antibody fusion protein 中文意思是什麼

antibody fusion protein 解釋
抗體融合蛋白(質)
  • antibody : n. 【醫學】抗體。
  • fusion : n. 1. 熔解,熔化;【物理學】(核)聚變,合成。2. 〈美國〉融合;(政黨等的)合併,聯合。
  • protein : n. 【化學】朊,蛋白(質)。
  1. In order to get further evidence of the localization and distribution of emt - 1 in cells, we have prepared emt - 1 his6 - fusion protein and intend to abtain emt - 1 antibody for immuno - histochemistry assay

    為了進一步證實emt l在細胞內的定位及組織分佈,擬制備抗emt l抗體,進行免疫組化驗證。
  2. Purified fusion protein gst - hnadc3 was used as an immunogen to inoculate rabbits and the antibody against the gst - hnadc3 fusion protein was raised, and was purified by gst sepharose 4b affinity chromatography to remove the antibody against gst

    Ptg誘導表達,超聲破碎細胞后,採用親和層析方法純化融合蛋白gst十nadc3 ,並以此為抗原免疫紐西蘭株白兔制備融合蛋白抗體。應用親和層析的方法對gst十nadc3融合蛋白抗體進行純化,以去除抗gst抗體。
  3. Ability to a - complement of the ea / ed protein was determined by the addition of onpg western blot test with rabbit to e. coli p - galactosidase pcab as first antibody was used to verify the fusion proteins

    以兔抗p半乳糖昔酶抗體做western blot以證實與gst融合表達的ea工d蛋白是p半乳糖昔酶的成分。實驗結果1
  4. Get the inclusion bodies 2 ) western blot analysis of fusion protein expression ( 1 ) electrophoresis ( 2 ) transfer proteins from gel to membrane ( 3 ) blocking ( 4 ) incubation with primary antibody ( 5 ) enzyme conjugate incubation ( 6 ) substrate incubation. 3 ) gst detection module with cdnb enzymatic assay 3 purification of gst fusion proteins 1 the denaturalization of inclusion bodies. 2 purification using glutathione sepharose 4b column wash matrix with 1 pbs, prepare a 50 % slurry for batch purification method, pack column with matrix slurry

    三、 gst一hbrp重組蛋白的純化1 .超聲破碎細胞,離心,上清和沉澱進行sds一page電泳分析2 .樣品處理提取包涵體,變性后,加人用pbs平衡過的以utal腸onesepb抓脫4b ,室溫下孵育3 .以utadtionesepharose4b柱純化以utad雲onesepharose4b柱的準備根據毛山lel ,決定純化所需的gll衛ta1如oneseph娜se4b的柱床體積,用預冷的1xpbs清洗cldtathionese戶, se4b ,得到50 %的基質
  5. Ptxb1 - hng and ptxb1 - m - insulin are expressed in e. coli successfully. after sds - page and densitometric scan analysis, the results show that the expression level of hng fusion protein is above 40 % and m - insulin fusion protein above 50 % of total bacterial proteins. western - blot result demonstrated m - insulin fusion protein had specific reaction with mouse anti human insulin antibody ( igg )

    Pbv220 ? hng在大腸桿菌中未檢測到表達,后兩個克隆在大腸桿菌bl21 ( de3 )中獲得高效表達, hng及m - insulin融合蛋白表達量分別佔全菌蛋白的40及50左右;經western - blot鑒定m - insulin融合蛋白可以與小鼠抗人胰島素單克隆抗體( igg )發生抗原抗體結合反應。
  6. After sds - page and densitometric scan analysis, the expression level of hng fusion protein is above 40 % and m - insulin fusion protein above 50 %. western - blot result demonstrated m - insulin fusion protein had specific reaction with mouse anti human insulin antibody, we got hng fusion protein and m - insulin fusion protein with purity of above 80 %

    今士考個二目卜乙成功構建了ptxbi一hng及ptxbi一m一insulin原核表達克隆,並獲得了高效表達,經過純化得到純度人於80 %的融合蛋白,並對人胰島素突變體融合蛋白進行了初步活性測定。
  7. By immune the animal with the protein, the antibody which is anti - gst - cpti fusion protein was prepared. lt was testified that the antibody can special immunological recognition the protein gst - cpti, gstand cpti by indirect elisa. the coefficient of correlation is significant and the potency is more than 1 : 8000

    對其進行細菌表達后,利用glutathionesepharose4b親和柱純化獲得gst - cpti融合蛋白,免疫動物后制備了相應的抗gst - cpti融合蛋白抗體。
  8. Second, a prokaryotic expression construct, obtained from invitrogen transformed into prokaryotic and induced to express vp1 protein. the expressed vp1 fusion protein was purified by affinity chromatography using glutathione - agarose resin and used in elisa and western bolt analysis as the antigen. the elisa and western blot results showed that the anti - fmdv antibody was elicited specifically against vp1 antigen

    第二,為了得到抗原蛋白,將vp1的原核表達質粒pgex - 4t - vp1轉化入大腸桿菌bl21中,經iptg誘導,裂解細胞後用瓊脂糖珠進行純化,用elisa和westernblot進行檢測,結果表明誘導表達出所需大小的融合蛋白。
  9. After the lysate was purified with gst sepharose 4b affinity chromatography, a specific band of 34kd appeared in sds - page gel, the purity and the titer of the antibody against fusion protein gst - hnadc3 could reach up to 90 % and 1 : 32, respectively

    菌體裂解液經gst親和層析純化后, sds page上出現一分子量為34kd的特異蛋白條帶,純度可達90 。
  10. 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七三種原核重組表達質粒,並在大腸桿菌中誘導表達出相應的融合蛋白;用全長gstjqdrgz蛋白免疫兔,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多克隆抗血清,利用固定於硝酸纖維素膜上的ndrgz抗原親和吸附純化抗血清,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。
  11. Hisityl - trna synthetase catalyzes the aminoacylation of trnahis in the initial step of protein biosynthesis. the involumen of histidyl - trna synthetase in autoimmune diseases is another feature of the enzyme. in studies, it is reported that purified jo - 1 antigen can increase the detection rate of anti - jo - 1 antibody. but it is difficult to obtain a single component by biochemical extraction. genetic engineering can help us to desolve this problem. after looking up mrna sequence encoding histidyl - trna synthetase in genebank, we used rt - pcr technology to gain its full length dna sequence. the vestor ptybllwas used in the construction of expressing vestor. we transformed the jo - 1 gene into er2566 and used this system to express fusion jo - 1 antigen

    本實驗從人胎盤中提取總rna ,利用rt - pcr技術獲得了編碼jo - 1的基因整長序列,選用impact - cn系統中的ptyb11載體,構建了jo - 1基因的克隆與表達載體,並轉化大腸桿菌er2566 ,經過抗性篩選、分子量大小比較、雙酶切鑒定、和pcr鑒定等多種方法驗證,篩選出了5個陽性克隆。
  12. The recombinant pcr technic was used to introduce a linking peptide klgggg to the site between scfv single chain form of the monoclonal antibody sz - 51 specific for the glycoprotein gmp140 on activated platelet membrane and uk32 low molecular weight form of pro - urokinase, to make the scfv - linker - uk32 chimeric gene. this gene was cloned into the transfer vector pbacpak9, and cotransfected with bacpak6 bsu36i digest into sf 9 cells. the fusion protein was secreted into the medium. in the fifth day after the cotransfection, the supernatant of the medium showed 107 iu ml fibrinolytic activity, higher than 25 iu ml fibrinolytic activity of scfv - uk32. elisa showed that the supernatant had the binding activity to activated platelet. wastern blotting also indicated that the supernatant could bind to the monoclonal antibody of urokinase b chain

    為了提高重組導向溶栓分子scfv - uk32的溶纖活性,通過重組pcr方法在編碼scfv與uk32的堿基之間引入編碼klgggg連接肽的堿基序列,並克隆到轉移載體pbacpak9上,通過與線性病毒dna bacpak6 bsu36i digest共轉染到昆蟲細胞sf 9內,進行表達。表達產物分泌到上清中,共轉染后第5d天用纖維平板法測得sf 9細胞上清溶纖活性達到107 iu ml ,比未引入連接肽的scfv - uk32的表達活性25 iu ml高。
  13. Using the monoclonal antibody to rev and the anti - sera against the rev env gp90 - gst fusion protein. the molecular cloned virus was detected by ifa. we also amplified the gp90 from the cells infected with the molecular cloned virus by polymerase chain reaction. all these results indicated the recombinant plasmid containing the total rev genome cdna is infectious

    對snv株前病毒全基因組cdna克隆進行酶切,將酶切產物分別克隆進puc18中,分別將各個亞克隆進行測序,按照酶切位點和已知的部分序列以及rev物理圖譜將測得的序列進行拼接,完成了rev全基因組序列。
  14. The fusion ( f ) protein and hemagglutinin - neuraminidase ( hn ) are the major virulence factors of the virus to which the host responds well with protective antibody production. recombinant plasmids containing the f or hn gene can induce specific immune responses against ndv. however, dna vaccination by injection or gene gun routes is rather inconvenient and costly in field applications in scaled animal farms

    融合蛋白( f )和血凝素-神經氨酸酶蛋白( hn )是ndv的主要宿主保護性抗原,以f基因和hn基因為免疫原研製的dna疫苗能誘導一定程度的免疫應答,但注射免疫或基因槍免疫途徑因實際操作和成本等問題難以推廣應用,而直介面服重組質粒dna免疫效果不理想。
  15. Constructed the fusion protein expression vector of echistatin, . and identify it by dna sequencing. the vector can express echistatin fusion protein at a high level, the fusion protein molecular weight is about 16000 da in sds - page analysis, and the fusion protein consists more than 30 % of total protein, the fusion protein has specific antigen - antibody reaction with rabbit anti - echistatin polyclonal antibody. the fusion protein include : hpk5. his + 6tag, and echistatin. echistatin can be released by cnbr cleavage

    構建了echistatin融合蛋白表達載體,經dna測序鑒定正確后,溫控誘導表達,獲得了高效表達,表達產物經505一隊ge分析,分子量為16000oa ,符合預計的融合蛋白分子量,表達產物. ll 』菌體總蛋白的30 %以上, westem一blotting結果顯示,該日的蛋白能夠和echistatin多克隆抗體發生特異性抗原抗體反應,表明我們成功構建了eohistatin的高效融合表達克隆。
  16. Expression of gst - snail fusion protein in prokaryotic cells and preparation of polyclonal antibody against snail

    融合蛋白的原核表達及其多克隆抗體制備
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