Department of Cell, Developmental and Integrative Biology, University of Alabama at Birmingham , Birmingham, Alabama.
Department of Veterinary Medicine, Virginia-Maryland Regional College of Veterinary Medicine, University of Maryland , College Park, Maryland.
Am J Physiol Cell Physiol. 2018 Jun 1;314(6):C675-C689. doi: 10.1152/ajpcell.00221.2017. Epub 2018 Feb 14.
Cellular life requires the activation of the ADP-ribosylation factors (ARFs) by Golgi brefeldin A-resistant factor 1 (GBF1), a guanine nucleotide exchange factor (GEF) with a highly conserved catalytic Sec7 domain (Sec7d). In addition to the Sec7d, GBF1 contains other conserved domains whose functions remain unclear. Here, we focus on HDS2 (homology downstream of Sec7d 2) domain because the L1246R substitution within the HDS2 α-helix 5 of the zebrafish GBF1 ortholog causes vascular hemorrhaging and embryonic lethality (13). To dissect the structure/function relationships within HDS2, we generated six variants, in which the most conserved residues within α-helices 1, 2, 4, and 6 were mutated to alanines. Each HDS2 mutant was assessed in a cell-based "replacement" assay for its ability to support cellular functions normally supported by GBF1, such as maintaining Golgi homeostasis, facilitating COPI recruitment, supporting secretion, and sustaining cellular viability. We show that cells treated with the pharmacological GBF1 inhibitor brefeldin A (BFA) and expressing a BFA-resistant GBF1 variant with alanine substitutions of RDR1168 or LF1266 are compromised in Golgi homeostasis, impaired in ARF activation, unable to sustain secretion, and defective in maintaining cellular viability. To gain insight into the molecular mechanism of this dysfunction, we assessed the ability of each GBF1 mutant to target to Golgi membranes and found that mutations in RDR1168 and LF1266 significantly decrease targeting efficiency. Thus, these residues within α-helix 2 and α-helix 6 of the HDS2 domain in GBF1 are novel regulatory determinants that support GBF1 cellular function by impacting the Golgi-specific membrane association of GBF1.
细胞的生命活动需要 ADP-ribosylation 因子(ARFs)的激活,这一过程由高尔基 Brefeldin A 抗性因子 1(GBF1)介导,后者是一种鸟嘌呤核苷酸交换因子(GEF),具有高度保守的催化 Sec7 结构域(Sec7d)。除了 Sec7d,GBF1 还包含其他保守结构域,但它们的功能尚不清楚。在这里,我们重点关注 HDS2(Sec7d 下游同源结构域 2)结构域,因为在斑马鱼 GBF1 同源物的 HDS2α-螺旋 5 内的 L1246R 取代会导致血管出血和胚胎致死(13)。为了剖析 HDS2 内的结构/功能关系,我们生成了六个变体,其中将α-螺旋 1、2、4 和 6 内最保守的残基突变为丙氨酸。在基于细胞的“替代”测定中评估了每种 HDS2 突变体支持 GBF1 正常支持的细胞功能的能力,例如维持高尔基体稳态、促进 COPI 募集、支持分泌和维持细胞活力。我们表明,用药理学 GBF1 抑制剂布雷菲德菌素 A(BFA)处理并表达具有丙氨酸取代 RDR1168 或 LF1266 的 BFA 抗性 GBF1 变体的细胞在高尔基体稳态方面受损,ARF 激活受损,无法维持分泌,并且在维持细胞活力方面存在缺陷。为了深入了解这种功能障碍的分子机制,我们评估了每种 GBF1 突变体靶向高尔基体膜的能力,发现 RDR1168 和 LF1266 中的突变显著降低了靶向效率。因此,GBF1 中的 HDS2 结构域的α-螺旋 2 和α-螺旋 6 内的这些残基是新型调节决定因素,通过影响 GBF1 与高尔基体特异性膜的结合来支持 GBF1 的细胞功能。
