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Direct binding of the Kex2p cytosolic tail to the VHS domain of yeast Gga2p facilitates TGN to prevacuolar compartment transport and is regulated by phosphorylation

机译:Kex2p胞质尾巴与酵母Gga2p的VHS结构域的直接结合促进TGN进入前真空区室转运并受磷酸化作用调节

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摘要

Human Golgi-localized, γ-ear–containing, ADP-ribosylation factor–binding proteins (Ggas) bind directly to acidic dileucine sorting motifs in the cytosolic tails (C-tails) of intracellular receptors. Despite evidence for a role in recruiting ubiquitinated cargo, it remains unclear whether yeast Ggas also function by binding peptide-sorting signals directly. Two-hybrid analysis shows that the Gga1p and Gga2p Vps27, Hrs, Stam (VHS) domains both bind a site in the Kex2p C-tail and that the Gga2p VHS domain binds a site in the Vps10p C-tail. Binding requires deletion of an apparently autoinhibitory sequence in the Gga2p hinge. Ser780 in the Kex2p C-tail is crucial for binding: an Ala substitution blocks but an Asp substitution permits binding. Biochemical assays using purified Gga2p VHS–GGA and TOM1 (GAT) and glutathione S-transferase–Kex2p C-tail fusions show that Gga2p binds directly to the Kex2p C-tail, with relative affinities Asp780 > Ser780 > Ala780. Affinity-purified antibody against a peptide containing phospho-Ser­780 recognizes wild-type Kex2p but not S780A Kex2p, showing that Ser780 is phosphorylated in vivo; phosphorylation of Ser780 is up-regulated by cell wall–damaging drugs. Finally, mutation of Ser780 alters trafficking of Kex2p both in vivo and in cell-free trans-Golgi network (TGN)–prevacuolar compartment (PVC) transport. Thus yeast Gga adaptors facilitate TGN–PVC transport by direct binding of noncanonical phosphoregulated Gga-binding sites in cargo molecules.
机译:人类高尔基体定位,含γ耳的ADP-核糖基化因子结合蛋白(Ggas)直接与细胞内受体胞质尾部(C-尾)中的酸性双亮氨酸分选基序结合。尽管有证据表明在招募泛素化货物中起作用,但尚不清楚酵母Ggas是否也通过直接结合肽分选信号起作用。两次杂交分析显示,Gga1p和Gga2p Vps27,Hrs,Stam(VHS)域都结合了Kex2p C-tail中的位点,而Gga2p VHS域则结合了Vps10p C-tail中的位点。绑定需要删除Gga2p铰链中的一个明显的自抑制序列。 Kex2p C-tail中的Ser780对于结合至关重要:Ala取代会阻断,而Asp取代则允许结合。使用纯化的Gga2p VHS-GGA和TOM1(GAT)以及谷胱甘肽S-转移酶-Kex2p C-tail融合物进行的生化分析表明,Gga2p直接与Kex2p C-tail结合,相对亲和力为Asp780> Ser780> Ala780。亲和纯化的含磷酸Ser­780肽的抗体可识别野生型Kex2p,但不能识别S780A Kex2p,表明Ser780在体内被磷酸化。破坏细胞壁的药物会上调Ser780的磷酸化。最后,Ser780的突变改变了体内和无细胞反式高尔基网络(TGN)–疏液前腔(PVC)运输中Kex2p的运输。因此,酵母Gga衔接子通过直接结合货物分子中非规范的磷酸化Gga结合位点来促进TGN-PVC的运输。

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