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Golgi targeting of Drosophila melanogaster β4GalNAcTB requires a DHHC protein family–related protein as a pilot

机译:果蝇靶向果蝇β4GalNAcTB的高尔基体需要DHHC蛋白家族相关蛋白作为先导

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摘要

Drosophila melanogaster β4GalNAcTB mutant flies revealed that this particular N-acetylgalactosaminyltransferase is predominant in the formation of lacdiNAc (GalNAcβ1,4GlcNAc)-modified glycolipids, but enzymatic activity could not be confirmed for the cloned enzyme. Using a heterologous expression cloning approach, we isolated β4GalNAcTB together with β4GalNAcTB pilot (GABPI), a multimembrane-spanning protein related to Asp-His-His-Cys (DHHC) proteins but lacking the DHHC consensus sequence. In the absence of GABPI, inactive β4GalNAcTB is trapped in the endoplasmic reticulum (ER). Coexpression of β4GalNAcTB and GABPI generates the active enzyme that is localized together with GABPI in the Golgi. GABPI associates with β4GalNAcTB and, when expressed with an ER retention signal, holds active β4GalNAcTB in the ER. Importantly, treatment of isolated membrane vesicles with Triton X-100 disturbs β4GalNAcTB activity. This phenomenon occurs with multimembrane-spanning glycosyltransferases but is normally not a property of glycosyltransferases with one membrane anchor. In summary, our data provide evidence that GABPI is required for ER export and activity of β4GalNAcTB.
机译:果蝇黑腹果蝇β4GalNAcTB突变体蝇表明,这种特殊的N-乙酰半乳糖胺基转移酶是lacdiNAc(GalNAcβ1,4GlcNAc)修饰的糖脂形成的主要手段,但无法确认克隆酶的酶促活性。使用异源表达克隆方法,我们分离了β4GalNAcTB和β4GalNAcTB引物(GABPI),这是一种与Asp-His-His-Cys(DHHC)蛋白相关的跨膜蛋白,但缺少DHHC共有序列。在没有GABPI的情况下,无活性的β4GalNAcTB被捕获在内质网(ER)中。 β4GalNAcTB和GABPI的共表达产生活性酶,该活性酶与GABPI一起位于高尔基体中。 GABPI与β4GalNAcTB缔合,当以ER保留信号表达时,其在ER中保持活性β4GalNAcTB。重要的是,用Triton X-100处理分离的膜囊泡会干扰β4GalNAcTB活性。这种现象发生在跨膜糖基转移酶上,但通常不是具有一个膜锚的糖基转移酶的特性。总之,我们的数据提供了GABPI是ER出口和β4GalNAcTB活性所必需的证据。

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