陽性基質 的英文怎麼說

中文拼音 [yángxìngzhí]
陽性基質 英文
animus
  • : Ⅰ名詞1 (太陽; 日光) the sun 2 (山的南面; 水的北面) south of a hill or north of a river 3 (中...
  • : Ⅰ名詞1 (性格) nature; character; disposition 2 (性能; 性質) property; quality 3 (性別) sex ...
  • : Ⅰ名詞1 (性質; 本質) nature; character; essence 2 (質量) quality 3 (物質) matter; substance;...
  • 陽性 : 1. [醫學] positive 2. [語言學] (與陰性相對的) masculine gender
  1. In this study, iltv - nm98a strain and iltv - wanggang strain were multiplied in chorioallantois. a pair of primers were devised according to the nucleic acid sequence of iltv tk gene and the dna of multiplied virus was used as pattern to amplify the gene of tk by polymerase chain reaction ( pcr ). the product of pcr was linked with suitable plasmid. then, the recombined plasmid was converted to escherichia coli. the converted escherichia coli

    根據已發表的iltvtk因的核苷酸序列設計一對pcr引物,以增殖的兩株iltv的dna為模板,分別對它們的tk因進行pcr擴增。將回收的pcr產物連接到適當的粒載體上,轉化感受態大腸桿菌,通過篩選對iltvtk因的克隆進行擴增培養。
  2. 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

    擴增產物連接到pgem - teasy載體中,轉化大腸桿菌dh5菌株,篩選氨芐青霉素抗菌落,提取粒經酶切鑒定、 pcr分析以及確證測序證明,所克隆的1500bp左右的片段含有完整的3abc因,與國外參考序列相比,同源在99以上。將重組粒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載體上的片段於3abc因708bp處出現了17bp的缺失,碰巧在3ab因后形成一終止密碼子,但3ab因的閱讀框架完整,選出含有3ab因完整閱讀框架的克隆,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,並能被口蹄疫病毒血清識別。經薄層掃描分析,表達量占總蛋白量的26以上。
  3. Based on the residue monitoring results in the previous year, especially on the feedback information of the positive ( non - compliance ) results, and taking account of world - wide alert notifications, samples of some items to be taken will be duly increased year by year ; based on the reasonable suggestions in fvo inspection report and the problems of chloramphenicol and nitrofuran which had been notified by eu in recent years, the monitoring items are being added in order to meet the residue requirement of importing countries and regions such as the eu, japan, korea, switzerland and hk

    國家檢總局根據上一年度殘留監控結果反饋情況,特別是結果的檢出情況,結合各國預警通報的情況,每年適當增加對應監控的檢測項目的取樣數量;尤其是針對歐盟每次考察報告中對我殘留監控計劃提出的合理化建議和近年來歐盟通報的氯黴素和硝呋喃問題,增加了滿足歐盟、日本、韓國、瑞士、香港等國家和地區殘留監控要求的項目。
  4. The result showed that the homology rate of pila gene among the 5 avian pathogenic e. coli strains tested and one human e. coli were from 89. 8 % to 91. 1 %, and the homology rate of amino acid were from 88. 5 % to 91. 8 %. the homology rate of pila gene sequence among 5 avian pathogenic e. coli strains tested and avian pathogenic e. coli reported ( serotype o1, o2, o78 ) were from 87. 8 % to 90. 2 %, and the homology rate of amino acid were from 84. 6 % to 91. 2 %. there had homology in avian pathogenic e. coli. there had some common antigen side in type 1 pili of avian pathogenic e. coli

    結果表明:運用msha法檢測1型菌毛的檢出率為80 ( 36 45 ) , pcr法的檢出率為95 . 5 ( 43 45 ) , pcr方法用於1型菌毛的檢測比msha更加敏感、快速、特異強;選擇5株優勢血清型雞源致病大腸桿菌代表株( o _ ( 89 ) , o _ ( 119 ) , o _ ( 141 ) , o _ ( 127 ) )的1型菌毛pila因的pcr擴增片段經純化后,分別定向克隆到puc18粒的多克隆位點,構建了含有目的因片段的克隆粒,並轉化到dh5株大腸桿菌載體菌中,篩選獲得克隆菌株。
  5. In this paper, a field strain of infectious bronchitis virus was isolated from proventriculus tissue, morphological observation by electron - microscope and the biological characterizations of the virus were studied, pairs of specific primers are designed and synthesized in correspondence with them, according to the published sequences of infectious bronchitis virus three structural protein ( spike protein s membrane protein m nucleocapsid protein n ) genes, the cdna of si gene, s2 gene, m gene. n gene of ib v isolate lx4 were amplified by rt - pcr and full sequences were first reported

    在此礎上,根據國內外已發表的ibv因序列,分別設計特異引物,應用不同引物進行反轉錄合成cdna ,分片段對ibv的主要結構因進行pcr擴增,並分別將各個目的片段克隆到puc19載體上,在大腸桿菌dh5中實現目的因的分子克隆,經藍白斑篩選、限制內切酶分析、 pcr鑒定,篩選出重組粒,並對各個目的因片段進行序列測定,從而獲得ibv主要結構因全序列。
  6. Fos + / th + / gfap + and fos + / vp + / gfap + triple labeled n - asc could be found in the mvz, pvn and son respectively ; ( 2 ) under electronic microscope, the astrocytic processes connected closely with the dendrites or axons of the neurons, where the bilateral membranes became thick. we call transiently it electron - dense areas ( edas ). the number of edas increased remarkably following hyperosmotic stimulation ; ( 3 ) when trace retrogradely, wga - hrp was microinjected into the unilateral son, pvn or nucleus of solitary tract ( nts ) respectively using the stereotaxic method, the n - ascs formed by the neurons triple - labeled with hrp / fos / th ( or vp ) and astrocytes labeled with gfap could be found in the mvz, son and pvn respectively ; ( 4 ) after being treated with heperosmotic nacl solution, intracellular calcium concentration in cultured hypothamic neurons and astrocytes increased and then decreased

    腦內gfap結構也明顯增多,其分佈與fos細胞分佈本一致,表現為胞體肥大、突起粗長; ast緊密包繞在神經元周圍形成神經元- ast復合體( n - asc ) ;在mvz 、 pvn和son三重免疫組化染色切片上可見到fos + th + gfap +第四軍醫大學博士學位論文和fos vp gfap三重標記asc ; ( 2 )免疫電鏡下son內星型膠細胞突起與神經元樹突或軸突之間接觸部位出現增厚的膜結構一電于緻密區( edas ) ,高滲刺激后數量明顯增多: ( 3 )將們個mp注入大鼠一側n卜、卜卜或孤束核( ws ) ,分別在延髓內臟帶( mvz ) 、 so和pvn內出現fos hrp th 、 fos hrp八p三重標記神經元和gfap標記ast形成的n asc ; ( 4 )高滲刺激使培養神經元和ast內鈣水平先升高后降低,最後維持在比高滲刺激前稍高的靜息鈣水平上。
  7. The positive colonies that grew on the ampicillin ( amp ) plate ( lb agar medium contaning 100 g / ml amp ) were screened and identified. sds - page and western blot analysis were performed to study the expression profiles of target gene cein in e. coli

    從轉化的平板中篩選出重組子,進行不同iptg濃度和不同誘導時間的表達研究,並利用sds - page電泳和westernblotting蛋白印跡技術對外源因cei _ ( 12 )在大腸桿菌e
  8. Microbiology of food and animal feeding stuffs. horizontal method for the enumeration of coagulase - positive staphylococci staphylococcus aureus and other species. part 2 : technique using rabbit plasma fibrinogen agar

    食品和動物飼料微生物學.凝膠水平計數方法.葡萄球菌和其它屬.第2部分:兔原生血纖蛋白瓊脂培養技術
  9. The cloning cdna fragment was extracted from positive clones and sequenced. the results showed that the cdna fragment was 816bp in size, encoding a protein which included 272 amino acids. the sequence homology analysis was carried out via the software blast 2. 0 network service in the four large databases - genbank, embl, ddbj, pdb, which had recorded 1 337 978 nucleotide and protein sequences. the results of the analysis indicated that the nucleotide homologous rates between the rubber tree etr and 15 recorded etrl of other plants ( mango, passion fruit, persia plum, strawberry, grape. . etc ) were 75 % - 80 % ; the protein homologous rates between the rubber tree etrl and these recorded etrl genes were 90 % - 95 %. from the results mentioned above, we could confirm that the cdna of rubber tree etrl had been cloned

    克隆子中提取克隆片段,經序列測定分析,結果表明,克隆片段的cdna大小為816bp ,編碼的蛋白包含272個氨酸。因序列通過blast2 . 0networkservice軟體對genbank , embl , ddbj , pdb四個大型數據庫中記錄的1337978條核酸和蛋白序列進行序列相似檢索,結果表明與芒果、一西番蓮、波斯梅、草毒、葡萄、西洋梨等15種已報道的植物的etrl因cdnag的同源率為75 88 ;蛋白酸序列的同源率為90 95 ,表明本研究確實克隆到了橡膠樹etri因的cdna序列。 4
  10. Different amount of copies in different tissues attribute to the different density of positive signals. the result of the experiment suggested that the transgenic animals can be produced by spermatozoa - mediated gene transfer after the entrapment of liposome. and because the exogenous dna occurs losing the segments. partly integration, or existin g outside of genome dna, the rate of chimerism is relatively high

    結果表明: ( 1 )脂體包裹外源因轉染精子的方法,可將外源因導入受精卵中,能夠獲得轉因動物,並得到了較高的轉率; ( 2 )精子攜帶的外源dna的整合過程是隨機的,在受精過程和胚胎早期分化過程中可能發生了片段丟失、不完全整合或游離于因組存在而產生嵌合體。
  11. The hwtx - i gene was chemically synthesized according to its known cdna sequence, the gene was inserted into vector ppic9k which contained aoxj promotor and the sequence of a secreting signal peptide - a - factor, the cloning ppic9k / hwtx - i was constructed and confirmed by two - step pcr and dna sequence analysis, then it was transformed into host strain gs115, a his + muts cell line was screened and multicopy transformants were screened by various g418 concentrations, the multicopy transformant was named gh1. gh1 was cultivated in flasks. after 6 days of induction by 0. 5 % methanol, the supernatant was checked by 16. 5 % tricine - sds page, which showed there was a band in the position of 3. 5 - 6. 1kd, then it was isolated and desalted by ultrofiltration followed by ion exchange of cm column, after reverse phase hplc of ci8 and vacuum drying, the purified rhwtx - 1 was obtained which was proved to be correct recombinant hwtx - i by tricine sds - page, maldi - tof mass spectrometry, amino acid composition analysis, the n - terminal amino acid sequence and its biological activity, the final field of the purified rhwtx - i was about 80mg / l, accounting for 23. 6 % of it total secretory proteins

    將帶有hwtx -因的ppic9k經blgii線化后,轉化酵母宿主菌gs115原生體后經篩選克隆並經表型鑒定為his ~ + mut ~ s酵母菌,進一步用遺傳毒素g418篩選多拷貝的轉化菌株,命名為gh1 ;將gh1甲醇酵母菌用0 . 5的甲醇誘導表達,發酵上清經90飽和度的( nh _ 4 ) _ 2so _ 4沉澱, yw - 3 ( mwc03000 )的超濾膜超濾,再經cm離子交換, c _ ( 18 )反相hplc純化得到分子量為4kd左右的組分,其中4289 . 05的組分經譜鑒定,氨酸組成分析和序列測定為正確的表達產物,生物學活表明其活為天然毒素活70 % ,表達量為80mg / l 。
  12. When cotransforming pgbd - nifa and ad fusion genomic library into saccharomyces cerevisiae pj69 - 4a, 109 candidates interacting with nifa had been selected by testing for the expression of the his3, ade2 and lacz reporter genes

    誘餌粒和文庫粒共轉化釀酒酵母( saccharomycescerevisiae ) pj69 - 4a ,通過檢測報告因his3 、 ade2及lacz的表達進行篩選,初篩得到109個酵母菌落。
  13. Dna and rna dot blotting revealed that the f gene was transcribed into mrna in the vero cells. there was expression of the f protein as shown by indirect immunofluorescent assay. the expression began at 48h post - infection and increased thereafter, as indicated by elisa

    將真核表達粒pcdna3 - f高壓電轉化dam和phop因雙突變的減毒鼠傷寒沙門氏菌zj111株( zj111 / pcdan3 - f ) ,並直接轉染vero細胞,分別提取細胞總dna和總rna , dig標記探針均可檢測到雜交信號。
  14. Two strains of prrsv were isolated from the swine infected with prrsv in shangdong province and daqing area, in order to clarify the source and genetic background of porcine reproductive and respiratory syndrome virus ( prrsv ) from different parts of china, thus providing theoretic basis for the study of vaccine against it. the prrsv was cultured on mark - 145 cells for 5 ~ ~ 6 passages. when the cpe was obvious, the virus was harvested and purified

    為了弄清我國不同地區prrsv的來源以及其遺傳學背景,為疫苗學研究提供理論根據,本研究在ch - 1a株完整的因組獲得以後,從流行於我國山東( sd )和黑龍江大慶( dq )地區疑似prrs的豬體內分離到prrsv ,在mark - 145細胞上盲傳5 6代,細胞出現明顯病變以後,收獲病毒液,然後提純,提取全病毒rna ,經過反轉錄、 pcr擴增獲得結構因orf2 7的目的因片斷,然後與pmd - t載體連接,轉化,得到粒后進行測序,並將其與ch - 1a株進行了比較分析,同時對這兩個毒株的結構因組的理化進行分析。
  15. The interesting gene fragment with ecori and noti were amplified by overlapping pcr, which inserted into vector plasmid ppic9k after degisted by ecori and noti, and the recombinant plasmid was transformed into competent dh5cc. positive clones were screened by pcr from the lb plate with amp. digesting analysis resulte shows that the interesting gene were inserted into the vector ppic9k with correct direction

    目的因經雙酶切后連接載體ppic9k ,然後導入大腸桿菌dh5中,在含氨卞青霉素( amp )的lb板上用pcr反應篩選出菌落,雙酶切結果表明目的因已插入載體中,且方向正確,測序結果進一步證明人巨細胞病毒重組因表達粒成功地克隆了目的因片段。
  16. 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、標記因nptll 、抗除草劑因epsps 、 pat 、抗蟲因cry1ao )的粒作為轉因植物檢測的對照。
  17. Expression in vitro cos - 7 cells were transfected with pm, pms, pmi and pmsi constructs by cationic liposom, respectively. 48 hours later, mrna of targets gene were detected by rt - pcr and hil - 12 protein in culture supernatnant and cell lysates were detected by western blotting. p815 cells were transfected with pm and pms constructs and selected by g418

    2 .重組粒在真核細胞中的表達: ( 1 ) pm 、 pms轉染cos一7細胞, 48小時后,用ri 』 - pcr檢測目的因在mrna水平的表達;轉染p815細胞, g418篩選抗細胞克隆,用rt - pcr檢測目的因在mrna水平的表達,結果為,說明在轉錄水平有目的因的表達。
  18. The expression conditions of e2 gene in p. pastoris were optimized, the results indicated that the peak obtained after 72 hours ; pattern of inhibition / induction could improve expression level ; the best ph value were between 7. 5 and 8. 0 and the optimized methanol - induced concentration was 2 % - 3 % the e2 genes of the prevalent strain ( guangxi yulin strain ) and c strain derived from rabbit spleen tissue were amplified and cloned into e. coli the expression vector pproex - htb respectively, the recombinant plasmids pproex - gxyl and pproex - c were obtained and then were transformed into the dh5a e. coli competent bacteria respectively, the recombinant bacteria could express the major antigen region of e2 gene, the expression yields amount to 35 % and 38 % repectively

    豬瘟病毒ez因的原核表達: pcr擴增出當前豬瘟流行野毒株,中國豬瘟兔化弱毒( c株)兔脾組織毒ez因的主要抗原區,將其克隆到原核大腸桿菌表達載體pproex htb中誘導表達,經sds page檢測表明,重組粒能表達ez因主要區蛋白, westernblot檢測表明,誘導表達蛋白與豬瘟血清發生特異反應,表達量為35和38 ,可用於因工程診斷抗原。
  19. The research showed that their interactions in yeast two - hybrid system are still steady when the vector was exchanged, in contrast, the interaction was disappear when the reading frame of each positive had been changed. the four positives were subcloned into suicide plasmid so that gene mutant strains could be constructed via conjugation and homologous recombination

    為了進一步驗證這些克隆的編碼產物與nifa蛋白的相互作用,將它們與nifa因互換載體后共轉化酵母,仍然可以激活三個報告因的表達,而克隆移碼表達的重組粒和pgbd - nifa的共轉化物則不能在選擇平板上生長。
  20. Ir - ta - ti metal oxide coated titanium anodes of variable composition were prepared by thermal decomposition. their micro morphorogies and electrochemical properties were characterized by scanning electron microscope, open circuit potential, cyclic voltammetry, consumption rate measurements and accelerated life test. the sem results indicated that all coatings were of a porous and cracked - mud microstructure influenced greatly by the composition of coatings. the electrochemical measurements showed that the ir - ta - ti ternary oxide - coated anodes exhibited excellent electrochemical activity and electrochemical stability in both acidic media and seawater which were affected by the composition and microstructure of the coatings. owing to good corrosion resistance and low consumption rate in seawater, metal oxde coated anodes belong to insoluble material, and can be potentially applid in impressed current cathodic protection systems as an anode

    採用熱分解方法在鈦體上制備銥鉭鈦金屬氧化物極,用掃描電鏡對極塗層顯微形貌進行分析,通過強化電解壽命試驗、開路電位測試、消耗率試驗及循環伏安曲線研究了金屬氧化物極的電化學能. sem分析結果表明銥鉭鈦金屬氧化物極塗層呈現多孔多裂紋形貌結構.隨極塗層組成不同,塗層顯微形貌表現出很大差異,這種差異直接影響極電化學能.電化學能試驗結果表明銥鉭鈦金屬氧化物極在酸和海水中具有良好的電化學穩定和電化學活.此外,銥鉭鈦金屬氧化物極在海水中的消耗率很低,屬于不溶極材料,作為外加電流陰極保護用輔助極具有廣泛的應用前景
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