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利用神经氨酸酶的底物特异性进行靶向糖组学分析,鉴定包括 Sda/CAD 抗原在内的内源性唾液酸化糖肿瘤标志物候选物。

Identification of internally sialylated carbohydrate tumor marker candidates, including Sda/CAD antigens, by focused glycomic analyses utilizing the substrate specificity of neuraminidase.

机构信息

Department of Molecular Biology.

Department of Medical Checkup.

出版信息

Glycobiology. 2018 May 1;28(5):247-260. doi: 10.1093/glycob/cwy010.

DOI:10.1093/glycob/cwy010
PMID:29390163
Abstract

In our previous study, 14 sulfated carbohydrate tumor marker candidates were identified by focused glycomic analyses. Here, glycomic analyses focused on internally sialylated glycans to identify novel marker candidates. Internally sialylated glycans were enriched by digestion of pyridylaminated glycans prepared from sera with α-neuraminidase from Salmonella typhimurium, which did not cleave sialic acids linked to internal residues, followed by anion-exchange chromatography. Next, internally sialylated O-glycan profiles were constructed using two types of high performance liquid chromatography, which were compared between 20 healthy controls and 11 patients with gastric cancer and 9 patients with pancreatic cancer. In all, 17 marker candidates were identified. The structures of glycan candidates were precisely analyzed using enzymatic digestion, glycan synthesis, 2D mapping and mass spectrometry. Among 17 candidates, one was STn, and the other 16 comprised 10 core1, 1 core2 and 5 core3 glycans. The various structures included a α2,6-sialylated reducing terminal GalNAc and α2,6-sialylated type1 N-acetyl-lactosamine. Eight candidates possessed the Sda/CAD antigen. The levels of these candidate glycans in sera from all 40 subjects were quantified using a selected reaction monitoring assay and found to be elevated in at least one or more patients. Although the serum levels of each candidate glycan varied between patients, those candidates having the same backbone or determinant, such as core3 backbone and core1 structures with extended type1 N-acetyl-lactosamine, displayed similar patterns of elevation. These results suggest that analysis of multiple markers may be an effective means of diagnosing various cancers.

摘要

在我们之前的研究中,通过聚焦糖组学分析鉴定了 14 个硫酸化碳水化合物肿瘤标志物候选物。在这里,糖组学分析集中于内部唾液酸化聚糖,以鉴定新的标记物候选物。内部唾液酸化聚糖通过用鼠伤寒沙门氏菌的α-神经氨酸酶消化从血清中制备的吡啶氨化聚糖进行富集,该酶不会切割与内部残基相连的唾液酸,然后进行阴离子交换层析。接下来,使用两种类型的高效液相色谱法构建内部唾液酸化 O-聚糖图谱,在 20 名健康对照者、11 名胃癌患者和 9 名胰腺癌患者之间进行比较。总共鉴定出 17 个候选标志物。使用酶消化、聚糖合成、二维图谱和质谱精确分析糖候选物的结构。在 17 个候选物中,一个是 STn,另一个是 16 个核心 1、1 个核心 2 和 5 个核心 3 聚糖。各种结构包括α2,6-唾液酸化的还原末端 GalNAc 和α2,6-唾液酸化的 type1 N-乙酰乳糖胺。有 8 个候选物具有 Sda/CAD 抗原。使用选择反应监测分析定量测定所有 40 名受试者血清中的这些候选糖水平,发现至少一种或多种患者的水平升高。尽管每个候选糖在患者之间的血清水平不同,但具有相同骨架或决定簇的候选物,如核心 3 骨架和具有扩展的 type1 N-乙酰乳糖胺的核心 1 结构,显示出相似的升高模式。这些结果表明,分析多个标志物可能是诊断各种癌症的有效方法。

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