sulfur [美國] (16號元素, 符號s)
  • : 酸構詞成分。
  • : 名詞[生物化學] (生物體的細胞產生的有機膠狀物質) enzyme; ferment
  • 硫酸 : [無機化學] sulphuric acid; sulphoacid; vitriol; vitriol oil; dipping acid; sulfuric acid; hydric ...
  1. Zhang y, xie q, guo y, et al., a study on adsorption of electrogenerated cystine precipitate onto au electrode using electrochemical quartz crystal impedance system. chinese chem. lett., 1999, 10, 1057

    張友玉,謝青季,袁玉等.溶菌在裸金電極和巰基乙或正十二烷基醇修飾金電極上的吸附.應用學, 2002 , 19 , 4
  2. Foodstuffs - determination of sulfite - enzymatic method

    食品.亞鹽的測定.
  3. Established in 1991, mainly produce human choroinic gonadotrophin ( hcg ), human menopausal gonadotrophin ( hmg ), urofollitropin ( fsh ), heparin sodium, chondroitin sulfate, sodium benzoate, polyaluminchloride ( water clarified reagent ) etc., we are the largest and the only enterprise which produce urinary items from crude to the injectable

    成立於1991年,主要生產絨促性素、尿促性素、卵胞激素、尿激、肝素鈉、軟骨素、苯甲鈉、聚合氯鋁凈水劑等,是中國最大的唯一的從尿液做到原料藥的生產廠家。
  4. This enzyme was different with the ones reported in the past. a phosphatase was isolated from the chloroplast thylakoid membrane of ipomoea aquatica, by nacl extration, ammonium sulfate precipitation, ion - exchange chromatography and hydrophic chromatography through butyl - toyopearl 650m column

    使用nacl抽提、銨分步沉澱、離子交換和butyl - toyopearl650m疏水柱層析等方法,從蕹菜葉綠體類囊體膜中分離純到一種蛋白磷
  5. Foodstuffs. determination of sulfite. part 2 : enzymatic method

    食品.亞鹽的測定.第2部分:
  6. Northern blot results show that nos. 66 - 1, 84, 89 - 1, 97, 108, 152, 175 and 233 have stronger signal in sp6 - tester than in sp6 - driver ; and no. 23 has weak signal only in sp6 - tester, nos. 94, 165, 172, 185 and 191 have similar hybridization signals in both sp6 - tester and sp6 - driver ; nos. 4, 17, 18, 28, 6 9, 101, 156 - 1, 157 - 1 and 183 do not reveal hybridization signals in both sp6 - tester and sp6 - driver ; the results of sequencing and blastn and blastx on ncbi indicate that no. 23 cdna ( 846bp ) has significant alignments with nicotiana tabacum mrna for elicitor inducible beta - 1 - glucanase nt - sube76, and arabidopsis thaliana clone 7119 for glycosyl hydrolase family 17 ( protein id : at5g55180. 1, supported by cdna : 7119, supported by cdna : gi _ l 87001 54 ) and arabidopsis thaliana beta - 1 - glucanase - like protein ( gi _ 2 1594590 ) ; no. 84 cdna ( 560bp ) has significant alignment with lotus corniculatus aspartate aminotransferase mrna ( complete cds length = 1685, gi | 2605931 | gb | af029898. 1 | af029898 ) for aspartate aminotransferase ; no. 89 - 1 cdna has significant alignment with arabidopsis tha

    與同源性最高的擬南芥類似晚期胚胎發生高豐度蛋白比較,二者都具有lea 2結構域、保守分泌蛋白cog5608結構域和低復雜度區,都具有pkc磷位點、酪蛋白激位點、 n十四酞位點和酚胺位點,所不同的是: ( )在結構功能域上, 152全長cdna編碼的蛋白質序列中多了1個lea 2結構域、 l個保守分泌蛋白cog5608結構域和1個低復雜度區; ( 2 )在功能位點上, 152全長cdna編碼的蛋白質具有酪氨位點、多了l個酪氨位點和1個可能的天冬氨富集區,但沒有n糖基位點; ( 3 )擬南芥類似晚期胚胎發生高豐度蛋白的lea 2結構域具有顯著性( e
  7. Medium experiments were arranged under uniform design, and then an optimum medium was got accordingly. the culture liquid was centrifugalized at 3, 500r / min for 30min, then ammonium sulfate was added into the supernatant to a final concentration of 30 % to precipitate the others

    通過銨分級沉澱、 deaesephadexa - 50陰離子交換凝膠層析和sephadexg - 75凝膠柱層析對發酵液進行分離和純,並得到電泳純的
  8. Thioredoxins, an ubiquitous small proteins with a redox active disulfide bridge in its conserved motif - cp ( g ) pc -, are universally distributed in eucaryote and procaryote and have a molecular mass of approximately 12kda. by its disulfide / dithiol interchange reaction, this protein can transmit the regulatory signals to seleted targets ( enzymes, transcription factors etc ) and plays an important role in many plant physiological processes that includes photosynthesis, dna synthesis, transcription, protein disulfide reduction, protein repair, filamentous phage assembly, cell apoptosis and seeds germinating and so on

    該蛋白質中含有保守的- cp ( g ) pc -氨基活性基序,該基序中的兩個半胱氨殘基可通過巰基二鍵的轉換實現其氧還原狀態的變和電子氫的傳遞,對細胞中與氧還原相關的多種生理過程的調節起重要作用。通過同許多類、蛋白類、細胞內活性因子相藕連, trx能對光合作用、 dna復制、基因轉錄、細胞凋亡和生長、噬菌體組裝、蛋白質的還原和修復信號傳導等生理過程產生影響和調節。
  9. Purification and characterization of phytase from a. niger an 01001 a. niger an01001 was inoculated on solid media and cultivated at 30 for 5 days. proteins were extracted from solid - state fermentation with 50mm acetate buffer ( ph5. 5 ). the molecule weight of the phytase protein was determined as about 78kd by sds - page. the purification procedures include ammonium sulfate precipitation, deae - cellulose ion - exchange chromatography, gel electrophoresis and electroelution

    3 .植的分離純及其性質研究黑麴黴ano1001經固體發酵,用緩沖液抽提后,經按沉澱, deae一纖維素離子交換層析,聚丙烯酞胺凝膠電泳和電洗脫等純步驟獲得的植,用sds一page檢測為一條均一譜帶,其分子量約為78kd 。
  10. - acetolactate decarboxylase is purifed from cell extract by 50 % - 80 % ammonium sulfate - fractionation, 50, 2min heat treatment and deae - sepharose fast flow column chromatography, which we study the different ph and different buffer of deae - sepharose fast flow column chromatography and conclude ph 6

    對其學性質進行了研究。 -乙酰乳脫羧經50 80銨分級沉澱、 50 , 2min熱處理、 deae - sepharosefastflow離子交換柱層析方法分離純
  11. - acetolactate decarboxylase are widely found among bacterial strains but not in other groups of organisms. the enzyme has been demonstrated to be effective for removal of acetolactate and widely used in beer product. in this paper, - acetolactate decarboxylase from bacillus subtilis was purifed to homogeneity from cell extract by ammonium sulfate - fractionation, heat treatment, deae - sepharose fast flow column chromatography

    本文對來源於枯草芽孢桿菌( bacillussubtilis ) 3226 - 5的-乙酰乳脫羧銨分級沉澱、熱處理、 deae - sepharosefastflow離子交換柱層析等分離純步驟,得到sds - paeg電泳純,通過n末端氨基序列分析驗證蛋白的純度。
  12. This paper stuffed with twelve important grain and vegetable crops, studied the injury symptom, dose reaction, injury threshold value and influential factor of main pollutant so2 on various plants, tested the dynamic transformation of pod, cat, mda, soluble protein, free pro and chlorophyll of resistant plant and sensitive of these physiological biochemical transformation with plant resistant ability. meanwhile, simply studied the protective role of the five compounds on plant. the result indicated the followings

    本實驗以12種重要的糧食和蔬菜作物為研究對象,研究了主要大氣污染物二氧( so _ 2 )對不同植物的傷害癥狀、劑量反應、傷害閾值以及影響因素,測定了抗性和敏感植物在受到so _ 2污染后植物體內過氧( pod ) 、過氧( cat ) 、丙二醛( mda ) 、可溶性蛋白質、游離脯氨和葉綠素的動態變,並分析了這些生理生和植物抗性的相互關系,同時還對5種合物溶液對植物的保護作用進行了初步研究,結果表明: 1
  13. The isolation and purification of dnaase in the earthworm the earthworm dnaase was purified from the tissue extract of earthworm by denaturing the protein with low ph buffer, high temperature, ammonium sulfate precipitation, deae - cellulose ( de52 ) chromatography and ultra - filter membrane

    雙胸蚓組織中dna的分離純雙胸蚓組織粗提取液經過選擇性變性、選擇性熱變性、按分段鹽析、 deae一纖維素( de52 )柱層析、超濾膜分級分離后得到一個電泳純的dna
  14. A novel aqueous two - phase system can be formed by the mixtures of a polymer and cationicanionic surfactants. such a system can be used as a partitioning system of proteins. in this work, we investigated the formation, phase behavior and protein partitioning in aqueous two - phase systems formed by dodecyltriethylammonium bromide / sodium dodecylsulfate / peg and dodecyltriethylammonium bromide / sodium dodecylsulfate / dextran. the ligands with affinity were attached to the polymers and the affinity partitioning of proteins was investigated. it was shown that the surfactants and polymers are enriched in different phases of aqueous two - phase systems. phase separation are promoted by increasing temperature and adding inorganic salts. different proteins are partitioned in different phases. the selectivity of protein partitioning is increased by adding ligands with affinity

    報道了由正負離子表面活性劑與高聚物混合溶液形成的一種可用於蛋白質的分離及分析的新型雙水相萃取體系.研究了正負離子表面活性劑(溴十二烷基三乙銨/十二烷基鈉)分別與葡聚糖和聚乙二醇混合雙水相體系的形成規律、相行為及牛血清蛋白和溶菌在雙水相體系中的分配.通過在高聚物分子中接上親和配基,研究蛋白質在雙水相體系中的親和分配.結果表明,在該體系中,表面活性劑與高聚物分別富集於不同相中.升高溫度及加入無機鹽均可促進雙水相體系的形成,不同蛋白質可分配于不同的相中.親和配基的引入極大地增強了蛋白質分配的選擇性
  15. To isolate and purify dnaase in the earthworm first, the tissue extract of earthworm was prepared by dissolving the earthworm with sucrose and denaturing the protein with low ph buffer. then dnaase was purified by denaturing the protein with higher temperature. the following steps were ammonium sulfate precipitation, deae - cellulose ( de52 ) chromatography and filtration by ultra - filter membrane

    雙胸蚓組織中dna的分離純採用蔗糖溶解雙胸蚓,並選擇性變性制備雙胸蚓組織粗提取液,再經選擇性熱變性、銨分段鹽析、 deae ?纖維素( de52 )柱層析及超濾膜分級分離對雙胸蚓組織中dna進行分離純
  16. This study was to investigate the effects of sulfur dioxide inhalation at different concentrations on some glutathione - related enzymes such as glutathione s - transferase ( gst ), glucose 6 - phosphate dehydrogenase ( g6pd ) and glutathione reductase ( gred ) in brain, lung, heart, liver, kidney and spleen of mice by the technology of biochemical toxicology. the results were showed as follows, so2 exposure at different concentrations caused the changes of glutathione redox system. moreover, the activities of antioxidative enzymes and the contents of reduced glutathione ( gsh ) were decreased significantly in different tissues at higher concentrations of soa

    本研究利用生毒理學技術研究了不同濃度二氧吸入( 22 2mg m ~ 3 , 64 3mg m ~ 3 , 148 23mg m ~ 3 )對純系昆明小鼠腦、肺、心、肝、腎、脾六種組織的谷胱甘肽還原( glutathionereductase , gred ) 、谷胱甘肽轉移( glutathiones - transferase , gst )和葡萄糖- 6 -磷脫氫( glucose6 - phosphmedehydrogenase , g6pd )活性的影響,結果表明so _ 2吸入使小鼠不同組織的谷胱甘肽氧還原系統發生了改變,表現為隨著so _ 2吸入濃度的增加,該系統中的抗氧活性的顯著變和抗氧物質水平的顯著降低,且存在著組織差異性。
  17. The enzyme retained full activity after being treated at room temperature for 1 hour at ph between 4. 0 and 11. 5. the enzyme can be incubated at 50 for 4h with only less 50 percent loss of activity and is stable in the frozen state. when streptomyces griseus atcc14811 was cultured in 10. 3 % sucrose yeme liquid medium, production of extracellular cholesterol oxidase increased for 5 days before decrease

    利用銨鹽析及deae -纖維素離子交換柱層析提取純灰色鏈黴菌atcc14811發酵上清液中的膽固醇氧,理性質研究表明作用晟適ph為8 . 0 ,最適溫度為45 , ph穩定范圍在ph4 . 0 - 11 . 5之間,在50條件下保溫4h ,仍保留54活力。
  18. The brine shrimp he was prepared and purified by 67 % ammonium sulfate precipitation, deae - sepharose fast flow ion - exchange chromatography, and sephacryl column gel - filtration, and its biochemical and enzymological properties were identified in this study. it was found that the deduced molecular weight of he in sds - page is about 98. 5 kda, and its proteolytic activity was optimized at ph of 7. 5 - 8. 5 and at temperature of 40, respectively

    我們利用67銨沉澱、 deae - sepharosefastflow陰離子交換柱層析和sephacryl凝膠過濾柱層析,並以酪蛋白為其蛋白水解活性的檢測底物、以卵膜為其卵殼裂解活性的特異性底物,從鹵蟲胚胎孵液中分離純出了鹵蟲的孵分子,其在sds - page電泳中的分子量約為98 . 5kda 。
  19. 3. the extracellular phb depolymerase was purified from 09 by using hydrophobic column chromatography and gel filtration technique in sephadex g - 100. the specific activity of the purified enzyme was increased by 37. 9 folds over crude extract, and the recovery yield was 8. 9 %

    以粗液為起始,經銨分級沉澱、 sephadexg - 100凝膠過濾后,分離純了該,純倍數約為37 . 9 ,活力回收率8 . 9 。
  20. The crude cellulases from liquid fermentation of b - 6 and ass. 3711 were isolated and purified by ( nh4 ) so4 precipitation, sephadex g - 100 and deae - sepharose cl 6b column chromatography. the cmcase components were purified and some of their physical and chemical properties were studied

    本文將液體發酵的液經銨分級沉澱、柱層析后得電泳純cmcase組分,並對as3 . 3711和b - 6來源的cmcase解動力學和理性質作了比較研究。
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