Department of Pharmacology and Toxicology, University of Vienna, Vienna, Austria (W.S., P.S.-H., R.L.-G.); APEPTICO Forschung und Entwicklung GmbH, Vienna, Austria (S.T., B.F., H.F., H.P.); and Division of Pulmonary Medicine, Department of Pharmacology and Toxicology, Vascular Biology Center, Medical College of Georgia, Georgia Regents University, Augusta, Georgia (R.L.).
Mol Pharmacol. 2013 Dec;84(6):899-910. doi: 10.1124/mol.113.089409. Epub 2013 Sep 27.
AP301 [Cyclo(CGQRETPEGAEAKPWYC)], a cyclic peptide comprising the human tumor necrosis factor lectin-like domain (TIP domain) sequence, is currently being developed as a treatment for lung edema and has been shown to reduce extravascular lung water and improve lung function in mouse, rat, and pig models. The current paradigm for liquid homeostasis in the adult mammalian lung is that passive apical uptake of sodium via the amiloride-sensitive epithelial Na⁺ channel (ENaC) and nonselective cyclic-nucleotide-gated cation channels creates the major driving force for reabsorption of water through the alveolar epithelium in addition to other ion channels such as potassium and chloride channels. AP301 can increase amiloride-sensitive current in A549 cells as well as in freshly isolated type II alveolar epithelial cells from different species. ENaC is expressed endogenously in all of these cell types. Consequently, this study was undertaken to determine whether ENaC is the specific target of AP301. The effect of AP301 in A549 cells as well as in human embryonic kidney cells and Chinese hamster ovary cells heterologously expressing human ENaC subunits (α, β, γ, and δ) was measured in patch clamp experiments. The congener TIP peptide AP318 [Cyclo(4-aminobutanoic acid-GQRETPEGAEAKPWYD)] activated ENaC by increasing single-channel open probability. AP301 increased current in proteolytically activated (cleaved) but not near-silent (uncleaved) ENaC in a reversible manner. αβγ- or δβγ-ENaC coexpression was required for maximal activity. No increase in current was observed after deglycosylation of extracellular domains of ENaC. Thus, our data suggest that the specific interaction of AP301 with both endogenously and heterologously expressed ENaC requires precedent binding to glycosylated extracellular loop(s).
AP301 [环(CGQRETPEGAEAKPWYC)],一种包含人肿瘤坏死因子凝集素样结构域(TIP 结构域)序列的环状肽,目前正在被开发为一种治疗肺水肿的药物,并已被证明可减少肺外水并改善小鼠、大鼠和猪模型中的肺功能。目前,成年哺乳动物肺中液体动态平衡的范例是,通过阿米洛利敏感的上皮钠通道(ENaC)和非选择性环核苷酸门控阳离子通道被动地顶端摄取钠,除了钾和氯通道等其他离子通道外,还为通过肺泡上皮重吸收水创造了主要驱动力。AP301 可以增加 A549 细胞以及来自不同物种的新鲜分离的 II 型肺泡上皮细胞中的阿米洛利敏感电流。ENaC 在内皮细胞中均有表达。因此,进行了这项研究以确定 ENaC 是否是 AP301 的特定靶标。在贴附斑实验中测量了 AP301 在 A549 细胞以及异源表达人 ENaC 亚基(α、β、γ 和 δ)的人胚肾细胞和中国仓鼠卵巢细胞中的作用。同源 TIP 肽 AP318 [环(4-氨基丁酸-GQRETPEGAEAKPWYD)] 通过增加单通道开放概率激活 ENaC。AP301 以可逆的方式增加蛋白水解激活(切割)但不是近沉默(未切割)ENaC 的电流。αβγ-或 δβγ-ENaC 共表达是最大活性所必需的。ENaC 细胞外结构域的糖基化缺失后,没有观察到电流增加。因此,我们的数据表明,AP301 与内源性和异源表达的 ENaC 的特异性相互作用需要预先与糖基化细胞外环结合。