連接片段 的英文怎麼說

中文拼音 [liánjiēpiānduàn]
連接片段 英文
joining segment
  • : Ⅰ動詞1 (連接) link; join; connect 2 (連累) involve (in trouble); implicate 3 [方言] (縫) ...
  • : Ⅰ動詞1 (靠近;接觸) come into contact with; come close to 2 (連接; 使連接) connect; join; put ...
  • : 片構詞成分。
  • : Ⅰ量詞(部分) section; segment; part; paragraph; passage Ⅱ名詞(姓氏) a surname
  • 連接 : connect; fit together; link; marry; mate; joint; association trail; linkage; concatenate; concate...
  • 片段 : part; passage; fragment; extract; segment; bit; episode; snatch; section
  1. Third, it is this " moment " of the segment of space - time which based on the the philosophy of the nature and describing the mechanical movement that symbolize the transform from the view of integralization in classical atomism of mathematics to the view of integralization of modern real number

    另外,正是基於新的自然哲學的、作為描述機械運動的時空的「瞬」標志著古典數學原子論的積分觀向現代的分割實數續統的積分觀的轉化,而現代數學的微分概念更是直源於描述機械運動的速度和與運動軌跡密切相關的曲線的切線問題。
  2. This time, using cdna of zmcdc5 as template, we amplify a sequence by means of pcr technology. and then, using restrict endoenzyme and ligase, we conjunct the 0. 8kb length dna sequence in a expression vector, pet - 30a. after induction, expression and purification, we obtained a 35. 4kda truncated fusing zmcdc5 protein which contains 267aa ( 647 to 914aa in zmcdc5 ). with the purified protein, we got its antibody and testified the antibody by means of western blotting and dot blotting

    本實驗是以zmcdc5的cdna為模板,使用pcr獲得基因,再通過酶切,將得到的0 . 8kb的基因構建於pet - 30a表達載體上,經過誘導表達和純化,獲得zmcdc5的融合蛋白,其中包括了zmcdc5925個氨基酸中647 914共267個氨基酸殘基
  3. In this paper, first strand cdna of 3abc gene was synthesized using template rna extracted from cells infected with fmdv. the complete 3abc gene about isoobp was amplified by pcr and ligated into pgem - t easy vector. after transforming e. coli dh5 a, ampicillin resistant colonies were isolated and plasmid dna was prepared and analyzed by restriction analysis and pcr. presence of the full length 3abc gene was verified by nucleotide sequence analysis and the plasmid containing the expected sequence was named as pgem - 3abc. comparing the aquired sequence of 3abc with that of reference strains, the homology is more than 99 percent. the pgem - 3abc was digested with sal i and bgl ii and ligated into xho i and bgl ii - digested expression vector ptriex - 4 neo. lt was identified by restriction analysis and pcr and sequencing that this fragment had a 17bp deletion hi the nucleotide sequence 708bp of 3abc gene, which happened to form a terminator codon behind 3ab gene, but it contained the complete open reading frame ( orf ) of 3ab gene. positive clones were selected and induced with lmmol / l isopropyl - d - galactoside ( iptg ), bacteria were detected by sds - page and western blotting after properly treated. the results showed that the 3ab gene expressed successfully in e. coli and 33. 5ku fusion protein can be recognized by the positive bovine serum of fmdv. the amount of target protein is over 26 % of the total bacteria protein by gel thin layer scanning analysis

    擴增產物到pgem - teasy載體中,轉化大腸桿菌dh5菌株,篩選氨芐青霉素抗性菌落,提取質粒經酶切鑒定、 pcr分析以及確證性測序證明,所克隆的1500bp左右的含有完整的3abc基因,與國外參考序列相比,同源性在99以上。將重組質粒pgem - 3abc和表達載體ptriex - 4neo分別用sal和bgl與xho和bgl消化后,亞克隆3abc基因至原核表達載體ptriex - 4neo中,通過酶切鑒定、 pcr擴增以及序列分析,發現克隆到ptriex - 4neo載體上的於3abc基因708bp處出現了17bp的缺失,碰巧在3ab基因后形成一終止密碼子,但3ab基因的閱讀框架完整,選出含有3ab基因完整閱讀框架的陽性克隆,用iptg誘導表達,收集菌液進行sds - page電泳、 westernblotting分析,結果表明, 3ab基因在大腸桿菌中成功表達,其表達產物為分子量33 . 5ku的融合蛋白,並能被口蹄疫病毒陽性血清識別。經薄層掃描分析,表達量占總蛋白量的26以上。
  4. Reclamation, purification and linkage of them respectively, then sequencing and analyses of according gene structure were made, results show that the complete sequence length of corresponding pcr product from brussel sprouts, kohlrabi and kale are 1665bp, 1650bp and 1650bp, containing the first two exons and introns and 22bp of the third exon

    對各pcr產物分別進行回收、純化、載體和序列測定及基因結構分析等,結果表明,該在抱子甘藍、羽衣甘藍和球莖甘藍三種作物中的全長分別為1665bp 、 1650bp和1650bp ,包括相應基因的前兩個外顯子和內含子以及第三個外顯子的22bp序列。
  5. 4. the construction of middle - clone vector and expression vector the puc - cp and pgem - 7z plasmid were digested by kpnl and bamhi, and collected the digested cpti fragment and the pgem - 7z, then ligated by t4 dna ligase and formed the pgem - cp

    中間載體及表達載體的構建將puc - cp質粒和pgem ? 7z質粒,用kpni和bamhi酶切,分別回收cpti斷和酶切后的載體,用t _ 4構建成中間載體pgem - cp 。
  6. Healthy rabbits were inoculated each with vaccine of the recombinant fused pili - el - 2 protein at 250ul per dose to potentiate the immunogenicity. rabbits inoculated two times at one week interval

    擴增此質粒,回收bamh切出的2 . 5kb的基因,與pme290 ( bamh酶切後去磷酸化)載體
  7. Secondly, the effort is made to develope new type of transition element for multi - scale fatigue damage simulaton of long - span structures for the transition between elements for the hot spot stress analysis and the structural element. the linear and piecewise linear interplotion function for displacement interplotion are used for the transition element formulation according to the displacement compatibility requirement between element interfaces

    在綜合已有的構造過渡單元模型關于位移插值形式的基礎上,通過採用分線性位移插值模式和線性位移插值方式,並在位移模式中引入非協調位移模式,強迫構造單元通過分試驗,構造了一種用於疏密網格單元過渡單元。
  8. The c - phycocyanin ( cpc ) operon of blue - green alga ( or cyanobacteria ) arthrospira platensis fachb341 was cloned, sequenced and characterized by using chromoseme walking method. the sequence includes cpcb gene ( 519 bp ), cpca gene ( 489 bp ), cpch gene ( 357 bp ), and upstream sequence of cpcb ( 427 bp ) and upstream sequence of cpch genes ( 184 bp ), 111 bp of phycocyanin intergenetic spacer ( pc - igs ). upstream sequence of cpcb gene was ligated into promoter - probe vector pegfp - 1 and transformed into three systems : e. coli, synechocystis pcc 6803 and a. platensis fachb341 by supersonic and electrophoresis methods

    根據genbank中報道的節旋藻藻藍蛋白基因序列設計引物,首先克隆了鈍頂節旋藻( arthrospiraplatensisfachb341 )藻藍蛋白操縱子中亞基基因、亞基基因部分序列及二者之間的間隔區序列( pc - igs )並進行序列測定,然後根據此測序結果設計引物,通過染色體步移法克隆得到藻藍蛋白操縱子長度為2086bp的基因,其中包括藻藍蛋白亞基基因( cpcb , 519bp ) ,亞基基因( cpca , 489bp ) ,蛋白h基因( cpch , 357bp ) ,亞基基因上游啟動子序列( 427bp )以及各基因之間的間隔區( pc - igs , 111bp ; cpch與cpca間隔區, 184bp ) 。
  9. An infectious eiav clone was recovered by transfecting fatal donkey dermal ( fdd ) cell cultures and donkey leukocyte ( dl ) culture in vitro with the full - length gene clone of dv. the virus ( designed pd70344v ) derived from the third passage in dl culture was observed by electron microscope and the reverse transcriptase ( rt ) activity was determined

    將包含全基因的三個基因克隆以限制性內切酶消化后順次克隆到載體ptz18r上,構建了4個全長基因的分子克隆,分別命名為pd30343 、 pd70333 、 pd70343 、 pd70344 ,其中兩個轉移到低拷貝載體plg338上,命名為plgd30343 、 plgd70344 。
  10. Artificially using t - a cloning techniques and initiated one - step ligation of multi - fragments method were the main factors in the process of full - length cdna construction

    T - a克隆的巧妙運用和多一步法的成功運用是全長cdna得以快速構建的主要原因。
  11. Using rt - pcr with two degenerate primes designed from conserved amino acids of cdpk kinase and autoinhibitory domains, three 618 bp cdna fragments ( 618 - 1. 618 - 2 and 618 - 3 ) were also isolated from broad bean leaves, and a partial cdna vjcpk2 lacking 5 " end was isolated from broad bean leaves with two gene - specific primers designed according to the 618 - 1 sequence

    用rt - pcr技術,以cdpks激酶區和區的保守氨基酸設計的一對簡並引物,從蠶豆葉中還擴增到了3個618bp ( 618 - 1 、 618 - 2和618 - 3 )的cdna;用race技術,以618 - 1序列設計的一對基因特異性引物,克隆到了還缺少5 』末端的cdnavfcpk2 。
  12. Thirdly, the hyl gene was cloned to puc19 and pbr322 respectively. then the fragment containing ampr derived from puc19 and hasa came from pse380 - has were inserted into hyl either or both in vitro. transformed the recombinated vectors into s. equi by electro - operation, then plating on hag solid medium containing ampicillin, and selected clones hi which the hyl gene was inactivated by gene replacement through homologous recombination

    ( 1 )直插入外源基因滅活hyl方法:將hyl與載體puc19 pbr322后,用來自puc19的amp ~ r抗性基因從hyl基因的中部插入將載體上的hyl分為兩部分; ( 2 )用hasa替換hyl部分的方法:將hyl與載體pucl9 pbr322后,用hasa替換部分hyl ,再將amp ~ r入到hasa上游。
  13. Clone human wnk4 full length cdna into pgem - t vector human kidney total una was extracted and used as template to amplify wnk4 full length cdna with the forward primer ( 7 - 27 ) and reverse primer ( 3808 - 3833 ) with the long template expanded pcr system kit

    5 .原位雜交以小鼠腎臟總翩a為模板,擴增wnki基因外顯子1 , 24一28 ,以a和wnk4基因外顯子13一16,純化后在pgem一t載體上。
  14. What we thought was that, it would be nice if kima could schedule the screening a little earlier and made the interval in between longer, especially the interval between the first and the second screening, so that people could have time to go for dinner

    他認為電影不是拍出來的,而是從逐格逐格的或畫面組合而成的。如果要電影產生意思,必須在組合上做到作用,而非相互沖突。
  15. After watching three films in a row, k. lui and i were both exhausted. what we thought was that, it would be nice if kima could schedule the screening a little earlier and made the interval in between longer, especially the interval between the first and the second screening, so that people could have time to go for dinner

    在他眼中,蒙太奇不是沖突,而是。他認為電影不是拍出來的,而是從逐格逐格的或畫面組合而成的。如果要電影產生意思,必須在組合上做到作用,而非相互沖突。
  16. 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為基礎,將1 . 5kb的安普黴素抗性基因插入到avec基因中的sphi酶切位點,再將此插入失活的avec基因到具有合轉移功能(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,由此得到重組質粒pc05 。
  17. In order to check if it is the aim gene, we devised pcr with a new pair of primer, sequenced and registered the product with registration number : af449446. moreover we forecast and analysis the primary, secondary, tertiary and quaternary structure of the three protein : osftszi, crftszi and crftsz2 which has already cloned by our team before. after that we construct ftsz molecular evolution tree to site them in

    又將生物信息學技術同實驗技術相結合,針對ftsz保守區設計引物擴增出一條衣藻ftsz,進行est搜索、比對、拼,最終克隆出新基因crftsz1 ;同本試驗室曾經獲得的另一個衣藻crftsz2基因進行蛋白質的一、二、三、四級結構預測、分析及比較尋找進化線索,建立了ftsz蛋白的氨基酸進化樹作進一步的進化定位。
  18. 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,然後插入到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回收純化的目的與3301質粒進行,再對重組子進行平板篩選和酶切分析確定ta29 - hsp70sensecdna - nos和ta29 - hsp70antisensecdna - nos插入到3301質粒中,構建成3301 + 650和3301 + 651表達載體。
  19. This method has several strong points : ( 1 ) eliminating the possibility of ringing self of vector. ( 2 ) the inserting fragments ca n ' t ligate each other. ( 3 ) the translating rate with the partially filled in method is equal to phosphatase method

    末端半補齊技術的優點有: ( 1 )徹底消除載體自環化的可能性; ( 2 )消除了插入自身相互的可能性; ( 3 )同常用的堿性磷酸酯酶法相比較,採用半補齊技術其產物的轉化率不受影響。
  20. Then, the plasmid was transformed into jm109. the full length pstvd cdna recombinant plasmid was further identified by restriction mapping analysis and the nucleotide sequence of cdna cloned in pmd 18 - t vector was analyzed with ab1 377 dna sequence. test showed that the cdna of this chinese pstvd isolate was the same as pstvd - kf - 6 mild " type " isolate which originated from naturally infected potatoes in field of cornell university potato breeding program

    利用rt - pgr技術,設計一對引物,對田間採集的經鑒定含pstvd的陽性樣品進行全序列擴增,並將所得產物純化回收,到pmd18t - vector中,並轉化至大腸桿菌jm109中,挑選白斑進行雙酶切( saci / ecorv )鑒定證明插入為359bp大小,進行序列測定,所得克隆基因為pstvd全序列負鏈,大小為359bp 。
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