插入重組 的英文怎麼說

中文拼音 [chāzhòng]
插入重組 英文
additive recombination
  • : 動詞1. (把細長或薄的東西放進、擠入、刺進或穿入; 插上; 插進) stick in; insert 2. (中間加進去; 加進中間去) interpose; insert
  • : Ⅰ動詞1 (進來或進去) enter 2 (參加) join; be admitted into; become a member of 3 (合乎) conf...
  • : 重Ⅰ名詞(重量; 分量) weight Ⅱ動詞(重視) lay [place put] stress on; place value upon; attach im...
  • : Ⅰ名詞1 (由不多的人員組成的單位) group 2 (姓氏) a surname Ⅱ動詞(組織) organize; form Ⅲ量詞(...
  • 插入 : insert; infix; run in; break in; patch; insertion; plug in; intercalate; intercalation; intromiss...
  • 重組 : bpr
  1. The pcr product was inserted into expression plasmid pet - 32a ( + ) after restriction digest. then the recombinant plasmid was identified by endonuclease analysis, pcr ampliation and dna sequencing. the report showed that the recombinant plasmid had right open reading frame

    質粒經酶切鑒定, pcr鑒定和測序,結果證實豬肺炎支原體黏附因子p97基因的抗原決定簇r1區定向了質粒pet - 32a ( + ) ,且閱讀框架正確。
  2. 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 ,然後定向真核表達質粒pcdna3中,構建了含hn基因的質粒。
  3. 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基因原核表達質粒載體prset和pet28的bamhi / hind位點,成功構建表達質粒prt - p450nor和pet - p450nor ,並轉化到e . colibl21 。
  4. 4. engineering dhqase ( arod ) - deficient e. coli mutant with a second copy of the arob gene gene targeting technique was used to disrupt the arod gene in e. coli chromosome. the mutant 31bk was engineered, in which homologous recombination of the arobkanr gene cassette into the arod locus ( arod : : arobkanr ) of the e. coli strain atcc31884 genome utilized the helper plasmid pkd46 with red system. the host cell 31bk lacked catalytic activity of dhqase ( arod ) and had a second copy of the arob gene, so it improved carbon flow into the quinic acid biosynthesis direction

    構建宿主菌基因精確定位突變株31bk ( arod : : arobkan ~ r )為了改變代謝途徑脫氫奎尼酸( dhq )分支點上的代謝流量,使之充分流向目的產物奎尼酸合成方向,利用基因打靶技術構建了31884宿主菌arod基因精確定位突變體,使dhq脫水酶( dhqase )失活,阻斷了碳代謝流流向芳香氨基酸生成的方向,同時用同源的方法將arob基因定位整合染色體上,解除了限速酶對碳代謝流通過共同途徑到達dhq的阻遏影響,並減輕代謝負擔。
  5. 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,然後將基因(命名為bpap )到大腸桿菌-枯草桿菌穿梭質粒載體psugv4中,構建成表達質粒psu一bpap 。
  6. 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噬菌體抗體庫的容量和率。
  7. 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到轉移載體質粒pbac - pak8的多克隆位點中,獲得轉移載體質粒pbacpak - hbmp 。
  8. After linerization, the recombinant plasmid was transformed into pic hia pastoris by electroporation, which then were cultured in md plate free of histidine, from which the positive colones were propagated

    質粒線性化后,用電擊法將質粒轉化巴氏畢赤酵母,在缺氨酸的md板上篩選陽性菌落,然後用不同濃度的g418 ? ypd板篩選多拷貝單菌落。
  9. According to above consideration, experiments was carried out as below : first, targeted gene - human serum albumin ( hsa ) gene was obtained via pcr technology. secondly, the hsa gene was liganded with a plasmidprla22 whose two arms carry dna sequences necessary for crossing with the human a - lactalbumin yac to form an integration vector prla - hsa, then the integration vector plasmid was co - transformated into the right yac - bearing yeast with another plasmid plrh33 which carrys a selective gene

    因此,本試驗首先擴增出整合在酵母基因里的人血清白蛋白( hsa )基因作為目的基因,並將人血清白蛋白基因到一個含有人-乳白蛋白yac同源序列的型質粒載體,以構建整合型載體,再與另一個帶篩選基因的質粒共轉化含人-乳白蛋白yac的酵母細胞體內。
  10. Fabrication of the box beam is divided into such parts as reinforcement, formwork, concreting, prestressing, moving and storing of beam, pipe grouting under pressure, end sealing of the beam, water - proof layer on the bridge surface system, protective coating etc. the paper makes description of effective box beam construction technology and workmanship which can be adopted in other projects, such technologies as : manufacturing and fixing of reinforcement, steel reinforcement fixing baseplate, web plate and top plate respectively and lifting the steel skeleton into form, requirements of design and manufacturing and way of utilization for dismantling - erection type formwork and hydraulic formwork, optimization of concrete ratio, concrete pouring process of two ends of beam in priority over the middle, in sequence of first baseplate followed by web plate and top plate at last, concrete pouring in inclined section and in horizontal layer, concrete vibration mainly by external vibrator in assistance with internal vibrator, methods and regulation for steam curing of concrete, dual controls over stress and strain to ensure quality of prestressing workmanship, construction method of effective beam moving by heavy - weight special moving facility, some regulations and key notes about construction of grouting under pressure, beam ends sealing, water - proof layer on the bridge surface system, protective coating

    箱梁製造由鋼筋工程、模板工程、混凝土工程、預應力工程、移存梁工程、孔道壓漿工程、梁體封端工程、橋面防水層和保護層工程等施工環節成。文中介紹的採用胎具製作和綁扎鋼筋,分底腹板和頂板分別綁扎並吊裝鋼筋骨架模;拆裝式和液壓式兩種模板的設計、製作要求和使用方法;綜合考慮、優化混凝土配合比,混凝土灌注從兩端至中間、先底板、后腹板、再頂板的施工順序和斜向分段、腹板水平分層、附著式振搗為主、式搗固為輔的施工工藝,蒸汽養護的方法和規定;應力應變雙控制確保預應力施工質量的施工技術;採用物移運器有效移梁的施工方法;壓漿、封端、橋面防水層和保護層施工的一些規定和注意事項等都是對箱梁製造行之有效的施工技術和施工方法,並可為以後類似施工作借鑒。
  11. The pbacph - egf plasmid dna was used to co - transfect bmn cell with the modified bombyx mori baculovirus bm - bacpak dna, which was first linearized by aocl. after two rounds of plaque isolation, the recombinant virus ( named bmbacph - egf ) was further verified with pcr and dot hybridization. the recombinant bmbacph - egf virus was used to infect bmn culture cells at a moi of 10

    轉移載體dna與經bsu36i酶切線性化的修飾型病毒bm - bacpakdna共轉染家蠶bmn細胞,兩輪空斑篩選和純化,獲得病毒rbmbacph - egf ,經pcr擴增、 dna點雜交等方法鑒定證實病毒中已正確ph - egf融合基因。
  12. Therefore, blys, its receptor or related antagonists may find medical utility in the treatment of b cell disorders associated with autoimmunity, neoplasia, or immunodeficiency syndromes. in this study, epo signal peptide sequence and hsblys gene were linked by soe method. the fusion product was cloned into eukaryotic plasmids. pcdna3, pcdna3. 1, pefneo, respectively. meanwhile, the epo signal peptide sequence was mutated so as to form a restriction enzyme cut site : bin i. thus the recombinant plasmid can be used as secreting plasmid expressing other gene

    本實驗通過3 』端互補,進行引物延伸合成epo信號肽序列:信號肽和hsblys基因採用疊延伸拼接法形成融合基因;融合基因分別pcdna3 . 0 、 pcdna3 . 1 、 pefneo真核載體:引物延伸合成信號肽時,利用亮氨酸同義密碼,將信號肽基因的倒數第二個密碼突變,在載體上的信號肽序列之後,形成bln酶切位點,使三種載體成為分泌表達載體。
  13. 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dnapsti片段為基礎,將1 . 5kb的安普黴素抗性基因片段到avec基因中的sphi酶切位點,再將此失活的avec基因片段連接到具有接合轉移功能(含有orit基因)的鏈黴菌-大腸桿菌穿梭質粒phjl401的多克隆位點區,由此得到質粒pc05 。
  14. Unfortunately, as changes are made to the data sources, maintaining the quotient cube is non - trivial since the partitioning of the cube cells must also be updated. in this paper, the authors design incremental algorithms to update a quotient cube efficiently for both sum and median aggregate functions

    然而,當數據源發生改變的時候, quotient數據立方體很難進行維護,尤其是針對median這樣的非分步型聚集函數,因為當新的元時, quotient數據立方體中的等價類有的需要進行拆分,有的還需要新生成。
  15. Construction of male sterility expression vector by integration of artificial sense and antisense cdnas of hsp70 into puc18 and puc19 respectively, we can obtain psc and pac. tapertal specific expression promoter ta29 and terminator nos are connected directionally with sense and antisense cdnas of hsp70 extrected and purified from psc and pac., then integrated into puc18 and puc19, by which we can build sense and antisense cdna nos ( respectively named plasmid 650 and plasmid 651 ) of ta29 - hsp70. for the sake of better screening and examination of transformed gene, we cut plasmid 650, plasmid 651 and 3301 ( containing gusgene bar screening marker gene ) with hindiii and ecor i enzymes, then connect purified fragments of 650and 651 with plasmid 3301 to construct the vector 3301 + 650 and 3301 + 651. corroboration of whether sense and antisense cdna - nos is integrated into plasmid3301 can be made by plate screening and enzye - cutting analysis

    分別將從psc 、 pac回收純化的hsp70正、反義cdna與絨氈層特異表達啟動子ta29及nos終止子定向連接,然後到puc18 、 puc19中,構建成花藥特異表達的ta29 - hsp70sensecdna - nos和ta29 - hsp70antisensecdna - nos ,分別稱作650和651質粒。為了更好地對轉化子進行篩選和檢測,用hind和ecor分別對650 、 651及3301質粒(含gus報告基因和bar篩選標記基因)進行酶切,將從650和651回收純化的目的片段與3301質粒進行連接,再對子進行平板篩選和酶切分析確定ta29 - hsp70sensecdna - nos和ta29 - hsp70antisensecdna - nos到3301質粒中,構建成3301 + 650和3301 + 651表達載體。
  16. Multicopy integrants were screened with g418 from pichia pastoris which contains recombinant plasmid, and induced with methanol to secrete interesting peptide. the supernate of pichia pastoris culture was analysed by sds - page and western blotting. a reactive band, which the apparent molecular weight is 36kd, can be detected with sheep anti - hcmv polyclonal antibodies

    質粒轉化巴氏畢赤酵母, g418篩選出多拷貝的單克隆,甲醇誘導多拷貝的單克隆酵母細胞分泌目的蛋白,培養液上清經sds - page電泳分析,在蛋白質印跡中檢測到培養液上清有一表觀分子量為36kd ,能與羊抗hcmv多克隆抗體發生發應的條帶。
  17. This article dealt with cloning and sequencing of chitinase and endoglucanase genes of bacillus spp. and recombinant biocontrol isolates of bacillus spp

    質粒分析證明克隆子中含有質粒,外源片段大小為2 . 6kb左右,與pcr最初產物的大小一致。
  18. In this study, we designed a pair of primers based on the sequence of the upstream and downstream of chicken il - 2 gene. about 600 bp chicken il - 2 cdna fragment was cloned from cona - stimulated chicken splenocytes by reverse transcription - polymerase chain reaction ( rt - pcr ) and was subcloned into puc18 vector. recombinant clone was demonstrated by restriction enzyme digestion and dna sequencing. next, we construct recombinant plasmid pproex ? t - il - 2. the cdna of chicken il - 2 gene was subcloned into bamh i / hind iii sites of vector. the recombinant plasmid pproex ? t - il - 2 was transformed into e. coli dh5a and the bacteria was induced with iptg. it was demonstrated by sds - page and western blot that a 18kda protein which was equal to chicken il - 2 protein in molecular weight was expressed in e. coli dh5a. the expression level was up to 30 % of the total bacterial proteins. the purified protein was used to prepare the antibody against chicken il - 2 protein

    經酶切鑒定及dna序列測定,該基因為雞il - 2基因,其序列與sundick等報道的完全一致。在此基礎上,我們把雞il - 2基因亞克隆到大腸桿菌原核表達載體pproex ~ ( tm ) ht中,構建表達質粒並進行確證性序列測定,質粒測序結果表明將編碼雞il - 2成熟蛋白的基因正確地到原核表達載體pproex ~ ( tm ) ht的目的位點。質粒轉化受體菌dh5後用iptg於37進行誘導培養, sds - page和westernblot分析顯示,表達的雞il - 2融合蛋白分子量約為18kda ,表達的融合蛋白經薄層掃描發現目的蛋白表達量約占菌體蛋白的30 。
  19. One of them was identified as the beth gene of halobacillus sp. d8. a hydrophobicity plot of beth revealed an alteration of hydrophobic and hydrophilic segments that was characteristic for integral membrane protein, suggesting the presence of 12 transmembrane - spanning segments and belonged to bcct family

    質粒測序,片段大小為4kb左右,通過blast比較,結果顯示含有三個orf框,其中一個為甘氨酸甜菜堿轉運蛋白,對其氨基酸成進行疏水性分析,推測為含有12個跨膜域的跨膜蛋白,屬于bcct家族。
  20. Compared with a reported cmv - cp gene sequence, the homology of nucleotide sequences were 100 %. the sequencing result also demonstrated the recombinant vector pet - 22b - cp has a proper orf encoding 218 amino acids. the recombinant vector was transformed into bl21 ( de3 ) cells. transformants were grown and induced by the addition of isothiopropylgalactoside ( iptg ) to a concentration of imm with continued shaking at 37 ?

    酶切鑒定及序列測定表明,表達質粒pet - 22b - cp連接區域符合設計要求,具有正確的開放閱讀框架,片段含有218個氨基酸的完整編碼區,其核苷酸序列與報道的cmv - cp基因的同源性為100 。
分享友人
分享到 Line

分享到臉書