Implementation of plate reader-based indooxine and Nessler protocols for monitoring L-asparaginase serum activity in childhood acute lymphoblastic leukaemia.

IF 2.5 Q3 BIOCHEMICAL RESEARCH METHODS
Biology Methods and Protocols Pub Date : 2024-06-13 eCollection Date: 2024-01-01 DOI:10.1093/biomethods/bpae042
Bozhidar Vergov, Yordan Sbirkov, Danail Minchev, Tatyana Todorova, Alexandra Baldzhieva, Hasan Burnusuzov, Мariya I Spasova, Victoria Sarafian
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Abstract

Monitoring the blood serum activity of L-asparaginase in children with acute lymphoblastic leukaemia (ALL) has been highly recommended to detect enzyme inactivation that can cause relapse and to avoid unwanted toxicity. Nevertheless, perhaps at least partially due to the lack of clinically approved commercially available kits or standardized and independently reproduced and validated in-house protocols, laboratory assay-based determination of the optimal doses of L-asparaginase is not carried out routinely. In this study, we adapted previously published protocols for two plate reader-based colorimetric methods, indooxine and Nessler, to measure asparaginase activity. Mock samples with dilutions of the enzyme for initial optimization steps, and patient samples were used as a proof of principle and to compare the two protocols. For the first time the indooxine and the Nessler methods are adapted for a plate reader and L-asparaginase serum activity levels are compared by both protocols. Passing-Bablok and Bland-Altman's statistical analyses found very little difference, strong correlation (r = 0.852), and bias of only 6% between the data from the two methods when used for fresh patient samples. Furthermore, we demonstrate that the Nessler method could also be applied for frozen sera as the results, compared to fresh samples, showed little difference, strong correlation (r = 0.817), and small bias (9%). We successfully adapted and validated two methods for measuring L-asparaginase activity in cALL and provided the most detailed description to date on how to reproduce and implement them in other clinical laboratories.

在儿童急性淋巴细胞白血病中采用基于平板阅读器的indooxine和Nessler方案监测L-天冬酰胺酶血清活性。
人们强烈建议监测急性淋巴细胞白血病(ALL)患儿血清中 L-天冬酰胺酶的活性,以检测可能导致复发的酶失活,并避免不必要的毒性。然而,也许至少部分是由于缺乏临床认可的市售试剂盒或标准化、独立复制和验证的内部方案,实验室测定 L-天冬酰胺酶最佳剂量的工作并未常规化。在本研究中,我们改编了之前发表的两种基于平板阅读器的比色法(indooxine 和 Nessler),用于测量天冬酰胺酶的活性。我们用稀释了酶的模拟样本和病人样本作为初始优化步骤,并对两种方法进行了原理验证和比较。这是首次将吲哚辛法和奈斯勒法应用于平板阅读器,并通过两种方法比较 L-天冬酰胺酶的血清活性水平。Passing-Bablok 和 Bland-Altman 统计分析发现,在用于新鲜患者样本时,两种方法的数据差异很小,相关性很强(r = 0.852),偏差仅为 6%。此外,我们还证明奈斯勒方法也可用于冷冻血清,因为与新鲜样本相比,结果显示差异很小,相关性很强(r = 0.817),偏差很小(9%)。我们成功地调整并验证了两种测量 cALL 中 L-天冬酰胺酶活性的方法,并就如何在其他临床实验室中复制和实施这两种方法提供了迄今为止最详细的说明。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Biology Methods and Protocols
Biology Methods and Protocols Agricultural and Biological Sciences-Agricultural and Biological Sciences (all)
CiteScore
3.80
自引率
2.80%
发文量
28
审稿时长
19 weeks
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