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使用 2H 磁共振波谱测量琥珀酸代谢来对放疗后脑胶质瘤的反应进行成像。

Imaging Glioblastoma Response to Radiotherapy Using 2H Magnetic Resonance Spectroscopy Measurements of Fumarate Metabolism.

机构信息

Cancer Research UK Cambridge Institute, University of Cambridge, Cambridge, United Kingdom.

Department of Radiology, School of Clinical Medicine, Cambridge Biomedical Campus, University of Cambridge, Cambridge, United Kingdom.

出版信息

Cancer Res. 2022 Oct 4;82(19):3622-3633. doi: 10.1158/0008-5472.CAN-22-0101.

Abstract

UNLABELLED

Early detection of tumor cell death in glioblastoma following treatment with chemoradiation has the potential to distinguish between true disease progression and pseudoprogression. Tumor cell death can be detected noninvasively in vivo by imaging the production of [2,3-2H2]malate from [2,3-2H2]fumarate using 2H magnetic resonance (MR) spectroscopic imaging. We show here that 2H MR spectroscopy and spectroscopic imaging measurements of [2,3-2H2]fumarate metabolism can detect tumor cell death in orthotopically implanted glioblastoma models within 48 hours following the completion of chemoradiation. Following the injection of [2,3-2H2]fumarate into tumor-bearing mice, production of [2,3-2H2]malate was measured in a human cell line-derived model and in radiosensitive and radioresistant patient-derived models of glioblastoma that were treated with temozolomide followed by targeted fractionated irradiation. The increase in the [2,3-2H2]malate/[2,3-2H2]fumarate signal ratio posttreatment, which correlated with histologic assessment of cell death, was a more sensitive indicator of treatment response than diffusion-weighted and contrast agent-enhanced 1H MRI measurements, which have been used clinically to detect responses of glioblastoma to chemoradiation. Overall, early detection of glioblastoma cell death using 2H MRI of malate production from fumarate could help improve the clinical evaluation of response to chemoradiation.

SIGNIFICANCE

2H magnetic resonance imaging of labeled fumarate metabolism can detect early evidence of tumor cell death following chemoradiation, meeting a clinical need to reliably detect treatment response in glioblastoma.

摘要

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在接受放化疗后,早期检测胶质母细胞瘤中的肿瘤细胞死亡,有可能区分真正的疾病进展和假性进展。可以通过使用 2H 磁共振(MR)波谱成像来非侵入性地在体内成像[2,3-2H2]延胡索酸盐的产生来检测肿瘤细胞死亡。我们在这里显示,2H 磁共振波谱和[2,3-2H2]延胡索酸盐代谢的波谱成像测量可以在放化疗完成后 48 小时内检测到原位植入的胶质母细胞瘤模型中的肿瘤细胞死亡。在向荷瘤小鼠注射[2,3-2H2]延胡索酸盐后,在源自人细胞系的模型中以及在用替莫唑胺治疗后接受靶向分割照射的放射敏感和放射抵抗患者衍生的胶质母细胞瘤模型中测量了[2,3-2H2]苹果酸盐的产生。治疗后[2,3-2H2]苹果酸盐/[2,3-2H2]延胡索酸盐信号比的增加与细胞死亡的组织学评估相关,与已用于临床检测胶质母细胞瘤对放化疗反应的扩散加权和对比剂增强 1H MRI 测量相比,是对治疗反应更敏感的指标。总的来说,使用 2H MRI 检测延胡索酸盐代谢产物苹果酸盐的产生,可以早期检测胶质母细胞瘤细胞死亡,有助于改善对放化疗反应的临床评估。

意义

化学疗法后用标记的延胡索酸盐代谢的 2H 磁共振成像可以检测到肿瘤细胞死亡的早期证据,满足了在胶质母细胞瘤中可靠检测治疗反应的临床需求。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/394e/9530651/0efd159740b5/overview_graphic_can-22-0101.jpg

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