Analysis of total microcystins and nodularins by oxidative cleavage of their ADMAdda, DMAdda, and Adda moieties

IF 2.5 Q1 Chemistry
Amanda J. Foss , Christopher O. Miles , Alistair L. Wilkins , Frode Rise , Kristian W. Trovik , Kamil Cieslik , Mark T. Aubel
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引用次数: 8

Abstract

Microcystins (MCs) and nodularins (NODs) exhibit high structural variability, including modifications of the Adda (3S-amino-9S-methoxy-2S,6,8S-trimethyl-10-phenyldeca-4E,6E-dienoic acid) moiety. Variations include 9-O-desmethylAdda (DMAdda) and 9-O-acetylDMAdda (ADMAdda) which, unless targeted, may go undetected. Therefore, reference standards were prepared of [ADMAdda5]MCs and [DMAdda5]MCs, which were analyzed using multiple approaches. The cross-reactivities of the [DMAdda5]- and [ADMAdda5]MC standards were similar to that of MC-LR when analyzed with a protein phosphatase 2A (PP2A) inhibition assay, but were <0.25% when analyzed with an Adda enzyme-linked immunosorbent assay (ELISA). Oxidative cleavage experiments identified compounds that could be used in the analysis of total MCs/NODs in a similar fashion to the 2R-methyl-3S-methoxy-4-phenylbutanoic acid (MMPB) technique. Products from oxidative cleavage of both the 4,5- and 6,7-ene of Adda, DMAdda and ADMAdda were observed, and three oxidation products, one from each Adda variant, were chosen for analysis and applied to three field samples and a Nostoc culture. Results from the oxidative cleavage method for total Adda, DMAdda, and ADMAdda were similar to those from the Adda-ELISA, PP2A inhibition, and LC-MS/MS analyses, except for the Nostoc culture where the Adda-ELISA greatly underestimated microcystin levels. This oxidative cleavage method can be used for routine analysis of field samples and to assess the presence of the rarely reported, but toxic, DMAdda/ADMAdda-containing MCs and NODs.

Abstract Image

氧化裂解ADMAdda、dadda和Adda片段分析总微囊藻毒素和结核素
微囊藻毒素(MCs)和结节蛋白(NODs)具有高度的结构变变性,包括Adda (3s -氨基- 9s -甲氧基- 2s, 6,8s -三甲基-10-苯基十二- 4e, 6e -二烯酸)片段的修饰。变异包括9- o -去甲基adda (DMAdda)和9- o -乙酰基DMAdda (ADMAdda),除非靶向,否则可能无法检测到。为此,制备了[adadda5]和[DMAdda5]MCs的参比标准,并采用多种方法对其进行分析。用蛋白磷酸酶2A (PP2A)抑制试验分析,[DMAdda5]-和[adadda5]MC标准物的交叉反应性与MC- lr相似,但用Adda酶联免疫吸附试验(ELISA)分析时,交叉反应性为<0.25%。氧化裂解实验确定了可用于总MCs/NODs分析的化合物,类似于2r -甲基- 3s -甲氧基-4-苯基丁酸(MMPB)技术。对Adda、DMAdda和ADMAdda的4,5-和6,7-烯氧化裂解产物进行了观察,并从每个Adda变体中选择了三个氧化产物进行分析,并应用于三个现场样品和Nostoc培养。氧化裂解法测定总Adda、DMAdda和ADMAdda的结果与Adda- elisa、PP2A抑制和LC-MS/MS分析的结果相似,除了在Nostoc培养中,Adda- elisa大大低估了微囊藻毒素的水平。这种氧化裂解方法可以用于野外样品的常规分析,并评估很少报道但有毒的含有DMAdda/ adadda的mc和nod的存在。
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
Analytica Chimica Acta: X
Analytica Chimica Acta: X Chemistry-Analytical Chemistry
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3
审稿时长
16 weeks
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