瓊脂糖酶 的英文怎麼說
中文拼音 [qióngzhītáng]
瓊脂糖酶
英文
agarfitine-
Fourthly, according to the activity, collect, dialyse, freeze, dry respectively the sod protein through deae - sepharose column chromatog - raphy ; process the sod protein through sephacryl s - 200 column chromatography with the preceding method. at last, process the pure sod protein with same functional enzyme electrophoresis and active dye, isoelectric focusing electrophoresis and sds - page
將粗酶液過deae -瓊脂糖柱層析,得三個活力峰,分別收集、透析、乾燥濃縮后;再上sephacryls - 200凝膠柱層析,按與deae -瓊脂糖柱層析后同樣的方法收集處理。The page revealed the culture supernatant of the initial strain and the mutant contained different protein bands, which exactly demonstrated at protein level that a. niger j 506 was surely a mutant of a. niger m1. zymogram stained with xylan - remazol brilliant blue for detecting xylanase showed there are three different xylanases in the mutant culture, while two xylanases in initial strain. what is important, the third xylanase in a. niger j 506 have higher activity and more production levels from page and zymogram of xylanase
尤其是在木聚糖酶譜帶檢測中發現,突變株發酵液中有三種類型的木聚糖酶,而出發菌株中只有兩種類型的木聚糖酶,並且通過考馬斯亮藍g250染色和瓊脂糖板上的透明圈發現,突變株中第三種類型的木聚糖酶不僅表達量很大,活力也很高。To find dnaase in the earthworm the tissue extract of earthworm with different concentration reacted with rna, circular dna, linear dna for an hour at 37, then the producetion was detected by 1 % agrose gel. the tissue extract of earthworm, the tissue protein extract of earthworm and the tissue extract of earthworm without protein reacted with pbv220 - r - inf for an hour at 37, then the producetion was detected by 1 % agrose gel. 2
雙胸蚓組織中dna酶的發現用不同濃度的雙胸蚓組織提取液與rna 、環狀dna及線狀dna在37反應1小時後用1的瓊脂糖凝膠電泳對其反應產物進行觀察;雙胸蚓組織粗提取液、雙胸蚓組織蛋白粗提取液及雙胸蚓組織去蛋白提取液分別與pbv220 - ? inf質粒37反應1小時後用1的瓊脂糖凝膠電泳對其反應產物進行觀察。Extraction of large - fragment genomic dna in order to gain dna template of pcr amplification ( long pcr amplification and salvage pcr amplification ) which was high purity and large fragment, three methods were used to extract genomic dna of bacillus subtilis, i. e. low melting - point agarose embedding method, sds - proteinase k - phenol chloroform extraction method and bacterial genomic dna extraction kit method. the genomic dna of bacillus subtilis were gained by these methods, and the operated programs of the methods were improved. the results showed that the genomic dna extracted by low melting - point agarose embedding method were obviously biggest than that of another two methods
大片段基因組dna的提取為了獲得用於pcr擴增(長距離pcr擴增和分段pcr擴增)的高純度、大片段(至少為pcr產物長度的4倍)的dna模板,應用三種方法:低熔點瓊脂糖包埋法, sds -蛋白酶k -酚氯仿抽提法和細菌基因組dna提取試劑盒法,分別提取獲得了枯草桿菌基因組dna ,並對3種方法的操作程序進行了不同程度的改進,結果表明:低熔點瓊脂糖包埋法提取的基因組dna片段明顯大於后兩種方法,採用0 . 5瓊脂糖凝膠電泳3h ,仍然跑不出加樣孔。A method for preparation of antithrombin ( at - ) concentrated from human plasma ' s fraction has been described. after preliminary treatment of plasma with the cold ethanol, the isolation of at - iii from the precipitate was performed by affinity chromatography on heparin - sepharose cl - 6b ; desalted by dialysis and concentrated
從人體血漿中提取較高純度的抗凝血酶( at - )的,通過低溫乙醇處理血漿,得到的沉澱經肝素-瓊脂糖兩次親和層析,並透析、濃縮獲得at -的初品。Recovered the agarose and identified by agarose gelelectrophoresis. the producys of pcr fragments and pcambial303 plasmid ligation were transformed into e. coli ( dh5a ). the result of pcrof positive recombinant and restriction analysis demonstrated that the plant expressing vector of tps is attained
Pcr產物經回收后,經瓊脂糖凝膠電泳鑒定后,與pcambia1303連接並轉化大腸桿菌dh5a ,陽性重組子經pcr和限制性內切酶酶切圖譜分析,表明已獲得海藻糖- 6 -磷酸合成酶基因的植物表達載體。I and hindlll respectively. after the digested products were run via agarose gel electrophoresis and transferred into nylon membrane, the southern blot was carried out using the cdna of rubber tree etrl as probe. the result of the southern blot showed that a hybridization band ( - 3. 0kb ) turned up from the ecor i digested product and another band ( - 4. 8kb ) turned up from the hindi ]
從橡膠樹pr107品系的嫩葉提取基因組dna ,用限制性內切酶ecor 、 hinofll分別酶切,瓊脂糖凝膠電泳分離並轉膜后,用克隆的橡膠樹etri基因的cdna片段作探針進行southern雜交分析,結果表明, ecor酶切在約3 okb處有一條雜交帶出現, hi 。Main works and their important results are showed as following. firstly, the cdna encoding bullfrog gh is amplified by use of the total rna, extracted from adult bullfrog ' s pituitary, as the template, pi ( 5 ' - cggatcc atg gct tca ggg tta ggc ) and p2 ( 5 ' - cgaattc tta aaa ggt gca gtt gct ) as the primer pair and one particular cdna product, 660bp, was obtained after the rt - pcr - the product was purified by using dna agarose gel extraction method. after the purified cdna and pmd18 - t vector were ligated at 16 over night, the ligation products were transformed into e. coli strain dh5a and then the transformants were screened by clone pcr method
首先,以成體牛蛙的腦垂體總rna為模板,進行rt ? pcr擴增得到約660bp的特異性pcr產物帶,切下瓊脂糖凝膠中的特異產物帶進行cdna膠回收,將cdna與pmd18 ? t載體進行t ? a克隆連接並轉化到dh5 e . coli后,進行菌落pcr 、質粒酶切鑒定,篩選出陽性菌株,測序結果經blast分析,與已報道的牛蛙生長激素基因高度同源,證實此陽性克隆為牛蛙生長激素基因轉化子,命名為pbfgh 。The purified products were cloned into pgem - t - easy vector successfully, the cloned plasmids were transformed into e. coli. tgl. the specific recombinant plasmid was identified by molecular weight, pcr and restriction endonuclease analysis. the results indicated that the resultant construct contained the gene of interest hn at right orientation of the insert
經瓊脂糖電泳檢測,將大小與預計分子量一致的片段純化后連接到pgem - t - easy克隆載體中,再轉化大腸桿菌tgi感受態細胞,得到的轉化子經分子量比較、 pcr鑒定和酶切分析篩選陽性克隆。Construction, preparation and quantity of cea dna vaccine : plasmid pgem4 - cea containing full - length of cea cdna was cleaved by ecori, 2. 4kb fragment was recovered, and ligated with ecori - cleaved plasmid pci - neo
Pci n的構建制備和定量: ecori酶切含仍a全基因的質粒pgem 。 cea ,瓊脂糖電泳回收2The purified production was cloned into pmd18 - t vector. the cloned plasmids were transformed into jm109. the specific recombinant plasimid was identified by molecular weight, pcr and restriction endonuclease analysis. the results indicated that the resultant construct contained the gene of ibdv a fragment at right orientation
經瓊脂糖電泳檢測,將大小與預計分子量一致的片段純化后連接到pmd18 - t載體中,再轉化到jm109感受態細胞,得到的轉化子經分子量比較、 pcr鑒定和酶切分析篩選陽性克隆,結果表明,得到的陽性重組子中含有a節段全長基因,插入到載體中的方向正確。分享友人