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A convenient HPLC assay for the determination of fructosamine-3-kinase activity in erythrocytes

机译:方便的HPLC测定法测定红细胞中的果糖胺-3-激酶活性

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Fructosamine-3-kinase (FN3K) mediates the regeneration of lysine from fructosamines formed on proteins as a result of the ‘early’ Maillard reaction. As fructosamines and advanced glycation endproducts derived therefrom are supposed to play an adverse role in the development of diabetic complications, FN3K is discussed as a protein-repairing enzyme. In this study, a method for the determination of FN3K activity in erythrocyte lysate is described which overcomes the complexity of currently known assays. The assay is based on the FN3K-dependent conversion of the synthetic UV-active fructosamine N α-hippuryl-N ε-(1-deoxy-D-fructosyl)lysine (BzGFruK) to N α-hippuryl-N ε-(phosphofructosyl)lysine (BzGpFruK). The FN3K activity was quantified by measuring the formation of BzGpFruK using RP-HPLC with UV detection. Identification of the metabolite BzGpFruK was achieved by means of UV and mass spectroscopy. The results are related to the content of haemoglobin for standardisation. First activity measurements with a chosen number of normoglycaemic subjects confirmed the convenient applicability of the method and showed distinctly different individual activities, as already discovered recently. The new established assay needs only the equipment of a routine laboratory with HPLC instrumentation. This should facilitate further studies about a possible relationship between the FN3K activity and the development of diabetic complications.
机译:果糖胺3激酶(FN3K)介导了蛋白质的果糖胺中赖氨酸的再生,而果糖胺是“早期”美拉德反应的结果。由于果糖胺和由其衍生的高级糖基化终产物在糖尿病并发症的发生中起着不利的作用,因此人们将FN3K作为一种蛋白质修复酶进行了讨论。在这项研究中,描述了一种确定红细胞裂解物中FN3K活性的方法,该方法克服了目前已知测定方法的复杂性。该测定基于FN3K依赖性,将合成的UV活性果糖胺Nα-尿嘧啶-Nε-(1-脱氧-D-果糖基)赖氨酸(BzGFruK)转化为Nα< / sup> -hippuryl-Nε-(磷酸果糖基)赖氨酸(BzGpFruK)。 FN3K活性通过使用RP-HPLC和UV检测测量BzGpFruK的形成来定量。代谢物BzGpFruK的鉴定是通过UV和质谱法完成的。结果与血红蛋白含量有关。如最近已经发现的,对一定数量的正常血糖受试者进行的首次活动测量证实了该方法的便利性,并且显示出明显不同的个体活动。新建立的测定方法仅需要配备HPLC仪器的常规实验室的设备。这应有助于进一步研究FN3K活性与糖尿病并发症发生之间的可能关系。

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