59 resultados para 867
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通过单克隆抗体制备技术得到三株特异结合半抗原 4 ( GSH-S-DNP二苄酯 )的单克隆抗体 HB4 ,HB5和 HB7.抗体经两步化学诱变得到具有细胞谷胱甘肽过氧化物酶 ( c GPX)活性的含硒抗体酶 m HB4 ,m HB5和 m HB7,活力分别为 1 70 ,1 867,32 U/μmol.其中 m HB5的活力是天然兔肝 c GPX的 0 .32倍 ,m 4 A4的1 .51倍 .等离子体 -质谱 ( ICP/MS)测得每分子含硒抗体酶分子中大约存在 2个硒原子 .m HB5的最适 p H为8.6~ 8.8.在 p H值范围为 7.0和 37℃条件下 ,m HB5催化 GSH和 H2 O2 或 t-ROOH反应的二级速率常数为 :k+ 1 ( H2 O2 ) 9.71× 1 0 6 L /( mol· min) ,k+ 1 ( t-ROOH) 5.99× 1 0 5 L/( mol· min) . m HB5使非酶催化反应速率提高了 9.8× 1 0 6和 3.7× 1 0 5倍.
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建立了麻醉镇痛药物的电子轰击/串联质谱分析方法,得到了电子轰击/串联质谱 (EI/MS/MS)条件下16种麻醉镇痛药物标准品的碰撞诱导解离(CID)-子离子谱,适合于复杂基质中这类化合物的定性分析。并利用所建方法对一肌注度冷丁者的尿样进行了检测。
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利用气相色谱-质谱联用技术对夜来香种子油中的脂肪酸(经甲酯化后)进行分离和定性,共鉴定出二十种脂肪酸。并用归一化法确定出各成分在夜来香种子油中的相对含量。对所得的结果进行了讨论。
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In this article, we report the rare earth ion selective electrodes developed in our laboratory. Rare earth containing functional copolymers, rare earth oxides, and chelates have been used as active materials. Methods for preparing raw materials, behavior of electrodes, and application of rare earth ion selective electrodes in flow injection analysis have been discussed as well.
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catena-Poly[{pentaaqua(L-proline-O)-erbium-mu-(L-proline-O:O')} trichloride], {[Er(C5H9-NO2)2(H2O)5]Cl3}n, M(r) = 594.0, monoclinic, P2(1), a = 8.294 (1), b = 10.981 (3), c = 11.934 (3) angstrom, beta = 107.04 (2)degrees, V = 1039.2 (4) angstrom3, Z = 2, D(x) = 1.90 g cm-3, lambda(Mo Kalpha) = 0.71069 angstrom, mu = 45.2 cm-1, F(000) = 586, T = 298 K, R = 0.0244 for 1711 unique reflections [I > 3 sigma(I(o))]. The crystal consists of one-dimensional chains of infinite length in which one L-proline ligand bridges two neighboring Er ions, the other L-proline ligand being monodentate.
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本文介绍用兰州化物所制备的Ag_2WO_4,MgO/AgVO_3催化剂分析含氟量很高的高分子化合物中的碳、氢的方法。该法的优点是快速、简便、燃烧温度低。测定的绝对误差不大于0.3%。 2 仪器和试剂: Carlo Erba 1106型元素分析仪,精度为lμg的天平,锡箔压制的样品小舟。Ag_2WO_4,MgO/AgVO_3兰州化物所制,镀银还原铜自制。氧气、氦气的纯度为99.999%。
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The surface structure of glassy carbon electrode subjected to "galvanostat" pretreat- ment and its electrocatalytic behaviour in the presence of ascorbic acid, catechol and hydroquinone were studied by means of cyclic voltammetry, chronoamperometry, chronocoulometry and scanning electron microscopy. The electrocatalytic mechanism was discussed, which was due to the adsorption and the catalysis of functional groups at the electrode surface. Three separated peaks from the mixture of catecnol, hydroq...
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用循环伏安法、计时电流法、计时库仑法和X射线先电子能谱法研究了恒电流法电化学预处理玻炭电极上的表面性质及其对抗坏血酸、儿茶酚和对苯二酚的电催化效应。讨论了电催化机理,证明电极表面吸附及表面功能团的催化是发生电催化的主要原因。儿茶酚、对苯二酚和抗坏血酸的混合物在预处理电极上的波峰明显分开,有可能应用于儿茶酚和抗坏血酸的同时测定。
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Recently, beta-thymosin-like proteins with multiple thymosin domains (defined as thymosin-repeated proteins) have been identified from invertebrate. In the present study, the cDNAs of two thymosin-repeated proteins (designated EsTRP1 and EsTRP2) were cloned from Chinese mitten crab by expressed sequence tags (EST) techniques. BLAST analysis presented three and two thymosin domains in EsTRP1 and EsTRP2, respectively, with the identities amongst the five domains varying from 47% to 100%. Both EsTRP1 and EsTRP2 shared high similarities with previously identified vertebrate beta-thynnosins and invertebrate thymosin-repeated proteins (TRPs) with the identities ranging from 43% to 78%, indicating that EsTRPs were new members of the beta-thymosin family. Real-time RT-PCR assay was adopted to determine the tissue distribution of EsTRPs and their temporal expression profile in hemocytes after pathogen stimulation and injury challenge. The expression of EsTRP1 transcript was predominantly detectable in the tissues of hemocytes, hepatopancreas and gonad with the highest expression in hemocytes, while the highest expression level of EsTRP2 was found in heart. EsTRP1 mRNA expression in hemocytes significantly increased at 3 and 48 h after Listonella anguillarum challenge, but there was no significant variation in EsTRP2 temporal expression profile. The injury challenge reduced the mRNA expression of EsTRPs, with the down-regulation of EsTRP2 expression occurred earlier than that of EsTRP1. The cDNA fragments encoding their mature peptides of EsTRP1 and EsTRP2 were recombined and expressed in Escherichia coli. The activities of recombinant proteins (rEsTRP1 and rEsTRP2) were examined by MTT (3-(4,5-dimethylthiazol-2-yl)-2, 5-diphenyltetrazoliumbromide) and lysoplate assay. rEsTRP2 could significantly accelerate the growth of human hepatocellular carcinoma cell line, but there was no significant effect of rEsTRP1 on the tumor cell proliferation. Both rEsTRP1 and rEsTRP2 did not possess the ability of killing Micrococcus luteus and L. anguillarum. The differences in the tissue distribution of mRNA transcripts, the response to pathogen stimulation and injury challenge, and the effect of recombinant proteins on human cell proliferation, indicated that there were functional diversity between the two structurally different molecules, EsTRP1 and EsTRP2. (C) 2009 Elsevier Ltd. All rights reserved.
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能量代谢指动物在进行生理活动(如摄食、消化以及动物的活动等)时所消耗能量的总和,一般以动物的呼吸率利排泄率来估计动物的能量代谢。其主要研究内容是闸明生物能量代谢的基木规律以及与环境闪子的关系。菲律宾蛤仔(Ruditapesphil ippmarum)是我国一种重要的养殖贝类,关于其能量代谢的研究却较少,这种状况妨碍了菲律宾蛤仔养殖生态理论的完善和养殖技术的提高。本研究主要对菲律宾蛤仔呼吸率和排泄率的基本规律(能量代谢与体重的关系、能量代谢的昼夜变化)及其与环境因子(饵料浓度、水温、栖息底质环境)的关系进行探讨。研究结果如下:1.不同体重菲律宾蛤仔代谢率小同。实验川菲律宾蛤仔分三种大小:l(干肉重为0.07-0.14g)、ll(干肉重0.27-0.34g)、III(干肉重0.45~0.63g)。温度包括:26℃(八月)、20℃(十月)、1 5℃(十二月)、9℃(一月)。实验共设四个饵料浓度:2.28±0.25,6.454±0.44,10.284±0.82,15.414±1.56mgTPM/L(TPM,总颗粒物),饵料中POM(颗粒有机物)含量都为4.68±1.64 mg/L。常温下菲律宾蛤仔代谢率随着体重的增大而增大。15℃、20~C、26℃时蛤仔呼吸率与干肉重呈明显的幂函数关系R=aW~b,a值变动范围为0.1076-0.3309;b值变动范围为0.239l~0.8381;蛤仔排泄率与干肉重也呈明显的幂函数关系N=aW~b,a值变动范围为14.213~68.362:b值变动范围为0.3673-1.1 532。9℃(饵料浓度为2.28±0.25mgTPM/L)、20℃(饵料浓度为10.284-0.82mgTPM/L)、26℃(饵料浓度为6.454±0.44mgTPM/L)时不同体重蛤仔氧氮比差异显著,其它情况下不同体重蛤仔氧氮比差异不显著。2.常温下菲律宾蛤仔代谢率受饵料浓度的影响,不同大小蛤仔受饵料浓度的影响程度不同。I组蛤仔呼吸率受饵料浓度的显著影响,II组III组蛤仔呼吸率只在9℃(一月)和26~C(八月)时受饵料浓度的显著影响。26℃时影响最显著,26℃时I组蛤仔在饵料浓度为2.28±0.25,6.45±0.44,l0.28±0.82,15.4l±1.56mgTPM/L时呼吸率分别是O.086,0.146,0.073,0.093(mlO_2/h);ll组蛤仔在上述浓度饵料中呼吸率分别是0.138,0.214,0.J 26,0.12l(mlO_2/h);III组蛤仔在上述浓度饵料中呼吸率分别是0.129,0.266,0.186,0.192(mlO_2/h)。菲律宾蛤仔呼吸率在饵料浓度为6.45±0.44 mgTPM/L时最高,蛤仔呼吸率在其它饵料浓度时都会降低。菲律宾蛤仔排泄率在饵料浓度为10.28±0.82 mgTPM/L和15.4l士1.56mgTPM/L时显著高于其它浓度组,9℃时这种趋势更明显,9℃时饵料浓度为2.28±0.25,6.454±044,lO.284±0.82,15.41±1.56mgTPM/L中I组蛤仔排泄率分别是4.297,2.874,8.003,6.658(μgNH_3-N/h);II组蛤仔在上述浓度饵料中排泄率分别是4.011,3.609,10.427,12.732(μgNH_3-N/h);III组蛤仔在上述浓度饵料中排泄率分别是2.28 l,6.452,10.283,15.417(μgNH_3-N/h)。3.菲律宾蛤仔代谢率受自然温度的显著影Ⅱ向。I组蛤仔在9℃、15℃、20℃、26℃时呼吸率平均为0.057,0.085,0.039,O.099;II组蛤仔在上述四个温度中呼吸率平均为0.08,O.128,0.089,0.149(mlO_2/h),I组和II组蛤仔在9℃和20~C时呼吸率较低,在26℃时呼吸率最高。III组蛤仔在上述四个温度中呼吸率平均为0.09,O.1 59,O.143,O.193(mlO_2/h),在9℃时llI组蛤仔呼吸率显著低于其它温度组。温度为9℃、15℃、20℃、26℃时l组蛤仔排泄率平均为5.458,13.169,4.946,11.138(μgNH_3-N/h):II组蛤仔在上述温度中排泄率平均为7.695,23.578,8.319,23.90l(μgNH_3-N/h);III组蛤仔在上述温度中排泄率平均为11.738,27.443,15.658,35.407(μgNH_3-N/h),蛤仔排泄率在15℃和26℃时均高于9℃和20℃。4.摄食状态与饥饿状态菲律宾蛤仔代谢率有明显不同。26℃时蛤仔静止状态呼吸率平均为0.336(m102/g干重.h),摄食状态呼吸率平均为0.656(ml0_2干重.h),摄食状态呼吸率比静止状态平均升高了0 32(ml0_2/g干重.h);26℃时蛤仔静止状态排泄率平均为39.471(μgNH_3-N/g干重.h),摄食状态排泄率平均为88.08(μgNH_3-N/g干重.h),摄食状态排泄率比静止状态排泄率平均升高了48.6(μgNH_3-N/g干重.h)。摄食状态代谢率平均是静止状态的2~3倍。根据摄食引起的呼吸率和排泄率升高量得出每氧化产生lμgNH_3-N需0_2量平均为7.05μl。5.人工控制温度对菲律宾蛤仔代谢率有明显影响。不同大小蛤仔受温度的影响程度不同。在温度5℃、10℃、l 5℃、20℃、26℃,I组和II组蛤仔呼吸率都随着温度的升高而升高,在10℃~l5℃和20℃~26℃这二个温度变化范围内呼吸率变化最大,在20℃~26℃时I组蛤仔呼吸率变动范围为O.85~1.04(m10_2/g干重.h)、II组蛤仔变动范围为0.57~0.86(ml0_2/g干重.h)。III组蛤仔呼吸率只在5℃~l0℃时明显增高,变动范围为0.09~0.5l(m10_2/g干重.h),在10℃~26℃范围内变化不大。I组和II组蛤仔排泄率随着温度的升高而升高,变动幅度较大,在5℃~26℃范围内其排泄率变动范围为10.32~81.53(μgNH_3-N/g干重.h);而 III组蛤仔排泄率只在5℃~15℃时随着温度的升高而升高,其排泄率变动范围为6.75~23.77(μgNH_3-N/g干重.h),在15℃~26℃范围内几乎不变。III组蛤仔的适温范围比I组和II组蛤仔广。菲律宾蛤仔在5℃和10℃时氧氮比变化明显,变动范围为2.76~11.44,在15~26℃时变化不大。6.菲律宾蛤仔代谢率有明显的日节律性,呈正弦曲线型变化。蛤仔夜问代谢率明显升高。I组蛤仔夜间呼吸率平均为0.867(m10_2/g干重.h),白天呼吸率平均为O.504(m10_2/g干重.h);II组蛤仔夜间呼吸率平均为0.438(m10_2/g干重.h),白天呼吸率平均为0.36l(m102/g干重.h);III组蛤仔夜间呼吸率平均为0.409(m10_2/g干重.h),白天呼吸率平均为0.252(m102/g干重.h)。在22:00-23:00菲律宾蛤仔呼吸率最高。7.底质环境对菲律宾蛤仔的代谢率有明显影响。在饥饿状态下菲律宾蛤仔在泥沙底质中呼吸率平均为l 406(m10_2/g干重h),在无泥沙环境中呼吸率平均为O.963(ml0_2/g干重.h);摄食状态下菲律宾蛤仔在泥沙底质中呼吸率平均为1.59l(m102/g干重.h),在无泥沙环境中呼吸率平均为1.115(m10_2/g干重.h)。在饥饿状态下菲律宾蛤仔在泥沙底质中排泄率平均为78.934(μgNH_3-N/g 干重.h),在无泥沙环境巾排泄率平均为45.043(μgNH_3-N/g干重.h);摄食状态下菲律宾蛤仔在泥沙底质中排泄率平均为87.12l(μgNH_3-N/g干重.h),在无泥沙底质中排泄率平均为58.354(μgNH_3-N/g干重.h)。蛤仔在泥沙环境中呼吸率和排泄率都明显升高。
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首次记载了毛冠菊属 2种 4居群的核形态资料。两种植物的染色体间期和前期染色体为复杂型和中间型。狭舌毛冠菊两居群的染色体数目与核型公式为 2n =1 8=1 4m + 2sm + 2st( 2SAT) ;毛冠菊两居群的染色体数目与核型公式为 2n =1 8=1 4m + 2sm( 2SAT) + 2st。它们分别代表了整个毛冠菊属的两组植物 ,并包含了形态学上最原始的种类 ,因此 ,该属的染色体基数可能为x =9。核形态证据表明毛冠菊属放在紫菀族比放在旋覆花族和千里光族中更为合理。
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主要从岩石学,矿物学,岩石分类,C,O,Sr同位素,碳酸岩与矿化的关系等各方面对(碱性)碳酸岩的研究进行了较为全面的总结,并结合近20年来实验岩石等,流体包裹体研究,CO2^- H2O-NaCl流体体系的性质的研究,对碳酸岩岩浆的来源及成因,岩浆-热液的演化进行了分析和探讨,碳酸岩形成至少经历了三个阶段,即岩浆阶段,岩浆期后阶段(气相碳酸岩/岩浆热液阶段),交代碳酸岩阶段,而作为与碳酸岩在空间和成因上有密切联系的基性,超基性岩,碱性岩杂岩体,则经历了碳酸岩成岩阶段以前的岩浆不混熔作用,结晶分异作用,岩浆结晶作用以及碳酸岩形成之后的围岩蚀变(霓长岩化)作用.
