幫忙翻譯一段英語(yǔ)

粵du社長(zhǎng)嘔 2008-02-19 03:32:04 529 瀏覽

Plant material and culture conditions have been described (7). Briefly， a diploid tissue culture line， WOO1C， of wild carrot， Daucus carota L.， was maintained in Murashige and Skoog medium supplemented with 0.1 mg of 2，4-dichlorophenoxy... Plant material and culture conditions have been described (7). Briefly， a diploid tissue culture line， WOO1C， of wild carrot， Daucus carota L.， was maintained in Murashige and Skoog medium supplemented with 0.1 mg of 2，4-dichlorophenoxyacetic acid (2，4-D). To regenerate plants from the culture， callus tissue was transferred to the same medium devoid of 2，4-D (embryogenic medium). All experiments were performed with cultures grown in liquid medium. For convenience， cultures grown in 2，4-D-containing medium are referred to as "callus cultures"， and those grown in medium without 2，4-D as "embryo cultures." The growth of callus cultures was measured by the sidearmturbidity method (7). The number of cells at any time point of growth was estimated from turbidity in a Klett-Summerson calorimeter and was expressed in arbitrary units. For example， Klett 100 corresponds to ="2 X 106 cells per ml. The relationship is linear up to Klett 150 in our Klett-Summerson colorimeter. Suspension cultures ofWOOLC cell line are normally maintained at cell densities between 106 and 107 cells per ml in 0.1 mg of 2，4-D per liter (high-density culture) in shake flasks. During a quantitative study on embryogenesis， we found that maximal embryo production can be achieved by first incubating the culture at high density in medium without 2，4-D for one generation time and then diluting it to 2-3 x 104 cells per ml (low-density culture). To compare cultures of comparable density， callus cultures and embryo cultures were subjected to the same procedure. To initiate low-density embryo or callus cultures， an 8-day-old high-density culture grown at the logarithmic phase was washed three times with fresh callus or embryogenic medium and resuspended at 8 x 105 cells per ml for one generation (3 days) in its corresponding medium. It was then diluted to 2 x 104 cells per ml; 20 ml of the culture was incubated in a plastic Petri dish (9 cm in diameter) at 240C. The morphogenetic events of the cultures were examined and photographed under a dissecting microscope. 請(qǐng)不要用google的那個(gè)，我看不懂~~ 展開

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fsq9264543 2008-03-02 00:00:00

quite professional

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新北方極地1 2008-02-20 00:00:00

植物材料與文化條件已被描述（ 7 ）。簡(jiǎn)單來(lái)說(shuō)，二倍體組織文化線， woo1c ，野生蘿卜，胡蘿卜，是保持murashige和skoog培養(yǎng)基用0.1毫克的2，4 -二氯苯氧乙酸（ 2，4 -四）。再生植物從文化，愈傷組織被移送到同一個(gè)中等空洞2，4三維（胚中等）。所有實(shí)驗(yàn)均與文化成長(zhǎng)在液體中等。為方便起見(jiàn)，文化的成長(zhǎng)，在2，4三維含中等稱為"愈傷組織培養(yǎng)" ，而那些成長(zhǎng) 在培養(yǎng)基2，4三維"胚胎文化" 。生長(zhǎng)愈傷組織培養(yǎng)，是衡量該sidearmturbidity 法（ 7 ）。細(xì)胞數(shù)量在任何時(shí)間點(diǎn) 增長(zhǎng)估計(jì)從濁度在klett -薩默森熱量表，并有人表示，在任意單位。舉例來(lái)說(shuō)， klett 100對(duì)應(yīng)= " 2 × 106細(xì)胞每毫升。關(guān)系是直線上升，以klett 150我們klett -薩默森色。懸浮培養(yǎng)ofwoolc細(xì)胞系通常保持在細(xì)胞密度之間的106和107細(xì)胞每毫升0.1 毫克的2，4三維每公升（高密度文化），在搖瓶。在定量研究胚胎發(fā)生后，我們發(fā)現(xiàn) Z大的胚胎生產(chǎn)，可以取得diyi孵化文化，在高密度的媒體2，4三維1 一代人的時(shí)間，然后再稀釋至2-3 x 104個(gè)細(xì)胞中每毫升（低密度文化）。比較文化比較的密度，愈傷組織培養(yǎng)及胚胎文化遭到了同樣的程序。發(fā)起低密度胚或愈傷組織培養(yǎng)，為期8天的歲高密度培養(yǎng)的速度增長(zhǎng)，對(duì)數(shù) diyi階段被沖至3倍，與新鮮愈傷組織或胚中型及懸浮于8 × 105個(gè)細(xì)胞每毫升1 一代人（ 3天）在其相應(yīng)的媒介。當(dāng)時(shí) 稀釋至2 × 104個(gè)細(xì)胞，每毫升， 20毫升的文化孵育在一個(gè)塑料皮氏培養(yǎng)皿（ 9公分），在240c 。該形態(tài)發(fā)生的事件，其文化的人進(jìn)行檢查和拍照根據(jù)解剖顯微鏡

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幫忙翻譯一段英語(yǔ): Plant material and culture conditions have been described (7). Briefly， a diploid tissue culture line， WOO1C， of wild carrot， Daucus carota L.， was maintained in Murashige and Skoog medium supplemented with 0.1 mg of 2，4-dichlorophenoxy... Plant material and culture conditions have been described (7). Briefly， a diploid tissue culture line， WOO1C， of wild carrot， Daucus carota L.， was maintained in Murashige and Skoog medium supplemented with 0.1 mg of 2，4-dichlorophenoxyacetic acid (2，4-D). To regenerate plants from the culture， callus tissue was transferred to the same medium devoid of 2，4-D (embryogenic medium). All experiments were performed with cultures grown in liquid medium. For convenience， cultures grown in 2，4-D-containing medium are referred to as "callus cultures"， and those grown in medium without 2，4-D as "embryo cultures." The growth of callus cultures was measured by the sidearmturbidity method (7). The number of cells at any time point of growth was estimated from turbidity in a Klett-Summerson calorimeter and was expressed in arbitrary units. For example， Klett 100 corresponds to ="2 X 106 cells per ml. The relationship is linear up to Klett 150 in our Klett-Summerson colorimeter. Suspension cultures ofWOOLC cell line are normally maintained at cell densities between 106 and 107 cells per ml in 0.1 mg of 2，4-D per liter (high-density culture) in shake flasks. During a quantitative study on embryogenesis， we found that maximal embryo production can be achieved by first incubating the culture at high density in medium without 2，4-D for one generation time and then diluting it to 2-3 x 104 cells per ml (low-density culture). To compare cultures of comparable density， callus cultures and embryo cultures were subjected to the same procedure. To initiate low-density embryo or callus cultures， an 8-day-old high-density culture grown at the logarithmic phase was washed three times with fresh callus or embryogenic medium and resuspended at 8 x 105 cells per ml for one generation (3 days) in its corresponding medium. It was then diluted to 2 x 104 cells per ml; 20 ml of the culture was incubated in a plastic Petri dish (9 cm in diameter) at 240C. The morphogenetic events of the cultures were examined and photographed under a dissecting microscope. 請(qǐng)不要用google的那個(gè)，我看不懂~~ 展開

英語(yǔ)高手幫忙翻譯一下: ThequalitysystemofthecompanyisinconformitywithISO9002.Makingcomprehensiveuseofbiotechnology，thecompanyspecializesinmanufacturingandsellingC-4seriesorganicacidsandchiralpr... The quality system of the company is in conformity with ISO 9002 . Making comprehensive use ofbiotechnology， the company specializes in manufacturing and selling C-4series organic acids and chiral products. These products are widely used in many fields such as food， phamaceutical and chemical industries， and are well accepted by the overseas markets. The man products are L-Malic acid ， DL-Malic acid， L(+)-Tartaric acid ， Fumaric acid， Maleic acid and other organic acids. Annual productivity amounts to 20，000 tones. The company has become an important manufacturer of C-4 series organic acids in the world . All the products of the company have respectively met the different international aadvanced standards such as Food chemicals Codex， U.S. Pharmacopoeia ，British Pharmacopoeia and the products have obtained Star-K Kosher certificate. Above 70% of the Companys products are exported to Japan， Europe， Australias， the United states and middle East ， and they are renown and well recognized in the international markets. The company will devote itself to research and development of enzyme technology and organic electrochemistry. It will continuously introduce new food additives， chiral pharmaceutical intermediates， chiral auxiliaries and chiral drugs. Depending on superior quality， good service and high reputation， the company is willing to establish a long-term mutually beneficial business partnership with overseas customers and continue contribute to the happy life of humans. 展開

請(qǐng)翻譯一段簡(jiǎn)單的英語(yǔ)（務(wù)必準(zhǔn)確）: 用翻儀器的走遠(yuǎn)！Thetissueishomogenizedwithchloroform/methanol(2/1)toafinalvolume20timesthevolumeofthetissuesample(1gin20mlofsolventmixture).Afterdispersion，thewholemixtur... 用翻儀器的走遠(yuǎn)！ The tissue is homogenized with chloroform/methanol (2/1) to a final volume 20 times the volume of the tissue sample (1 g in 20 ml of solvent mixture). After dispersion， the whole mixture is agitated during 15-20 min in an orbital shaker at room temperature. The homogenate is either filtrated (funnel with a folded filter paper) or centrifuged to recover the liquid phase. The solvent is washed with 0.2 volume (4 ml for 20 ml) of water or better 0.9% NaCl solution. After vortexing some seconds， the mixture is centrifuged at low speed (2000 rpm) to separate the two phases. Remove the upper phase by siphoning and kept it to analyze gangliosides or small organic polar molecules. If necessary (need of removing labelled molecules...)， rinse the interface one or two times with methanol/water (1/1) without mixing the whole preparation. After centrifugation and siphoning of the upper phase， the lower chloroform phase containing lipids is evaporated under vacuum in a rotary evaporator or under a nitrogen stream if the volume is under 2-3 ml. 展開

求助：幫忙幫忙，機(jī)械英語(yǔ)NB的幫忙翻譯下: The effect of beam diameter on the electron skirt in a high pressure scanning electron microscope R. Belkorissata， A. Kadouna， B. Khelifab， C. Mathieub，* aLaboratoire d’Elaboration et de Caracte′risation des Mate′riaux， Univ... The effect of beam diameter on the electron skirt in a high pressure scanning electron microscope R. Belkorissata， A. Kadouna， B. Khelifab， C. Mathieub，* aLaboratoire d’Elaboration et de Caracte′risation des Mate′riaux， Universite′ Djilali Liabe`s de Sidi Bel-Abbes， BP 89， 22000 Sidi Bel-Abbe`s， Algeria bCentre de Calcul et de Mode′lisation de Lens， University D’Artois， Faculte′ Jean Perrin， SP 18 Rue Jean Souvraz， 62307 Lens cedex， France Received 9 February 2004; accepted 19 March 2004 Abstract Helium gas and air are commonly used in the high pressure scanning electron microscope (HPSEM). The presence of a gaseous environment in the specimen chamber modifies the electron beam profile. In order to fully understand the beam-gas interaction， we have investigated the beam-diameter effect for two gases (helium and air) by Monte Carlo simulation. In this calculation， we have assumed that the electron beam is Gaussian and we have explored the influence of the nature of the gas at low voltage. When the beam diameter varies between 1 and 100 nm， there is no influence on the beam profile for these two gases. The resolving power of the HPSEM is not affected by the beamgas interaction. These theoretical results have been compared with experimental images obtained at low voltage under air and helium gases. The variation of image quality at low voltage has confirmed the interest of helium for use in a Field Emission Gun SEM (FEGSEM) in high pressure (or low vacuum) conditions. q 2004 Elsevier Ltd. All rights reserved. Keywords: High pressure scanning electron microscope; Monte Carlo; Electron scattering; Electron profile; Skirting 展開

英語(yǔ)高手幫忙翻譯段英文謝謝?。?: In this paper， the degradation of an azo dye Orange G (OG) on nitrogen-doped TiO2 photocatalysts has been investigated under visible light and sunlight irradiation. Under visible light irradiation， the doped TiO2 nanocatalysts demonstrated ... In this paper， the degradation of an azo dye Orange G (OG) on nitrogen-doped TiO2 photocatalysts has been investigated under visible light and sunlight irradiation. Under visible light irradiation， the doped TiO2 nanocatalysts demonstrated higher activity than the commercial Dugussa P25 TiO2， allowing more ef?cient utilization of solar light， while under sunlight， P25 showed higher photocatalytic activity. According to the X-ray diffraction (XRD)， X-ray photoelectron spectroscopy (XPS) and UV–vis spectra analyses， it was found that both the nanosized anatase structure and the appearance of new absorption band in the visible region caused by nitrogen doping were responsible for the signi?cant enhancement of OG degradation under visible light. In addition， the photosensitized oxidation mechanism originated from OG itself was also considered contributing to the higher visible-light-induced degradation ef?ciency. The effect of the initial pH of the solution and the dosage of hydrogen peroxide under different light sources was also investigated. Under visible light and sunlight， the optimal solution pH was both 2.0， while the optimal dosage of H2O2 was 5.0 and 15.0 mmol/l， respectively. Azodyes， which are characterized by the presence of one or more azo bonds ( N N )， are among the most notorious widespread environmental pollutants associated with textile，cosmetic， food colorants， printing， and pharmaceutical indus-tries. Because of their non-degradability， toxicity， potential mutagenicity and carcinogenicity， wastewaters originating from these dyes production or application industries pose a major threat to the surrounding ecosystems and human beings’ health.[1–3].Environmental concerns and the need of meeting the strin-gent international standards for rejecting wastewaters has made the development of novel and cost-effective processes for the puri?cation of azo dyes ef?uents an issue of major technological importance. 展開

幫忙翻譯一哈文章（翻譯成英語(yǔ)）: 摘要本文采用環(huán)氧氯丙烷、乙二胺、對(duì)氨基苯磺酸等物質(zhì)合成了一種新的活性染料耐氯水牢度提升劑，并對(duì)經(jīng)多種類型活性染料染色的織物進(jìn)行固色處理，再進(jìn)行氯漂處理。經(jīng)過(guò)對(duì)織物K/S值、Z大吸收波長(zhǎng)λmax、摩擦牢度及皂洗牢度的分析，確定提升劑處理的Z佳工... 摘要本文采用環(huán)氧氯丙烷、乙二胺、對(duì)氨基苯磺酸等物質(zhì)合成了一種新的活性染料耐氯水牢度提升劑，并對(duì)經(jīng)多種類型活性染料染色的織物進(jìn)行固色處理，再進(jìn)行氯漂處理。經(jīng)過(guò)對(duì)織物K/S值、Z大吸收波長(zhǎng)λmax、摩擦牢度及皂洗牢度的分析，確定提升劑處理的Z佳工藝。實(shí)驗(yàn)表明:織物的K/S值有很大的提高，織物的耐氯牢度大致可提升2～3級(jí)，并且不會(huì)改變織物色光。但是提升劑對(duì)色織物的摩擦牢度和皂洗牢度影響不是很大。關(guān)鍵詞：活性染料；耐氯色牢度；提升劑；染色工藝展開

請(qǐng)教英語(yǔ)高人，幫忙翻譯一下．急用，謝謝?。。?: Theelementalcontentofrawmaterials，phosphogypsum，substrate(potassiumsalt)，products(superphosphateand“Amofoska”)，soil，andgrasswasdeterminedusingconventionalandepithermaln... The elemental content of raw materials， phosphogypsum， substrate (potassium salt)， products (superphosphate and “Amofoska”)， soil， and grass was determined using conventional and epithermal neutron activation analysis using the IBR-2 pulsed fast reactor at Frank Laboratory of Neutron Physics (FLNP)， Joint Institute for Nuclear Research (JINR)， Dubna， Russia. The analytical procedure was described elsewhere by Frontasyeva and Pavlov [15]. Quality control was based on the application of certified reference materials (CRMs): IAEA-336 (lichens)， IAEA-SDM (lake sediment) and IAEA-SL1 (soil). The certified values and the results obtained by NAA were compared (Table 2). Concentrations of most elements were in good agreement with the CRMs except for Ti， Ni， Ce， Eu， Dy and Rb， which differed from the certified value as follows: Ti - 41.7 %， Ni - 26.5 %， Ce - 24.3 %， Eu - 32.9 % and Dy - 33.3 % in IAEA-SL1 (soil) and Rb - 20.6 % in IAEA-336 (lichens). For the 21 elements in agreement with the certified values the bias observed was below 20 %. For 11 elements (Al， V， Mn， As， Br， Sc， Cr， Sm， Na， Co and Sb)， the bias ranged from 0.03 % to 5 %， for 5 elements (Fe， Zn， Ba， Th and Cs) the bias was greater than 5 % but lower than 10 %， and for 5 elements (La， Tb， Hf， Ta and U) the bias was determined to be between 10 % and 20 %. Samples of raw materials， phosphogypsum， substrate， products， soil (of about 0.1 g)， and grass (0.3 g) were irradiated in cadmium-screened channels 1 and 2 of the pneumatic “Regata” system described elsewhere by Frontasyeva and Pavlov [15]. In order to determine elements associated with long-lived radionuclides， samples were irradiated for 100 hours. Spectra of induced gamma activity were recorded after 4 and 20-24 days of cooling. Short irradiations， 5 minutes for grass samples and 60 seconds for the remaining samples， allowed determination of Al， Ca， Cl， I， K， Na， Mg， Mn， Ti and V. Gamma-ray spectra were recorded after 5 and 12 minutes after irradiation. Data processing was performed using software developed at FLNP JINR [16， 17]. All gamma-spectrometers and counting electronics were made at JINR [16]. The software developed at FLNP JINR for peak searching， peak fitting， and nuclide identification routines were used for processing the amplitude spectra [16]. In the case of the lack of analytical data， there was a half of the detection limit inserted for each analyte [18]. Principal component analysis (classical PCA and fuzzy PCA) was performed as a tool for searching the possible correlations between environmental and industrial samples that could implicate the impact of phosphatic fertilizer production on the environment adjacent to the plant. 請(qǐng)給一個(gè)比較能看懂的翻譯，謝謝. 展開

幫忙翻譯一下化工方面的單詞英語(yǔ): 堿值測(cè)定器試劑移液管錐形瓶酸式滴定管甲基黃溴甲酚綠混合指示劑鹽酸標(biāo)準(zhǔn)溶液摩爾/升酸式滴定管... 堿值測(cè)定器試劑移液管錐形瓶酸式滴定管甲基黃溴甲酚綠混合指示劑鹽酸標(biāo)準(zhǔn)溶液摩爾/升酸式滴定管展開

幫忙翻譯下化工的英語(yǔ)。。用在線詞典翻譯部正確: A reversed-phase ion-pairing high-performance liquid chromatography (RP-HPIPC) method for the separation of a complex mixture of heparin-derived oligosacchrides has been developed by a stepwise optimization of the mobile phase， in which the... A reversed-phase ion-pairing high-performance liquid chromatography (RP-HPIPC) method for the separation of a complex mixture of heparin-derived oligosacchrides has been developed by a stepwise optimization of the mobile phase， in which the concentration of ion-pairing reagent， mobile phase pH， and acetonitrile concentration were varied. The resolution of more than 30 oligosaccharide components was obtained， under optimized conditions， in an analysis time of less than 30 min. This represents the first RP-HPLC method that can separate a complex mixture of both small and large sulfated oligosaccharides in a single chromatographic step. The heparin-derived oligosaccharides， in this mixture， can also be separated under a second set of RP-HPIPC conditions using a volatile ion-pairing reagent， tributylammonium acetate， to aid in the recovery of individual sulfated oligosaccharides. Moreover， it was possible to replace sodium chloride gradient， required for eluting highly sulfated oligosaccharides， with a fixed， low concentration of a volatile salt， ammonium acetate， by utilizing an acetonitrile gradient. This solvent system might make it possible to directly interface this RP-HPIPC separation with mass spectral analysis. ??2003 Elsevier B.V. All rights reserved. Keywords: Ion-pairing reagents; Gradient elution; Oligosaccharides 展開

幫忙翻譯: AttachingtheSampleChuckYouwillneeda#2Phillipsscrewdriverforthisstep.FollowingthedetailsshowninFig.2-4，installthesamplechuckbyfirstaligningthepinsonthebottomofthesamplechu... Attaching the Sample Chuck You will need a #2 Phillips screwdriver for this step. Following the details shown in Fig. 2-4， install the sample chuck by first aligning the pins on the bottom of the sample chuck with the receptacles on the alpha- SE base. Then tighten the upper two captive thumb screws. Next， use the Phillips screwdriver to tighten the lower two captive screws. Don’t over tighten the screws! It will make it difficult to remove them in the future; just ensure that the screws are snug. Finally， connect the vacuum line from the sample chuck to the vacuum fitting on the alpha-SE base. Releasing the Z-stage Shipping Lock To access the Z-stage shipping lock， first loosen the captive screw on the lamp/shipping lock access door， then open the access door by rotating 180°， as shown in Fig. 2-5. To release the Z-stage shipping lock， stand in front of the ellipsometer and use your left hand to balance the weight of the Z-stage (you will feel it lift up slightly). It will be difficult to release the shipping lock if you apply too much or not enough upward force. Next， use your right hand to move the shipping lock to the operating position (to the right， see Fig. 2-6). If the lock is hard to move， you can use a tool to gain more leverage. The shipping lock will move about 1/3” [8mm] to the right. Checking the Lamp Check that the QTH lamp in fully seated in the lamp housing. The lamp is located behind the actuator screw (see Fig. 2-6) and has two white wires protruding from the back of the lamp. Simply push down on the lamp ensuring that the lamp is fully seated in the lamp housing. Rotate the lamp/shipping lock access door to the closed position and hand tighten the captive screw. 拒絕翻譯軟件，翻譯軟件我自己也會(huì)用不是用翻譯軟件我就看不懂，只是，上來(lái)找人翻譯就是希望翻譯出比較容易看懂，不需要自己對(duì)照就可以看的說(shuō)明書，如果用翻譯軟件，根本就詞不達(dá)意，還是要自己對(duì)著原文件核實(shí) 既然用了那么多積分，就希望有相當(dāng)?shù)某晒绻梅g軟件混積分，那就是人品問(wèn)題了還有，某些人不要不懂亂說(shuō)混積分展開

麻煩哪位英語(yǔ)牛人幫忙翻譯下~~藥學(xué)的翻譯成英語(yǔ) 謝謝了: 目的制備足浴液并對(duì)其進(jìn)行質(zhì)量考察。方法采用正交試驗(yàn)優(yōu)選苦參中苦參堿和紫草中紫草素的提取工藝，通過(guò)紫外分光光度法對(duì)苦參堿與紫草素的含量進(jìn)行測(cè)定，并將苦參堿、紫草素、水楊酸、苯甲酸和硼酸按一定比例進(jìn)行溶解實(shí)驗(yàn)?；瘜W(xué)成分分析采用薄層色譜法及試管... 目的制備足浴液并對(duì)其進(jìn)行質(zhì)量考察。方法采用正交試驗(yàn)優(yōu)選苦參中苦參堿和紫草中紫草素的提取工藝，通過(guò)紫外分光光度法對(duì)苦參堿與紫草素的含量進(jìn)行測(cè)定，并將苦參堿、紫草素、水楊酸、苯甲酸和硼酸按一定比例進(jìn)行溶解實(shí)驗(yàn)。化學(xué)成分分析采用薄層色譜法及試管實(shí)驗(yàn)法對(duì)苦參中苦參堿與紫草中紫草素進(jìn)行化學(xué)成分檢測(cè)。結(jié)果通過(guò)薄層色譜法和試管實(shí)驗(yàn)法得出苦參堿為生物堿、紫草素為蒽醌。通過(guò)正交試驗(yàn)和紫外分光光度法選出Z優(yōu)提取方案。通過(guò)溶解實(shí)驗(yàn)使中化學(xué)藥物形成混懸液，Z后得到足浴液樣品。結(jié)論通過(guò)T濃度實(shí)驗(yàn)，溶解實(shí)驗(yàn)選用95%乙醇為溶媒。通過(guò)L9(33)正交實(shí)驗(yàn)確定Z佳提取工藝，即提取時(shí)間為30min，溫度為60℃，乙醇濃度為60%，以苦參堿作對(duì)照品，用分光光度法測(cè)定其苦參堿得率3.07%。經(jīng)過(guò)實(shí)驗(yàn)摸索，得到超聲提取紫草工藝的Z佳條件，即乙醇濃度為70%，超聲功率為400w，料液比為1：40時(shí)提取率較高。足浴液制備方法簡(jiǎn)便，有利于實(shí)際生產(chǎn)，降低能源、節(jié)約時(shí)間，有較大的開發(fā)利用價(jià)值和廣泛的市場(chǎng)前景。關(guān)鍵字：紫草；苦參；正交設(shè)計(jì)；薄層色譜展開

英語(yǔ)課文翻譯: Ifyouhadtochoosethesinglemostimportantdiscoveryofthe20thcentury，youwouldhavearealdilemmaonyourhands.Injust100years，theworldchangedcompletely.Amazingdiscoveriesweremadeinm... If you had to choose the single most important discovery of the 20th century， you would have a real dilemma on your hands. In just 100 years， the world changed completely. Amazing discoveries were made in medicine， communications and transport， not to mention our knowledge of the world and space . Medical advances ranged from discovering the causes of diseased under microscopes to surgical procedures replacing diseased organs with donated ones.Communications changed with the introduction of mobile phones and the way we correspond went from writing letters to emailing. We started flying around the world and meanwhile， scientists figured out how to spilt the atom， previously thought to be the smallest particle of matter in the universe. Although it is impossible to choose the most important discovery， it is possible to single out a few pioneers of the 20th century.Here are five of them. 展開

想請(qǐng)有理工科背景的英文強(qiáng)人幫忙翻譯一段英文信件！: The support module's APD bias has come factory set for an APD multiplication gain between 10 and 20. The APD bias monitor via the BNC connector is provided as a way to check the bias and adjust it as desired. You do not need to have... The support module's APD bias has come factory set for an APD multiplication gain between 10 and 20. The APD bias monitor via the BNC connector is provided as a way to check the bias and adjust it as desired. You do not need to have the APD bias monitored while the module is in operation， but it is good idea to double check its value at least intermittently. A simple voltmeter can be used to check the bias， and any BNC type connection and cabling should work fine. The specifications sheet has a chart showing the APD's DC current and gain versus it bias， as well as a table listing the bias at M=10 and M=20. While a current-limiter in the support module protects from damaging the APD， you must keep the APD bias below breakdown to prevent a noisy output. The SMA outputs are designed for 50-Ohm coax cabling. Since your receiver has 300 MHz output filters most cabling should work fine. Higher frequency RF or microwave rated cabling is not required. Closely matching cable length for the two outputs is required when you are terminating the two outputs differentially， otherwise when using single ended outputs ensure that both outputs are terminated similarly. In terms of the support module's ground， it should be provided through the power supply's IEC connector to a safety earth. For signal integrity the receiver's outputs should be grounded through the SMA coax cabling to whatever instrument you are using read the output， i.e. oscilloscope or counter. The ground plug is an optional ground connected directly to the outputs' SMA coax ground， but it is not required for operation. I am also attaching an electronic copy of the specifications and operations sheets if more copies of it are needed. 展開

求專業(yè)的英語(yǔ)達(dá)人幫忙翻譯下萬(wàn)分感謝: Caution:Do not place your finger over the vent(it pressurizes the sensor) to test the flow indicator when gas is flowing to the sensor.removing your finger (the restriction) generates a vacuum on the sensor and maydamage the sensor(voiding ... Caution:Do not place your finger over the vent(it pressurizes the sensor) to test the flow indicator when gas is flowing to the sensor.removing your finger (the restriction) generates a vacuum on the sensor and maydamage the sensor(voiding the sensor warraty). Positive pressure applications: If the sample pressure is greater than 30 psign an external pressure regulator(optional) is required upsteram of the analyzer to control of sample flow.a pressure regulator with a metallic diaphragm is recommended to prevent high oxygen reading that cuold result from the use of diaphragms constructed of more gas permeable materisls. If other optionoal sample system components such as coiled metal tubing(samples must be colled to at least 35-40℃ for continuous use)，coalescing filters ，scrubbers，etc.are required install the pressure rugulator after the coiled tubing and bofore the other components and the analyzer.a scrubber requires a flow valve upstream for optimum efficiency and response time and that the analyzer flow valve is opened completely. Atmospheric or slightly negative pressure applications: For accurate high ppb and/or low ppm range measurements，an optional simple pump is required downstream of the analyzer to draw the sample through the analyzer.The cacuum drawn on the analyzer and sensor should not exceed 4”of water. Caution:Use ofpump downstream of the sensor requires the floe control valve upstream of the sensor be completely opened to avoid drawing ercessive vacuum in the sensor，which can damage the sensor. If pump over-loading(due to the limitation of low flow rate of the sample gas)is a comsideration，a second throttle valve on the pump’s inlet side may be necessary to provide a bypass path，as illustrated below，to prevent the pump from over-loading and over-heating while miantaining the required sample flow rate within the above-mentioned parameters 展開

幫忙翻譯一句話: Catalysts were prepared by pore volume impregnation of ?-alumina

幫忙翻譯2: 3.6. Advantages of chromia as promoter in copper-based Catalysts It should also be noted from Figs. 5 and 6 that in the steam reforming reaction to produce hydrogen for fuel cell applications， trace quantities (<0.4 wt.%) of Cr2O3 on Cu... 3.6. Advantages of chromia as promoter in copper-based Catalysts It should also be noted from Figs. 5 and 6 that in the steam reforming reaction to produce hydrogen for fuel cell applications， trace quantities (<0.4 wt.%) of Cr2O3 on Cu not only doubled the activity for the MSR but also halved the amount of CO formed， thereby enhancing H2 production. This improved selectivity reduces the problem of H2 separation from the reaction products in fuel cell applications. An important finding in this research is the role that very small amounts of Cr2O3 play in all the reactions investigated， namely， methanol synthesis， water gas shift and methanol steam reforming. In commercial co-precipitatedcopper-based methanol synthesis catalysts， copper is known to be the active component [3]. More recently， it has becomeestablished that ZnO promotes methanol synthesis and that surface species formed by Cu-ZnO interaction are responsible for methanol synthesis [42]. The role of Cr2O3 in commercial catalysts is thought to be similar to that of Al2O3， which is to act as stabilizer of the structure of the copper catalyst， thereby reducing sintering. In this study， as in a previous one [18] using a different technique todeposit chromia on the surface of skeletal copper， we have shown that Cr2O3 has a significant role in copper-based methanol synthesis from CO2. That role is to improve the methanol yield by reducing the RWGS reaction (Fig. 3) aswas observed in the earlier study [18]. A major finding of this study has been the very strong evidence the Cr2O3 has a synergistic effect on the activity of copper for methanol synthesis， methanol steam reforming and the water gas shift reactions. From Figs. 4 and 5 it can be seen that 0.85 wt.% Cr2O3 enhances the specific activity (mol/hm2 Cu) of skeletal copper 270% for the WGS and 150% for methanol steam reforming. In the case of methanol synthesis (Fig. 2) 0.61 wt.% Cr2O3 increases the specific activity of copper by 67%. The results for the WGS and MS reactions are similar to those obtained under the same reaction conditions using skeletal copper promoted by Cr2O3 which was deposited from sodium chromate in the caustic leach liquor [28]. In that study， the effect of chromia was more pronounced， with an increase in activity of 950% for theWGSand 168% for the MSR reaction， respectively， using skeletal copper containing 0.75 wt.% Cr2O3. For methanol synthesis over Cr2O3 promoted skeletal copperprepared using sodium chromate in the leach liquor， Ma et al. [18] observed no increase in the specific activity of copper. 展開

幫忙翻譯成英語(yǔ): 1.掌握量熱裝置的基本組合及電熱補(bǔ)償法測(cè)定熱效應(yīng)的基本原理2.用電熱補(bǔ)償法測(cè)定KNO3或KCL在不同濃度水溶液中的積分溶解熱3.用作圖法求KNO3或KCL在水中的微分沖淡，積分沖淡熱和微分溶... 1.掌握量熱裝置的基本組合及電熱補(bǔ)償法測(cè)定熱效應(yīng)的基本原理 2.用電熱補(bǔ)償法測(cè)定KNO3或KCL在不同濃度水溶液中的積分溶解熱 3.用作圖法求KNO3或KCL在水中的微分沖淡，積分沖淡熱和微分溶解熱還有：1。測(cè)定蔗糖轉(zhuǎn)化的反應(yīng)速率常數(shù)和半衰期 2.掌握旋光儀的使用方法不要用翻譯網(wǎng)站翻啊······麻煩各位了展開

有英語(yǔ)高手或者會(huì)labview的高手幫忙翻譯下: LabVIEW就是基于虛擬儀器的開發(fā)環(huán)境，本文闡述了基于虛擬儀器技術(shù)在阻抗參數(shù)測(cè)量中的應(yīng)用，根據(jù)電子測(cè)量的基本原理、計(jì)算方法和流程，利用了LabVIEW的特有語(yǔ)言—G語(yǔ)言—對(duì)被測(cè)對(duì)象進(jìn)行... LabVIEW就是基于虛擬儀器的開發(fā)環(huán)境，本文闡述了基于虛擬儀器技術(shù)在阻抗參數(shù)測(cè)量中的應(yīng)用，根據(jù)電子測(cè)量的基本原理、計(jì)算方法和流程，利用了LabVIEW的特有語(yǔ)言—G語(yǔ)言—對(duì)被測(cè)對(duì)象進(jìn)行程序編譯、運(yùn)行、修改并Z終顯示運(yùn)行結(jié)果有高手幫忙翻譯下展開

文章繼續(xù)求翻譯1，生物/英語(yǔ)達(dá)人來(lái)幫忙！: Residues of malachite green (MG) were extracted from homogenized animal tissues with a mixture of McIlvaine buffer (pH 3.0)–acetonitrile， and purified over an aromatic sulfonic acid solid-phase extraction column followed by ... Residues of malachite green (MG) were extracted from homogenized animal tissues with a mixture of McIlvaine buffer (pH 3.0)–acetonitrile， and purified over an aromatic sulfonic acid solid-phase extraction column followed by HPLC or LC–ESI-MS–MS analysis. Ascorbic acid and N，N，N9，N9-tetramethyl-1，4-phenylenediamine dihydrochloride were added to reduce de-methylation of the dye. Responses were recorded at 620 nm (HPLC) or by multiple-reaction-monitoring (LC–MS–MS) after post-column oxidation using PbO2 . MG and its primary metabolite leuco-malachite green (LMG) were successfully determined at 2.5–2000 mg / kg in catfish， eel， rainbow trout， salmon， tropical prawns and turbot， with a limit of detection at 1 mg / kg (HPLC) and 0.2 mg / kg (LC–MS–MS) for both MG and LMG. Recoveries for LMG were between 86±15% (prawn) and 105±14% (eel). Freeze–thawing cycles， and storage at 4°C and -20°C affected the recovery of both MG and LMG. Analyses of eel， trout and (processed) salmon field samples collected at local retailers， fish-market and -shops demonstrated trace levels of MG-residues. A McIlvaine solution at pH 3.0 was prepared by mixing 18.9 ml 0.2 M sodium hydrogen phosphate and 81.1 ml 0.1 M citric acid， whereas these volumes were 62.5 and 37.5 ml， respectively， to obtain a McIlvaine solution at pH 6.0. The SPE-eluent was prepared just before use and consisted of a mixture of 2.5 ml 25% (m/v) ammonium hydroxide， 2.5 ml 1.0 mg/ml methanolic ascorbic acid and 45 ml methanol. The sample-solvent was composed， just before use， from 2.5 ml 1.0 mg/ml methanolic ascorbic acid， 20 ml 50 mM sodium perchlorate containing 25 mM sodium acetate and 25 mM 1-pentanesulfonic acid adjusted to pH 4.0 with acetic acid， and 27.5 ml acetonitrile. Chemicals and solutions containing the dyes were protected from light. Fish were bought at the fish market and local stores. Blank trout were collected from aquaria at Utrecht University (The Netherlands). Tropical prawns were collected by the Dutch Inspectorate for Health Protection and Veterinary Public Health. 展開

急求英語(yǔ)達(dá)人幫忙翻譯段文章，在線等謝謝: The incorporation of silicon from the quartz-made growth chamber， characteristic of NIRIM-type reactor is insignificant in our samples， if any. The peak at 1.681 eV from the Si–V defect is totally absent from our films (not shown here)， wh... The incorporation of silicon from the quartz-made growth chamber， characteristic of NIRIM-type reactor is insignificant in our samples， if any. The peak at 1.681 eV from the Si–V defect is totally absent from our films (not shown here)， which supports the good quality of these films. The improvement of the crystalline quality of {111} films is explained by the weak ion bombardment of the sample during its growth outside the plasma ball. Raman measurements (not shown in this work) have also confirmed the high crystalline quality of our films， in particular in the low doping range. Very high boron concentrations (up to 5×1021 cm?3) have been reached at this growth position， outside the plasma ball. 展開

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