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使用薄层层析(f-TLC)法检测分枝杆菌酸 A/B 时的替代硼酸,用于诊断布鲁里溃疡。

Alternative boronic acids in the detection of Mycolactone A/B using the thin layer chromatography (f-TLC) method for diagnosis of Buruli ulcer.

机构信息

Department of Chemistry, School of Physical and Mathematical Sciences, College of Basic and Applied Sciences, University of Ghana, P.O. Box LG 56, Legon, Accra, Ghana.

Department of Chemistry, University of Sheffield, Dainton Building, Sheffield, S3 7HF, UK.

出版信息

BMC Infect Dis. 2023 Jul 27;23(1):495. doi: 10.1186/s12879-023-08426-2.

DOI:10.1186/s12879-023-08426-2
PMID:37501134
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10373253/
Abstract

BACKGROUND

Mycobacterium ulcerans is the causative agent of Buruli ulcer. The pathology of M. ulcerans disease has been attributed to the secretion of a potent macrolide cytotoxin known as mycolactone which plays an important role in the virulence of the disease. Mycolactone is a biomarker for the diagnosis of BU that can be detected using the fluorescent-thin layer chromatography (f-TLC) technique. The technique relies on the chemical derivatization of mycolactone A/B with 2-naphthylboronic acid (BA) which acts as a fluorogenic chemosensor. However, background interferences due to co-extracted human tissue lipids, especially with clinical samples coupled with the subjectivity of the method call for an investigation to find an alternative to BA.

METHODS

Twenty-six commercially available arylboronic acids were initially screened as alternatives to BA using the f-TLC experiment. UV-vis measurements were also conducted to determine the absorption maximum spectra of mycolactone A/B and myco-boronic acid adducts followed by an investigation of the fluorescence-enhancing ability of the boronate ester formation between mycolactone A/B and our three most promising boronic acids (BA15, BA18, and BA21). LC-MS technique was employed to confirm the adduct formation between mycolactone and boronic acids. Furthermore, a comparative study was conducted between BA18 and BA using 6 Polymerase Chain Reaction (PCR) confirmed BU patient samples.

RESULTS

Three of the boronic acids (BA15, BA18, and BA21) produced fluorescent band intensities superior to BA. Complexation studies conducted on thin layer chromatography (TLC) using 0.1 M solution of the three boronic acids and various volumes of 10 ng/µL of synthetic mycolactone ranging from 1 µL - 9 µL corresponding to 10 ng - 90 ng gave similar results with myco-BA18 adduct emerging with the most visibly intense fluorescence bands. UV-vis absorption maxima (λ) for the free mycolactone A/B was observed at 362 nm, and the values for the adducts myco-BA15, myco-BA18, and myco-BA21 were at 272 nm, 270 nm, and 286 nm respectively. The comparable experimental λ of 362 nm for mycolactone A/B to the calculated Woodward-Fieser value of 367 nm for the fatty acid side chain of mycolactone A/B demonstrate that even though 2 cyclic boronates were formed, only the boronate of the southern side chain with the chromophore was excited by irradiation at 365 nm. Fluorescence experiments have demonstrated that coupling BA18 to mycolactone A/B along the 1,3-diols remarkably enhanced the fluorescence intensity at 537 nm. High-Resolution Mass Spectrometer (HR-MS) was used to confirm the formation of the myco-BA15 adduct. Finally, f-TLC analysis of patient samples with BA18 gave improved BA18-adduct intensities compared to the original BA-adduct.

CONCLUSION

Twenty-six commercially available boronic acids were investigated as alternatives to BA, used in the f-TLC analysis for the diagnosis of BU. Three (3) of them BA15, BA18, and BA21 gave superior fluorescence band intensity profiles. They gave profiles that were easier to interpret after the myco-boronic acid adduct formation and in experiments with clinical samples from patients with BA18 the best. BA18, therefore, has been identified as a potential alternative to BA and could provide a solution to the challenge of background interference of co-extracted human tissue lipids from clinical samples currently associated with the use of BA.

摘要

背景

溃疡分枝杆菌是导致布鲁里溃疡的病原体。分枝杆菌疾病的病理学归因于一种称为mycolactone 的有效大环细胞毒素的分泌,该毒素在疾病的毒力中起着重要作用。Mycolactone 是 BU 诊断的生物标志物,可使用荧光薄层色谱 (f-TLC) 技术检测。该技术依赖于用 2-萘硼酸 (BA) 对 mycolactone A/B 进行化学衍生化,BA 作为荧光化学传感器。然而,由于与临床样本一起提取的人组织脂质引起的背景干扰,特别是与该方法的主观性,需要进行调查以寻找 BA 的替代品。

方法

最初使用 f-TLC 实验筛选了 26 种市售的芳基硼酸作为 BA 的替代品。还进行了 UV-vis 测量,以确定 mycolactone A/B 和 myco-硼酸加合物的最大吸收光谱,然后研究了 mycolactone A/B 与我们最有前途的三种硼酸 (BA15、BA18 和 BA21) 之间硼酸盐酯形成的荧光增强能力。LC-MS 技术用于确认 mycolactone 和硼酸之间的加合物形成。此外,还使用 BA18 和 BA 对 6 个聚合酶链反应 (PCR) 确认的 BU 患者样本进行了比较研究。

结果

三种硼酸 (BA15、BA18 和 BA21) 产生的荧光带强度优于 BA。在使用三种硼酸的 0.1 M 溶液和各种体积的 10 ng/µL 合成 mycolactone 进行的薄层色谱 (TLC) 上进行的络合研究中,从 1 µL 到 9 µL 的 10 ng 到 90 ng 范围内,与 myco-BA18 加合物一起出现的荧光强度最强。游离 mycolactone A/B 的最大紫外可见吸收峰 (λ) 为 362nm,myco-BA15、myco-BA18 和 myco-BA21 的加合物的 λ 值分别为 272nm、270nm 和 286nm。mycolactone A/B 的可比实验 λ 值为 362nm,与 mycolactone A/B 的脂肪酸侧链的计算伍德沃德-菲舍尔值 367nm 相当,表明即使形成了 2 个环状硼酸酯,只有带有生色团的南部侧链的硼酸盐被 365nm 辐射激发。荧光实验表明,mycolactone A/B 与 BA18 的偶联沿着 1,3-二醇显著增强了在 537nm 处的荧光强度。高分辨率质谱仪 (HR-MS) 用于确认 myco-BA15 加合物的形成。最后,与原始 BA 加合物相比,f-TLC 分析患者样本时,BA18 的分析结果显示 BA18 加合物的强度得到了改善。

结论

研究了 26 种市售硼酸作为 BA 的替代品,用于 BU 诊断的 f-TLC 分析。其中三种 (3) BA15、BA18 和 BA21 给出了更好的荧光带强度分布。在形成 myco-boronic 酸加合物后,它们的分布更容易解释,并且在使用 BA18 的患者临床样本实验中,效果最好。因此,BA18 已被确定为 BA 的潜在替代品,并可能为当前与 BA 一起使用时与临床样本中提取的人组织脂质相关的背景干扰提供解决方案。

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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a4bb/10373253/3c451cc4c29a/12879_2023_8426_Fig6_HTML.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a4bb/10373253/3125f05f5507/12879_2023_8426_Fig7_HTML.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a4bb/10373253/81c95ddb070b/12879_2023_8426_Fig8_HTML.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a4bb/10373253/d774e3c46e4c/12879_2023_8426_Fig9_HTML.jpg
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