熒光掃描 的英文怎麼說
中文拼音 [yíngguāngsǎomiáo]
熒光掃描
英文
fluorescent scanning-
The amount by which the dot deflects past the end of the screen is called the screen-overscan.
光點偏轉超過熒光屏邊緣的總數叫做熒光屏過掃描。We used fission yeast schizosaccharomyces pombe ( s. pombe ), an unicellular eukaryotic organism, as research material. electroporation was adopted to load ca2 + fluorescent indicator into yeast cell and under the laser scanning confocal microscopy ( lscm ), we observed cytosolic ca2 + distribution and relative content as well as fluorescence intensity of gfp - cam in different phases of cell cycle of yeast cell. flow cytometry provided a way of determining the relative dna content of populations of fission yeast
本文以單細胞的真核模式生物裂殖酵母( schizosaccharomycespombe )為研究材料,通過激光掃描共聚焦顯微鏡觀察酵母細胞胞質內游離ca ~ ( 2 + )的分佈及相對濃度,以及不同周期時相細胞中gfp - cam的熒光強度變化,並採用細胞流式法對酵母細胞的相對dna含量進行測定以確定細胞所處周期時相。By sds - page and immuno - blotting, we found that a monoclonal antibody of anti - chick brain cytoplasmic dynein intermediate chain antibody could react with cytoplasmic dynein intermediate chain - like protein at 67 kda in lily pollen. under confocal laser scanning microscopy after immunoflurescence labeling, we found that the dynein intermediate chain - like protein appeared punctated and was co - localization partly with microtubules in cytoplasm of lily pollen tube
免疫熒光標記及激光共聚焦掃描顯微鏡觀察發現,類細胞質力蛋白中間鏈在百合花粉管中存在於顆粒狀細胞器上;免疫熒光雙標及激光共聚焦掃描顯微鏡觀察發現,百合花粉管中類細胞質力蛋白中間鏈和微管存在部分共分佈。On the backgrounds of researches inside and outside country, and cooperating experiments with theories analyses, the influence of different processing technology parameters and different sbs modifier sorts on the sbs modified asphalts " properties has been studied. at the same time, their microstructure are observed through fluorescence optical microscopy and scanning electronic microscopy, thus to direct modified asphalt production. on the above conclusion ' s basement, analysing some disadvantages of the storage stability test of sbs modified asphalt in the current specification, a new storage stability test apparatus is developed
本文在參考國內外研究的基礎上,採用理論、試驗相結合的方法,研究加工工藝參數以及改性劑種類等對sbs改性瀝青性能的影響,並通過熒光顯微鏡、掃描電鏡分析其微觀形態,從而指導sbs改性瀝青的生產;在此基礎上,分析我國現行規范用來評價sbs改性瀝青儲存穩定性方面的不足,開發了新的試驗儀,根據動態剪切流變試驗結果和微觀狀態分析,提出一個新的指標? ?離析率r _ s來評價sbs改性瀝青的儲存穩定性;最後,針對不穩定的改性瀝青提出改善措施,研究證明摻加增容劑和穩定劑是行之有效的方法。The shadow mask is the critical component of the colour picture tube and the important component for the choice of colour, its function concentrates on the limitation of electronics bound diameter and the screening direction, the electronics bound which is sent by the electronics gun goes scanning, during the scanning process, we should guarantee every bound gathering into the small holes situated on the screen, then these bounds will point to the regularized position through the small holes on the flat mask, and then three basic colours will be produced, at the same time, those useless electronics will be blocked by the mask board
平板蔭罩是彩色顯像管的關鍵部件之一,是一個重要選色元件,其作用是限制電子束直徑和上屏方向,由電子槍發射的電子束在偏轉磁場的作用下進行掃描,掃描過程中必須使每個電子束只能射中熒光屏上的為該束指定的那些小孔上會聚,並通過蔭罩上諸多的小孔分別打到各自對應的熒光質點上,發出三種基色(紅,綠,藍) ,而無用的電子則被蔭罩板截獲。Usb2. 0 - based fluorescent image acquisition system of the biochip scaner
0技術在生物晶元掃描儀熒光圖像採集中的應用This study was focused on the occurrence characteristics of the cryptomelane - bearing ores and the mineralogical characteristics of natural cryptomelane. the morphology, chemical and structure features of natural cryptomelane were characterized by means of powder x - ray diffraction, scanning electron microscopy, electron probe microanalyzer, energy dispersive spectrometer and x - ray fluorescence
利用x -射線粉晶衍射掃描電鏡電子探針電子能譜和x熒光光譜對天然錳鉀礦的形貌特徵化學成分結構特徵進行研究,結果表明天然錳鉀礦晶體形態主要為針狀纖維狀,沿The epitaxial growths of ingaas / gaas / algaas fundamental material and the fabrication of 45 - deflector are extensively studied in our work. some measuring methods are used to evaluate the growth quality of our grown structure by pl, cv, x - ray double crystal diffraction, sem etc. property analysis are provided for it
利用高能電子衍射、電化學c - v 、掃描電鏡( sem ) 、 x射線雙晶衍射儀、光熒光譜儀( pl ) 、原子力顯微鏡等多種方法對制備的器件進行了檢測,同時對實驗結果進行了必要的分析。3. observe the binding of oligochitosan labeled with 2 - amac with macrophages under confocal laser microscope and analysis the fluorescence intensity by flow cytometer using the cell quest software
在激光掃描共聚焦顯微鏡下觀察2 -氨基吖啶酮標記殼寡糖與巨噬細胞的結合,用流式細胞儀分析熒光強度。After treatment with bfa, immunoflurescence labeling and confocal laser scanning microscopy indicated that the cytoplasmic dynein intermediate chain - like protein in lily pollen tube was insensitive to bfa treating, but spectrin - like protein was sensitive to it under the same condition
用bfa處理百合花粉管后,通過免疫熒光標記及激光共聚焦掃描顯微鏡觀察發現類細胞質力蛋白中間鏈對bfa不敏感;同樣的處理發現類紅膜肽對bfa敏感。In this paper, wheat cultivars lovrin 10 ( resistant ) and 5389 ( susceptible ) were selected as materials in this system. the mesophyll protoplasts of wheats ( mpw ) were isolated using cellulase and pectolase digestion. by the indirect immune fluorescent labeling, microtubules ( mts ) pattern in mpw were showed clearly under the confocal laser scanning microscope ( clsm )
本試驗以抗(洛夫林10 ) 、感( 5389 )不同的兩小麥( triticumaestivuml . )品種為材料,採用酶解法制備小麥葉肉原生質體,利用間接免疫熒光方法結合激光共聚焦掃描顯微技術對小麥葉肉細胞原生質體的微管骨架進行了清晰的標記,並探索了微管骨架標記的影響因素。Twophoton laser scanning fluorescence microscopy and its applications
雙光子激光掃描熒光顯微鏡及其應用At that time, cytosolic fluorescence intensity decreased to normal level, which shows that most of cells get through the gl / s point and enter the log phase. when cultured in medium that neucl was omitted, most of the cells were synchronized at gl stage of cell cycle. with flow cytometry, we found that cytosolic cam content of gl cells was higher than that of normal cells at log stage
在激光掃描共聚焦顯微鏡下觀察不同周期時相裂殖酵母細胞中cam的濃度及分佈變化,結果表明,分裂期細胞總體熒光強度強于間期細胞;而對同一細胞內熒光強度的分析說明,間期細胞的熒光主要分佈於胞質中,細胞核內則分佈較少;而正在進行有絲分裂的細胞內熒光主要集中於赤道板處;剛完成有絲分裂的細胞內熒光則相對集中於兩端或其中的一端。Polarized microscopy, sem - eds, xrf, uv - vis, pl, ftir, epr have been used in this study to investigate two chameleon diamonds and a synthetic diamond which show color - change effects
摘要對具有變色效應的兩顆變色龍金剛石與一顆鮮黃色合成金剛石進行了掃描電鏡能譜、 x射線熒光光譜、顯微紅外光譜、紫外可見吸收光譜、光致發光譜、電子順磁共振譜等測試研究,以探討引起金剛石變色的原因。Part i this paper has minutely studied the interaction between ag ( i ) and serum albumin. the binding of ag ( i ) to human serum albumin ( hsa ) or bovine serum albumin ( bsa ) has been studied by equilibrium dialysis at ph ( 5. 4 ). the scatchard analysis indicates that there exists several strong binding sites of ag ( i ) in both hsa and bsa. a notable hysteretic effect has been observed in the interaction of ag ( i ) with hsa or bsa using uv - visible spectrometry at ph ( 5. 4 ), which shows that the binding between ag ( i ) with hsa or bsa may induce a slow transition of hsa or bsa from the conformation of weaker affinity for ag ( i ) to one of stronger affinity ( a - b transition ). the rate constants and activation parameters of this transition parameters of this tansition were measured and discussed. the binding equilibrium has been also studied by resonance light - scattering spectrum ( rls ) and flurescence quenching
第一部分:等離子點ph ( 5 . 4 )條件下,用平衡透析法和紫外光譜,熒光光譜,共振散射光譜研究了ag ( )與人血清白蛋白( humanserumalbumin ,簡稱hsa )或牛血清白蛋白( bovineserumalbumin ,簡稱bsa )的結合。 scatchard圖分析表明, ag ( )在hsa或bsa中有強弱兩類結合部位,通過計算機擬合獲得結合的逐級穩定常數值。紫外掃描發現ag ( )與hsa或bsa的結合存在滯後效應,表明ag ( )與hsa或bsa的結合可能誘導蛋白質構象發生緩慢變化( a - b ) ,測得並討論了這一構象變化的速度常數和活化參數。Sections were stained by he and were observed under light microscope. ( 4 ) observation on cell - matrix complex with confocal microscope. cell - matrix complex was stained by fluorochrome cfda - am ( loug / ml, looul ) after 7 days incubation, the sample was scanned by confocal microscope to observe cell - growth in the matrix
細胞一多孔膜復合物的激光共聚焦顯微鏡觀察:取培養7天的細胞一多孔膜復合物,以10ug inl的熒光染料cfad am100ul染色,檄光共聚焦顯微鏡檢測激光激發的綠色熒光,掃描成像觀察活細胞生長倩況。Laser scanning confocal microscope combined with fluorescence probe and fluorescence resonance energy transfer techniques has become a very effective tool of researching the behavior of massive molecules in living cells
摘要激光掃描共聚焦顯微鏡結合熒光探針以及熒光共振能量轉移技術,已成為近年來應用在活細胞中研究大分子行為的一種非常有效的研究工具。H2o2 generation in guard cells was examined by laser scanning confocal microscopy based on fluorescence probe h2dcfda. the fluorescence intensity in guard cells of wild type and ios5 was essentially the same before treatment
以h2o2熒光探針h2dcfda結合激光掃描共聚焦顯微技術直接檢測了保衛細胞內的h2o2產生情況。未加任何處理之前,野生型與los5保衛細胞內熒光強度幾乎相等。A 30 u 1 sample of a 34mm solution of amac and loou 1 of a l. om solution of nabh3cn were added
沖洗后在激光掃描共聚焦顯微鏡下觀察實驗組和對照組巨噬細胞的熒光強弱差異。After flushing the fluorescence intensity difference between treatment group and control group was observed under fluorescence microscope
沖洗后激光掃描共聚焦顯微鏡下觀察實驗組和對照組巨噬細胞的熒光強弱的差異。分享友人