prokaryotic 中文意思是什麼

prokaryotic 解釋
初核質
  1. Prokaryotic expression of vp2 gene of infectious bursal disease virus and antigenicity of expressed product

    2基因的原核表達與抗原性分析
  2. Prokaryotic expression of dnaj - homologous chaperon pbp and preparation of rabbit antibody against pbp

    的融合表達及其抗體的制備
  3. Compared to the prokaryotic gene expressing systems and mammalian gene expressing systems, insect gene expressing systems possess the stronger ability of the transcription and post - translation processing, which also has high production. we can anticipate it will be a kind of potent effective ectogenesis eukaryotic gene expressing system

    與原核表達系統和哺乳動物細胞表達系統比較,昆蟲細胞表達系統既有較強轉錄和翻譯后加工修飾能力,又有高表達量等特點,可望成為基因產業中一種比較理想的外源真核基因表達系統。
  4. Prokaryotic expression and characterization of n - terminal truncated glycoprotein gp85 of epstein - barr virus

    端片段的原核表達與初步鑒定
  5. Since the important roles of eo protein in the viral infection. immunity and virus - host interaction. the homology of 21 csfv strains was investigated by sequence analysis of eo genes in this study, which will provide some evidence for epidemiological study. in addition, the eo gene of hog cholera lapinized vaccine ( hclv ) strain was expressed in the prokaryotic and eucaryotic systems, and the recombinant proteins were preliminarily analyzed by immunological method

    鑒于eo蛋白在病毒感染,誘導機體免疫及與宿主細胞相互關系中的作用,本研究克隆了2株豬瘟病毒eo基因並將其與其它毒株eo基因進行了序列分析,揭示了我國豬瘟病毒流行株之間的遺傳演化關系,為豬瘟病毒的流行病學研究提供依據。
  6. Conclusions : prokaryotic and eukaryocytic expression plasmids of the shortened hepatitis b surface antigen were successfully constracted, and the target proteins expressed by iptg induced in escherichia coli. as well as in eukaryocyte ( hepg2 and cos - 7 ), then their antigenity were detected

    結論:截短的乙型肝炎表面抗原分子的原核和真核表達』重組質粒成功被構建及分別在人腸桿菌efl得到誘導表達和存貞核細胞ifj表達,並檢測劍其表達產物的抗原特性。
  7. Prokaryotic expression of neural cell adhesion molecule l1 - ig and its function

    的原核表達及其功能
  8. Cloning, prokaryotic expression of the mink prp precursor gene

    水貂朊蛋白前體基因的原核表達
  9. Construction of the prokaryotic expression vector of mtb lhp gene and its expression

    基因原核表達載體的構建和表達
  10. Polymer his - tagged peac1 - gfp efficiently activated myosin mg - atpase activity, which indicated that peacl might take part in correlative living activities in vivo. moreover, this result provided experimental proof in vitro for fusing gfp to actin isoform directly to study the dynamics of microfilaments and its regulation in vivo. we prepared rabbit anti - pea actins polyclonal antibodies using peacl as antigen which being expressed and purified from prokaryotic cells, and the antibodies possessed better immunity activity to pea actins

    通過肌動蛋白體外對dnase以及肌球蛋白atpase活性影響的研究,發現單體his - taggedpeac1 - gfp能顯著抑制dnase活性,在肌動蛋白聚合條件下能有效激活肌球蛋白atpase活性,這一結果預示著peac1在體內可能參與相關的生命活動,為利用gfp直接與肌動蛋白異型體融合來研究體內微絲的動態變化及其調節提供了實驗依據。
  11. 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基因插入原核表達質粒載體prset和pet28的bamhi / hind位點,成功構建重組表達質粒prt - p450nor和pet - p450nor ,並轉化到e . colibl21 。
  12. Prokaryotic microbial diversity of the ancient salt deposits in the kunming salt mine, p. r. china

    昆明鹽礦古老巖鹽沉積中的原核生物多樣性
  13. Cloning and construction of prokaryotic expression vector of vp1 gene of foot - and - mouth disease virus serotype o

    1基因的克隆及原核表達載體構建
  14. Full - length or truncated cdna was subcloned into prokaryotic expression vector pet30a and expression induced in e. coli bl21 ( de3 ). no squalene synthase polypeptide of expected molecular mass was observed in e. coli containing the putative full - length squalene synthase cdna, however, overexpression in e. coli was achieved by truncating 30 hydrophobic amino acids at the carboxy terminus

    但在含有全長的鯊烯合酶cdna的大腸桿菌中並沒有觀察到預期大小的鯊烯合酶表達,而c末端截短30個疏水氨基酸的鯊烯合酶可在大腸桿菌中過量表達。
  15. This paper is a study on the expression of the protective gene of bont / a in the prokaryotic and eukaryotic. it indicates the possibility to produce the recombinant protein in quantities. it has also laid down a good foundation for the further research on vaccine or antibody of bont / a

    本論文進行了人工合成的a型肉毒毒素hc段基因在原核和真核表達系統中的表達研究,使制備大量bont a保護型抗原的重組蛋白成為可能,為進一步進行a型肉毒毒素的疫苗或抗體研究奠定了一定的基礎。
  16. Human bone morphogenetic protein 3 is a member of tgf - b superfamily. lt can induce the differentiation of cartilage and bone tissue in mesenchymal cell. and is important to bone self - repairment and bone development during embryo morphogenesis. in addition, some other biological activities of hbmp - 3 have also been found. such as inducing development of embryo and stimulating differentiation of neural and blood cells. therefore, there is a great prospect in the use of hbmp - 3. there is trace content of hbmp - 3 in human body. it has been expressed in the expression system of eukaryotes and prokaryotes respectively, but its application is restricted because of defects in the process and modification after translation in prokaryotic cells and higher costs and lower yields existed in eukaryotic expression system

    人骨形成蛋白3 ( hbmp - 3 )屬于tgf -超家族的一員,可以誘導間充質細胞分化為軟骨和骨,在胚胎時期骨骼發育和骨再生修復中起著重要的作用,而且對胚胎發育過程中中胚層的誘導和分化、造血組織的發育以及神經系統的發育和修復等都起著重要作用,因而hbmp - 3有廣闊的市場前景。它在人體內含量極微,盡管研究人員已經在原核細胞和真核細胞表達系統中分別進行了表達,但是由於原核表達系統缺乏翻譯后的加工修飾,真核表達系統存在成本高、產量低等特點,限制了其在臨床上的應用。
  17. After adding culture mediem of stably transfected jurkat cells to hepatocarcinoma cells, the binding specificity of the scfvs with hbsag was further confirmed by observation by fluorescence microscope, indirect immunofluorescence and flow cytometer analysis. prokaryotic expression plasmids ptat - ha - scfvs were successfully constructed

    建系細胞培養上清與肝癌細胞作用后,經熒光顯微鏡觀察、間接免疫熒光及流式細胞儀檢測進一步確定表達的scfv融合蛋白具有與hbsag特異性結合的活性。
  18. One was cloning, sequence analysis and expression of the fragment containing the b and c antigenic sites locating at the 5 " terminus in spike gene of tgev in prokaryotic expression system ( fused with gst ), the other was preparation of non - radioactive probe labeled by digoxigenin for detecting the rna extracted from tgev by assay of dot - blot

    為了鑒別診斷tgev與prcv及對tgev進行流行病學調查,本研究採用原核表達系統( gst融合表達系統)表達tgev纖突蛋白( s蛋白)中含有b和c抗原位點的多肽,並且制備了非放射性地高辛標記的核酸探針,通過斑點雜交( dot - blot )檢測tgev核酸rna 。
  19. As fomentation of temperature - sensitive protein, ftsz is a normal protein in prokaryotic

    Ftsz蛋白是一類普遍存在於原核生物中的溫度敏感型骨架蛋白。
  20. Expression and identification of truncated 56kda protein of orientia tsutsugamushi gilliam strain in prokaryotic cells

    蛋白部分基因的原核表達及初步鑒定
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