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基于琼脂的微生物群落的定量 SIMS 成像。

Quantitative SIMS Imaging of Agar-Based Microbial Communities.

机构信息

Department of Chemistry and Beckman Institute for Advanced Science and Technology , University of Illinois at Urbana-Champaign , Urbana , Illinois 61801 , United States.

Department of Chemistry and Biochemistry and Department of Chemical and Biomolecular Engineering , University of Notre Dame , Notre Dame , Indiana 46556 , United States.

出版信息

Anal Chem. 2018 May 1;90(9):5654-5663. doi: 10.1021/acs.analchem.7b05180. Epub 2018 Apr 13.

Abstract

After several decades of widespread use for mapping elemental ions and small molecular fragments in surface science, secondary ion mass spectrometry (SIMS) has emerged as a powerful analytical tool for molecular imaging in biology. Biomolecular SIMS imaging has primarily been used as a qualitative technique; although the distribution of a single analyte can be accurately determined, it is difficult to map the absolute quantity of a compound or even to compare the relative abundance of one molecular species to that of another. We describe a method for quantitative SIMS imaging of small molecules in agar-based microbial communities. The microbes are cultivated on a thin film of agar, dried under nitrogen, and imaged directly with SIMS. By use of optical microscopy, we show that the area of the agar is reduced by 26 ± 2% (standard deviation) during dehydration, but the overall biofilm morphology and analyte distribution are largely retained. We detail a quantitative imaging methodology, in which the ion intensity of each analyte is (1) normalized to an external quadratic regression curve, (2) corrected for isomeric interference, and (3) filtered for sample-specific noise and lower and upper limits of quantitation. The end result is a two-dimensional surface density image for each analyte. The sample preparation and quantitation methods are validated by quantitatively imaging four alkyl-quinolone and alkyl-quinoline N-oxide signaling molecules (including Pseudomonas quinolone signal) in Pseudomonas aeruginosa colony biofilms. We show that the relative surface densities of the target biomolecules are substantially different from values inferred through direct intensity comparison and that the developed methodologies can be used to quantitatively compare as many ions as there are available standards.

摘要

经过几十年在表面科学中广泛用于元素离子和小分子片段测绘的应用,二次离子质谱(SIMS)已成为生物学中分子成像的强大分析工具。生物分子 SIMS 成像主要用作定性技术;虽然可以准确确定单个分析物的分布,但很难测绘化合物的绝对数量,甚至很难比较一种分子物质的相对丰度与另一种分子物质的相对丰度。我们描述了一种用于琼脂基微生物群落中小分子的定量 SIMS 成像方法。微生物在琼脂薄膜上培养,在氮气下干燥,然后直接用 SIMS 成像。通过光学显微镜,我们表明在脱水过程中琼脂面积减少了 26 ± 2%(标准偏差),但生物膜形态和分析物分布总体上得到保留。我们详细介绍了一种定量成像方法,其中每个分析物的离子强度(1)归一化为外部二次回归曲线,(2)校正同系物干扰,(3)针对样品特定噪声和定量下限进行过滤。最终得到每个分析物的二维表面密度图像。通过对铜绿假单胞菌菌落生物膜中的四种烷基-喹诺酮和烷基-喹啉 N-氧化物信号分子(包括假单胞菌喹诺酮信号)进行定量成像,验证了样品制备和定量方法。我们表明,目标生物分子的相对表面密度与通过直接强度比较推断的值有很大不同,并且所开发的方法可用于定量比较尽可能多的离子,只要有可用的标准。

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