標記基因 的英文怎麼說

中文拼音 [biāoyīn]
標記基因 英文
labelled gene
  • : Ⅰ名詞1 [書面語] (樹梢) treetop; the tip of a tree2 (枝節或表面) symptom; outside appearance; ...
  • : Ⅰ動詞1 (把印象保持在腦子里) remember; bear in mind; commit to memory 2 (記錄; 記載;登記) writ...
  • : Ⅰ動詞[書面語] (沿襲) follow; carry on Ⅱ介詞1 [書面語] (憑借; 根據) on the basis of; in accord...
  • 標記 : (標志; 記號; 貨物標記) tab; sign; stamp; peg; label; mark; flag; blip; notation; fleck; track; ...
  1. Hitchhiking effects also play a role in experiments with marker genes.

    附加效應在以標記基因作試驗中也是起作用的。
  2. Three methods for rapid selection of transgenic cotton plants in laboratory with kanamycin as indirect marker

    標記基因的轉抗蟲棉室內快速鑒定方法
  3. Methods : ( 1 ) the segregation of foreign target gene in the t1 by histochmical gus assays ; ( 2 ) identification of pure line from transgenic tomatoes ( tl ) through examining gus expression in pollens in conjunction with pcr analysis of marker gene ( npt ) ; ( 3 ) the transcript levels of leetrl or leetr2 in anti - sense transgenic plants ; ( 4 ) the phenotypes of the transgenic plants in tomato during whole life cycle under ethylene - treated and non - treated conditions

    本研究以反義乙烯受體leetr1 , leetr2番茄t _ 0代種子為實驗材料,利用gus表達研究外源的遺傳規律,並藉助于pcr技術對目的和標記基因的鑒定獲得轉t _ 1代材料。利用gus在t1花粉中的表達鑒定獲得轉純合植株。研究了轉後代的生長發育模式、對外源乙烯敏感性,以及靶的表達特性,初步探明了它們在乙烯受體系統中的功能。
  4. 7. at the first time, the reporter dye, fam was linked to the 5 " - end of the oligonucleotides of the probes, and the tamra was located at the 3 " - end as quencher dye. we use camv35s and fmv promoter, nos terminater, mark gene nptii, and aim gene pat, epsps and cryla ( b ) genes as target sequences, design pairs of sp

    7 、首次以fam熒光素探針5 』端作為發光團,以tarma探針3 』端為淬滅團,以camv35s 、 fmv啟動子、 nos終止子、標記基因nptll 、抗除草劑epsps 、 pat 、抗蟲cry1a )為檢狽目,設計、篩選出特異性引物和探針,優化實驗參數,建立了轉植物通用性熒光pcr定性檢測方法體系。
  5. Sv40 polya signal and two loxp sites was added consecutively after the termination codon taa, and then a gfp gene was inserted between the two loxp sites

    在三個終止密碼子taa之後,連上sv40polya 。 sv40polya之後,又連上兩個loxp位點。在兩個loxp位點,插入標記基因gfp 。
  6. Transgenic plants and their marker gene knock - out

    農作物及其標記基因的消除
  7. As part of the project to improve isoflavone contents of legume forage by introducing isoflavone synthase ( ips ) gene, in this work, we have established the agrobacterium - mediated transformation system of white clover

    A311帶有pbi121質粒,該質粒攜有gus,其啟動子為35s啟動子,篩選標記基因為npt 。
  8. We constructed a binary vector carrying a modified human afgf gene and a mana gene that allows the use of pmi selection system, an antibiotic and herbicide - free system, during the transformation procedure

    我們構建的雙元表達載體帶有一個經過改構的人類酸性成纖維細胞生長( afgf ) ,載體上的選擇標記基因為mana ,它使得轉化過程中可以使用pmi這種不含抗生素及除草劑的選擇系統。
  9. To target this mitochondrial enzyme into chloroplast, the cdna sequence of mnsod was fused to a chloroplast transit peptide from a pea rubisco small subunit gene, whereas expression of the chimeric gene was driven by the camv 35s promoter

    Pchlsod質粒含有煙草mnsod的cdna序列,與豌豆核糖體小亞葉綠體引物肽( tp )的編碼序列構成融合,由35s啟動子調控。 npt為選擇標記基因, pgv2260為輔助質粒。
  10. ( 2 ) the interest gene in pcar is under the control of acti which is the strong promoter in rice. the selectable marker gene is hyg gene

    ( 2 )表達載體pcar中目的由單子葉強啟動子水稻act1啟動子調控,選擇標記基因為潮黴素抗性
  11. The new measures are a function of the genetic distance between the marker locus and a qtl. through simulations, we found that when marker allele frequencies vary across loci, the previous hwd measures are biased and not powe

    計算機模擬表明,當各標記基因頻率不同時,用以前的hwd指數精細定位會產生偏差,新的指數可以有效的進行精細定位,使用y > u和y < t的樣本的lcd的功效普遍比僅僅使用y > u的樣本的氣回,的功效高。
  12. Finally the expression cassette of the two genes were inserted into binary vector pbin19

    最後得到的植物表達載體pbm含目的及植物選擇標記基因npt 。
  13. 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。
  14. Kurstaki strain hd73, were inserted into two copy sets of res sites. the res sites have same direction. when - the recombinant plasmid was introduced into crystal negative b. thuringiensis host bmb171, antibiotic resistance genes and other non - 5, thuringiensis dna can be selectively eliminated after the selection by antibiotic resistance marker

    將crylac10或壯觀黴素和蘇雲金芽胞桿菌的質粒復制起始區oril030連接在一起,置於兩個同向的解離區之間,再將操作中所必需的大腸桿菌質粒復制起始區和抗生素標記基因等與之相連構成解離載體。
  15. Based on the foundation research of the interaction of virus and host actin, we recombine gfp gene - a reporter gene - with 5c actin gene of drosophila melanogaster, a gfp - actin fusion gene was obtained

    本文在總結前人關于病毒與宿主肌動蛋白相互作用的研究的礎上,利用綠色熒光蛋白標記基因,與果蠅肌動蛋白5cactin融合,構成gfp - actin融合
  16. On the development and its safety management of the agricultural transforming gene biological products

    植物中的標記基因
  17. 5. in this study, we have cloned camv35s and fmv promoter, nos terminater, mark gene nptii, and aim gene pat, epsps and cryia ( b ) genes used as positive collate

    5 、克隆了camv35s 、 fmv啟動子、 nos終止子、標記基因nptll 、抗除草劑epsps 、 pat 、抗蟲cry1ao )的陽性質粒作為轉植物檢測的陽性對照。
  18. Linkage analysis plays an important role in gene mapping. the foundation : the two gene locuses which locate on the same chromosomal ( eg. disease gene and marker gene ) happen to cross over and recombine. the farther the distance between two locuses is, the higher the probability happening to cross over is, the lower the probability that the two locuses are inherited to offspring together is, that is, the degree of linkage is not strong. so we can estimate the distance and the degree of linkage by the recombination fraction between the two locuses to locate gene

    連鎖分析是定位主要策略之一,其本原理是位於同一染色體上兩個位點(例致病標記基因)在減數分裂的過程中會發生交換與重組,染色體上的兩個位點間距離越遠,發生重組的概率就越大,兩個位點在一起傳給後代的機會就越少,即連鎖程度弱,這樣由位點與疾病位點間的重組率可估算出兩者間的距離以及連鎖程度,達到定位的目的。
  19. If we study on the phylogenetic relationship in intra - genus or intra - species using gapdh as a target gene, it may be make a discrepancy

    對于距現今較近的動物,用其作為近親緣關系的屬內種間的標記基因,可能產生偏差。
  20. This expression vector plbcas - hsa - lgl has the following advantages : i ) the 1. 7kb promoter is able to drive cell - specific and hormone - dependent expression ; ii ) the inclusion of intron - 1 can increase expression level of fusion genes ; iii ) the 5 ' utr of bovine p - casein mrna may have a positive role in both transcriptional and post - transcriptional regulation ; iv ) the gfp gene make the selection of positive clone among embryos possible ; v ) the gfp gene can be easily excised via cre - mediated recombination between the two loxp sites after the expression vector has been integrated into chromosome ; vi ) the two incompatible lox sites, loxp and lox2272, would facilitate cre - recombinase mediated cassette exchange ( rmce ), which in theory will leading to develop a technology of site - specific gene expression in animal mammary glands

    該載體的特點是:具有可以調控外源在乳腺中特異表達的牛-酪蛋白5 `端側翼區和包括第一外顯子及內含子在內的5 `端調控區;將人血清白蛋白cdna準確地置於牛-酪蛋白第二外顯子中的翻譯起始密碼子atg之後,而且沒有增加額外的序列和使人血清白蛋白cdna移碼;引入標記基因gfp ,便於在胚胎期鑒定陽性胚胎,減少受體;引入cre lox重組系統: ( ? )標記基因gfp的兩端的兩個loxp位點可以在表達載體整合到組后,刪除標記基因; ( ? )餘下的一個loxp位點可以和前面的lox2272位點組成cre重組酶介導的盒式交換系統。
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