鼠疫血清 的英文怎麼說
中文拼音 [shǔyìxiěqīng]
鼠疫血清
英文
pest sera-
Second, ca - np30 conjugate was made by binding ca with np30. then immunized balb / c mice with ca - np30, and evaluated its effects on protective immunity, serum specific igg antibody levels and delayed type hypersensitivity ( judged by footpad test )
將鈣納米顆粒ca與np30制備成ca皿30結合物( ca np30 ) ,主動免疫b從b兒, j 、鼠,觀察其對, j 、鼠抗血吸蟲感染的保護作用、對血清特異性屹g抗體的影響和足墊反應。The western blot analysis show that the antiserum induced by the new antigen plus hemocyanin could bind with the 22kd and 55kd proteins, which were existed in the testis tissue protein of mouse, rat and human. 2 ) the purified peptide emulsified in an equal volume of freund ' s adjuvant and immunized the female balb / c mice with 8 - 10 weeks old. the antiserums and the washings of vaginal membrane were detected by elisa, and shown the highest level of the specific antibody igg was 1 : 6000, while the iga was 1 : 300
二、 p3多肽與弗氏佐劑混懸后免疫近交系balb c小鼠后,在血清和陰道粘膜沖洗液中可檢測出特異性lgg 、 lga ,最高效價分別達到1 : 6000和1 : 300 ;免疫后的小鼠脾臟淋巴細胞增殖率升高,淋巴細胞培養上清液中分泌的il 4和inf y也升高,且以il 4更明顯。This modification includes : ( 1 ) selecting two important molecules as candidates, ( 2 ) choosing a promiscuous t - cell epitope, and two b - cell epitopes or conserved amino acid sequences from the two important molecules, ( 3 ) connecting them adequately through analysis by the molecule designing software. therefore, the synthetic new antigen may interfere with the process of fertilization by multiple ways and its contraceptive effects may be enhancing. based on the molecule designing methods, the b - lymphocyte cell epitope of sperm / testis specific protein sp17 and cyritestin which interfere with fertilization in mouse, as well as the promiscuous th cell epitope of the ribonuclease ( rnase ) in bovine were selected
本研究以蛋白質分子設計的理論和方法研究避孕疫苗,將sp17和cyritestin關鍵表位和牛核糖核酸酶非選擇性th細胞表位合理組合,獲得新抗原- 35肽序列;並在合成、純化後分別與弗氏佐劑、免疫刺激復合物( iscoms )混合后免疫不同遺傳背景的雌性小鼠,觀察血清和生殖道內的特異性抗體滴度的動態變化、生育力的改變以及免疫后小鼠重要臟器的組織病理學改變:以及在ivf下,新抗原的特異性抗血清對精卵相互作用的影響及抗原在精子表面的特異性定位。On the base of i. acidophilus strains pb1 mixed with enterococcus strains m1, pb2, a30, a31, bifidobacteria pba and inf were added in the culture. the results suggested pba and inf were limited on the co - cultures, its indicated that pba and inf grew badly with other probiotics in vitro each mice were given 0. 5ml fermentative liquor of probiotics strains pbl + a30, pba, pb1, m1, pb1 + m1, pb1 + a30 for one month
將幾株體外性狀好的菌株pba 、 pb1 、 m1 、 pb1 + m1 、 pb1 + a30 ,每天以0 . 5ml每隻發酵液的量灌胃給正常小白鼠,時間30天,測定小鼠免疫器官指數和血清中細胞因子的變化,並觀察小鼠脾臟的變化。Anti - melatonin monoclonal antibodies of higher titer, affinity and good sensitivity were obtained by coupling mt to bovine serum albumin with formaldehyde and by immunizing mice with multifocal intra - dermal injections. we obtained 6 strains of hybridoma, all of them secreting specific antibodies to mt, we apply antibodies to determinate free mt inhuman serun with group - selective immunoassay technique. an inhibition curve for mt was obtained in the range of 50pg to30ng, and 1. 4ng of mt inhibited the value of the assay by half. we evaluate the specificity of antibodies by determination of cross - reactivity of several analogues, the moabs recognized mt but
通過將mt用甲醛作連結劑連結到牛血清白蛋白上sa採用皮下多點注射兔疫小鼠得到了高效價,高親和力,較好特異性的抗mt單克隆抗體,最後獲得了5株單克隆細胞株,都能分泌針對mt的特異性抗體,建立了選擇性基團免疫分析法,用制備的抗體測定了人血清中mt的含量,作了mt的抑制標準曲線,其抑制范圍從50pg ? 30ng ,半抑制量為1In order to study the function of cycling2 in vitro culturing cell line, we used pires - g2 eukaryotic expression vector transfecting human gastric cell line sgc - 7901 and human embryo kidney hek - 293 cells by lipofectamine plus reagent, and studied the function of cycling2 expression on the cell proliferation in vitro, further investigated the regulation mechanism of cycling2. at the same time, we made a study on the expression level change of cycling2 in normal gastric tissue and different type and different stage of gastric carcinoma tissue. material and method 1 material : piresneo vector was purchased from clonetech, plasmid extraction and purification kit was purchased from qiagen company ; rpmi 1640, dmem fetal calf serum were obtained from gibco / brl ; lipofectamine plus and g418 were purchased from life technologies ; ultrasensitive ? s - p kit, mouse monoclonal antibody p21wafl ( in use ), dab staining kit were purchased from maixin company
實驗材料與方法1 .實驗試劑高糖dmem 、 rpmll640和胎牛血清購自美國g山eo / brl公司; dmewf12 ( 1 : 1 )混合培養液購自美國hyclone公司;胰蛋白酶購自美國si目叮a公司; hepes由美國amersco公司分裝;脂質體轉染試劑( upofectalnineplusreageni )和以18為美國玩vitrogen公司產品; piresneo載體購自美國cloneteeh公司;質粒提取及純化試劑盒購自德國qiagen公司; ultresensitive翎s一p免疫組織化學試劑盒;鼠單克隆抗體戶3 ( do一7 )蛋白(即用型) ;鼠單克隆抗體p21waf , (即用型) ; dab染色試劑盒均購自福建邁新公司;鼠單克隆抗體pziwa曰(濃縮型) ;辣根過氧化酶標記羊抗鼠二抗購自北京中山公司; ecl試劑盒購自美國santacruze公司; dcproteinassay試劑盒購自bi 。Conditioned immunosuppression to rabbit anti - rat lymphocyte serum in rats
以兔抗鼠淋巴細胞血清為非條件刺激的條件性免疫抑制By genetic engineering methods, ureb gene and ureb - hspa fusion gene were amplified by pcr and cloned into a prokaryotic expression plasmid ptrc99a - asd, and identified recombinant plasmid was then
口服、鼻飼免疫balb / c小鼠,在腸液和血清中可以分別檢測到針對hpylori的特異性分泌型iga和址g抗體。S, . antibodies were monitored at interal of one week, the results showed that it is positive between 2 to 4 weeks after inoculation ; the mice were weighed every 5 day, the results showed that weight difference is significant between the inoculated and control group. seroreaction of test group is positive using hbsag elisa kit, but control group is negative
6 、動物試驗:將重組矗因工程苗苗誘導表達波免疫家兔,然後每周采血分離血清測邑鉆抗體,結果在免疫后2周,血渝中檢出ss抗體;兔疫注射10日齡小白鼠,每5天稱重一次,結果表明:注射誘導表達液的試驗組比對照組槽重差異顯著叩0Following the 7d, 14d, 21d, 28d feeding period, in each treatment, one mouse was killed to count the ratio of peripheral anae + t lymphocyte, serum igg content, serum cu, zn - sod activity, serum cp activity, immune organ index, copper concentration in liver and spleen
在正式試驗期第7天、 14天、 21天、 28天,每重復選取1隻小鼠,測定外周血t淋巴細胞百分比、血清igg含量、血清銅鋅超氧化物歧化酶和銅藍蛋白活性、免疫器官指數及肝臟和脾臟銅含量。Investigation of serum epidemiology from the plague foci population in leizhou island, guangdong
廣東省雷州市鼠疫疫源地人群血清流行病學調查及分析Serum immunopharmacological assessment of effects of rubia yunnanensis on murine immune cell stimulated with streptococcal antigens
小紅參含藥血清對鏈球菌抗原刺激小鼠的免疫藥理學研究Methods five tests, including hypoxia tolerance test, serum content determination of sod and mda in mice, carbon clearance and weight determination of immune organ, content determination of serum hemolysin, and delayed - type hypersensitivity test were carried out to evaluate the main pharmacological indexes of lilium brownii polysaccharide
方法通過耐缺氧實驗及小鼠血清中sod 、 mda含量測定,網狀內皮系統的碳粒廓清速度及免疫器官重量測定,血清溶血素含量測定,遲發型超敏反應等實驗對百合多糖的主要藥理指標進行考察。Methods : in cultured lung explants without serum, the lipid component synthesis of pulmonary surfactant was evaluated in [ 3h ] - choline incorporation ; mrna content of phosphocholine cytidylyltransferase ( cct ) in lung explants was investigated in rt - pcr ; the changes of the ultrastructure of the at ii cells were observed with electron microscope ; the expression of nmdar1 subtype was observed in immunohistochemistry staining ; nitric oxide synthase ( nos ) activity, nitric oxide ( no ) content, superoxide dismutase ( sod ) level, malondialdehyde ( mda ) content and lactae dehydroase ( ldh ) level were determined by biochemistry methods. results : 1. influence of glutamate on synthesis of the lipid component of pulmonary surfactant ? with l - arginine, glu inhibited [ 3h ] - choline incorporation with good dose - dependence and time - dependence ; ( 2 ) mrna content of cct of the glu treatment groups was decreased ; ( 3 ) glu increases the release of ldh in cultured lung explants ; ( dwith electron microscope histochemistry, glu induced the changes of the ultrastruture of at ii iv cells
方法:採用成年大鼠肺組織無血清培養,運用[ ~ 3h ] -膽堿摻入法測定ps主要脂質磷脂酰膽堿( pc )合成量; rt - pcr擴增檢測肺組織中pc合成限速酶磷酸膽堿二胞苷酰基轉移酶( cct ) mrna含量;透射電子顯微鏡法觀察肺泡型上皮細胞和ps系統超微結構的變化;免疫組織化學染色檢測glu的受體nmdar1亞單位的表達;生化測定肺組織乳酸脫氫酶( ldh )釋放量和肺組織勻漿中一氧化氮合酶( nos )活性、一氧化氮( no )生成量、超氧化物歧化酶( sod )水平以及丙二醛( mda )含量。Then protein crystal of eif - 5a was observed using atomic force microscopy. further, the polyclonal and monoclonal antibodies were gained from immunized rabbits and rats. hypusine - contained eif - 5a plays a role in cell growth and differentiation
用得到的重組蛋白分別免疫家兔和小鼠,獲得兔的抗血清和三株持續分泌單抗的雜交瘤細胞株,為進一步分析eif - 5a的功能提供了檢測手段。These indicated that the porcine il - 6 gene was correctly transcribed and translated in the recombinant bacteria. the fusion protein was recovered from polyacrylamid gel and used to immunize the rabbit, and the liter of rabbit anti - porcine il - 6 serum from immunized rabbit was 1 : 128, 000
從制備性聚丙烯酰胺凝膠中回收融合蛋白,用mtt法測定重組蛋白刺激小鼠脾淋巴母細胞增殖反應活性,並以重組蛋白免疫家兔制備抗豬il - 6滴度為128 , 000的高免兔血清。The recombinant was transformed into e. co2i ' bl21 strain for expression with the induce of iptg
將表達產物從凝膠中回收,免疫4周齡小白鼠,五次免疫后,采血分離血清。Antigen in me was stable after treated with gastric juice for 6h. me has significantly enhanced the immune efficiency of rhp. in this study, high specific antibodies levels were induced in serum, gastric and intestinal mucosa of balb / c mice immunized with rhp by oral, rectal and intranasal route
Rhp疫苗經鼻腔、直腸及口服免疫小鼠后,均在小鼠的血清、胃粘膜、小腸粘膜沖洗液中產生了較強的特異性免疫應答,並產生了明顯的抗hp的免疫保護。In addit ion, effect of so2 inhalation on the serum cytokine of peripheral blood was determined through the methods of molecular immunology. these studies further indicated that oxidative stress maybe plays an important role in the mechanisms of sulfur dioxide toxicity
另外還從分子免疫學角度研究了二氧化硫吸入后小鼠血清中細胞因子的變化,上述研究結果進一步明確了氧化應激很可能是二氧化硫的重要毒性作用機制。In order to study immunization of genetic vaccine by inoculation, two kinds of dna vaccine of ndv are constructed and analysed their sequense, which will express f protein in eukaryotic cell ( hela cell ) in vitro with the method of transfection by cationic liposome the results testify that two sorts of plasmids dna successfully expressed the f protein of ndv in hela cell, but the expressed content of pc4. 0f is higher than ones of pc3. 1f
將構建的基因疫苗pc3 . 1f大量提取和純化,採取肌肉注射和腹腔注射兩種途徑、不同劑量免疫小鼠,用elisa方法檢測小鼠血清中抗f基因表達產物的抗體水平。研究結果表明,基因疫苗pc4 . 0f和pc3 . 1f均在hela細胞中成功表達,其中pc4 . 0f的表達量比pc3 . 1f高。分享友人