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通过一种新的 LC-MS/MS 方法提高干血斑中视黄醇的长期稳定性及其水平的定量。

Improving long-term stability of retinol in dried blood spots and quantification of its levels via a novel LC-MS/MS method.

机构信息

Beijing Municipal Key Laboratory of Child Development and Nutriomics, Capital Institute of Pediatrics, Beijing, 100020, China.

Department of Biochemistry and Immunology, Capital Institute of Pediatrics, Beijing, 100020, China.

出版信息

Anal Bioanal Chem. 2019 Dec;411(30):8073-8080. doi: 10.1007/s00216-019-02183-5. Epub 2019 Nov 25.

Abstract

Vitamin A deficiency (VAD) is a major micronutrient deficiency in children. Although plasma and serum retinol levels are proposed as the key indicators of VAD, collecting and transporting plasma and serum are difficult and inconvenient in field studies. Dried blood spot (DBS) retinol has been used as an alternative to plasma retinol in several epidemiological and clinical studies. A limitation of methods that use DBS retinol is the instability and apparent loss of retinol in DBSs. Therefore, an accurate, reliable method for stabilizing retinol in DBSs and quantifying and comparing DBS retinol concentrations with equivalent plasma retinol levels is required. In this study, antioxidants on paper combined with vacuum treatment were found to greatly increase the stability of DBS retinol during 120 min of air drying and 30 days of room-temperature storage. A surrogate matrix of whole blood prepared using a mixture of human erythrocytes and 2% BSA in PBS was firstly used in DBS retinol determination based on the fact that retinol is excluded from erythrocytes. The method was linear in the concentration range of 0.04-300 μg/mL. Both the between-run (n = 5) and within-run (n = 6) precision (relative standard deviations, RSD%) were below 8.42%. The spiked recoveries at 3 concentrations ranged from 86.48 to 98.13%. The internal standard (IS)-normalized matrix factor (MF) was 99.72% with a RSD% of 10.50% (n = 3). The accuracy was calibrated using two National Institute of Standards and Technology (NIST) serum-generated calibrants at concentrations of 0.1962 and 0.3948 g/mL, and relative errors (RE% values) of 0.07% and 4.95% were found, respectively. A simple calibration model was first developed to convert DBS retinol concentration to the equivalent plasma retinol concentration, thereby enabling comparisons with clinical reference ranges and with studies using serum or plasma samples. Graphical abstract.

摘要

维生素 A 缺乏症(VAD)是儿童中一种主要的微量营养素缺乏症。虽然血浆和血清视黄醇水平被提议作为 VAD 的关键指标,但在现场研究中收集和运输血浆和血清是困难和不方便的。干血斑(DBS)视黄醇已在几项流行病学和临床研究中被用作血浆视黄醇的替代品。使用 DBS 视黄醇的方法的一个限制是 DBS 中视黄醇的不稳定性和明显损失。因此,需要一种准确、可靠的方法来稳定 DBS 中的视黄醇,并定量和比较 DBS 视黄醇浓度与等效血浆视黄醇水平。在这项研究中,发现与抗氧化剂结合的纸张与真空处理相结合,可以大大提高 DBS 视黄醇在 120 分钟空气干燥和 30 天室温储存过程中的稳定性。首先,根据视黄醇从红细胞中排除的事实,使用红细胞和 2%BSA 在 PBS 中的混合物制备全血的替代基质,用于 DBS 视黄醇的测定。该方法在 0.04-300μg/mL 的浓度范围内呈线性。批内(n=5)和批内(n=6)精密度(相对标准偏差,RSD%)均低于 8.42%。在 3 个浓度下的加标回收率范围为 86.48-98.13%。内部标准(IS)归一化基质因子(MF)为 99.72%,RSD%为 10.50%(n=3)。使用浓度为 0.1962 和 0.3948 g/mL 的两个美国国家标准与技术研究院(NIST)血清生成校准标准对准确性进行校准,发现相对误差(RE%值)分别为 0.07%和 4.95%。首先开发了一个简单的校准模型,将 DBS 视黄醇浓度转换为等效的血浆视黄醇浓度,从而能够与临床参考范围以及使用血清或血浆样本的研究进行比较。

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