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采用气相色谱-串联质谱法快速定量检测昆虫保幼激素及其生物合成途径中的中间产物。

A rapid quantitative assay for juvenile hormones and intermediates in the biosynthetic pathway using gas chromatography tandem mass spectrometry.

机构信息

School of Chemical and Environmental Engineering, Shanghai Institute of Technology, Shanghai, 201418, PR China.

School of Chemical and Environmental Engineering, Shanghai Institute of Technology, Shanghai, 201418, PR China; Institute of Agro-Food Standards and Testing Technologies, Shanghai Academy of Agricultural Science, Shanghai, 201403, PR China.

出版信息

J Chromatogr A. 2018 Feb 23;1538:67-74. doi: 10.1016/j.chroma.2018.01.030. Epub 2018 Jan 18.

Abstract

A method for rapid quantitation of insect juvenile hormones (JH) and intermediates in the biosynthetic pathway, both in vitro and in vivo (hemolymph and whole body), has been developed using GC-MS/MS. This method is as simple as the radiochemical assay (RCA), the most commonly used method for measurement of JH biosynthesis in vitro, without need for further purification and derivatization, or radioactive precursors or ligands. It shows high sensitivity, accuracy and reproducibility. Linear responses were obtained the range of 1-800 ng/mL (approximately 4-3000 nM). Recovery efficiencies for farnesol, farnesal, methyl farnesoate and JH III were approximately 100% in vitro and over 90% in vivo, with excellent reproducibility at three different spike levels. Titer of JH III in the hemolymph was relatively low at day 0 (adult female emergence) (79.68 ± 5.03 ng/mL) but increased to a maximum of 1717 ng/mL five days later. In whole body, JH III quantity reached a maximum on day 4 (845.5 ± 87.9 ng/g) and day 5 (679.7 ± 164.6 ng/g) and declined rapidly thereafter. It is in agreement with the hemolymph titer changes and biosynthetic rate of JH in vitro. Comparison with the results of inhibition of JH biosynthesis by two known inhibitors (allatostatin (AST) mimic H17 and pitavastatin) using RCA and GC-MS/MS, showed that there was little difference between the two methods In contrast to other methods, the present method with GC-MS/MS can be used to elucidate the mechanism of inhibition by inhibitors of JH biosynthesis without any derivatization and purification. This method is applicable to screening of JH inhibitors and the study of inhibitory mechanisms with high sensitivity and accurate quantification. It may also be useful for the determination of JH titer in other Arthropods.

摘要

一种用于快速定量昆虫保幼激素(JH)及其生物合成途径中的中间产物的方法,无论是在体外还是体内(血淋巴和整个机体),均已通过 GC-MS/MS 建立。该方法与最常用于体外测量 JH 生物合成的放射性化学测定法(RCA)一样简单,无需进一步纯化和衍生化,也无需放射性前体或配体。它具有高灵敏度、准确性和重现性。在线性范围内,其范围为 1-800ng/mL(约 4-3000nM)。法呢醇、法呢醛、甲基法呢酯和 JH III 的体外回收率约为 100%,体内回收率超过 90%,在三个不同的加标水平具有出色的重现性。血淋巴中 JH III 的含量在第 0 天(成虫雌虫出现)相对较低(79.68±5.03ng/mL),但 5 天后增加到 1717ng/mL 的最大值。在整个机体中,JH III 的含量在第 4 天(845.5±87.9ng/g)和第 5 天(679.7±164.6ng/g)达到最大值,此后迅速下降。这与血淋巴中的含量变化和体外 JH 的生物合成速率一致。与 RCA 和 GC-MS/MS 两种已知的 JH 生物合成抑制剂(保幼激素激动素(AST)模拟物 H17 和匹伐他汀)的抑制作用的结果进行比较,表明两种方法之间几乎没有差异。与其他方法相比,本方法使用 GC-MS/MS 可以在无需衍生化和纯化的情况下阐明抑制剂对 JH 生物合成的抑制机制。该方法适用于高灵敏度和准确定量筛选 JH 抑制剂和研究抑制机制。它也可能对其他节肢动物中 JH 含量的测定有用。

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