核清蛋白 的英文怎麼說

中文拼音 [qīngdànbái]
核清蛋白 英文
nucleoalbumin
  • : 核構詞成分。
  • : Ⅰ形容詞1 (純凈) unmixed; clear 2 (寂靜) quiet 3 (清楚) distinct; clarified 4 (一點不留) w...
  • : 名詞1. (鳥類或龜、蛇類所產的卵) egg 2. (像蛋形的東西) an egg-shaped thing 3. (辱罵之詞)
  • : Ⅰ形容詞1 (似雪的顏色) white 2 (清楚; 明白; 弄明白) clear 3 (空的; 沒加他物的) pure; clear; ...
  • 蛋白 : 1. (卵中透明的膠狀物質) egg white; albumen; gary2. [生物化學] (蛋白質) protein
  1. 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左右的片段含有完整的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,並能被口蹄疫病毒陽性血識別。經薄層掃描分析,表達量占總量的26以上。
  2. " now we want to understand how the nucleoprotein regulates viral rna replication

    陶一之說: 「我們打算進一步搞調節病毒rna復制的機制。
  3. This modification includes : ( 1 ) selecting two important molecules as candidates, ( 2 ) choosing a promiscuous t - cell epitope, and two b - cell epitopes or conserved amino acid sequences from the two important molecules, ( 3 ) connecting them adequately through analysis by the molecule designing software. therefore, the synthetic new antigen may interfere with the process of fertilization by multiple ways and its contraceptive effects may be enhancing. based on the molecule designing methods, the b - lymphocyte cell epitope of sperm / testis specific protein sp17 and cyritestin which interfere with fertilization in mouse, as well as the promiscuous th cell epitope of the ribonuclease ( rnase ) in bovine were selected

    本研究以質分子設計的理論和方法研究避孕疫苗,將sp17和cyritestin關鍵表位和牛酸酶非選擇性th細胞表位合理組合,獲得新抗原- 35肽序列;並在合成、純化後分別與弗氏佐劑、免疫刺激復合物( iscoms )混合后免疫不同遺傳背景的雌性小鼠,觀察血和生殖道內的特異性抗體滴度的動態變化、生育力的改變以及免疫后小鼠重要臟器的組織病理學改變:以及在ivf下,新抗原的特異性抗血對精卵相互作用的影響及抗原在精子表面的特異性定位。
  4. Later work clearly showed that a ribosome contains many different proteins.

    近的工作楚地表明了體包括許多不同的質。
  5. The sucking mouse brain were inoculated with mdj - 01 strain to make electron microscopic examination, results showed that the virus was a spheral particle with membran which had a diameter of about 40 nm. by indirect fluorescent antibody test mdj - 01 strain was identified with tbev. a part of region encoding e protein was expanded by rt - pcr and sequenced. the nucleotide sequences of two strain viruses were compared with sequences in genbankjsequence homology analyses revealed mdj - 01 strain and senzhang strain had the highest homology with tbev oshima5 - 10, respectively, which were 95 %, 94 %. mdj - 01 strain was identified with tbev again

    應用間接免疫熒光試驗進行血學鑒定,結果表明mdj - 01株為tbev 。通過rt - pcr技術擴增部分e序列並測序,在genbank上進行同源性比較,發現mdj - 01株和森張株與tbevoshima5 - 10株的同源性最高,分別為94 、 95 ,從分子生物學水平上進一步證明mdj - 01株病毒為tbev 。在鑒定的基礎上,本實驗對兩株病毒進行了苷酸全序列測定。
  6. After the recombinant plasmid pcdna3. 1 / ts87 was identified by digestion of hindlll and bamh i, it transformed into cos7 by lipofectamine. expression product was identified by immunohistochemical method, sds - page and western - blot. the immunocytochemistry result has shown that specific brown - staining grains were found in the cytoplasm of cells transformed by recombinant plasmid versus not seen in cells transformed by pcdna3. 1 or normal cells ; the sds - page result has revealed that a band about 3 8kb was found in cell lysis transformed by recombinant plasmid versus not in cells transformed by pcdnas. l or normal cells ; the western - blot result has showed that only the band about 38kd was recognized by sera from rabbit infected by t. s artificially and sera from rabbit immunized with soluble antigen of t. s and with protein expressed by ts87 gene and by a monoclonal antibody of t. s

    通過細胞的免疫組化,細胞裂解物的sds - page電泳, westem - blot分析檢測目的基因的表達情況。免疫組化結果顯示:重組質粒轉染的細胞質中有棕褐色顆粒,而空載體轉染細胞及正常細胞無此現象;細胞裂解物sds - page電泳結果顯示:只有重組質粒轉染的細胞在約38kd處有明顯的帶,這與理論計算的ts87基因表達的分子量為38kd基本一致; western - blot分析結果顯示:約38kd的帶能夠分別被旋毛蟲感染兔血,成蟲蟲體可溶性抗原免疫兔血, ts87基因原表達免疫兔血( ts87血)以及一株具保護性的旋毛蟲單抗特異識別。
  7. The effects of glp - 1 ( 7 - 36 ) nh2 on insulin secretion glp - 1 ( 7 - 36 ) nh2 with the concentration of 2. 5nmol / l, 5. 0nmol / l, l0. 0nmol / l, 20. 0nmol / l, 40. 0nmol / l respectively were added to the medium as different experimental groups, 24 hours later, insulin amount are 68. 76 ? 1. 71 72. 30 ? 3. 13 104. 16 ? 5. 57 110. 98 ?. 29 111. 58 ? 0. 65miu / l respectively, and the insulin account is 55. 53 ?. 63miu / lin the control group. there was no significant difference between the groups with 2. 5nmol / land 5. 0nmol / l glp - 1 ( 7 - 36 ) nh2 respectively ; and there was not significant difference among the groups with lo. onmol / l, 20. 0nmol / l and 40. 0nmol / l glp - 1 ( 7 - 36 ) nh2 respectively. but the difference is significant between experimental groups and control group ( p < 0. 05 ). the data show that with the rising concentration of glp - 1 ( 7 - 36 ) nh2, there is an increasing amount of insulin

    對照組培養液中不含g廿一1 ( 7一36 ) nhz ,實驗組培養液中含有20nmol / lglp一1 ( 7一36 ) nhz ,培養24h后,用0 . 25 %胰酶消化胰島分散細胞,塗片后利用針對胰島素mrna的寡甘酸探針進行細胞原位雜交, dab顯色,高晰度病理圖文分析系統( highpathologiealimageanalysissystem , hp認s )對細胞著色的平均光密度( mean即tiealdensity , mod )量化分析,觀察實驗組和對照組胰島素mrna的表達情況。
  8. By using western - blot, the fusion protein could not be react with antiserum to prrsv, whereas it presented a reactivity with swine antisera against prrsv and mab ge3 by elisa the results implied that the epitope might be one conformational epitope that was mainly composed of aa50 ~ aa55 domain on n protein

    Western - blot分析表明表達產物與prrsv陽性血沒有反應性,而elisa分析表明表達產物可與prrsv陽性血和單克隆抗體發生反應。由此說明單克隆抗體ge3所識別的抗原表位可能是存在於n上以kphf為心的構象型表位。
  9. 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基因的原表達: 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基因的主要抗原區,將其克隆到原大腸桿菌表達載體pproex htb中誘導表達,經sds page檢測表明,重組質粒能表達ez基因主要區, westernblot檢測表明,誘導表達與豬瘟陽性血發生特異性反應,表達量為35和38 ,可用於基因工程診斷抗原。
  10. Change of immunosuppressive acidic protein in sera of patients with pulmonary tuberculosis and its clinical significance

    肺結患者血中免疫抑制酸性變化及其臨床意義
  11. The main differences in sod exist in two stages - 6 - from darkly - pigmented eye to hatching, which showed two more bands ( sodl " and sod2 " ) in the isozyme pattern of embryo activated by heterogeneous sperm than that activated by homogenous sperm. meanwhile, the other two isozymes ( est and me ) detected in this paper did not show apparent differences between the embryo activated by homogenous sperm and that activated by heterogeneous sperm

    對異精激發彭澤鯽雌發育子代及其母本彭澤鯽和父本海鯉的血、肌肉以及心、肝、腎、腦、眼等組織的酯酶( est ) 、蘋果酸脫氫酶( mdh ) 、蘋果酸酶( me ) 、超氧化物歧化酶( sod )和乳酸脫氫酶( ldh )電泳圖譜的比較研究。
  12. With serum arylesterase as the topics of teaching, small biomolecules, enzyme and protein, nucleic acids and genes as well as the techniques for their researches were covered

    以血芳香酯酶為研究對象可覆蓋小分子、酶和大分子、酸和基因等對象和相應研究技術。
  13. 24, 48, 72 hours later after transfection, we testified the expression of pp38 with mab h19, and pp24 with the antiserurn of pp24 expressed in e. coli. the tests justified the expression of pp24 in prokaryotic and eukaryotic expressing systems. in order to study the correlation of pp38 and pp24, we cloned pp38 gene and pp24 gene into pbudce4

    為研究pp38和pp24之間的關系,將型mdvmd11株的pp38基因和pp24基因的完整orf克隆到真雙表達載體pbudce4 . 1中,轉染cef后,通過ifa檢測和用抗pp24多克隆血進行western - blotting試驗檢測到了pp38和pp24磷的共表達。
  14. The high titer specific ndrg2 antibody is indispensable to reseach deeply the functions or the tissue and subcellular distribution features of ndrg2, ha order to prepare ndrg2 antibody, the whole ndrgl sequence was cloned into prset - a vector and two truncated sequences of ndrg2 were cloned into pgex - 4t - l vector. after induced by iptg, the fusion proteins were expressed in e. coli ; rabbits immunized with the whole length ndrg2 protein were reinforced with two shortened fragments of ndrg2 ; after immunization, rabbits produced high titer antiserum against ndrg2. then antisemm was absorbed using ndrg2 antigen immobilized on nc filters, the purified product of antiserum shows high special to ndrg2 protein, and the separated inclusion body of 6his - ndrg2 will be useful for the further reseach

    為制備高效價的ndrgz抗體,分別構建了prset a雌、 pgex4t d唾倉和pgex4tl七三種原重組表達質粒,並在大腸桿菌中誘導表達出相應的融合;用全長gstjqdrgz免疫兔,然後用gst ndrgz人和gstjqdrgze片段加強免疫,經免疫得到了較高效價的兔抗人ndrz多克隆抗血,利用固定於硝酸纖維素膜上的ndrgz抗原親和吸附純化抗血,提高了ndrgz抗體的特異性;並對包涵體形式表達的6his ndrgz進行初步的分離純化。
  15. The cdna expression library that contains no intron theoretically include all expressed genes and conserve resource genes permanently. lt can be used to find out and clone some genes which can express particular protein with modern molecular biological techniques, such as immunological screening, drug - prob screening, southern et al. lt is very important to study the life nature of plasmodium falciparum in molecular level. with the developments of these studies, the drug - resistant mechanism of the plasmodium falciparum and the genes of some specific medicine binding protein can be made well - known. at the same time, the researches will do good to explain the mechanism of some specific medicines in order to design and screen new anti - malaria drugs

    建立cdna表達文庫在一次永久保存基因資源的同時,可以利用功能篩選、免疫學篩選、藥物探針篩選、 southern雜交和大規模序列測定等現代分子生物學技術尋找特異性活性基因,進而克隆和表達這些基因,對從酸及質等分子水平研究瘧原蟲的生命活動規律,對揭示其抗藥性分子機理,搞某些特效藥物結合的基因及此類藥物的作用機制,對新型抗瘧藥物的合理設計及篩選都具有極其重要的現實意義。
  16. The activity of the antiserum was tested by dot enzyme immunization assay ( diba ) with purified antigen. western blot of hela nuclear protein extract, which contained natural hbaf53, showed that the antiserum is also a specific antiserum to natural hbaf53. therefore the highly specific and sensitive antiserum can be applied to various studies

    用純化的抗原,經斑點印跡試驗測得baf53抗血的效價,又用提取的hela細胞(含有天然baf53)進行免疫印跡分析( westernblotting ) ,證明天然baf53也是該抗血的抗原,說明獲得的多抗血具有高特異性和敏感性,可用於多方面的研究。
  17. Through three rounds of screening, seventeen clones were selected and used in competitive test. the mab ge3 could specifically inhibit eight out of seventeen clones from binding to swine antisera. based on the amin acid sequences deduced from the foreign sequence inserted in the phage, it was indicated that all clones shared the core sequence - p / ekphf, that was similar to aa50 ~ aa55 domain of n protein of prrsv

    從第三輪親和篩選的噬菌體中隨機挑取17個克隆進行功能鑒定,結果表明8個克隆與mabge3具有較強的特異性結合力並可以被prrsv陽性血阻斷,測序發現7個克隆具有心序列: p ekphf ,該序列與prrsvnaa50 aa55 ( p ekphf )具有較高的同源性。
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