phage antibody造句

"phage antibody"是什么意思   

例句与造句

  1. A murine phage antibody library containing 1 . 710
    成功构建一库容量为1 . 710
  2. Then the biotin - labelled n - peptide interacted with the phage antibody library
    对其研究可能有助于了解成瘾机制和有临床应用价值。
  3. The murine phage antibody library was amplified and then panned by human chorionic gonadotropin for four rounds . the last round enriched phage clones were used to reinfect
    由鼠源噬菌体抗体库淘选到展示有人绒毛膜促性腺激素单链抗体的噬菌体克隆。
  4. One n - peptide - binding scfv clone was selected from the phage antibody library using affinity panning . the target antigen , n - peptide was biotinylated using photobiotin first
    N -肽是一种新发现的神经肽,其n端与阿片肽高度同源,可与阿片肽受体相互作用。
  5. In the present paper the application of dna library , phage display random peptide library , phage antibody library , etc . in the research of serodiagnostic reagents and their special values were reviewed
    本文综述了基因文库、噬菌体展示肽库及噬菌体抗体库技术在血清学诊断试剂研制中的应用及其各自的优点。
  6. It's difficult to find phage antibody in a sentence. 用phage antibody造句挺难的
  7. 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龄balb c小鼠,从其脾脏组织分离总rna ,应用重组噬菌体抗体库技术,构建了一个针对牛精子的噬菌体抗体文库。
  8. 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
    取阳性重组噬菌体抗体克隆株pcsa1 , pcr扩增其scfv基因,筛选重组子进行序列测定,发现其序列符合小鼠抗体基因的一般特征,并且与几株抗磷酸胆碱的抗体重链和轻链可变区序列的同源性达80以上;推测pcsa1scfv针对的抗原是磷酸胆碱类物质。
  9. Methods : a set of oligonucleotide primers were designed and used to amplify the vh and vl gene from anti - hbsag fab antibodies screened from phage antibody library . the products were cloned into puc19 vector and their sequences were analysed . the vh and vl gene fragments were tethered by a peptide linker and a leader sequence coding region , with the leader sequence added at 5 " terminus of each gene ( l - vh - linker - vl ) and designated as l - scfv
    方法以从噬菌体抗体库中筛选获得的抗hbsag的fab抗体基因为模板,分别扩增出其轻、重链可变区( v _ l 、 v _ h )基因,通过重组pcr方法将轻、重链可变区基因用连接肽( gly _ 4ser ) _ 3的编码序列连接,并引入前导肽编码序列,构建具有l - v _ h - linker - v _ l结构的单链抗体基因。
  10. Detection of antigen - binding affinity of mg7 recombinant phage antibody elisa was repeated to confirm the antigen - binding affinity of positive clones screened out in the former procedure ; these positive phages were examined by restriction analysis ( ecor i and hind iii ) ; competitive elisa was performed to test the inhibitory ratio of these positive clones to the binding affinity of mg7mab and its relevant antigen , the positive dones possessing apparent inhibitory effect were singled out for later use
    X阳性克到驶知烘扳原kbbjg )浊对阳性克隆进行限制陇卧赐析( uwi和hedlll )鉴定三用竞争elisatoljmg7重组噬菌体抗体性克隆对mg7单扶与其相应抗原结合忙的喇率,从中j ) ed出对mg7单抗与期眩抗原结合有抑余j效应的克隆用于进一涉研究。
  11. 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重组噬菌体抗体库的淘筛用m13ko7辅助噬菌体感染转化菌,以挽救出噬菌体形式的抗体库;用高表达mg _ 7抗原的胃癌细胞系kato对抗体库进行三轮淘筛;用elisa筛检呈现有mg _ 7scfv的噬菌体单克隆。
  12. 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重组噬菌体抗体库的构建及鉴定从培养的mg _ 7杂交瘤细胞中提取并分离mrna ,反转录成cdna ;利用pcr分别扩增mg _ 7单抗的重链及轻链可变区基因,并通过? dna连接子将二者连接起来形成mg _ 7单链抗体基因;将mg _ 7单链抗体基因插入pcantab5e ;将连接产物转化感受态tg1大肠杆菌,制备细菌形式的mg _ 7重组噬菌体抗体库;通过菌落计数和限制性酶切分析( ecor和hind )评估mg _ 7重组噬菌体抗体库的容量和重组率。

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