例句與造句

1. Expression of crylac in transgenic tobacco plants was assayed with elisa . the results showed that pinll signal peptide sequence enhanced the expression of crylac protein in transgenic tobacco
   熒光顯微觀察到gfp在植物細(xì)胞間隙高效表達(dá)， westernblot結(jié)果顯示crylac蛋白也在植物細(xì)胞間隙表達(dá)。
2. Gfp gene was also fused behind the signal peptide sequence to construct plasmid p3301ubisiggfp and transformed to tobacco . the results of fluorescent detection showed gfp localization in the apoplast
   Elisa結(jié)果顯示，馬鈴薯蛋白酶抑制劑基因的信號(hào)肽序列使crylac基因在轉(zhuǎn)基因煙草中的表達(dá)量顯著提高。
3. We generated a recombinant eukaryotic gene expressing vector harboring a full - length hgh gene , 2 . 4 kb genomic dna with four introns and the signal peptide sequence cloned to the eukaryotic gene expressing vector pcdna3 . 0
   我們直接將含有4個(gè)內(nèi)含子和自身信號(hào)肽的2 . 4kb全長(zhǎng)人生長(zhǎng)激素基因直接克隆至真核表達(dá)載體pcdna3 . 0 ，然后利用脂質(zhì)體轉(zhuǎn)染家蠶bmn細(xì)胞，瞬時(shí)表達(dá)hgh 。
4. To allow secretion of the crylac protein into the intercellular space , potato proteinase inhibitor ii ( pinll ) signal peptide sequence was n - terminally fused to the crylac coding region to construct plasmid p3301ubisigac
   運(yùn)用pcr技術(shù)克隆了馬鈴薯蛋白酶抑制劑基因的信號(hào)肽序列，并將其分別連到crylac 、 gfp基因的5 ’端，構(gòu)建植物轉(zhuǎn)化載體p3301ubisigac和p3301ubisiggfp 。
5. In order to explore transgenic plants for production of recombinant scfv specific for presl ( 20 - 47 ) , nicotiana tabacum was transformed with a gene encoding anti - presl of hepatitis b surface antigen scfv and bearing an / / - terminal endoplasmic reticulum protein signal peptide sequence
   在用煙草作為生物反應(yīng)器時(shí)，分別將該單鏈抗體靶向細(xì)胞質(zhì)和內(nèi)質(zhì)網(wǎng)。經(jīng)westernblot分析，靶向細(xì)胞質(zhì)中表達(dá)時(shí)，可溶單鏈抗體最高占總的可溶蛋白的0 . 06 。
6. It's difficult to find signal peptide sequence in a sentence. 用signal peptide sequence造句挺難的
7. ( 3 ) at post - translation level plant mutual sequence of starting translation aaca and eukaryotic secretory signal peptide sequence was added to 5 ' - flanking region of t - pa gene and kdel ( sequence located to endoplastic reticulum ) to 3 ' - flanking region by pcr amplication and plant expression vector pbemt was constructed
   ( 3 )翻譯后水平通過(guò)pcr擴(kuò)增的方式在t - pa基因5端添加了真核分泌信號(hào)肽序列和植物翻譯起始共有序列aaca ，在3端添加了內(nèi)質(zhì)網(wǎng)定位序列kdel ，構(gòu)建了植物表達(dá)載體pbemt 。
8. The new synthesized protein was led to endoplastic reticulum cavity by eukaryotic secretory signal peptide sequence and then anchored to innerwall of endoplastic reticulum by kdel sequence , which interdicted the process of protein entering golgi body and cytoplasm , and then avoided heterogeneous glycosylation modification of foreign protein and prolonged the disappearance of half life of protein in organism . 2
   真核分泌信號(hào)肽序列可以引導(dǎo)新合成的蛋白質(zhì)進(jìn)入內(nèi)質(zhì)網(wǎng)腔， kdel序列將進(jìn)入內(nèi)質(zhì)網(wǎng)腔的蛋白質(zhì)錨定在內(nèi)質(zhì)網(wǎng)內(nèi)壁上，從而阻斷了蛋白質(zhì)進(jìn)入高爾基體和細(xì)胞質(zhì)的過(guò)程，進(jìn)而避免了外源蛋白質(zhì)的異源糖基化修飾，延長(zhǎng)了蛋白質(zhì)在生物體內(nèi)的半衰期。
9. The length of this phytase gene is1506bp interrupted once by an intron of 102bp in the 5 " part of the gene , this intron contains donor sequence - gtatgc , lariat sequence - gctgac and acceptor sequence - cag which are typically conserved sequence of the intron of fungal phytase gene . this gene encodes a peptide of 467amino acid residues with molecular weight of 51 . 37kda , containing 13 potential n - glycosylation sites and a signal peptide sequence made up of 19 amino acid residues at n teminal of the peptide
   核苷酸序列分析表明， pcr擴(kuò)增產(chǎn)物中包含有完整的phya基因，該基因全長(zhǎng)1506bp ，其中包含一段長(zhǎng)102bp的內(nèi)含子，該內(nèi)含子具有真菌植酸酶基因內(nèi)含子的特征保守序列： donor序列? gtatgc ， lariat序列? gctgac及acceptor序列? cag 。該基因編碼467個(gè)氨基酸，理論分子量為51 . 37kda ，其上有13個(gè)潛在的n -糖基化位點(diǎn)， n端19個(gè)氨基酸為信號(hào)肽序列，植酸酶活性位點(diǎn)序列( crvtfaqvlsrhgaryptdskgk )位于氨基酸序列的+ 71 + 93 。
10. In comparison with genbank data , the homologies of the nucleotide sequence and amino acid sequence were as following : hc was 98 . 4 % and 100 % ; ha was 97 . 2 % and 99 . 3 % respectively . 4 . two recombinant prokaryotic expression vector were constructed which has complete open reading occlusing initation codon , leader signal peptide sequence and termination codon
    序列分析表明，所克隆獲得的基因與genbank中已經(jīng)登錄的核苷酸和氨基酸的同源性分別為： hc98 . 4和100 ， ha97 . 2和99 . 3 ，證明本試驗(yàn)蟲(chóng)株與國(guó)外報(bào)道的同源性很高。
11. Therefore , blys , its receptor or related antagonists may find medical utility in the treatment of b cell disorders associated with autoimmunity , neoplasia , or immunodeficiency syndromes . in this study , epo signal peptide sequence and hsblys gene were linked by soe method . the fusion product was cloned into eukaryotic plasmids . pcdna3 , pcdna3 . 1 , pefneo , respectively . meanwhile , the epo signal peptide sequence was mutated so as to form a restriction enzyme cut site : bin i . thus the recombinant plasmid can be used as secreting plasmid expressing other gene
    本實(shí)驗(yàn)通過(guò)3 ’端互補(bǔ)，進(jìn)行引物延伸合成epo信號(hào)肽序列：信號(hào)肽和hsblys基因采用重疊延伸拼接法形成融合基因；融合基因分別插入pcdna3 . 0 、 pcdna3 . 1 、 pefneo真核載體：引物延伸合成信號(hào)肽時(shí)，利用亮氨酸同義密碼，將信號(hào)肽基因的倒數(shù)第二個(gè)密碼突變，在重組載體上的信號(hào)肽序列之后，形成bln酶切位點(diǎn)，使三種載體成為分泌表達(dá)載體。
12. The signal peptide sequence which was used for secretedly expressing divergent gene in mammary gland cells was ligated to the e2 gene , the e2 gene with signal sequence was obtained by pcr . the gene resisting kanamycin was cut down from pgfp - cl vector and inserted into p22 vector , a p22 vector with gene resisting kanamycin was constructed , it was tried to construct an expression vector for transforming go
    豬瘟病毒ez基因的乳腺特異表達(dá)載體構(gòu)建：將在乳腺細(xì)胞中特異分泌的信號(hào)肽序列連接到ez基因， pcr得到了目的片段，再將pgfpci載體上的kana基因切下與在乳腺細(xì)胞中特異表達(dá)的p22載體連接，使其帶有篩選標(biāo)記，然后將帶有信號(hào)肽的ez插入到p22中，試圖構(gòu)建山羊乳腺上皮細(xì)胞的特異性表達(dá)載體。