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Purification cloning and characterization of a GPI inositol deacylase from Trypanosoma brucei

机译:布鲁氏锥虫GPI肌醇脱酰基酶的纯化克隆和鉴定

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摘要

Inositol acylation is an obligatory step in glycosylphosphatidylinositol (GPI) biosynthesis whereas mature GPI anchors often lack this modification. The GPI anchors of Trypanosoma brucei variant surface glycoproteins (VSGs) undergo rounds of inositol acylation and deacylation during GPI biosynthesis and the deacylation reactions are inhibited by diisopropylfluorophosphate (DFP). Inositol deacylase was affinity labelled with [3H]DFP and purified. Peptide sequencing was used to clone GPIdeAc, which encodes a protein with significant sequence and hydropathy similarity to mammalian acyloxyacyl hydrolase, an enzyme that removes fatty acids from bacterial lipopolysaccharide. Both contain a signal sequence followed by a saposin domain and a GDSL-lipase domain. GPIdeAc–/– trypanosomes were viable in vitro and in animals. Affinity-purified HA-tagged GPIdeAc was shown to have inositol deacylase activity. However, total inositol deacylase activity was only reduced in GPIdeAc–/– trypanosomes and the VSG GPI anchor was indistinguishable from wild type. These results suggest that there is redundancy in T.brucei inositol deacylase activity and that there is another enzyme whose sequence is not recognizably related to GPIdeAc.
机译:肌醇酰化是糖基磷脂酰肌醇(GPI)生物合成中的必不可少的步骤,而成熟的GPI锚通常缺乏这种修饰。布鲁氏锥虫变体表面糖蛋白(VSG)的GPI锚点在GPI生物合成过程中经历了几轮肌醇酰化和去酰化作用,并且去酰化反应被氟代磷酸二异丙酯(DFP)抑制。用[ 3 H] DFP亲和标记肌醇脱酰基酶并纯化。肽测序用于克隆GPIdeAc,它编码与哺乳动物的酰氧基酰基水解酶具有显着序列和亲水性相似性的蛋白质,该酶可从细菌脂多糖中去除脂肪酸。两者均包含信号序列,其后是saposin结构域和GDSL-脂肪酶结构域。 GPIdeAc – / – 锥虫在体外和在动物中都是可行的。亲和纯化的HA标记的GPIdeAc被证明具有肌醇脱酰基酶活性。但是,总肌醇脱酰基酶活性仅在GPIdeAc – / – 锥虫中降低,而VSG GPI锚与野生型没有区别。这些结果表明布鲁氏球菌肌醇脱酰基酶活性存在冗余,并且存在另一种酶,其序列与GPIdeAc不能识别。

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