library of recombinant 中文意思是什麼

library of recombinant 解釋
重組基因文庫
  • library : n. 1. 圖書館,圖庫;藏書樓;藏書。2. 叢書,文庫。
  • of : OF =Old French 古法語。
  • recombinant : n. 【遺】重組器官,復合器官。
  1. Culture of mg7 hybridoma cells and detection of antigen - binding affinity of mg7 mab by elisa 2. construction and identification of mg7 recombinant phage antibody library mrna was isolated from cultured mg7 hybridoma cells and converted into cdna ; the variable fragments of heavy and light chain were separately amplified and assembled into scfvs with a specially constructed dna linker by pcr. the scfvs dma was ligated into the phagmid vector pcantabse and the ligated sample was transfered into competent e. co / / tg1 to generate a bacterial form of mg7recombinant phage antibody library ; volume and recombinant ratio of the library were evaluated by means of bacterial colony counts and restriction analysis ( ecor i and hind iii )

    Mg _ 7重組噬菌體抗體庫的構建及鑒定從培養的mg _ 7雜交瘤細胞中提取並分離mrna ,反轉錄成cdna ;利用pcr分別擴增mg _ 7單抗的重鏈及輕鏈可變區基因,並通過? dna連接子將二者連接起來形成mg _ 7單鏈抗體基因;將mg _ 7單鏈抗體基因插入pcantab5e ;將連接產物轉化感受態tg1大腸桿菌,制備細菌形式的mg _ 7重組噬菌體抗體庫;通過菌落計數和限制性酶切分析( ecor和hind )評估mg _ 7重組噬菌體抗體庫的容量和重組率。
  2. Constructing cdna expressing library of erythrocytic plasmodium falciparum from hainan : the total rna was obtained by using. triplix kit. a modified oligo ( dt ) primer ( cds ffi pcr primer ) was used in the single - stranded ( ss ) dna synthesis reaction. the ss - dna was reversely transcripted from total rna. double - stranded ( ds ) cdna was amplified by long - distance ( ld ) pcrafter the digestion with proteinase k and sfi i, the cdna with no less than 200bp was collected and purified by glass - milk kitthe library was constructed after the ligation of cdna to tiplex2 phage particle packaged with the packaging extract system in vitro. a high titer and high recombinant ratio of cdna library was constructed

    構建惡性瘧原蟲海南株紅內期cdna表達文庫提取紅內期惡性瘧原蟲海南株總rna ,直接以總rna為模板使用cdna文庫構建試劑盒,首先反轉錄合成ss一dna ,再擴增合成ds一dna ( cdna ) ,對擴增產物用蛋白酶k消化及左z丁i酶切,抽提蛋白、去除rna后,用玻璃奶試劑盒純化、回收20obp以上的片斷,經與載體連接再用蛋白包裝物包裝后形成未擴增文庫,最後擴增完成惡性瘧原蟲海南株紅內期cdna表達文庫的構建。
  3. The full length cdnas of 17 - hsd1 and 17 - hsd3, 17 - hsd8 were obtained by library screening and race, respectively. expression patterns ( tissue distribution ) of three types 17 - hsds were checked by rt - pcr and northern blot. the recombinant constructs of 17 - hsdl / pet blue2 and 17 - hsd8 / pcdna 3. 1 were made and subsequently transformed into the corresponding host expression cell of ( de3 ) placi and mammalian hek 293 cell

    首先從genebank下載在其他脊椎動物中已被克隆17 - hsd1 , 17 - hsd3的氨基酸和核甘酸序列,並在序列保守區域設計簡並引物,然後分別以羅非魚卵巢和精巢cdna為模板進行rt - pcr擴增得到17 - hsd1 , 17 - hsd3的中間片段。
  4. The library was rescued with phage m13k07 in order to display scfv on the surface of the phage and to form the recombinant phage antibody library. one of positive scfv clones, named pcsal, was selected with phage - elisa after panning and screening by bull sperm three times. scfv fragment, amplified from pcsa1, was ligated to pmd18 - t vector for sequencing analysis

    取陽性重組噬菌體抗體克隆株pcsa1 , pcr擴增其scfv基因,篩選重組子進行序列測定,發現其序列符合小鼠抗體基因的一般特徵,並且與幾株抗磷酸膽堿的抗體重鏈和輕鏈可變區序列的同源性達80以上;推測pcsa1scfv針對的抗原是磷酸膽堿類物質。
  5. Its genomic dna was partially digested by sauial. dna fragments from 4 to 16 kb were collected after electrophoresis and ligated with bamhi - digested puc18 to construct genomic library. the total number of recombinant plasmids is about 9000

    進一步在opua基因的上下游序列分別設計引物,從h . trueperi基因組dna中擴增出所預期大小的片段,測序驗證已獲得opua基因的全序列。
  6. The patterns of sds - page indicated more than 30 % of recombinant proteins could be obtained from the extract of e. coli bl21. furthermore, library of recombinant phage antibodies was constructed from total rna isolated from spleen of the female balb / c mice immunized by bull sperm

    首先用牛精子免疫雌性四周齡balb c小鼠,從其脾臟組織分離總rna ,應用重組噬菌體抗體庫技術,構建了一個針對牛精子的噬菌體抗體文庫。
  7. Panning and enrichment ofmg7 recombinant phage antibody the transformed cells were infected with m13k07 helper phage to produce a phage form of mgy recombinant phage antibody library ; after three rounds panning of the library with the mgrbinding antigen highly expressed gastric cancer cell line kato iii, the mg7 scfv displayed phage dones were selected from the enriched recombinant phages by elisa

    3 mg _ 7重組噬菌體抗體庫的淘篩用m13ko7輔助噬菌體感染轉化菌,以挽救出噬菌體形式的抗體庫;用高表達mg _ 7抗原的胃癌細胞系kato對抗體庫進行三輪淘篩;用elisa篩檢呈現有mg _ 7scfv的噬菌體單克隆。
  8. On the bases of designing a primer pair, we obtained the coding domain sequence of rbp by pcr from cdna library. then the gene was cloned into pgem - t vector, the dna sequencing showed that the cloned gene was in agreement with the reported sequence. then the tageted gene of rbp was further subcloned into a procaryotic expression vector pbv220 and constructed recombinant plasmids was named pbv220 - rbp. in order to expresse rbp in procaryotic cell efficiently, the recombinant plasmids was introduced into e. colidhs a straints. expression of rbp was induced by temperature induction

    本實驗在合成該蛋白基因上下游引物的基礎上,利用pcr技術,從人睪丸cdna庫中釣取目的基因,並克隆于pgem - t載體中,經序列測定證明與文獻報道基本一致,再將目的基因從重組克隆質粒中亞克隆于pbv220原核表達載體中,轉化宿主菌,經溫度誘導后,進行sds - page電泳分析,發現在約21kd位置上出現了一條明顯的蛋白帶,與預期相符。
  9. On account of vaccination purpose, the neutralizing protection of anti - ns5 antibodies should be tested. ( 3 ) screening antagonistic peptide of ns5 protein a library of phage - displayed disulfide - constrained random peptides was incubated with a plate coated with the recombinant ns5 protein

    ( 3 ) nss蛋白小分子結合膚的篩選:以活性表達的nss蛋白為配基,從噬菌體展示的構象約束性隨機膚庫中篩選相應的配體分子,共進行了4輪篩選。
  10. Then the recombinant dna was packaged in vitro. identification of cdna library was followed, such as clone efficiency, recombinant efficiency, library integrality and the size of inserts

    第二部分:以gt11為載體構建乳腺癌細胞t47d的cdna表達文庫;對構建的文庫進行克隆效率、重組效率、完整性以及插入片段的鑒定;並進行文庫擴增。
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