首页> 美国卫生研究院文献>Frontiers in Endocrinology >Assay of Endogenous 35-diiodo-L-thyronine (35-T2) and 33′-diiodo-L-thyronine (33′-T2) in Human Serum: A Feasibility Study
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Assay of Endogenous 35-diiodo-L-thyronine (35-T2) and 33′-diiodo-L-thyronine (33′-T2) in Human Serum: A Feasibility Study

机译:人血清中内源性35-二碘-L-甲状腺素(35-T2)和33-二碘-L-甲状腺素(33-T2)的测定:可行性研究

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摘要

3,5-diiodo-L-thyronine (3,5-T2) is an endogenous derivative of thyroid hormone with potential metabolic effects. It has been detected in human blood by immunological methods, but a reliable assay based on mass spectrometry (MS), which is now regarded as the gold standard in clinical chemistry, is not available yet. Therefore, we aimed at developing a novel ad-hoc optimized method to quantitate 3,5-T2 and its isomers by MS in human serum. Serum samples were obtained from 28 healthy subjects. Two ml of serum were deproteinized with acetonitrile and then subjected to an optimized solid phase extraction-based procedure. To lower background noise, the samples were furtherly cleaned by hexane washing and acetonitrile precipitation of residual proteins. 3,5-T2 and its isomers 3,3′-T2 and 3′,5′-T2 were then analyzed by HPLC coupled to tandem MS. Accuracy and precision for T2 assay were 88–104% and 95–97%, respectively. Recovery and matrix effect averaged 78% and +8%, respectively. 3,5-T2 was detected in all samples and its concentration averaged (mean ± SEM) 41 ± 5 pg/ml, i.e., 78 ± 9 pmol/l. In the same samples the concentration of 3,3′-T2 averaged 133±15 pg/ml, i.e., 253±29 pmol/l, while 3′,5′-T2 was not detected. 3,5-T2 concentration was significantly related to 3,3′-T2 concentration (r = 0.540, P < 0.01), while no significant correlation was observed with either T3 or T4 in a subset of patients in which these hormones were assayed. In conclusion, our method is able to quantify 3,5-T2 and 3,3′-T2 in human serum. Their concentrations lie in the subnanomolar range, and a significant correlation was detected between these two metabolites in healthy individuals.
机译:3,5-二碘-L-甲状腺素(3,5-T2)是甲状腺激素的内源性衍生物,具有潜在的代谢作用。已经通过免疫学方法在人血中检测到了它,但是基于质谱(MS)的可靠测定法(目前被认为是临床化学中的金标准)尚不可用。因此,我们旨在开发一种新型的临时优化方法,以通过MS在人血清中定量3,5-T2及其异构体。从28名健康受试者获得血清样品。用乙腈使2 ml血清脱蛋白,然后进行基于固相萃取的优化程序。为了降低背景噪音,通过己烷洗涤和残留蛋白质的乙腈沉淀进一步清洁样品。然后通过与串联质谱联用的HPLC分析3,5-T2及其异构体3,3'-T2和3',5'-T2。 T2分析的准确度和精密度分别为88–104%和95–97%。回收率和基质效应分别平均为78%和+ 8%。在所有样品中均检测到3,5-T2,其平均浓度为41±5 pg / ml(平均值±SEM),即78±9 pmol / l。在相同样品中,3,3'-T2的平均浓度为133±15 pg / ml,即253±29 pmol / l,而未检测到3',5'-T2。 3,5-T2浓度与3,3'-T2浓度显着相关(r = 0.540,P <0.01),而在分析了这些激素的一部分患者中,与T3或T4均未发现显着相关性。总之,我们的方法能够定量检测人血清中的3,5-T2和3,3'-T2。它们的浓度在亚纳摩尔范围内,并且在健康个体中这两种代谢物之间检测到显着相关性。

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