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Plasma degradome affected by variable storage of human blood

机译:血浆降解受人血储存量变化的影响

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摘要

BackgroundThe successful application of—omics technologies in the discovery of novel biomarkers and targets of therapeutic interventions is facilitated by large collections of well curated clinical samples stored in bio banks. Mining the plasma proteome holds promise to improve our understanding of disease mechanisms and may represent a source of biomarkers. However, a major confounding factor for defining disease-specific proteomic signatures in plasma is the variation in handling and processing of clinical samples leading to protein degradation. To address this, we defined a plasma proteolytic signature (degradome) reflecting pre-analytical variability in blood samples that remained at ambient temperature for different time periods after collection and prior to processing.MethodsWe obtained EDTA blood samples from five healthy volunteers (n = 5), and blood tubes remained at ambient temperature for 30 min, 8, 24 and 48 h prior to centrifugation and isolation of plasma. Naturally occurred peptides derived from plasma samples were compared by label-free quantitative LC–MS/MS. To profile protein degradation, we analysed pooled plasma samples at T = 30 min and 48 h using PROTOMAP analysis. The proteolytic pattern of selected protein candidates was further validated by immunoblotting.ResultsA total of 820 plasma proteins were surveyed by PROTOMAP, and for 4 % of these, marked degradation was observed. We show distinct proteolysis patterns for talin-1, coagulation factor XI, complement protein C1r, C3, C4 and thrombospondin, and several proteins including S100A8, A9, annexin A1, profiling-1 and platelet glycoprotein V are enriched after 48 h blood storage at ambient temperature. In particular, thrombospondin protein levels increased after 8 h and proteolytic fragments appeared after 24 h storage time.ConclusionsThe overall impact of blood storage at ambient temperature for variable times on the plasma proteome and degradome is relatively minor, but in some cases can cause a potential bias in identifying and assigning relevant proteomic markers. The observed effects on the plasma proteome and degradome are predominantly triggered by limited leucocyte and platelet cell activation due to blood handling and storage. The baseline plasma degradome signature presented here can help filtering candidate protein markers relevant for clinical biomarker studies.
机译:背景技术组学技术在发现新颖的生物标志物和治疗干预目标方面的成功应用,是通过大量存储在生物库中的精心挑选的临床样品的促成的。开采血浆蛋白质组有望改善我们对疾病机制的了解,并可能代表生物标志物的来源。然而,定义血浆中疾病特异性蛋白质组学特征的主要混杂因素是临床样品处理和加工中的差异,导致蛋白质降解。为了解决这个问题,我们定义了血浆蛋白水解特征(降解组),反映了采集后和处理前不同时间在环境温度下保持在室温下的血样的分析前变异性。方法我们从五名健康志愿者(n = 5)中获得了EDTA血样。 ),在离心和分离血浆之前,将血管在环境温度下保持30分钟,8、24和48小时。通过无标记定量LC-MS / MS比较了血浆样品中天然生成的肽。为了描述蛋白质降解,我们使用PROTOMAP分析在T = 30分钟和48小时分析了合并血浆样品。结果通过PROTOMAP检验了820种血浆蛋白,其中4%的蛋白降解明显。我们显示了talin-1,凝血因子XI,补体蛋白C1r,C3,C4和血小板反应蛋白的独特蛋白水解模式,并且在48 h血液储存后,包括S100A8,A9,膜联蛋白A1,profiling-1和血小板糖蛋白V在内的几种蛋白质被富集。环境温度。特别是血小板反应蛋白的水平在8 h后增加,在24 h后出现蛋白水解片段。结论在室温下不同时间储血对血浆蛋白质组和降解组的总体影响相对较小,但在某些情况下可能导致在识别和分配相关蛋白质组学标记方面存在偏见。观察到的对血浆蛋白质组和降解组的影响主要是由于血液处理和储存引起的有限的白细胞和血小板细胞活化而触发的。此处呈现的基线血浆降解组学特征可以帮助过滤与临床生物标志物研究相关的候选蛋白质标志物。

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