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尿调蛋白的纳升液相色谱-串联质谱法分离及其糖基化分析。

Uromodulin Isolation and Its -Glycosylation Analysis by NanoLC-MS/MS.

机构信息

Department of Urology and The Proteomics Center, Boston Children's Hospital and Harvard Medical School, Boston, Massachusetts 02115, United States.

Broad Institute of MIT and Harvard, Cambridge, Massachusetts 02142, United States.

出版信息

J Proteome Res. 2021 May 7;20(5):2662-2672. doi: 10.1021/acs.jproteome.0c01053. Epub 2021 Mar 2.

DOI:10.1021/acs.jproteome.0c01053
PMID:33650863
Abstract

The glycoprotein uromodulin (UMOD) is the most abundant protein in urine, and -glycans are critical for many biological functions of UMOD. Comprehensive glycan profiling of UMOD provides valuable information to understand the exact mechanisms of glycan-regulated functions. To perform comprehensive glycosylation analysis of UMOD from urine samples with limited volumes, we developed a streamlined workflow that included UMOD isolation from 5 mL of urine from 6 healthy adult donors (3 males and 3 females) and a glycosylation analysis using a highly sensitive and reproducible nanoLC-MS/MS based glycomics approach. In total, 212 -glycan compositions were identified from the purified UMOD, and 17% were high-mannose glycans, 2% were afucosylated/asialylated, 3% were neutral fucosylated, 28% were sialylated (with no fucose), 46% were fucosylated and sialylated, and 4% were sulfated. We found that isolation of UMOD resulted in a significant decrease in the relative quantity of high-mannose and sulfated glycans with a significant increase of neutral fucosylated glycans in the UMOD-depleted urine relative to the undepleted urine, but depletion had little impact on the sialylated glycans. To our knowledge, this is the first study to perform comprehensive -glycan profiling of UMOD using nanoLC-MS/MS. This analytical workflow would be very beneficial for studies with limited sample size, such as pediatric studies, and can be applied to larger patient cohorts not only for UMOD interrogation but also for global glycan analysis.

摘要

尿调蛋白(UMOD)是尿液中含量最丰富的蛋白质,其β-聚糖对于 UMOD 的许多生物学功能至关重要。UMOD 的全面聚糖谱分析为了解糖基化调控功能的确切机制提供了有价值的信息。为了从有限体积的尿液样本中对 UMOD 进行全面的糖基化分析,我们开发了一种简化的工作流程,该流程包括从 6 名健康成年供体(3 名男性和 3 名女性)的 5 毫升尿液中分离 UMOD,以及使用高度敏感和可重现的基于 nanoLC-MS/MS 的糖组学方法进行糖基化分析。总共从纯化的 UMOD 中鉴定出 212 种β-聚糖组成,其中 17%为高甘露糖聚糖,2%为去岩藻糖基/去唾液酸基,3%为中性岩藻糖基,28%为唾液酸化(不含岩藻糖),46%为岩藻糖基和唾液酸化,4%为硫酸化。我们发现,与未耗尽尿液相比,UMOD 的分离导致高甘露糖和硫酸化聚糖的相对含量显著减少,而 UMOD 耗尽尿液中中性岩藻糖基聚糖的相对含量显著增加,但耗尽对唾液酸化聚糖的影响很小。据我们所知,这是首次使用 nanoLC-MS/MS 对 UMOD 进行全面β-聚糖谱分析的研究。这种分析工作流程对于样本量有限的研究(如儿科研究)非常有益,并且不仅可以应用于更大的患者队列来研究 UMOD,还可以用于进行全面的聚糖分析。

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