inclusion body造句
造句与例句
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- 3 r hpf4 was expressed as inclusion body in e . coli , after washing with reagent i ( 50mm tris - cl ph 8 . 0 ; 100mmnacl ; 0 . 5mm edta ; 2m carbamide ; 0 . 2 % tritonx - 100 ; 0 . 2 % doc ) and reagent ii ( 50mol / l , ph8 . 0 tris
3超卢结合溶由酶法破碎人肠杆菌后,经分析rhpf4主要以包涵体的形式存在,包涵体经洗涤液iuommtrk mphs - The results showed that infected chicken not only had charateristic pathologic changes such as serious degeneration , necrusis , formation of intranuclear inclusion bodies in the hepatic cells , but its immune organs were also seriously injured
结果表明,病鸡发生以肝脏严重变性、坏死,并在肝细胞核内形成核内色涵体的特征性病变。 - Isolate and purify the target protein . prepare 50ml e . coli expressing the interesting proteins and harvest the cells and determinate the solubility of the target protein . completely solubilize inclusion bodies with 8m urea
溶解包涵体,将包涵体溶解物上ni一taslurry ,利用该融合蛋白表达时带有的his一tag与ni +的亲和作用分离、纯化表达蛋白。 - We find that the fusion proteins are inclusion bodies when the bacteria lysised by the lysozyme . the product of pet - 32a ( + ) - igf - i was analyzed by western blotting , which confirmed that the hybrid protein was expressed as expected
菌体采用溶菌酶裂解,融合蛋白以包涵体形式存在;对higf -融合蛋白进行了westernblot分析,确认所表达蛋白为目的蛋白。 - Section hi : purify & refold recombinant hpk - 5 protein was efficiently expressed in e . coli jm109 as inclusion bodies . after bacteria were smashed by ultrasound , te buffer , 1 % ttiton x - 100 and 2 m urea was used to efficiently extract inclusion bodies
用含sm尿素溶液洗涤包涵体, 8000r / min转速下分离包涵体,能最大限度去除杂蛋白,同时不会降低目的蛋白的损失。 - After the expression form analysis , the insoluble recombinant proteins was purified by destraction and abstersion of inclusion bodies . to study the abstersion condition of the inclusion bodies , we adopted ultrasound crushing and freezing - melting methods
采用超声加洗涤液破碎菌体;离心加冻融分离纯化融合蛋白,研究不同的超声次数和冻融对包涵体洗涤效果的影响。 - After dissolving inclusion bodies , renaturing inclusion bodies and further purification by immobilized metal ion affinity chromatography ( imac ) , the fusion protein trx - scfv of electrophoretic purity was obtained , they still possessed antigen - binding activity
经变性复性,用固相金属离子亲和色谱法一步分离纯化了具有功能的单链抗体,在一升的发酵液中得到78mg的重组蛋白。 - The inclusion bodies of recombinant protein were purified with washing buffer consisting of various urea ( 2mol / l and 4mol / l ) for several times , and then dissolve the fusion protein in the denature buffer using 8mol / l urea as denaturant
用含有2mol l和4mol l尿素的包涵体洗涤液洗涤包涵体,在37条件下,洗去了大部分菌体蛋白及其它核酸物质。用8mol l尿素作为变性剂溶解包涵体,包涵体在8mol l尿素中的溶解性非常好。 - Although some pga precursors formed inclusion bodies in the cytoplasm of dh5a / pkkfpga , the amount only made up 5 - 10 % of all the afpga peptides , this explained why the expression level of afpga in dh5 / pkkfpga was a little lower than that in dh5 / psmlfpga
虽然青霉素g酰化酶在菌株dh5 pkkfpga中形成包涵体,但其量只占总酶的5 - 10 ,解释了为什么菌株dh5 pkkfpga的表达量虽然比菌株dh5 pkkfpga低,但差距不大。 - The virus could multifly on the mdck cells . and induce regular cytopathic effect ( cpe ) . observed by negative staining electron microscope , the virus could be seen with coroniform spike . in the ultrathin sections , the viruses were found to multiply and induce inclusion body forming in the cytoplasm
本研究从某动物园两只死亡大熊猫的肝、脾等脏器分离病毒,经mdck细胞适应培养,获得一株病毒(命名为dxmv ) ,在该细胞上可形成有规律的病变。 - It's difficult to see inclusion body in a sentence. 用inclusion body造句挺难的
- Its content was about 9 . 8 % among total cell protein by gene genius bio imaging system . the fusion proteins were found largely in an insoluble inclusion bodies . the purified fusion proteins was obtained by his6 technique used to immunize rabbits to obtain polyclonal antiserum with titer of 1 * 105
经工ptg诱导,重组质粒在点co力‘ blzi中表达出了c端融合了6xhis的融合蛋白,过量表达的蛋白主要以不溶性蛋白形式存在,其表达量占菌体总蛋白的9 . 8 % 。 - Different hosts " response suggested that tumv - sd1 could infect plants of 10 species in 3 families . tumv - sd1 formed pine - wheel inclusion bodies in plant cells . the coat protein of the tumv - sd1 contains 3 components whose estimated molecular weight are 45kd , 38kd and 14kd respectively
寄主反应特性表明, tumv - sd1 6能侵染3科10种植物, tumv - sd1在寄主细胞内形成风轮状内含体,外壳蛋白为3组分,分子量分别为45kd 、 38kd和14kd ;提纯的病毒粒体为长线条状。 - After washing with reagent , adopt the newest purification technology source30rpc , sds - page and densitometric scan analysis , the result show that expression level is 90 % of total bacterial proteins . after renaturation , ifnr , hgfa , hgfb , hpk5 were purified by akta purifier chromatogram instrument , sepharose fast flow , ssphacrayl series gel , selecting optimize condition . finally establish a kind of high efficient purification model of recombinant proteins produced in escherichia coli as inclusion bodies , purification product purity > 98 %
结论:总之,通过对发酵罐中重组工程菌各种培养因素的研究,建立了一种高密度、高表达发酵工艺体系,为重组蛋白的后续纯化提供了大量、稳定的原料供应;通过对不同目的蛋白的色谱行为的系统研究,建立了一种高效稳定、快速简洁、易于放大的包涵体重组蛋白分离纯化体系。 - Sectionii : to research and establish a kind of high efficient purification model of recombinant proteins produced in escherichia coli as inclusion bodies . to raise separate efficiency and biological active efficiency is especially important in the purification model of recombinant proteins . in accordance with these questions , we raise inclusion bodies purity before the purification as far as possible , and select the suitable chromatogram technology
研究并建立一种包涵体中高效分离纯化目的蛋白的优化模式重组蛋白分离纯化工艺中分离效率的提高、生物活性效率的提高及工艺的稳定性是尤其重要的,针对这些问题,我们在层析纯化前尽山西医科大学生物化学与分子生物学2003届硕士学位论文可能地提高包涵体纯度,并选择合适层析方法的同时合理的组合色谱分离单元。 - The steady dead generation and time that was caused by the isolated virus was certain by chicken embryo which was inoculated on seven or nine days . the histopathological changs of the infectious stunting syndrom were studied by the way of ordinary paraffin section and he dying . the experimental result were as follows : the test proved that the changes of the chicken embryo were different in different stage . the chicken embryo dead in a week after it inoculated . the body was dropsy and hemorrhage . dead before it hatched out , the embyo body were dropsy , pale and slime . the liver was yellow and swolled , gallbladder ( vesica fellea ) was filled with bile . bursa and glandula thymus analosis . the kindey dropsy . bowel lamina were humble , dilatation . gas and yellow foam were filled the bowel . histopathological changes were that , in early stage , obvious changes of liver and kindey were dropsy , hemorrhage and necrosis . two types eosinophilic intranuclear inclusion bodies including large round and little granular were present in cells of the above organs . the obvious changes of bursa were dropsy , adverse folliiculated growth and little lymphocytes proliferating , 19 - 21 days chicken embryo , one or two big empty vacuoles were prensent in cells of liver and kindey . the number of the folliculi was growing , the vacuoles between cells were larger
胆囊充盈、其内充满稀薄的胆汁;法氏囊、胸腺萎缩,肠道扩张、肠壁菲薄、内充满气体及黄色泡沫状物;肾脏肿大。病理组织学变化方面,早期肝脏、肾脏、肠主要以出血、水肿和坏死为主,且肝细胞核及肾小管的上皮细胞核内均发现有核内包涵体,包涵体呈嗜酸性,为大型圆形包涵体或不规则的颗粒状;法氏囊则以水肿、滤泡发育不良、小型淋巴细胞数量增多为主。 19 21日龄鸡胚肝细胞、肾小管上皮细胞的胞浆内出现1 2各大的空泡,法氏囊滤泡数目增多细胞间有较大空隙。 - This subject uses the genetic engineering technology and the newest modern biotechnology to study the genetic engineering lower reaches stage , in order to research and establish the optimum , high density fermentation technology pattern and high efficient isolation and purification model of recombinant proteins from inclusion bodies
本课题利用基因工程技术,重点从基因工程下游阶段着手研究,利用最新现代生物技术研究并建立经优化的高密度发酵工艺模式及高效分离纯化包涵体重组蛋白模式。一 - The recombinant b . thuringiensis subsp . israelensis b - pmpx2 can produce a rhombus crystalline inclusion body during its sporulation sds - page analysis proved that cytlaa had overexpressed during the sporulation of the recombinant . it was found that b - pmpx2 strain remained stable toxicity , whatever during vegetative phase or sporulation phase , which was similar to the expression of mtxl gene in the strain of protease ( s ) - deficient b . sphaericus
同时,将来源于苏云金芽孢杆菌以色列亚种( b . thuringiensissubsp . israelensis , b . t . i )的cytlaa基因和p20伴侣蛋白基因克隆连接到质粒pmt9中,并转化到苏云金芽孢杆菌无晶体型中得到重组转化子b - pmpx2 ,电镜观察发现重组转化子b - pmpx2形成一菱形晶体。 - The more favorable experiment conditions of preparing anatase nanometer tio2 powder are obtained from a lot of data . preparation technology of rutile nanometer tio2 powder is researched on the base of experiment of anatase nanometer tio2 powder . the influences of enclosure dose ' s quantity , preroasting temperatures phase - transition accelerant ' s quantity and calcining intensity and so on on the properties of inclusion body - zntio3 / ti ( oh ) 4 , granule size and properties of rutile nanometer tio2 powder are discussed
在锐钛型纳米tio _ 2粉体的制备基础之上,进一步研究了金红石型纳米tio _ 2粉体的制备工艺,探讨了包覆剂用量、预焙解温度、晶型促进剂量及焙烧温度和保温时间等因素对znco _ 3 / ti ( oh ) _ 4沉淀包覆体性能、金红石型纳米tio _ 2粉体产品的粒度和性能的影响。 - The reults of sds - page and western blot dermonstrated that the insoulable component of the induced e . coli culture contained protein 3a . the results of the study indicated that protein 3a existed in the form of inclusion body . the content of the expressed protein in the induced bacteria protein was 29 . 2 % and 22 . 1 % respectively
Sds - page和westernbolt结果证实,大肠杆菌菌体不可溶性蛋白中富含3a蛋白,且此融合蛋白的分子量符合预期设计,说明3a蛋白在表达产物中以包涵体的形式存在,所表达的蛋白含量分别占菌体蛋白的29 . 2和22 . 1 。 - The purified enzyme had a specific activity of 68 . 6 u / mg protein . overproduction of pga was often limited by translocation and / or periplasmic processing steps , subsequently resulted in intracellular accumulation of various types of pga precursors and then formed inclusion bodies in the cytoplasm and / or periplasm
经deae - sepharosecl6b离子交换层析和butyl - sepharosecl4b疏水层析,即可得纯度提高20倍、比活为68 . 6u mg的青霉素g酰化酶,两步纯化的总得率达91 。
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