細菌結構基因 的英文怎麼說

中文拼音 [jūnjiēgòuyīn]
細菌結構基因 英文
bacterial structural gene
  • : 形容詞1 (條狀物橫剖面小) thin; slender 2 (顆粒小) in small particles; fine 3 (音量小) thin ...
  • : 菌名詞1. (蕈) mushroom2. (姓氏) a surname
  • : 結動詞(長出果實或種子) bear (fruit); form (seed)
  • : Ⅰ動詞1 (構造; 組合) construct; form; compose 2 (結成) fabricate; make up 3 (建造; 架屋) bui...
  • : 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...
  • 細菌 : germ; bacterium (pl. bacteria); fungus (pl. fungi)
  • 結構 : 1 (各組成部分的搭配形式) structure; composition; construction; formation; constitution; fabric;...
  1. Quinic acid, used shikimate pathway in e. coli, it is necessary to extend metabolic pathway by introduction of a heterogenous gene qutb into the host cell. double specific enzyme genes arog, qutb or three ones arog, qutb, arob were co - expressed in a single plasmid pbv220 to improve the enzymes " rate - limiting reactions. modifications of e. coli chromosome by both disruption of the arod gene and directed - site insertion of the arob gene resulted in the change of carbon flow redirected into the quinic acid biosynthesis branch

    利用大腸桿莽草酸途徑合成新的代謝物奎尼酸,須在宿主胞引入異源酶擴展代謝途徑;串聯表達酶,同時適量增加不同種屬的多個關鍵酶酶量,改善限速反應;利用同源重組進行整合和破壞,改造染色體定向改變微生物代謝途徑;目的是將碳代謝流最大程度的引向奎尼酸生成的方向。
  2. The deleted mutant pap gene was also cloned into yeast secreted expression ppic9k vector to form ppic9k ~ 3, then the vector was transferred into pachia pastoris gs115 strain. the specific expression protein was secreted into the medium after inducing with methanol and the protein amount reached about 50 - 60 u g per millilitre measured by uv - absorbed methods in the supernatant of the medium via high density fermentation. sds - page results showed that there was one protein band in the gel which molecular weight was about 34ku

    將缺失型pap克隆于酵母分泌型表達載體ppicgk成重組載體,然後導入畢赤酵母( p8chianastoris )株gslls胞中,在甲醇的誘導下,經過酵母高密度發酵進行pap的表達,經sds page分析,果表明,在培養上清液中含有一明顯的特異性蛋臼條帶,大小為34ku ,經western blotting分析,該蛋白與法國pap抗血清有特異性反應,體外活性檢測表明該蛋白對tmv的侵染性具有高度的抑制性,說明該pap在畢赤酵母gs中也得到了正確表達。
  3. In terms with the principle of fusarium oxysporiun caused plant disease : bundles were blocked and fusarid acid killing cells was formed by hyphae so that caused water metabolism abnormal and plant wilting. in order to find out effective method of anti - fiisarium oxysporuin, long ya lillium was taken as material with plant tissue culture and genetic transformation techniques in this paper

    針對尖孢鐮刀的致病機理:絲阻塞維管束引起水分代謝失常和絲在植物體內產生毒素(鐮刀酸)損害膜造成代謝失常,從而導致植物萎焉。本實驗以龍牙百合為研究對象,應用胞工程中的離體培養方法並合轉技術,以期找到抗尖孢鐮刀的有效途徑。
  4. Objectives to improve the effect of a single mtb8. 4 dna vaccine, we constructed a chimeric mtb8. 4 / hil - 12 eukaryotic plasmid by linkage of mycobacterium tuberculosis mtb8. 4 gene to human il12 gene with a simple linker ( gly4 - ser ) 3. we analyzed the immunogenicity of chimeric dna vaccine and investigated the immune responses elicited when mtb8. 4 / hil12 was presented as endogenous ag

    目的:以il - 12作為分子佐劑,與核桿新抗原mtb8 . 4連接形成嵌合分子,將其克隆到真核表達質粒中,建成嵌合dna疫苗,研究其在小鼠體內誘導胞免疫應答的效果及對c57bl 6n小鼠的免疫保護作用,為尋求安全、有效、廉價的核病新疫苗打下礎。
  5. The photoabsorption properties of three kinds of br molecule films ( the wild - type br, the chemical enhanced br, the gene - variant br ) are investigated by measuring their absorption spectrum. using the gene - variant br film as a light - modulator, by the experiment of write - readout image and the analysis of image contrast, the light - modulated property of the modulator is studied. the relationship between wavelength of the modulated light and response time of the modulator is discussed emphatically

    本論文概述了視紫紅質分子、功能特性及研究發展的歷史與現狀,介紹了目前已有的和潛在的一些重要應用,通過對吸收光譜響應特性的測試研究了三類br分子薄膜(野生型,化學修飾型,修飾型)的光吸收特性,通過圖像的記錄/讀取實驗及圖像的對比度分析探討了改性型br分子薄膜的光調制特性,著重研究作為一個光調制器件對調制波長和調制時間的響應特性。
  6. In this experiment hcv structural gene was amplified by polymerase chain reaction ( pcr ), and was inserted into baculovirus expression vector pfastbacl to construct a recombinant transposing vector pfbl - cee. the plasmid pfb 1 - cee was transformed into dh1 obac competent e. coli cells. high molecular weight dna was prepared from the overnight cultures from the selected e. coli colonies, which was recombinant baculovirus shuttle vector containing hcv structural gene, named bac - cee

    本實驗用pcr擴增hcv,克隆到桿狀病毒表達載體pfastbacl中,建成重組轉座載體pfb1 - cee ,轉化dh10bac大腸桿感受態胞,篩選陽性落,抽提大分子質粒dna ,獲得含hcv的重組桿狀病毒穿梭載體bac - cee ,脂質體介導轉染sf9昆蟲胞,出現胞病變后,收集含有重組桿狀病毒顆粒的培養上消,重新感染sf9胞,收集sf9胞,進行12 . 5 sds -聚丙烯酰胺凝膠電泳,可見表達的蛋白條帶。
  7. In order to further investigate the role of axudl in human tumor carcinogenesis and the potential association between the axudl gene expression status and the stimulation of transforming growth factor beta in human cancers, the present study was performed in three aspects as follows : ( 1 ) cloning full length enconding region cdna of axudl and construction of eukaryotic vector that expression the fusion protein of axud1 and influenza virus hemagglutin ha epitope tag ; ( 2 ) exploring the time and dose effects of tgf - 1 on the expression - of axudl gene in hepg2 hepatoma cells and spc - a1 lung carcinomas cells, and studying the effects of overexpression of axud1 on the expression of cell cycle and apoptosis related protein in hepg2 hepatoma cells ; ( 3 ) construction and expression of human axudl in e. coli m15. the following main results and conclusions can be obtained from the present study : 1. the full length ecnoding region of human axudl cdna from human peripheral blood lymphocytes was successfully cloned using one step rt - pcr method, and constructed into a eukaryotic expression vector which can be expressed a ha - axud1 fusion protein with axud1 and influenza virus hemagglutin ha epitope tag. the recombinant plasmid was identified by polymerase chain reaction, restriction endonuclease maping and sequencing, this expression vector might be instrumental to further study the function of axud1 protein in tumor cells

    為了進一步研究axud1在人類腫瘤發生中的作用及axud1的表達狀況與tgf -介導的信號通路的關系,本實驗研究分為三個部分: ( 1 ) axud1cdna全長編碼區的克隆和ha表位標記的axud1表達載體的建; ( 2 )探討肝癌胞hepg2和肺腺癌spc - a1胞中tgf - 1誘導的axud1表達的時間、劑量效應以及誘導表達的可能機理,並研究axud1的過表達對胞周期和胞凋亡相關蛋白表達的影響; ( 3 ) axud1原核表達載體的建及其在大腸桿中的表達。本實驗的主要果和論如下: 1利用一步法rt - pcr成功地從人類外周血淋巴胞中克隆出axud1編碼區cdna ,並將其建入真核表達載體中,編碼的ha - axud1融合蛋白帶有流感病毒凝血素ha的表位標記肽段。
  8. With bacterial cgc as main subject, the tests had been done to elucidate mechanism of self - organization for macroscopic rhythmic structure. the dynamics of cgc forming was observed by special techniques of waving culture and microscopic culture ; the differences in outer structure of cell wall and flagella number had been observed by atomic force microscope scanning ; integrity of cell wall was examined under tem ; outer membrane protein was analysed by sds - page and various substance and factors for cgc formation were determined

    採用特殊的波動培養和顯微培養技術觀察潛生體形成動態;應用原子力顯微鏡掃描,比較潛生體與繁殖體在胞壁外層和鞭毛數量的差別;用透射電鏡觀察胞壁完整性,以十二烷硫酸鈉?聚丙烯酰胺凝膠電泳分析外膜蛋白的改變,並通過實驗分析多種物質和素對潛生體形成的影響。
  9. In order to get some functional clues from their structures, the upstream regulation region of ndrgl gene and second structure of ndrg2 protein are performed bioinformatics analysis ; we found that there are several binding sequences of some diffirent transcription factors, their functions include regulating tissue - specific gene expression, regulating expression of genes related to growth and early development of cells, besides this, regulating expression of genes under some stimulated conditions, and so on. predict in protein fold classification shows that ndrg2 belongs to alpha / beta hydrolase fold family, and there are high similarity between ndrg2 and epoxide hydrolase from bacteria, this suggests that ndrg2 protein may has enzymatic functions associated with resisting the oxidative stress, maintaining the balance of cell redox potential, involving in the metabolism process of xenobiotics or intracellular toxic molecules

    研究發現呷的調控區存在多種轉錄合位點,功能主要涉及組織特異性表達調控,胞生長發育相關的表達調控,刺激反應的表達調控等; ndrgz蛋白在上屬于a小水解酶類折疊,折疊分類預測表明ndrg2與其中的的環氧化物水解酶的二級極為相似,提示ndrgz蛋白具有一定酶活性,可能參與胞抗氧化應激反應,維持, an ) armtbffiofbfochmilsyn ) mdafblechmrbfobo4第四軍醫大學碩士學位論文胞內氧還電勢平衡,參與內外源有毒物質的代謝等。
  10. These phage display peptides may be the tnfa mimotopes. part iii specific c7c tnfa mimotope phage clone as target for screening of tnfa specific binding - peptides from 12mer phage display peptide library : by using the specific c7c tnfa mimotope as target, we developed a novel approach for screening phage peptide library targeting specific phage display peptides. we used c7c tnfa mimotope phage clone lcs - 7 ( c - rrpaqsg - c ) as target to screen 12mer phage peptide library and identify the positive clones by phage elisa

    3 、以特異性噬體克隆為靶篩選肽庫的研究? ?一種肽庫篩選新方法的建立:為了深入研究於與配(受體或抗體)相互作用的關鍵殘及其空間象,在上述研究礎上,我們以tnfa表位模擬肽克隆為靶篩選噬體十二肽庫,找尋與之合的tnfa合肽噬體克隆;並以此拓寬了噬體肽庫的應用范圍。
  11. Hsp70, a kind of molecular chaperone, has the main functions of taking part in protein folding, protein degredation and reparation of dna damadge and has important effects on the constructure and function of mitochondria. it has already been proved that there is a close correlation between hsp70 and the development of plants and animals. this paper deals with integrating sense and antisense cdnas of hsp70 into tobacco dna by constructing an expression vector of sense and antisense cdnas of hsp70 and gene - transforming methods - genegun bombarding and agrobacterium mediation. provided expression of hsp70 gene is inhibited by sense and antisense cdnas of hsp70 we can get male sterile plants so as to prove that antisense cdna of hsp70 leads to male sterility 1

    Hsp70是一種分子伴侶,主要功能是參與胞有關蛋白新生肽的折疊、亞組裝、胞內運輸、蛋白質降解及dna損傷的修復,對線粒體和功能發揮重要作用,已有研究證明hsp70與動植物的發育有密切的關系,本研究將hsp70正、反義cdna建成表達載體,並運用槍和農桿介導法將hsp70正、反義cdna導入煙草,試通過hsp70反義cdna抑制hsp70的表達從而創造雄性不育株,以證明hsp70反義cdna能創造雄性不育系。
  12. In this study, the recombinant plasmid pmd - 18t - pea - h3 was cleavaged with ncoi, xhoi and inserted into the expression vector pet - 28c and subsequently subjected to restriction endonuclease analysis and sequencing, the result indicated that the prokaryotic expression vector pet - 28c - pea - h3 was constructed successfully. after the expression plasmid was extracted and transformed into expression hosts bl21 ( de3 ) of e. coli, the transformed hosts were induced by iptg, bysds - page and elisa analysis of host protein. the expression of the objective gene was detected, and it could account for 16. 28 % of the total host protein. inclusion body was prepared from the incubating expression hosts induced by iptg

    同時將原核表達載體pet - 28c用nco , xho雙酶切,回收酶切產物,將回收的酶切產物pea , h3 ,載體進行連接,並轉入dh5感受態胞內,培養12 - 18小時后,挑取陽性落,經nco , xho雙酶切分析及pcr檢測,篩選到陽性克隆,其質粒測序果表明成功地建了毒性缺失的pea與人組蛋白h3融合的原核表達載體。
分享友人
分享到 Line

分享到臉書