表達質粒 的英文怎麼說

中文拼音 [biǎozhí]
表達質粒 英文
expression plasmid
  • : Ⅰ名詞1 (外面;外表) outside; surface; external 2 (中表親戚) the relationship between the child...
  • : Ⅰ動詞1 (暢通) extend 2 (達到) reach; attain; amount to 3 (通曉; 明白) understand thoroughly...
  • : Ⅰ名詞1 (性質; 本質) nature; character; essence 2 (質量) quality 3 (物質) matter; substance;...
  • : Ⅰ名 (小圓珠形或小碎塊形物) small particles; grain; granule; pellet Ⅱ量詞(用於粒狀物)
  • 表達 : deliver; express; show; voice; convey; communicate
  1. Stable suppression of afp gel expression by rnai in smmc - 7721 cells

    表達質粒穩定轉染肝癌細胞克隆的構建
  2. Methods : an artificial gene for fl extracellular domain cdna was synthesized by using favored genetic codons of pichia pastroris. by inserting human fl extracellular domain cdna coding 156 amino acid resi dues into pichia pastoris expression vector ppic9k containing aox1 promoter and the sequences of alpha secreting signal peptides, a recombinant expression plasmid ppic9k - fl was constructed, and integrated into the alcohol oxidase region of the host genome

    為了提高外源基因的量,我們根據畢赤氏酵母偏愛密碼子人工合成了編碼fl胞外區156個氨基酸的cdna序列,目的序列被定向克隆到酵母分泌型載體ppic9k上,構建ppic9k - fl表達質粒
  3. Protective immunity to schistosoma japonicum elicited by co - immunization of cathepsin b dna vaccine with eukaryotic plasmid encoding il

    4真核表達質粒聯合免疫誘導小鼠保護性的研究
  4. According to these problems, we adopt to the method of mending material, optimize to fermentation media and partly ferment condition. finally, we excogitate a kind of fermentation technology that is suitable for target gene efficiency expressed and is advantageous of product purified. with the plasmid pbv220 - ifnr, pbv220 - hgfa, pbv220 - hgfb, pbv220 - hpk5 that expresses serve as the model, adopting the biostat - c15l of b. braun company, utilize the method of mending material to ferment, through optimization fermentation media and optimization partly ferment condition ( ventilate quantity, stir speed, mend material speed ), eventually establishment a kind of fermentation technology that is suitable for target gene efficiency expressed and is advantageous of product purified

    以我室構建並穩定的重組pbv220 - - ifn 、 pbv220 - hgf 、 pbv220 - hgf 、 pbv220 - hpk5為模型,分別從不同的宿主菌中篩選出一種適合大規模生產的菌種bl21 ( de3 ) ,該工程菌株連續傳代100代表達質粒不丟失,量穩定;採用b . braun公司的biostat - c15l自控發酵罐,運用分批補料技術分別進行四種工程菌的高密度發酵,通過優化工程菌發酵的培養基配方及優化部分發酵條件(通氣量、攪拌速度、補料速度) ,最終建立一種適于目的基因高效的高密度發酵工藝模式。
  5. In this study five recombinant plasmids containing hn ( hemagglutinin - neuraminidase ) genes of ndv ( newcastle disease virus ) were constructed, hn genes were amplified by reverse transcriptase - polymerase chain reaction ( rt - pcr ) and were inserted directly into eukaryotic expression plasmid pcdna3

    應用反轉錄-聚合酶鏈反應( rt - pcr )獲得兩株新城疫病毒( ndv )血凝素-神經氨酸酶( hn )基因cdna ,然後定向插入真核表達質粒pcdna3中,構建了含hn基因的重組
  6. The highest antiviral litre of rpoifn - a was l l08iu / mi. the rpoifn - a protected pk - 15 cells against virulent hog cholera virus ( hcv ) infection in vitro

    Sds - page分析明,構建的重組表達質粒pqe30 poifn在大腸桿菌jm109中的rpoifn占菌體蛋白總量的20 26 。
  7. Construction of eukaryotic expression vector of human telomerase reverse transcriptase in immortalized hepatocytes

    構建永生化人肝細胞系人端酶反轉錄酶真核表達質粒
  8. The recombinant expression plasmids prt - p450nor and pet - p450nor were constructed by inserting p450nor gene into the bamh i / hind iii site of the prokaryotic expression vector prset and pet28, then they were transformed into e. coli bl21

    本研究將已克隆的真菌細胞色素p450nor基因插入原核表達質粒載體prset和pet28的bamhi / hind位點,成功構建重組表達質粒prt - p450nor和pet - p450nor ,並轉化到e . colibl21 。
  9. In order to express alkaline protease gene ( ap gene ) in bacillus subtil is, the recombinant expression plasmid was constructed. this plasmid contains a promoter bp53, also from b. pumilus un - 31 - c - 42, ap gene and the shuttle vector psugv4. after introduced into b. subtilis wb600, the transformants displayed the hydrolyzed zone on milk plate

    將來自短小芽抱桿菌un一31一c礴2的基因啟動子( bp53片段)和脫毛蛋白酶全基因( ap )進行融合,然後將重組基因(命名為bpap )插入到大腸桿菌-枯草桿菌穿梭載體psugv4中,構建成表達質粒psu一bpap 。
  10. Gfral was high expressed in e. coli after iptg induction. by ni2 + chelation affinity chromatography, the purified recombinant gfral protein were obtained. based on the evolutionary trace method, multiple sequence alignment and dendrogram construction were then carried out by the clustalx program and constructed a phylogenetic tree from a multiple sequence alignment for a protein family

    2 . gdnf的及其對pc12基因工程細胞的影響用本教研室已構建好的表達質粒pet一gdnf轉化大腸桿菌bl21 ( de3 ) ,經lmmipto誘導gdnf,並在niz氣nta柱上進行純化,稀釋復性后,純度90 %以上。
  11. Secondly, the hyaluronate lyase gene ( hyl ) was cloned into the vector puc19 by pcr using the total ona sample ofs. equi as template and partially sequenced, too

    Equi的總dna為模板,通過pcr方法,克隆了透明酸分解酶基因( hyl ) ,測序后連接到載體pse380的trc啟動子下游,構建表達質粒pse380 - hyl 。
  12. Thus, immunologists have sought smaller molecules with the antigen - recognition capability of antibodies. the variable domains of the heavy ( h ) and light ( l ) chains are sufficient for antigen recognition but the non - covalent complex of the two variable domains ( fv ) is unstable. it is possible to genetically engineer a single - chain fv ( scfv ) with the h chain v region connected to the l chain v region via a 15 amino acid linker composed of serine and glycine amino acid residues

    二、日本血吸蟲單克隆杭獨特型抗體np30的單鏈狐( scf )的構建、及對balbic小鼠誘導保護性作用研究l 、日本血吸蟲單克隆杭獨特型抗體np0的單鏈抗體歸cfv )的構建、通過pcr方法體外擴增並經測序驗證的重鏈、輕鏈可變區( vh 、 vl )基因先後重組入原核表達質粒ptha90相應的位點上,中間通過一連接肽( gly在er ) 。
  13. Cea gene was transferred into human dcs, and specific anti - cancer effecs induced by the vaccine was observed. this test is part of my tutor ' s. hang you - tian has observed the induction of crcinembryonic antigen ( cea ) - specific cytotoxic t - lymphocyte responses in vitro when he transfected dcs with pcdna3 - cea, and has observed the immunity effects of the dcs ( pcea ) inoculateing against to ct 26 ( hcea + ) loaded in balb / c mice. after vaccination with the cea gene - modified dc, the survival time of the mice vaccinated with ct26 + ( cea + ) ws prolonged more potently than that of the mice vaccinatd with other dcs

    癌胚抗原( carcinoebryonicantigen , cea )是一種研廠鄭州大學2002年碩士畢業論文轉染人癌胚抗原真核表達質粒的人樹突狀細胞的抗瘤作用究最為深入的腫瘤相關抗原( tumorassociatiednigen , taa ) ,在90的胃腸道腫瘤、 50的乳腺癌及70的非小細胞肺癌中有高水平的,是目前國際上公認的腫瘤標志物。
  14. Salmonella typhimuriwn, one of the invasive bacterial species, can be attenuated without loss of invasiveness and thus used for delivery of eukaryotic expression vectors into host cells in vivo. the recombinant plasmid containing the target gene is released inside the host cells and gain entry into the nucleus, resulting in expression of encoded antigens and subsequent induction of humoral and cellular immune responses

    沙門氏菌( salmonellatyphimurium )是一種較為常見的侵襲性胞內菌,通過基因工程方法減毒后對宿主致病性顯著降低,但仍保留良好的侵襲力,可直接將真核表達質粒攜帶進入動物細胞內相應的蛋白而誘導特異性的免疫應答反應。
  15. The 496 bp fragment of the orf of p22 gene and a 561 bp fragment were amplified from the genomic dna of zs strains of toxoplasma gondii. both 496 bp and 561 bp fragments were successfully cloned into the plasmid pthiohisa, b, c and pbudce 4. 1 respectively. 2

    從弓形蟲zs株基因組中擴增出p22編碼基因的一長496bp ,另一長561bp的片段,並成功構建含p22編碼基因的原核重組體pthiohisa , b , c / p22 ,及真核重組表達質粒pbudce4 . 1 / p22 。
  16. Conclusion : a 496 bp fragment of the gene encoding t gondii p22 surface protein was successfully cloned into the plasmid pthiohisa, b, c and expressed in the e. coli top 10, and the fusion proteins can be purificated effectively

    結論:成功構建弓形蟲zs株膜抗原p22編碼是因pthiohisa , b , c p22表達質粒,誘導弓形蟲農牧抗原p22蛋白,兒g 。
  17. An expression vector carrying a fragment encoding the amino - terminal part of an fr - 008 type i pks module, containing a keto - synthase ( ks ) and part of an acetyl - transferase ( at ) domain was constructed for trial expression of the extremely high g + c content ( 76 % ) pks gene in plant

    為探索在植物中極高g + c含量的pks基因的可能性,構建了攜帶有編碼fr - 008型pks模塊氨基端部分的基因的表達質粒,包括一個酮基合酶( ks )和部分酰基轉移酶( at )活性結構域。
  18. Dna and rna dot blotting revealed that the f gene was transcribed into mrna in the vero cells. there was expression of the f protein as shown by indirect immunofluorescent assay. the expression began at 48h post - infection and increased thereafter, as indicated by elisa

    將真核表達質粒pcdna3 - f高壓電轉化dam和phop基因雙突變的減毒鼠傷寒沙門氏菌zj111株( zj111 / pcdan3 - f ) ,並直接轉染vero細胞,分別提取細胞總dna和總rna , dig標記探針均可檢測到陽性雜交信號。
  19. In the study, several recombinant expression vectors were constructed in vitro by using the technique of gene engineering, making pheromone 3 be expressed under the control of different promoters and signal pcptides

    本研究利用基因工程的方法,體外構建重組表達質粒,探索用不同的啟動子和信號肽序列八肋游仆蟲信息素3蛋白。
  20. Cloning of the pten mmac1 cdna and construction of its expression plasmid

    克隆及其表達質粒的構建
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