共查询到19条相似文献,搜索用时 125 毫秒
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以磁性壳聚糖作为载体,戊二醛作为交联剂,对乳酸脱氢酶(LDH)进行固定化.固定化的最适条件为:戊二醛浓度6%,pH值7.5,酶的偶联时间2 h.对游离及固定化LDH酶学性质的研究表明,酶促反应的最适pH值为9.2,最适温度分别为37℃和50℃,对乳酸的表观米氏常数分别为1.6 mmol/L和0.9 mmol/L.游离酶和固定化酶在40℃放置150 min后,其活力分别为最初的56.5%和76.1%.固定化酶在4℃贮存4周后,活力仍保留50%以上.固定化酶在室温下与底物重复反应6次后,活力仍保留60%以上,说明固定化酶具有较好的热稳定性、贮存稳定性和复用性. 相似文献
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基于丙酮酸/还原型辅酶I/乳酸脱氢酶(LDH)/乳酸/氧化型辅酶I荧光猝灭体系和荧光毛细管分析技术,建立了可用于微量样品中LDH酶活性测定的方法。优化的测定条件为:激发及发射波长分别为350和460nm;测定温度为25℃;酸度为pH 6.5;NADH浓度为300μmol/L;丙酮酸浓度为1.2mmol/L。本方法的测定范围为50~1500IU/L,检出限为30IU/L,相对标准偏差2.1%~2.2%(n=10),回收率在96.4%~105%范围内。本方法操作简单,每次测定仅需样品2.0μL、试剂18.0μL,分析速度约为30样/h,利用本方法测定了微量血清中LDH的活性。 相似文献
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以壳聚糖为载体对醇脱氢酶(ADH)和脲酶(UASE)进行固定化。固定化的最适条件:ADH和UASE的偶联时间分别为2.5h和1.5h,交联剂戊二醛浓度为0.6%和0.5%,偶联pH值为6.8和5.0。对游离酶及固定化酶的性质研究表明,ADH酶促反应的最适宜pH为8.0和8.4,最适宜温度为33℃和35℃,米氏常数为48mmol/L和13mmol/L;UASE酶促反应的最适宜pH均为7.0,最适宜温度为60℃和72℃,米氏常数为0.4mmol/L和2mmol/L。固定化酶与游离酶相比在复用性上具有优势,用固定化酶测定了试样中尿素含量以及模拟样中银离子含量。 相似文献
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乙酰鸟氨酸脱乙酰酶固定化细胞拆分D,L-缬氨酸 总被引:3,自引:1,他引:3
报道了一种利用具有乙酰鸟氨酸脱乙酰酶活性的固定化细胞拆分D,L-缬氨酸的新方法. 该酶促反应最适条件: pH=6, 反应温度50 ℃, 底物N-乙酰-D,L-缬氨酸浓度200 mmol/L, 固定化细胞用量0.2 g/mL(或100 U/mL). 0.1 mmol/L CoCl2条件对该酶促反应有显著的激活作用. 在以上条件下反应2~3 h, 测得产物L-缬氨酸浓度95 mmol/L. 该固定化细胞连续10次使用, 平均转化率为90.8%(以N-乙酰-L-缬氨酸计), 显示出了良好的工业化应用前景. 相似文献
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在荧光毛细分析法(FCA)的基础上开发了一种用于DNA快速检测的DNA-FCA法.在毛细管内表面将DNA探针固定化,制成荧光毛细生物反应器(DNA-CBR).测定时,用DNA-CBR吸入含Cy-5标记的靶DNA样品液进行杂交反应,然后在646 nm激发波长、664 nm发射波长下进行荧光测定;Cy-5标记的靶DNA浓度在0.1~1.0 μmol/L之间线性良好(y=139.73x+39.613,r=0.9985);RSD<5.5%;检出限为0.17 pmol,样品用量10 μL;DNA-CBR能够重复使用6次.本方法可用于靶DNA的定性和定量检测. 相似文献
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Diaphorase was immobilized covalently as a monolayer on a tin(IV) oxide electrode, and the diaphorase electrode thus obtained responded to NADH amperometrically in the presence of ferricyanide or 2,6-dichloroindophenol as the electron mediator. The response was one to two orders of magnitude larger than that of a bare electrode. Further derivatization of the diaphorase electrode with a dehydrogenase (glucose, lactate or alcohol dehydrogenase), which reduces NAD to NADH by reaction with the substrate, yielded dehydrogenase/diaphorase heterobilayer-modified electrodes. These electrodes functioned as sensors for the respective substrate with NAD and ferricyanide as the mediators. Each bilayer electrode responded to the substrate only in the presence of added NAD; this provides evidence for the essential contribution of diaphorase to the sensor performance. As much as 60 to 80% of the electron mediator reduced by the enzymatic reaction was utilized in the amperometric response. 相似文献
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微量乳酸脱氢酶毛细管电泳在线反应电化学检测方法的研究 总被引:5,自引:0,他引:5
以乳酸脱氢酶催化乳酸与NAD+反应生成丙酮酸与NADH和安培法检测NADH为基础,利用电泳中介微分析(EMMA)技术,研究了超微量乳酸脱氢酶的毛细管电泳在线反应的电化学检测方法,并从理论上对EMMA电泳图中的平台宽度和高度作了初步探讨.结果表明,在EMMA的恒高压和零高压两种模式下,使用直径为150μm和束状碳纤维电极,在+0.8V检测电位下,对LDH活性检测灵敏度分别为1.1nU和0.6nU;所导出的平台高度、宽度与实验条件的关系式对提高毛细管电泳分离效率和检测灵敏度有一定指导意义. 相似文献
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采用时间相关单光子计数技术, 结合紫外-可见吸收光谱和稳态荧光光谱, 对不同环境下的色氨酸和辅酶还原型烟酰胺腺嘌呤二核苷酸(NADH)之间的共振能量转移荧光动力学进行了研究. 单体色氨酸、 牛血清白蛋白以及乳酸脱氢酶蛋白与NADH之间相互作用的光谱数据表明, 只有存在NADH结合位点的乳酸脱氢酶和NADH之间发生了荧光共振能量转移. 进一步通过加入丙酮酸来阻断乳酸脱氢酶和NADH之间的荧光共振能量转移通道, 时间分辨荧光光谱和衰减相关光谱(DAS)证实, 蛋白结合位点的存在是NADH和色氨酸之间发生荧光共振能量转移的前提条件. DAS揭示了乳酸脱氢酶平均荧光寿命的减小主要是源于色氨酸中7.35 ns的荧光寿命成分与NADH之间的荧光共振能量转移, 同时给出了NADH和色氨酸之间的能量转移效率, 为研究NADH和蛋白之间的相互作用提供了新思路. 相似文献
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《Analytical letters》2012,45(7):1165-1175
Abstract An optical fibre probe based on glucose dehydrogenase immobilized on nylon was constructed. The probe was used to quantitate glucose through a measurement of the fluorescence of the NADH formed by the enzyme-catalyzed reduction of glucose in the presence of NAD. The probe response was reproducible and displayed good linearity in the concentration range of 1.1 to 11.0 mM glucose. The limit of detection was 0.6 mM glucose. The response was affected by pH and NAD concentration. 相似文献
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A method for determination of l-malate in wine is described. Malate dehydrogenase and oxaloacetate decarboxylase were immobilized on poly (vinyl alcohol) beads and incorporated in a flow-injection system with fluorescence detection. Sample solution (50 mul) was injected into the carrier stream [4mM NAD(+) in glycine buffer (pH 10.0)]. The fluorescence based on the NADH formed could be directly related to the amount of malate. The calibration graph was linear over the range 0.4-300muM. The detection limit was 0.2muM. Sampling throughout was 25 samples/hr. 相似文献
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Torabi F Ramanathan K Larsson PO Gorton L Svanberg K Okamoto Y Danielsson B Khayyami M 《Talanta》1999,50(4):787-797
An electrochemical method for the measurement of NAD(+) and NADH in normal and cancer tissues using flow injection analysis (FIA) is reported. Reticulated vitreous carbon (RVC) electrodes with entrapped l-lactate dehydrogenase (LDH) and a new redox polymer containing covalently bound toluidine blue O (TBO) were employed for this purpose. Both NAD(+) and NADH were estimated coulometrically based on their reaction with LDH. The latter was immobilized on controlled pore glass (CPG) by cross-linking with glutaraldehyde and packed within the RVC. The concentrations of NAD(+) and NADH in the tissues, estimated using different electron mediators such as ferricyanide (FCN), meldola blue (MB) and TBO have also been compared. The effects of flow rate, pH, applied potential (versus Ag/AgCl reference) and adsorption of the mediators have also been investigated. Based on the measurements of NAD(+) and NADH in normal and cancer tissues it has been concluded that the NADH concentration is lower, while the NAD(+) concentration is higher in cancer tissues. Amongst the electron mediators TBO was found to be a more stable mediator for such measurements. 相似文献
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A fluorescence high performance liquid chromatographic method using an immobilized 3 alpha-hydroxysteroid dehydrogenase column as a post-column enzymatic reactor was developed for the determination of corticosteroid metabolites in the urine of subjects with congenital adrenal hyperplasia. 3 alpha-Hydroxysteroids, such as pregnanetriol, pregnanediol and pregnanetriolone, in the eluate from mu-Bondapak phenyl column (300 x 3.9 mm I.D.) using 0.05% ammonium phosphate buffer (pH 7.1)-acetonitrile-methanol (100:55:15) as the mobile phase was mixed with NAD+ solution in the enzyme column at 30 degrees C to generate NADH, which was monitored by a fluorophotometric detector. Each steroid was measured at the 2.5 micrograms/dl at the highest sensitivity of the detector. The mean recoveries and reproducibilities were 91.5-108.2% with 0.9-6.5% (CV%). 相似文献
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A new method for the determination of lactic acid based on the immobilization enzyme fluorescence capillary analysis (IE-FCA) was proposed. Lactic dehydrogenase (LDH) was immobilized on inner surface of a capillary with glutaraldehyde, and an immobilized enzyme lactate capillary bioreactor (IE-LCBR) was formed for the determination of lactic acid. After nicotinamide adenine dinucleotide (NAD+) is mixed with lactic acid solution, it was sucked into the IE-LCBR and was detected at λex 353 nm/λem 466 nm. Optimized conditions are as follows: the temperature is 38 °C; the reaction time is 15 min; the concentrations of Tris buffer (pH 8.8) and NAD+ are 0.1 mol L−1 and 4 mmol L−1, respectively; the concentration of LDH used for immobilization is 15 kU L−1. The concentration of lactic acid is directly proportional to the fluorescence intensity measured from 0.50 to 2.0 mmol L−1; and the analytical recovery of added lactic acid was 99–105%. The minimum detection limit of the method is 0.40 mmol L−1 and sensitivity of the IE-CBR is 4.6 F mmol−1 L−1 lactate. Its relative standard deviation (R.S.D.) is ≤2.0%. This IE-FCA method was employed for determination of lactate in milk drink. 相似文献
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A novel fluorimetric method is described for the determination of ethanol by means of alcohol dehydrogenase immobilized on a stirrer. Ethanol is oxidized by alcohol dehydrogenase to aldehyde, with simultaneous conversion of NAD to NADH; the increase in fluorescence of NADH is measured at 465 nm (λex = 370 nm). The calibration curve is linear for ethanol concentrations up to . Deproteinization is required prior to the assay of blood samples; recoveries are 97–102.7%. Enzyme stability, reproducibility and selectivity are discussed. 相似文献