酰基載體 的英文怎麼說
中文拼音 [jīzǎitǐ]
酰基載體
英文
acyl carrier-
Recently, ldl apheresis has been applied in clinic and achieves a satisactory effect. in this dissertation, the tripeptide, serine - aspartic - glutamic acid ( sde ), which existes in the cooh - terminal end of the seven repeats in the ligand binding domain of the ldl receptor and plays an important role in identifying ldl, was synthetized and immobilized onto the polyacrylamide ( paam ) beads as a bionic adsorbent for selective removal of ldl from plasma
本論文以絲氨酰-天冬氨酰-谷氨酸( sde )負電性三肽(此三肽廣泛存在於ldl受體配體結合域7個重復序列的羧基末端,對ldl受體特異性識別ldl起著重要作用)作為配體固定到聚丙烯酰胺微球載體上製成仿生性ldl親和吸附劑,考察其對人血漿中ldl及hdl的吸附功效。The preparation method of methyl 1 - naphthylacetate catalyzed by sulphuric acid, hydrochloric acid, chlorosulfonic acid, p - toluene sulfonic acid, amino sulfonic acid, strongly acidic cationic exchange resin, ferric chloride hexahydrate, stannic chloride pentahydrate, aluminium chloride, ferric sulfate, aluminium sulfate, titanium sulfate, sodium bisulfate monohydrate, solid super acid, heterpoly acid, support heterpoly acid, composite titanate and p - toluene sulfo - chloride etc. catalyst were reviewed
摘要評述了硫酸、鹽酸、氯磺酸、對甲苯磺酸、氨基磺酸、強酸性陽離子交換樹脂、六水三氯化鐵、五水四氯化錫、三氯化鋁、硫酸鐵、硫酸鋁、硫酸鈦、一水硫酸氫鈉、固體超強酸、雜多酸、固載雜多酸、復合鈦酸酯和對甲苯磺酰氯等催化劑催化合成1 -萘乙酸甲酯的方法。In the experiment, the full code sequence of bar gene was cloned by pcr from transgenic herbicide resistant bobwhite wheat and checked. it was expressed in e. coli and its protein was determined. after having been properly modified, the bar gene which correctly codes pat was cloned into binary vector pbi121 and then transferred into lba4404 by triparantal crossing, which is the prerequisite work for genetic transformation
本實驗從抗除草劑轉基因bobwhite小麥中,利用pcr克隆的方法擴增出bar基因全長,並在原核表達系統中表達,鑒定表達蛋白的活性,將能夠正確編碼ppt乙酰轉移酶的bar基因片段,經過適當的修飾構建入真核表達載體。Considering alcaligenes faecalis pencillin g acylase ( afpga ), which possesses the attractive characteristics for beta - lactam antibiotics conversions, the gene of pga was cloned into two expressing vector pkkfpga and psmlfpga. both the constructed plasmids psmlfpga and pkkfpga contained the pga gene, trc promoter and rrnb transcript terminator, differ in the replicon and antibotic marker, pkkfpga contained multicopy replicon ( cole 1 ) and ampicillin marker. while psmlfpga contained medium - copy replicon ( p15a ) and tetracycline marker
本文將糞產堿桿菌青霉素g酰化酶( afpga )基因構建表達載體pkkfpga和psmlfpga , pkkfpga和psmlfpga均含trc啟動子、青霉素g酰化酶基因、 rrnb轉錄終止子,其中pkkfpga含有氨卞青霉素抗性基因和cole1高拷貝復制子;而psmlfpga含有四環素抗性基因和p15a中拷貝復制子。Price, a. c. et al. " inhibition of b - ketoacyl - acyl carrier protein synthases by thiolactomycin and cerulenin. " j. biol. chem. 276 ( 2001 ) : 6551 - 9
硫乳黴素與淺藍菌素對酮酰基酰基載體蛋白合成酶的抑制作用, 《生物化學期刊》 276 ( 2001 ) : 6551 - 9Acetylornithine deacetylase is the key enzyme of producting l - methionine. we mainly do research work on the construction of acetylornithine deacetylase gene - engineering strain and characteristic of proteinase. in order to get high expression deacetylase strain, we obtain the gene by pcr arge gene. the product ( 2800bp ) was cloned into puc19 plasmid and confirmed with blue / white dot screening > restriction enzyme analysis and pcr. then taking the nucleotide sequencing compared with the sequence at blast of u. s. a. we constructed a high expression of gene - engineering strain - pxj 128 which containing the arge gene on the high expressing system of pxji18 with activity of acetylornithine deacetylase above 20000u / g
為了獲得高效表達的脫乙酰鳥氨酸酶工程菌株,在工程菌技術改造及其固定化研究做了進一步的研究和探討。我們採用基因工程技術,通過pcr技術擴增出了酰化酶關鍵酶基因?脫乙酰鳥氨酸酶基因arge ,將其克隆到puc19載體中,經酶切鑒定、 pcr鑒定篩選出重組陽性質粒,並測序鑒定,通過美國blast程序進行了基因數據庫相似性比較分析。In this experiment hcv structural gene was amplified by polymerase chain reaction ( pcr ), and was inserted into baculovirus expression vector pfastbacl to construct a recombinant transposing vector pfbl - cee. the plasmid pfb 1 - cee was transformed into dh1 obac competent e. coli cells. high molecular weight dna was prepared from the overnight cultures from the selected e. coli colonies, which was recombinant baculovirus shuttle vector containing hcv structural gene, named bac - cee
本實驗用pcr擴增hcv結構區基因,克隆到桿狀病毒表達載體pfastbacl中,構建成重組轉座載體pfb1 - cee ,轉化dh10bac大腸桿菌感受態細胞,篩選陽性菌落,抽提大分子質粒dna ,獲得含hcv結構區基因的重組桿狀病毒穿梭載體bac - cee ,脂質體介導轉染sf9昆蟲細胞,出現細胞病變后,收集含有重組桿狀病毒顆粒的培養上消,重新感染sf9細胞,收集sf9細胞,進行12 . 5 sds -聚丙烯酰胺凝膠電泳,可見表達的蛋白條帶。Study on method of extracting lead through emulsion liquid membrane taking dodecylbenzene - sulfonamido quinoline as a carrier
十二烷基苯磺酰胺喹啉作載體的液膜法提取水中鉛的研究In this paper, the relationship on inherent viscosity, degree of deacetylation and degree of carboxymethyl has been studied ; the preparation process of cx - 2, the histocompatibility and the animal cell culture have been described. the results provide foundational theories for preparation of the mcs and application in large - scale animal cell culture. cm - ch is a water - soluble derivative of chitosan
依次進行了cm - ch特性粘度、脫乙酰度、羧基化度的研究; cx - 2微載體的制備工藝優化研究; cx - 2微載體的組織親和性研究以及動物細胞培養實驗,為新型微載體的規模化制備及應用提供了一定的理論依據。4. the expressed result of pbv - a, pbv - b and pbv - c showed that the expressed protein was soluble and no inclusion body was been found. sds - page analysis show the molecular weight of protein expressed by phaa was 42kda which was equal to 3 - ketohilase, the molecular weight of protein expressed by phab was 26kda which was equal to acetoacetyl - coa reductase, and the molecular weight of protein expressed by phac was 63kda which was equal to pha synthase
表達載體pbv - a 、 pbv - b和pbv - c經誘導表達,發現所表達的蛋白均為可溶性蛋白,沒有包涵體出現;蛋白經sds ? page分析表明,基因phaa表達的蛋白分子量為42kda ,與?酮硫裂解酶分子量大小一致;基因phab表達的蛋白分子量為26kda ,與乙酰乙酰coa還原酶分子量大小一致;基因phac表達的蛋白分子量為63kda ,與pha合成酶分子量大小一致。分享友人