電泳電位 的英文怎麼說
中文拼音 [diànyǒngdiànwèi]
電泳電位
英文
electrophoretic potential-
In our experiment, after light and dark adaptation, the retina of the macrobrachium rosenbergi was respective incubated in high calcium solution, physiological solution and low calcium solution. we studied the effect of calcium concentration on the content and subcellular localization of gq protein a subunit in the photoreceptor cell of macrobrachium rosenbergi on light adaptation and dark adaptation by sds - page technology and imunoelectron microscopy technology. our study results indicated : 一 、 effects of calcium concentration on the soluble gq protein a subunit in the photoreceptor cell of macrobrachium rosenbergi on light adaptation and dark adaptation
而鈣離子對gq蛋白亞基活性有無影響還未見報道。我們以光適應和暗適應條件下的羅氏沼蝦復眼視網膜為材料,分別用高鈣溶液、生理溶液、低鈣溶液孵育后,通過sds ? page電泳技術及免疫膠體金電鏡技術,研究鈣離子濃度對光暗適應時羅氏沼蝦感光細胞gq蛋白亞基含量的影響及亞基亞細胞定位的影響。First, three isozymic systems ( lactate dehydrogenase ( ldh ), esteraes ( est ), malate dehydrogenase ( mdh ) ) extracted from threepopulations of mandarinfishes were detected by discontinuous vertical plate polyacrylamide gel electrophoresis ( page ). several loci were tested but none polymorphic locus was detected in qiupu river population. the results showed that : ldh can be used as biochemical markers to identify these three populations of mandarinfishes
首先,本試驗採用聚丙烯酰胺凝膠電泳( page )對我省三個水域鱖魚群體3種同工酶( ldh 、 est 、 mdh )的不同基因座位進行了檢測,結果表明: ldh同工酶可以作為區分秋浦河鱖魚、長江鱖魚兩個群體與萬佛湖鱖魚群體的生化遺傳標記;其次,運用rapd技術分析了三群體鱖魚的基因組dna的多態性。Second, the population genetic structure and genetic diversity of e. mollis were studied by using allozyme eletrophoresis and the electrophoretic data for 6 loci from 3 populations being xiangning, yicheng and pinglu populations in shanxi were got. the level of polymorphism was relatively higher than that of the insect - pollinated outcrossing species ( he = 0. 375 )
用等位酶電泳法和biosys - 2軟體對山西翅果油樹種群的遺傳結構和遺傳多樣性進行了研究,通過對3個種群的6個等位酶位點的電泳分析,結果表明: 5個位點為多態位點, 1個單態位點。Keywords : sedimentation velocity and potential, electrophoretic mobility, electric conductivity, charged composite particle, charged porous particle, arbitrary double - layer thickne
關鍵詞:沉降速度與電位、電泳可動度、電導度、帶電復合粒子、帶電多孔性粒子、任意電雙層厚度。The expressed product was lysised with supersonic wave and purified by sds - page. elisa analysis revealed that the antigenicity of the vpi protein has been detected. the forth part - detection of aev - nh937 strain by in situ hybridization ( 1sh ) - probe was labelled with digoxigenin ( dig ). then the probe hybrid with 5d, 10d, and 20d postinfection brain tissue of chicken. the results of the ish showed that the positive signal was found in 3 cases, while control group was negative. there has been a reasonable correlatien between this method and other detection test
經超聲波裂解,用尿素溶解包涵體,電泳純化后,利用elisa檢測vp _ 1外殼蛋白,表明具有一定抗原性;第四部分:應用原位雜交檢測aevi用dig標記的探針與sd 、 10d 、 20d的攻毒雞腦組織雜交,來檢測那v的rna 。? as same as most other schizothoracinae fishes, qinghai - lake nakked car ps may be tetraploid that already were diploidization ; ? qinghai - lake nakked carps arose from some primitive barbinae fishes, which gradually became special population adapting to high altitude environment by involvement and natural selection, on protein electrophoresis, out of 20 protein loci among 132 individuals in the present experiment, only t mdh > amy est and pod showed polymorphism
在蛋白水平上,共檢測了132尾裸鯉的20個遺傳座位,僅發現tf , mdh 、 amy 、 est和pod五個座位表現出多態性,其中, tf 、 mdh 、 amy和est四個座位均有一對等位基因;而pod座位表現出復雜的電泳圖譜,未進行深入分析。Abstract : the polymorphism of angiotensinogen gene at position 174 was studied in 90 cases of essential hypertension patients and 109 controls by pcr, restriction enzyme analysis and electrophoresis methods. the results showed the distribution of genetypes in hypertension group was significantly different from that of controls group. this suggested there is a correlation between the variant of agt174 and hypertension
摘要本文採用pcr 、限制性酶切和電泳分型等方法,分別對90例原發性高血壓患者和109例正常人血管緊張素原基因多態位點agt174進行了檢測,結果表明,高血壓組中三種基因型的分佈與對照組顯著不同,提高該位點變異與原發性高血壓的發生相關。In the second part, polyphasic taxonomy methods such as morphological method, physiological and biochemical method, dna g + cmol %, soluble protein electrophoresis and 18s rdna sequence analysis were used for systematics of all strains isolated and purified with the method above
本論文第二部分採用形態學、生理生化特徵、 dnag + cmol 、可溶性蛋白電泳及18srdna序列分析等分類技術對所分離的16株甲真菌進行了系統的分類研究,從而初步確定了16株甲真菌的分類地位。Detected samples and ladder were added synchronously during page. compare the bands to classify and denominated them. 2
各y ? str位點檢測到的等位基因與該位點的等位基因梯階( ladder )同步電泳的結果參見圖2 ? 1 2 ? 6 。This understand of stored nitrogen compounds restricted seriously the progress in the investigation of vegetative storage proteins. in the dissertation, we studied more extensively the cytology, biochemical properties and biological roles of vegetative storage proteins in swietenia macrophylla and in hevea brasiliensis by light - and electron microscopy, sds - page, page, immuno - blotting, indirect immunohistochemical localization and colloidal gold labelling and cdna clone techniques
採用光鏡和電鏡技術、 page 、 sds - page和免疫印跡技術、電泳凝膠過碘酸? schiff試劑染色、間接免疫熒光和電鏡免疫細胞化學定位技術以及cdna克隆技術,較深入地研究了大葉桃花心木和巴西橡膠樹的營養貯藏蛋白質的細胞學、生物化學性質和生物學功能。57 protein spots out of about 1000 detectable spots on the 2 - d gels were indentified by the following two methods : l ) n ~ terminal edman degradation microsequencing after the protein spots were electro - transferred to pvdf membrane. 2 ) maldi - tof - ms peptide fingerprint analysis of the protein spots and protein database searching. the 2d protein maps of the rice spikelet during the sterile and fertile stages were compared
二是通過原位酶解,抽提蛋白質片段進行maldi - tof質譜分析,利用肽質量指紋圖數據在數據庫中進行檢索,在雙向電泳凝膠上取了57個點進行分析,有34個蛋白質點在數據庫得到歸屬鑒定。Ten isozymes and proteins were investigated by cellulose acetate membrane electrophoresis, the phylogenetic relationship among four groups of microtus fortis was analyzed based on the alleles frequency at these biochemical loci
應用乙酸纖維素膜電泳法分析了四類東方田鼠的10種同工酶及蛋白,並觀察了它們在這些生化基因位點上的基因分佈特徵以研究它們之間的遺傳關系。These 8 y - str loci were amplified with pcr and the products of pcr were analyzed using gel electrophoresis. each allele of these 8 y - str loci was sequenced and the allele ladders were constructed in house. alleles of these y - str loci were nominated according to recommends of the international society of forensic genetics
應用pcr方法擴增y - str ,電泳分型;對所有基因座的等位基因進行測序,構建等位基因分型標準物,按國際法醫遺傳學會( isfg )原則命名等位基因。Location of the hbrp gene in the chromosome according to stanford g3 rh panel, a pair of primers are designed in the 3 " - utr region of the gene which is to be localized and human genome dna is amplified in advance whose products are examined by electrophoresis. then g3 panel is amplified and this process is repeated twice. the pcr result is sent to stanford human genome center ( shgc ) http : / / www - shgc
Hbrp基因的染色體定位使用stanfordg3rhkadiationhybrid )嵌板,在所要定位基因的3 』非翻譯區( untranslatedregion , utr )設計引物,預先擴增人基因組dna ,電泳檢測產物大小,繼之擴增g3rhpanel ,重復兩次,將pcr結果輸人斯坦福人類基因組中心( shgc )的主頁( http : 、 shgcPcr - based analysis method was carried out in the following study. dna amplification by pcr in cgg repeats were performed on 154 people as normal control ( 73 males and 81 females ) and 23 members from four x - linked mental retardation ( xlmr ) families. after electrophoresed on a 6 % - denaturing polyacrylamide gel ( acr : bis = 19 : l ), genotypes of the objects were determined by analyzing pcr products
本研究採用較以往更為簡便有效的pcr技術方法,對隨機抽取的154人的正常群體(男性73人、女性sl人)及來自四個智力低下家系的23名成員進行了fmr基因cgg重復序列的擴增,利用變性聚丙烯酸胺凝膠電泳技術對不同等位基因類型進行分離和統計。There are at least three kinds of ep in petal : thiol - proteinase, metallo - proteinase, serine proteinase. they gather at the site between 43 kd and 66. 2 kd ( about 52 kd ) on the substrate gel electrophoresis. the optimum ph of thiol - proteinase, metallo - proteinase is ph 6, which are looked as acid ep, the serine proteinase has two forms, one is acid ep ( ph 6 ), and the other is alkali ( ph 10 )
花瓣中都至少有3種內肽酶:巰基蛋白酶、金屬蛋白酶、絲氨酸蛋白酶,三者聚集在底物膠電泳膠條的43kd 66 . 2kd之間的位置,約為52kd ;前兩種最適ph為6 ,是酸性內肽酶,后一種有酸( ph6 ) 、堿( ph10 )兩種存在形式,既是酸性內肽酶又是堿性內肽酶。When swims to these 163 wild soybeans and half wild soybean pod electricity the result carries on gathers a kind of analysis discovered that, the geographical position close also the habitat similar material its heredity distance approaches, the geographical position close but habitat different material its heredity is away from not necessarily closely, the habitat same but the geographical position different material its heredity distance is farther
在對這163份野生大豆和半野生大豆pod電泳結果進行聚類分析時發現,地理位置相近且生境相似的材料其遺傳距離較為接近,地理位置相近而生境不同的材料其遺傳距離不一定相近,生境相同而地理位置不同的材料其遺傳距離較遠。Method to collect respectively 180 unrelated males " venous blood 500ul, who lived in shanxi province, 120 unrelated mongolians " venous blood 500ul, who lived in the inner mongolia autonomous region, and the blood is anticoagulant with edta, then to extract dna by using the method of phenol - chloroform after ingested by proteinase k at 56 and amplify the dys413 site by using pcr
方法採集180例山西漢族和120例內蒙古蒙古族男性無關個體靜脈血各500ul , edta抗凝,用tkml液反復洗滌至無色,加入2蛋白酶k緩沖液180ul ,蛋白酶k ( 20mg ml ) 20ul ,在56消化至液體清亮為止,用酚-氯仿法抽提dna , pcr擴增dys413位點, 6非變性聚丙烯酰胺凝膠電泳, 1硝酸銀染色分型。A review is presented on the recent progress and the prospect of the determination of microamounts of iodine in table salt by different electrochemical methods, such as ion selective electrode, electrometric titration, polarography, stripping voltammetry, potentiometric stripping, adsorptive stripping voltammetry, pneumatoamperometry, spectroelectrochemistry and electrophoresis
摘要從離子選擇電極法、電化學滴定法、極譜法、溶出伏安法、電位溶出法、吸附溶出伏安法、揮氣電流法、光譜電化學法和電泳法出發,評述了食鹽中碘含量測定的電化學分析法研究現狀及發展方向。Indentificatiort is also the first step towards studies on protein co - and post - translational modification, and ultimately, function. in the present study, the total proteins of the photo - thermo sensitive genie male - sterile rice ( oryza sativa, peiai64s ) spikelet at meiosis stage were used as the material. by optimizing crucial factors and procedures such as sample treatment, electrophoresis parameters, and gel concentration, 2 - d maps with high quality and reproducibility were obtained
用兩種方法對經雙向電泳分離的凝膠上的蛋白質點進行了初步鑒定,一是通過電印跡轉移把蛋白質轉到pvdf膜上,再用edman降解的方法測得部分相對分子質量在10000 - 30000da的蛋白質點的n -端序列,通過網上搜索其同源性對其進行鑒定,並確定該點在凝膠上的位置。分享友人