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In Vivo Brain Glucose Measurements: Differential Normal Pulse Voltammetry with Enzyme-Modified Carbon Fiber Microelectrodes

机译:体内大脑葡萄糖测量:酶修饰的碳纤维微电极的差分正常脉冲伏安法。

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The enzyme glucose oxidase was immobilized on the surface of carbon fiber microeleetrodes (CFMEs) either by cross-linking in glutaraldehyde vapor or by enzyme entrapment in electropolymerized films of m-phenylene-diamine or resorcinol. The cross-linked enzymatic layer was, in the given conditions, covered with an additional membrane of Nafion or cellulose acetate. The prepared glucose sensors Were tested using differential normal pulse voltammetry (DNPV, in which the scan comprises successive doublepulses ("prepulse and pulse"), the prepulses are of increasing amplitude, and the current measured is the differential of the current existing between each prepulse and pulse). With properly chosen DNPV parameters, the response to glucose presented a peak at a potential of about 1 V versus an Ag/AgCl reference, owing to the oxidation of enzymatically produced hydrogen peroxide. The calibration curves obtained (peak height/glucose concentration) were linear from 0.3-0.5 up to 1.5-6.5 mM and showed a sensitivity ranging from 1.4 up to 34.5 mA M~(-1) cm~(-2), depending on the sensor type. The DNPV response to glucose exhibited an essential insensitivity toward easily oxidizable interfering substances such as ascorbic acid and acetaminophen present at physiological concentrations. Pep-tides, the interfering species typical of the cerebral medium, were effectively retained by the above additional membranes. Concentration values of glucose in plasma and cerebrospinal fluid, determined in vitro from the DNPVpeak height, agreed well with those measured by standard procedures. In the anesthetized rat, extracellular brain concentration of glucose was also monitored during administration of either insulin or glucagon. Under such pharmacological conditions, thechanges observed in the peak height were in perfect agreement with the known effects induced by both substances.
机译:通过戊二醛蒸汽中的交联或酶夹在间苯二胺或间苯二酚的电聚合膜中,将葡萄糖氧化酶固定在碳纤维微电极(CFME)的表面上。在给定条件下,交联的酶促层被Nafion或乙酸纤维素的附加膜覆盖。使用差分正常脉冲伏安法(DNPV)对准备的葡萄糖传感器进行测试,其中扫描包括连续的双脉冲(“预脉冲和脉冲”),预脉冲的振幅不断增大,测得的电流是每个预脉冲之间存在的电流的差和脉冲)。使用适当选择的DNPV参数,由于酶促产生的过氧化氢的氧化,对葡萄糖的响应相对于Ag / AgCl参比在约1 V的电位处出现一个峰值。所获得的校准曲线(峰高/​​葡萄糖浓度)在0.3-0.5 mM至1.5-6.5 mM之间呈线性,并且显示的灵敏度范围从1.4 mC至(34.5 mA)M〜(-1)cm〜(-2),具体取决于传感器类型。 DNPV对葡萄糖的反应对以生理浓度存在的易氧化的干扰物质(例如抗坏血酸和对乙酰氨基酚)表现出基本的不敏感性。潮汐是大脑介质的典型干扰物质,可通过上述附加膜有效保留。从DNPVpeak高度体外测定的血浆和脑脊液中葡萄糖的浓度值与标准程序测得的值非常吻合。在麻醉的大鼠中,在胰岛素或胰高血糖素给药期间还监测了细胞外葡萄糖的浓度。在这种药理条件下,观察到的峰高变化与这两种物质引起的已知效应完全吻合。

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