Nakayasu Ernesto S, Yashunsky Dmitry V, Nohara Lilian L, Torrecilhas Ana Claudia T, Nikolaev Andrei V, Almeida Igor C
Department of Biological Sciences, The Border Biomedical Research Center, University of Texas at El Paso, El Paso, TX 79968, USA.
Mol Syst Biol. 2009;5:261. doi: 10.1038/msb.2009.13. Epub 2009 Apr 7.
Glycosylphosphatidylinositol (GPI) anchoring is a common, relevant posttranslational modification of eukaryotic surface proteins. Here, we developed a fast, simple, and highly sensitive (high attomole-low femtomole range) method that uses liquid chromatography-tandem mass spectrometry (LC-MS(n)) for the first large-scale analysis of GPI-anchored molecules (i.e., the GPIome) of a eukaryote, Trypanosoma cruzi, the etiologic agent of Chagas disease. Our genome-wise prediction analysis revealed that approximately 12% of T. cruzi genes possibly encode GPI-anchored proteins. By analyzing the GPIome of T. cruzi insect-dwelling epimastigote stage using LC-MS(n), we identified 90 GPI species, of which 79 were novel. Moreover, we determined that mucins coded by the T. cruzi small mucin-like gene (TcSMUG S) family are the major GPI-anchored proteins expressed on the epimastigote cell surface. TcSMUG S mucin mature sequences are short (56-85 amino acids) and highly O-glycosylated, and contain few proteolytic sites, therefore, less likely susceptible to proteases of the midgut of the insect vector. We propose that our approach could be used for the high throughput GPIomic analysis of other lower and higher eukaryotes.
糖基磷脂酰肌醇(GPI)锚定是真核生物表面蛋白常见且重要的翻译后修饰。在此,我们开发了一种快速、简便且高度灵敏(高阿托摩尔至低飞摩尔范围)的方法,该方法利用液相色谱 - 串联质谱(LC-MS(n))对恰加斯病的病原体——真核生物克氏锥虫的GPI锚定分子(即GPI组)进行首次大规模分析。我们基于基因组的预测分析表明,约12%的克氏锥虫基因可能编码GPI锚定蛋白。通过使用LC-MS(n)分析克氏锥虫昆虫寄生型前鞭毛体阶段的GPI组,我们鉴定出90种GPI种类,其中79种是新发现的。此外,我们确定由克氏锥虫小黏蛋白样基因(TcSMUG S)家族编码的黏蛋白是在前鞭毛体细胞表面表达的主要GPI锚定蛋白。TcSMUG S黏蛋白成熟序列较短(56 - 85个氨基酸)且高度O - 糖基化,并且含有较少的蛋白水解位点,因此,不太可能被昆虫载体中肠的蛋白酶所作用。我们提出,我们的方法可用于对其他低等和高等真核生物进行高通量GPI组分析。
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