織免疫 的英文怎麼說
中文拼音 [zhīmiǎnyì]
織免疫
英文
active immunity-
From dead chickens, one virrus was isolated by using eggs and chicken embryo fibroblast. lt was able to agglutinate chicken ' s erythrocytes and this heamagglutination could be inhibited by newcastle disease antiserum. this strain ' s biological property was tested by barren spot, cross - enutralization and cross - heamagglution inhibited and it was found that it was homological with the standard newcastle disease virus ( ndv ) virulent strain and avirulent strain but it had some diference with the standard strain
本實驗採用spf雞胚及雞胚原代成纖維細胞,從河北省某雞場新城疫免疫抗體很高的病死雞的腦組織中分離得到一株病毒。此株病毒能凝集雞的紅細胞,並且這種凝集可以被特異性抗血清所抑制。The distribution of the brine shrimp hgcs varies greatly from the species studied till now. one hour after hatching, neither the dorsal - anterior area nor the other dorsal area remained positive immunoreactivity signal. and 2 hours after hatching, there was no typical hgcs in the body of the brine shrimp and the remained hatching enzymes may participate in digesting the left vitellin in the nauplius
鹵蟲hgc最初出現至孵化前1h時均為全身性分佈,從孵出到孵出后2h ,頭鹵蟲孵化酶的生物化學性質及孵化腺細胞的免疫組織化學研究部的孵化酶顆粒已經減少,而變為非全身性分佈,到孵出后sh ,孵化酶顆粒已基本消失殆盡。Yherefore, many researchers have shown great concern with the development of vaccines to against schistosomiasis. at early stage, the research of vaccines of schitosomiasis was centered on dead vaccine and athenuated cercaria of schistosomes while molecular vaccine and athenuated cercaria of schistosomes while molecular vaccine is currently the focus of research with anti - infection protective immunity as its main concern. guan xiaohong and zhao weixian ( 1986 ) certified that the allergen of egg granulonma of schistosoma japonicum might firstly come from gut associated antigen ( gaa ) of schistosomula and adult worm and that daa had cross reaction with soluble egg antigen ( sea ) and membrane associated antigen ( maa ) ; and the gaa of schistosoma japonicum might play a sensitizing role in egg granuloma formation
Np30主動免疫c57bl 6對尾蚴攻擊感染產生42 . 05的保護力,肝組織減卵率為66 . 63 ; balb c和昆明種小鼠的保護率分別為39 . 53和50 . 46 ;免疫山羊可誘導42 . 78的減蟲率,肝組織減卵率為35 . 83 ,糞減卵率為25 ,並可明顯抑制肝臟蟲卵肉芽腫的大小,肉芽腫數量明顯減少,纖維化減輕,體重明顯增加,因此np30是南京醫科大學博士學位論文很有希望的抗日本血吸蟲病疫苗侯選分子。Immunofluorescence - histochemical changes of the astrocytes in cribriform plate due to high intraocular pressure in rats
大鼠高眼壓后篩板區星形膠質細胞的免疫熒光組織化學變化Magical fire ( eye doctor ) looks at well - being cream of sticking drawing tradition traditional chinese medicine formula famous and precious in tsinghua, is tied in wedlock modern up - to - date medicine result of scientific research, the various chinese medicinal crop famous and precious being carefully chosen, adopt the modern nano - technology and target to poison a technology to being given to, let various active material, tiny molecule, nutrition factor glutathione etc. guide medicine it is all right for to go ahead, the brute force passes through blood eye parclose, make pesticide effect reach nidus directly location, prompt the nutrition replenishing an eye with the part ( include ciliary muscle, retina, crystalline lens, optic nerve ), active eye part cell, improve eye part immunocompetence and oxidation resistance, boost an eye part organizing an assimilation of the new and excretion of the old, microcirculation improving and restoring an eye part, thereby reach eliminate look at strain, purpose improving and improving sight
清華神火視康貼汲取傳統中藥名貴配方之精華,結合現代醫藥最新科研成果,精選多種名貴中藥材,採用現代納米技術和靶向給藥技術,讓多種活性物質、微分子、營養因子谷胱甘肽等引藥上行,強力穿透血眼屏障,使藥效直達病灶部位,迅速補充眼部(包括睫狀肌、視網膜、晶狀體、視神經)的營養,激活眼部細胞,提高眼部免疫能力和抗氧化能力,促進眼部組織新陳代謝,改善和恢復眼部微循環,從而達到消除視疲勞,改善和提高視力的目的。The rse was then grafted to the dorsum of scid mice to evaluate its biocompatibility by histologic and immunohistochemistry analysis
將人包皮的表皮細胞和真皮的成纖維細胞復合到上述材料上培養7天後,移植到裸鼠背部,進行生物相容性、組織學和免疫組織化學的分析。Study and clinical observation of connected enzymology and tissue immune complex before and after therapy of vulvar dystrophy with immune inhibitor and traditional chinese medicine
免疫抑制劑及中藥治療外陰營養不良前後相關酶學及局部組織免疫復合物的研究及臨床觀察Section two the evaluation of biocompatibility of the acellular dermal matrix by the method of cell culture. the new born rat ' s epdermic cells were cultured with the acellular dermal matrix together as experiment group, while the epdermic cell were cultured simply as control. 24 hours later, under the invert microscope, the epidermic cells anchored well and transparent flat cells were observed in both groups. 7 days later, both cultured cells were taked out and fixed in 95 % ethanol, stained with hematoxylin and were observed under light microscope. many cleaved cells were observed in both groups. during cell culture, no pathogenic microganism was observed. so we considered the acellular dermal matrix was aseptic and had good biocompatibility. section three subdermal implantation of the acellular dermal matrix. 24 rats were used in the experiments. a piece of acellular dermal matrix ( 1. 5 x 1. 5cm2 ) was implanted beneath the dorsum skin flaps of each rat, 1 week, 2 weeks, 3 weeks and 4 weeks after implantation, 6 pieces of acellular dermal matrix were harvested and the size of implanted acellular dermal matrix were measured, the sections were used for he staining and observed under light microscope. the result were as folio wing : 1 - 2 weeks after implantation, the acellular dermal matrix began to adhere to the tissue around and turned red gradually ; 3 - 4weeks after implantation, the acellular dermal matrix adhered closely to the tissue around and could be recognized easily, 1 - 3 weeks after implantation, the size of implanted acellular dermal matrix had no statistical difference ( p > 0. 05 ). 4 weeks after implantation implanted acellular dermal matrix contracted ( p < 0. 05 ). under light microscope, l - 2weeks after implantation, the fibroblast cells infiltrated the acellular dermal matrix and a small amount endothelial cells of vessel and lympho - histiocytic cells infiltrated the acellular dermal matrix. 3 - 4 weeks after implantation, infiltrating blood vessels were evident. so we think that the acellular dermal matrix had low immunological reactions and could induce the infiltration of fibroblast macrophage cell and the endothelial cells of vessel
結果如下:皮下包埋卜周者,無細胞真皮基質漸與周圍組織粘附,顏色由蒼白轉紅;皮下包埋3周者,無細胞真皮基質與周圍組織緊密枯附,盾晰葉辯;術后卜周,包埋的基質面積變化較包埋前無統計學差異o川0引,術后4周包埋的無細胞真皮基質面積較包埋前縮小j刃刀5 ) 。光鏡下術后卜周,宿主的淋巳組織細胞、成纖維細胞浸入生長,釉附在膠原纖維上,少量血管內皮細胞浸入基質;術后34周,無細胞真皮基質內較多的血管形成,故可認為無細胞真皮基質免疫原性低,能誘導宿主的成纖維細胞、巨噬細胞浸入生長,為一種新型的真皮替代物。第四部分無細胞真皮基質與自體斷層皮片復合移棺的研究, sd大鼠10隻,在其背部卜方造成全厚皮膚缺損的創面Nayak et al. (1965) studied the immunocytologic and histopatholgic development of experimental swine influenza virus infection in pigs.
Nayak等(1965)研究了豬的實驗性流感病毒感染的免疫細胞學和病理組織學發展。Muscarinic acetylcholine receptors in sjgrens syndrome sjgrens syndrome is a chronic autoimmune disease characterized by histological and functional alterations of exocrine
修格連癥候群是一種慢性自體免疫疾病,其特徵為外分泌腺體之功能及組織學變化,引起淚腺和Thus, in order to investigate the developmental pathways not only involved in the regulation of growth and patterning, but also in the determination of cell lineages and differentiation, we utilized the fluorescent immunohistochemical methods, flow cytometry analysis sorting ( facs ) and molecular methods to investigate the developmental law of mammary gland at the different developmental stages, distribution of the stem cells in mammary gland, the methods of isolation, culture and evaluation for the stem cells, the multipotent abilities in vivo and in vitro, and the efficient cultural system for stem cells enriched in vitro. the results showed below : 1
我們以小鼠為模型,運用組織化學、免疫熒光組織(細胞)化學、流式細胞儀分選方法( facs )以及分子生物學手段,研究了小鼠乳腺的發育規律:小鼠乳腺組織中類乳腺幹細胞:小鼠乳腺細胞的分離、培養以及類乳腺幹細胞的鑒定;小鼠類乳腺幹細胞分化的潛能;小鼠乳腺類腺體體外短期培養富集類乳腺幹細胞體系的優化等。研究結果表明: 1So it can induce stronger and earlier iga immune responses at almost all mucosal sites than oral route. the way induced by nasal route is similar to which gut associated lymphoid tissue ( galt ) induced
鼻腔含有的蛋白水解酶較少,抗原不易被破壞,鼻腔免疫可以在多個粘膜部位產生siga反應,誘導與胃腸相關淋巴組織( galt )形式上相似的粘膜免疫反應。In one word, the methods for producing acellulace matrix have not been standardized. in this study, we want to select the best way to produce acellular matrix. we also use immunohistochemical method for detecting the magor heterogenetic antigen a - galactosyl residues ( a - gal ) in acellular matrix
並應用免疫組化的方法檢測脫細胞后基質的主要異種抗原,用種植實驗觀察異種機體對脫細胞生物基質的組織反應倩況,另在其上種植鼠成纖維細胞以觀察脫細胞生物基質的細胞毒性和細胞相容問題。Study on immune histochemistry of penaeus chinensis artificial infection with explosive epidemic pathogen
中國對蝦暴發性流行病病原的免疫組織化學研究In order to get further evidence of the localization and distribution of emt - 1 in cells, we have prepared emt - 1 his6 - fusion protein and intend to abtain emt - 1 antibody for immuno - histochemistry assay
為了進一步證實emt l在細胞內的定位及組織分佈,擬制備抗emt l抗體,進行免疫組化驗證。Final diagnosis of mfh was achieved based on histopathology and immunohistochemical stains
最後的確定診斷有賴于組織病理切片以及免疫螢光染色等檢查。A immunohistochemical study of rabbit cornea after excimer laser photorefractive keratectomy
術后角膜創面的免疫組織化學研究Female mice serum and vaginal secretion antibodies, their fertility and the pathological changes were determined. on the other hand, the effects of the anti - serum against synthetic peptide on the sperm - egg interaction during ivf and the location of p3 peptide in sperm were watched. the main results and conclusions were as follows : 1 ) the new antigen p3 peptide which harvested from the 430a peptide synthesizer were verified by the mass spectrograph and hplc, that the ratio of mass / charge of the synthetic peptide was equal to the molecular weight in theory and its purity was above 95 %
本研究的主要結果和結論如下:一、經抗原分子設計,在430a自動肽合成儀上合成的新抗原p3 ,經質譜儀分析證明其荷質比與理論一致;純化后,其純度大於95 ;將新抗原與klh偶連后免疫小鼠,經westernblot證實其誘導的特異性抗體可識別小鼠、大鼠、人睪丸組織中分子量約為22kd和55kd左右的蛋白質。Objective to find the factors affecting the morphogenesis of tissue - engineered cartilage in animals who have inherent immunity
目的在有免疫力的動物體兔體內探索組織工程化軟骨生成的影響因素。Nogo - 66 receptor, ngr, cloned in 2001, is a leucine - rich - repeat glycophosphatidylinositol - anchored membrane protein which mediates nogo - 66 inhibition of axonal outgrowth. both the long acidic amino - terminal domain and the nogo - 66 fragment have strong neurite growth inhibitory activity suggest that nogo - a has at least two inhibitory domains. northern blot, in situ hybridization, western blot and immunocytochemistry analyses show that in addition to oligodendrocytes, nogo - a mrna and nogo - a protein are also expressed in neurons in developing and adult brain and spinal cord, nogo - a is also found in peripheral organs such as heart and testis
Northernblot 、原位雜交、 westernblot和免疫組化結果證明: nogo amrna和nogo蛋白除了在cns的寡突膠質細胞中表達,還表達于發育階段和成年的腦、脊髓和外周神經節的某些神經元中,在外周組織如睪丸和心臟也有表達; nogoe在cns和pns以及多種外周組織中有廣泛分佈; nogo (除表達于腦和心臟外,在骨骼肌中有較高表達。分享友人