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组织表面糖胺聚糖的质谱分析。

Mass spectral profiling of glycosaminoglycans from histological tissue surfaces.

机构信息

Center for Biomedical Mass Spectrometry, Department of Biochemistry, Boston University School of Medicine , Boston, Massachusetts 02118, United States.

出版信息

Anal Chem. 2013 Nov 19;85(22):10984-91. doi: 10.1021/ac402517s. Epub 2013 Oct 29.

Abstract

Glycosaminoglycans (GAGs) are found in intracellular granules, cell surfaces, and extracellular matrices in a spatially and temporally regulated fashion, constituting the environment for cells to interact, migrate, and proliferate. Through binding with a great number of proteins, GAGs regulate many facets of biological processes from embryonic development to normal physiological functions. GAGs have been shown to be involved in pathologic changes and immunological responses including cancer metastasis and inflammation. Past analyses of GAGs have focused on cell lines, body fluids, and relatively large tissue samples. Structures determined from such samples reflect the heterogeneity of the cell types present. To gain an understanding of the roles played by GAG expression during pathogenesis, it is very important to be able to detect and profile GAGs at the histological scale so as to minimize cell heterogeneity to potentially inform diagnosis and prognosis. Heparan sulfate (HS) belongs to one major class of GAGs, characterized by dramatic structural heterogeneity and complexity. To demonstrate feasibility of analysis of HS, 15 μm frozen bovine brain stem, cortex, and cerebellum tissue sections were washed with a series of solvent solutions to remove lipids before applying heparin lyases I, II, and III on the tissue surfaces within 5 mm × 5 mm digestion spots. The digested HS disaccharides were extracted from tissue surfaces and then analyzed by using size exclusion chromatography/mass spectrometry (SEC-MS). The results from bovine brain stem, cortex, and cerebellum demonstrated the reproducibility and reliability of our profiling method. We applied our method to detect HS from human astrocytoma (WHO grade II) and glioblastoma (GBM, WHO grade IV) frozen slides. Higher HS abundances and lower average sulfation level of HS were detected in glioblastoma (GBM, WHO grade IV) slides compared to astrocytoma (WHO grade II) slides.

摘要

糖胺聚糖(GAGs)以时空调节的方式存在于细胞内颗粒、细胞表面和细胞外基质中,构成了细胞相互作用、迁移和增殖的环境。通过与大量蛋白质结合,GAGs 调节从胚胎发育到正常生理功能的许多生物学过程。已经表明 GAGs 参与包括癌症转移和炎症在内的病理变化和免疫反应。过去对 GAGs 的分析主要集中在细胞系、体液和相对较大的组织样本上。从这些样本中确定的结构反映了存在的细胞类型的异质性。为了了解 GAG 表达在发病机制中的作用,能够在组织学尺度上检测和分析 GAGs 以最小化细胞异质性从而有可能提供诊断和预后信息非常重要。硫酸乙酰肝素(HS)属于 GAG 的主要类别之一,其特征是结构异质性和复杂性显著。为了证明分析 HS 的可行性,将 15μm 冷冻牛脑干、皮质和小脑组织切片用一系列溶剂溶液洗涤以去除脂质,然后在 5mm×5mm 的消化点内将肝素酶 I、II 和 III 应用于组织表面。从组织表面提取消化的 HS 二糖,然后通过尺寸排阻色谱/质谱(SEC-MS)进行分析。牛脑干、皮质和小脑的结果证明了我们的分析方法的可重复性和可靠性。我们将我们的方法应用于检测人星形细胞瘤(WHO 二级)和胶质母细胞瘤(GBM,WHO 四级)冷冻切片中的 HS。与星形细胞瘤(WHO 二级)切片相比,胶质母细胞瘤(GBM,WHO 四级)切片中 HS 的丰度更高,平均硫酸化水平更低。

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