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DESI-MSI 引导的代谢表型关系探索通过多模态成像的单节段配准揭示了在透明细胞肾细胞癌中 PI38:3 与增殖细胞之间的相关性。

DESI-MSI-guided exploration of metabolic-phenotypic relationships reveals a correlation between PI 38:3 and proliferating cells in clear cell renal cell carcinoma via single-section co-registration of multimodal imaging.

机构信息

School of Medicine, University of St Andrews, North Haugh, St Andrews, KY16 9TF, UK.

Department of Urology, Western General Hospital, Crewe Road South, Edinburgh, EH4 2XU, UK.

出版信息

Anal Bioanal Chem. 2024 Jul;416(18):4015-4028. doi: 10.1007/s00216-024-05339-0. Epub 2024 May 23.

DOI:10.1007/s00216-024-05339-0
PMID:38780655
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11249708/
Abstract

A workflow has been evaluated that utilizes a single tissue section to obtain spatially co-registered, molecular, and phenotypical information suitable for AI-enabled image analysis. Desorption electrospray ionization mass spectrometry imaging (DESI-MSI) was used to obtain molecular information followed by conventional histological staining and immunolabelling. The impact of varying DESI-MSI conditions (e.g., heated transfer line (HTL) temperature, scan rate, acquisition time) on the detection of small molecules and lipids as well as on tissue integrity crucial for integration into typical clinical pathology workflows was assessed in human kidney. Increasing the heated transfer line temperature from 150 to 450 °C resulted in a 1.8-fold enhancement in lipid signal at a scan rate of 10 scans/s, while preserving histological features. Moreover, increasing the acquisition speed to 30 scans/s yielded superior lipid signal when compared to 10 scans/s at 150 °C. Tissue morphology and protein epitopes remained intact allowing full histological assessment and further multiplex phenotyping by immunofluorescence (mIF) and immunohistochemistry (mIHC) of the same section. The successful integration of the workflow incorporating DESI-MSI, H&E, and immunolabelling on a single tissue section revealed an accumulation of ascorbic acid in regions of focal chronic inflammatory cell infiltrate within non-cancerous kidney tissue. Additionally, a strong positive correlation between PI 38:3 and proliferating cells was observed in clear cell renal cell carcinoma (ccRCC) showing the utility of this approach in uncovering molecular associations in disease pathology.

摘要

已经评估了一种工作流程,该流程利用单个组织切片获得适合人工智能驱动的图像分析的空间配准、分子和表型信息。解吸电喷雾电离质谱成像(DESI-MSI)用于获得分子信息,然后进行常规组织学染色和免疫标记。在人肾中评估了改变 DESI-MSI 条件(例如,加热传输线(HTL)温度、扫描速度、采集时间)对小分子和脂质检测的影响,以及对组织完整性的影响,这对于整合到典型的临床病理学工作流程至关重要。将加热传输线温度从 150°C 增加到 450°C,在扫描速度为 10 次/秒时,脂质信号增强了 1.8 倍,同时保持了组织学特征。此外,与在 150°C 时的 10 次/秒相比,将采集速度提高到 30 次/秒可获得更好的脂质信号。组织形态和蛋白质表位保持完整,允许对同一切片进行全面的组织学评估,并通过免疫荧光(mIF)和免疫组织化学(mIHC)进行进一步的多重表型分析。成功整合了包含 DESI-MSI、H&E 和免疫标记的工作流程,在非癌性肾组织中局灶性慢性炎症细胞浸润区域发现了抗坏血酸的积累。此外,在透明细胞肾细胞癌(ccRCC)中观察到 PI 38:3 与增殖细胞之间存在强烈的正相关,表明该方法在揭示疾病病理学中的分子关联方面具有实用性。

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