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ATPase inhibitor based luciferase assay for prolonged and enhanced ATP pool measurement as an efficient fish freshness indicator

机译:基于ATPase抑制剂的荧光素酶测定法可延长和增强ATP池的测量,作为有效的鱼类新鲜度指标

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摘要

The nucleotide degradation pathway in somatic cells leads to the accumulation of products such as hypoxanthine and inosine, which are commonly used as fish and meat freshness indicators. Assays based on these molecules cannot differentiate the postmortem time over a short period of time (5–10 h). Further, quantification of these degradation products is cumbersome, costly and time-consuming. For the proposed assay, optimal concentrations of 30 and 2 mM, respectively, for the ATPase inhibitors sodium orthovanadate and EDTA were found. Further, it was observed that a firefly luciferase based assay could enhance the sensitivity levels up to 165-fold at 30 °C. In addition, it was observed that the sensitivity for ATP assay was enhanced up to 60-fold even after 12 h. The limit of detection for the ATP assay was 1 pM, unlike other conventional methods, which are sensitive only up to micromolar levels. Moreover, as little as 0.044 g fish fillet was required for the assay, and no time-consuming sample preparation was necessary. Luminescence of prolonged duration was observed in harvested fish kept at -20 °C in comparison with fish kept at 4 and 30 °C, which reflects the shelf life of fish preserved at lower temperatures.
机译:体细胞中的核苷酸降解途径导致次黄嘌呤和肌苷等产物的积累,这些产物通常用作鱼类和肉类的新鲜指标。基于这些分子的分析无法在短时间内(5-10小时)区分死后时间。此外,这些降解产物的定量是麻烦的,昂贵的和费时的。对于拟议的测定,发现ATPase抑制剂原钒酸钠和EDTA的最佳浓度分别为30和2 mM。此外,已观察到基于萤火虫荧光素酶的测定法可将灵敏度水平在30°C下提高至165倍。此外,观察到即使在12 h后,ATP测定的灵敏度也提高了60倍。 ATP测定的检测限为1 pM,这与其他常规方法不同,后者仅对微摩尔水平敏感。而且,该测定仅需要0.044 g鱼片,并且不需要耗时的样品制备。与保持在4和30°C的鱼相比,保持在-20°C的鱼的发光时间延长。这反映了低温保存的鱼的保质期。

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