質粒轉移 的英文怎麼說

中文拼音 [zhízhuǎn]
質粒轉移 英文
plasmid transfer
  • : 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)
  • : 轉構詞成分。
  • : Ⅰ動詞1. (移動) move; remove; shift 2. (改變; 變動) change; alter Ⅱ名詞(姓氏) a surname
  • 轉移 : 1 (改換位置) shift; transfer; divert 2 (改變) change; transform 3 [醫學] (擴散) metastasis;...
  1. The recombinant plasmid puge dna and transfer vector pfastbacl dna were treated again in the same enzyme, were linked by means of t4 dna ligase and transformed into e. coli jm109 permissive cells, yielding recombinant transfer vector plasmid pfastbac - ge dna and were transformed into dhlobac containing vector bacmid

    將重組pugedna與載體pfastbacldna用bamhi和ecori雙酶切處理, t _ 4dna連接酶連接,用連接產物化大腸桿菌jm109感受態細胞,得到重組載體pfastbac - gedna 。
  2. In order to facilitate the study of biological function of add gene cluster, e. coli - s. avermitilis intragenus conjugation system was established. in addition, phz2114 for the replacement of the entire add gene cluster and phz2130 for disruption of adda were constructed

    建立了除蟲鏈黴菌的接合系統,並構建了用於置換全部基因簇的基因置換phz2114和adda的基因中斷phz2130 ,為研究除蟲鏈黴菌add基因簇的生物學功能奠定了基礎。
  3. The recombinant transfer vector pbacpak - hbmp was constructed by insertion of the hbmp coding sequences into the multiple cloning site of transfer vector pbacpak. 8. bmn cell line was co - transfected with pbacpak - hbmp plasmid and linearized baculovirus bacpak6 dna by dosper agent

    將克隆到的hbmp基因通過適當的酶切插入到載體pbac - pak8的多克隆位點中,獲得重組載體pbacpak - hbmp 。
  4. In this study, the recombinant fowl - poxvirus was transfected into expressing the vp3 gene of isolated gpv h1 strain into the cef cells with fpv - 017 by liposome, which have the lacz reporter gene, earlier / latter promoters lp2ep2 of fpv, promoters p7. 5 and p7. 1 of vaccinia virus, replication unnecessary region of fpv - 017. following 6 cycles screenings, clonings, purification of blue plaques, detection of pcr and dot - elisa, which verified the genetic stable vp3 - fowlpox virus recombinant constructed successfully. this study provided the theoretical and practical foundation for development of gpv recombinant fowl - poxvirus genetic engineering vaccine, as well as provided substance preparatory for prevention the high mortality gpv

    本研究採用脂染方法,將含有完整gpvh1分離株vp3基因、報告基因lacz 、禽痘病毒早晚期啟動子lp2ep2 、痘苗病毒啟動子p7 . 5 、 p11和fpv - 017復制非必須區的載體psy681vp3lacz與fpv - 017共染雞胚成纖維細胞,經6輪蝕斑克隆、篩選、表達, pcr鑒定和dot - elisa檢測,證明該重組病毒已構建成功,並獲得了遺傳性狀穩定的鵝細小病毒vp3基因的重組禽痘病毒。
  5. In the presented study, using h7721 human hepatocarcinoma cell line transfected with sense or antisense cdna of gnt - v, the effects of gnt - v on signal transduction an d its mechanism as well as the alteration of gene expression were investigated. we expected to elucidate whether and how the transfected glycosyltransferase modulate the cell signal transduction and gene expression

    本文以穩定染gnt - v正義或反義cdna的h7721人肝癌細胞為材料,從下列四個方面對gnt - v影響信號導及其機制以及引起基因表達的變化進行了研究,企圖闡明糖基染是怎樣調節細胞信號導的
  6. Vp3 gene of hl isolate of goose parvovirus derived from recombinant piasmid pproex htb - vp3 was subcloned into ecorl site of psy538, and the reporter gene lacz with promoter pll was cloned into smai site of recombinant piasmid. both vp3 gene and lacz gene were cloned into noti site of psy681, recombinan fpv transfer vector containing vp3 gene of gpv was obtained. the result is basis of construction of recombinant fpv expressing vp3 gene of gpv and gpv genetic engineering vaccine

    本研究另從含有gpvh1分離株主要結構蛋白vp3基因的重組pproexhtb - vp3中切取gpvh1株vp3基因片段,將其亞克隆于psy538的ecori位點,然後將帶有痘苗病毒啟動子p11的lacz報告基因平端克隆于上述重組子的smai位點,再用noti切下同時含有vp3基因和lacz報告基因的片段,再亞克隆于psy681的noti位點,構建出含有vp3基因的重組禽痘病毒載體,為構建表達vp3基因的重組禽痘病毒從而制備gpv基因工程疫苗奠定了基礎。
  7. 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

    為探索在植物中表達極高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,包括一個酮基合酶( ks )和部分酰基酶( at )活性結構域。
  8. Based on a 3. 1kb pst i fragment of genomic dna of a wild s. avermitilis, a 1. 5 kb apramycin resistance fragment was inserted into sph i site of avec gene in the 3. 1 kb fragment, then a recombinant plasmid pc05 was obtained by introducing above inactivated avec fragment into mcs region of phjl401. competent cells of et12567 were transformed by recombinant plasmid pid03 and pc05 respectively

    以含有avec基因的3 . 1kb基因組dnapsti片段為基礎,將1 . 5kb的安普黴素抗性基因片段插入到avec基因中的sphi酶切位點,再將此插入失活的avec基因片段連接到具有接合功能(含有orit基因)的鏈黴菌-大腸桿菌穿梭phjl401的多克隆位點區,由此得到重組pc05 。
  9. For mobile sources, meca members include manufacturers of catalytic converters ( catalysts, substrates, mounting sleeves, and converter housings ) for all fuels ; diesel particulate filters ; oxygen, nox, and temperature sensors ; thermal management strategies ; engine / fuel management technologies ; crankcase emission control technologies ; evaporative emission controls ; enhanced combustion technologies ; plasma / corona technologies ; and components for fuel cell technology

    動源方面,其成員主要從事下列產品或技術的生產或研發:各類燃料的催化化器(包括相關產品如催化劑、基、安裝袖和化器殼) ;柴油顆過濾器;氧氣、氮氣和溫度傳感器;熱處理系統;發動機/燃料操控技術;曲軸箱排放控制技術;蒸發排放控制;強化燃燒技術;等離子體/電暈技術。
  10. The abuses of antibiotics in medicine and livestock exposed to environmental bacteria lead to a large - scale dissemination of antibiotic - resistance bacteria in aquatic environment under selective pressure and the resistant organism could transfer resistance genes across the genus and species by plasmid and integron, antibiotic resistance microbes are common in aquatic environment and the aquatic environment has become a major reservoir for antibiotic - resistant microbes

    摘要臨床和畜禽業抗生素的濫用導致微生物在選擇性壓力作用下獲得並維持耐藥性,並有可能通過和整合子將耐藥基因在相同或不同種屬中廣泛傳播,最終導致多重耐藥。
  11. The research showed that their interactions in yeast two - hybrid system are still steady when the vector was exchanged, in contrast, the interaction was disappear when the reading frame of each positive had been changed. the four positives were subcloned into suicide plasmid so that gene mutant strains could be constructed via conjugation and homologous recombination

    為了進一步驗證這些克隆的編碼產物與nifa蛋白的相互作用,將它們與nifa基因互換載體后共化酵母,仍然可以激活三個報告基因的表達,而陽性克隆碼表達的重組和pgbd - nifa的共化物則不能在選擇性平板上生長。
  12. When deposit temperature is raised from 450 to 500, the size of nano - crystals is increased from l ~ 4nm to 5nm. a few 8162 nano - crystals are also found, which are derived from the amorphous oxide in the matrix. simultaneity, some special patterns appear while nano - crystals move and rearrange

    薄膜中的結晶程度隨沉積溫度的升高而提高,納米硅晶的尺寸由450時的1 4nm增大到5nm以上,氧化程度也隨之加深,非晶介中的氧化物逐漸向氧化硅的晶態變,同時納米顆在晶和重排過程中局部形成特殊形貌的團聚物。
  13. It was also proved that the biosynthestic genes of apramycin was linked to the apramycin resistant gene in s. tenebrarius

    Pcr實驗證明基因重組菌株中接合同源整合到黑暗鏈黴菌h6的染色體上。
  14. The gene recombinant strain no. 42 ca n ' t generate ampramycin, which indicated that the cloned gene is involved in apramycin biosynthesis in s. tenebrarius

    通過接合的方法將pzxb014導入黑暗鏈黴菌h6中,篩選基因發生重組的菌株。
  15. Pfge analysis of these 21 blocked strains revealed a common chromosomal deletion in the 300kb asel fragment which might be responsible for antibiotic 5102 - iii biosynthesis. so the 300kb fragment was recovered and used as probe to hybridize with 10 - 22 genomic library. cosmids in this region were aligned and suitable fragments in this region were selected and used further for the construction of gene replacement plasmids

    以此片段為探針釣出了位於該區域的文庫克隆,並利用指紋印跡和雜交技術將這些文庫克隆排列起來,進而以位於該區域的不同位置的片段做臂構建了用於化和接合用的基因置換,並試圖通過基因置換將該區域置換下來,但尚未得到最終結果。
  16. A 1. 5 kb apramycin resistance fragment was inserted into nru i site of aved gene and the inactivated aved gene fragment was then introduced into mcs region of phjl401 - an e. coli / streptomyces shuttle vector with conjugation function ( containing orit gene ). as a result of above procedures, a recombinant plasmid pid03 was obtained

    將1 . 5kb的安普黴素抗性基因片段插入到aved基因中的nrui酶切位點,再將此滅活的aved基因片段插入到具有接合功能(含有orit基因)的鏈黴菌?大腸桿菌穿梭phjl401的多克隆位點區,由此得到重組pid03 。
  17. A fragment, containing 2. 0kb cloned 5. tenebrarius dna and reported genes of erme and xyle, was inserted in plasmid phz132 ( an e. coli - streptomyces shuttle plasmid incorporating orit from rk2 ) to construct disruption plasmid pzxb0l4. the plasmid was transformed into e. coli et12567 ( puz8002 ) to construct recombinant e. coli et12867 ( puz8002, pzxb014 )

    將克隆到的鏈黴菌dna2 . 0kb片段以及報告基因erme 、 xyle插入到具有orit的大腸桿菌?鏈黴菌穿梭phz132中構建接合pzxb014 ,並將其入大腸桿菌et12567 ( puz8002 )中,獲得供體菌et12567 ( puz8002 , pzxb014 ) 。
  18. The recombinant plasmids pbmb121l, pbmb9821l and pbmb986l were constructed after transferring bacillus thuringiensis icps gene crylaal, crylaclo and crylca from their original plasmid vectors to different plasmid vector. the relevant recombinant strains were obtained after introducing the 3 recombinant plasmids into bacillus thuringiensis plasmid - free mutant strain 8mb 171 by electroporation. the transformation and expression properties of 8mb 171 were studied

    通過將蘇雲金芽胞桿菌殺蟲晶體蛋白基因cry1aal 、 cry1ac10和cry1ca至不同載體上,分別構建了重組pbmb121l 、 pbmb9821l和pbmb986l ,並分別導入無突變株bmb171 ,篩選得到攜帶相應icps基因的重組菌株。
  19. Hegf gene with his - tag at the end, which was derived from pet22 - egf, was in - frame fused to the carboxy - terminal of polyhedrin ( ph ) gene, which included the amino - terminal 116aa coding region. the polyhedrin - egf fusion gene ( named ph - egf ) was then cut out with ecorv and ecori, and was cloned between ecorv and ecori sites of pbacpak. 8 ( the result plasmid was named pbacph - egf and the ph - egf fusing gene was right under the control of ph promoter ). the pbacph - egf structure was verified with restriction enzymes digestion and pcr

    從pet22 - egf中分離出末端帶his - tag的egf基因,對位融合於多角體蛋白n端116個氨基酸基因序列的下游(命名為ph - egf ) ,並在兩段基因間設計了凝血酶xa蛋白酶切位點,經過酶切、測序等鑒定正確后,克隆至pbacpak8中,使ph - egf融合基因置於多角體蛋白( polyhedrin , ph )基因啟動子控制之下,構建成重組載體pbacph - egf 。
  20. The gd and ge gene was subcloned into puc18, resulting in pugdge. the fragment from pcdnas. 1 - including hcmv promoter / enhancer, mcs and neomycin resistance gene was inserted into the bamhi and bsteii restrication sites of pugdge, resulting in the universal transfer vector pgd - m - ge. the universal transfer vector pgd - m - ge has deleted the gi gene and 363bp in the 5 ' end of the ge orf of prv. there were 11 restrication sites for insertion of the foreign gene. the upstream and downstream flanking sequences were up to 1. 25kb and 1. 42kb. it will be useful for developing the recombinant prv expressing foreign gene ( s )

    將gd 、 ge基因連接于puc18獲得pugdge ,缺失pugdge的bamh和bste位點間391bp的片段。在此缺失位置插入來自pcdna3 . 1 -的一偽狂犬病病毒gd 、 ge 、 tk基因的克隆與通用載體的構建段含hcmv啟動子。多克隆位點和neo報告基因的片段,構建了通用載體ppd m pe 。
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