htb 中文意思是什麼
htb
解釋
華天牌-
Vp3 gene of hl isolate of goose parvovirus derived from recombinant piasmid pproex htb - vp3 was subcloned into ecorl site of psy538, and the reporter gene lacz with promoter pll was cloned into smai site of recombinant piasmid. both vp3 gene and lacz gene were cloned into noti site of psy681, recombinan fpv transfer vector containing vp3 gene of gpv was obtained. the result is basis of construction of recombinant fpv expressing vp3 gene of gpv and gpv genetic engineering vaccine
本研究另從含有gpvh1分離株主要結構蛋白vp3基因的重組質粒pproexhtb - vp3中切取gpvh1株vp3基因片段,將其亞克隆于psy538的ecori位點,然後將帶有痘苗病毒啟動子p11的lacz報告基因平端克隆于上述重組子的smai位點,再用noti切下同時含有vp3基因和lacz報告基因的片段,再亞克隆于psy681的noti位點,構建出含有vp3基因的重組禽痘病毒轉移載體,為構建表達vp3基因的重組禽痘病毒從而制備gpv基因工程疫苗奠定了基礎。 -
By recombinant dna techniques, the vp2 gene of gpv hi strain was fused in frame with 6his gene of prokaryotic expression vector pproex - htb. the recombinant expression plasmid of goose parvovirus vp2 gene pproex - htb - vp2 was transformed into e. coli dh5a and induced with iptg. sds - page analysis showed an induced expression product band about 72ku, which correspond to the sizes of vp2, reported in the literature
利用dna重組技術,將其結構蛋白vp2基因亞克隆至原核表達載體pproex - htb , iptg誘導后成功表達出與預期大小相符的約72ku的融合蛋白,光密度掃描對表達產物進行初步定量,表明表達產物約占菌體總蛋白的14 。 -
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基因的主要抗原區,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,重組質粒能表達ez基因主要區蛋白, westernblot檢測表明,誘導表達蛋白與豬瘟陽性血清發生特異性反應,表達量為35和38 ,可用於基因工程診斷抗原。 -
The gene was subcloned into the pproextm htb vector, then was transformed the vector into e. coli dh5. a biologically active recombinant pil - 10 was obtained after induction by iptg
然後將pil - 10編碼基因亞克隆到表達載體pproextmhtb中,轉化dh5后,用iptg誘導培養,表達了具有活性的重組pil - 10 。
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