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Isotopic labeling of terminal amines in complex samples identifies protein N-termini and protease cleavage products

机译:复杂样品中末端胺的同位素标记可鉴定N-末端蛋白和蛋白酶裂解产物

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Effective proteome-wide strategies that distinguish the N-termini of proteins from the N-termini of their protease cleavage products would accelerate identification of the substrates of proteases with broad or unknown specificity. Our approach, named terminal amine isotopic labeling of substrates (TAILS), addresses this challenge by using dendritic polyglycerol aldehyde polymers that remove tryptic and C-terminal peptides. We analyze unbound naturally acetylated, cyclized or labeled N-termini from proteins and their protease cleavage products by tandem mass spectrometry, and use peptide isotope quantification to discriminate between the substrates of the protease of interest and the products of background proteolysis. We identify 731 acetylated and 132 cyclized N-termini, and 288 matrix metalloproteinase (MMP)-2 cleavage sites in mouse fibroblast secretomes. We further demonstrate the potential of our strategy to link proteases with defined biological pathways in complex samples by analyzing mouse inflammatory bronchoalveolar fluid and showing that expression of the poorly defined breast cancer protease MMP-11 in MCF-7 human breast cancer cells cleaves both endoplasmin and the immunomodulator and apoptosis inducer galectin-1.
机译:区分蛋白质的N末端和其蛋白酶裂解产物的N末端的有效的全蛋白质组策略将加速鉴定具有广泛或未知特异性的蛋白酶底物。我们的方法被称为底物末端胺同位素标记(TAILS),它通过使用树突状聚甘油醛聚合物去除胰蛋白酶和C末端肽来解决这一挑战。我们通过串联质谱从蛋白质及其蛋白酶裂解产物中分析未结合的天然乙酰化,环化或标记的N-末端,并使用肽同位素定量来区分目标蛋白酶的底物和背景蛋白水解的产物。我们确定了小鼠成纤维细胞分泌蛋白组中的731个乙酰化和132个环化的N-末端以及288个基质金属蛋白酶(MMP)-2切割位点。我们通过分析小鼠炎症性支气管肺泡液,并证明MCF-7人乳腺癌细胞中定义较差的乳腺癌蛋白酶MMP-11的表达可裂解内质蛋白酶和内切酶,进一步证明了我们的策略将蛋白酶与复杂样品中定义的生物途径连接的潜力。免疫调节剂和凋亡诱导物半乳凝素-1。

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