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在立体定向针活检后进行探针清洗的可行性,作为一种开发 H3 K27 改变弥漫性中线脑胶质瘤的细胞系和异种移植物的新技术。

Feasibility of probe washing after stereotactic needle biopsy as a novel technique for developing cell lines and xenografts of H3 K27-altered diffuse midline gliomas.

机构信息

Departments of1Neurologic Surgery and.

2Molecular Pharmacology and Experimental Therapeutics, Mayo Clinic, Rochester, Minnesota.

出版信息

J Neurosurg Pediatr. 2023 Jul 14;32(4):413-420. doi: 10.3171/2023.5.PEDS22557. Print 2023 Oct 1.

Abstract

H3 K27-altered diffuse midline gliomas (DMGs) are frequently biopsied to obtain tissue diagnosis, inform clinical decision-making, and determine clinical trial eligibility. Tissue yield from biopsies is typically low, leaving little material available for research. To advance understanding of disease biology and promote preclinical testing of novel therapeutics, collecting viable cellular material from treatment-naive tumors is of paramount importance. Here, the authors report the feasibility of a practicable technique for creating DMG cell lines and patient-derived xenografts (PDXs) without the need for additional biopsy specimens. Tumor cells are obtained by probe washing immediately after completion of biopsy. Wash fluid is collected, and viable cells are expanded in vitro. Cultured cells are used to establish PDX rodent models. A total of 5 patient samples were collected by this technique. Viable tumor cells were obtained from 3 of the 5 samples, and cell lines suitable for experiments were obtained within 6-8 months. Orthotopic implantation and flank engraftment was successful in 1 of the 3 established cell lines. Animals harboring intracranial tumors were euthanized due to disease burden 6-7 months after stereotactic injection. Flank tumors formed within 4-5 months and were serially passaged. Molecular and tissue analyses confirmed retention of H3 K27M expression and loss of H3 K27me3 in all cell lines and PDXs.

摘要

H3 K27 改变的弥漫性中线胶质瘤(DMG)常通过活检获得组织诊断,为临床决策提供信息,并确定临床试验的资格。活检获得的组织产量通常较低,留下的研究材料很少。为了深入了解疾病生物学,并促进新型治疗方法的临床前测试,从未经治疗的肿瘤中收集可行的细胞材料至关重要。在这里,作者报告了一种可行的技术,可在无需额外活检样本的情况下创建 DMG 细胞系和患者来源的异种移植物(PDX)。在活检完成后立即通过探针洗涤获得肿瘤细胞。收集洗涤液,并在体外扩增活细胞。培养的细胞用于建立 PDX 啮齿动物模型。通过该技术共收集了 5 个患者样本。从 5 个样本中的 3 个获得了可行的肿瘤细胞,并且在 6-8 个月内获得了适合实验的细胞系。在 3 个建立的细胞系中,有 1 个成功进行了原位移植和侧腹植入。由于疾病负担,在立体定向注射后 6-7 个月,颅内肿瘤的动物被安乐死。在 4-5 个月内形成了侧腹肿瘤,并进行了连续传代。分子和组织分析证实所有细胞系和 PDX 均保留了 H3 K27M 表达,丧失了 H3 K27me3。

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