Department of Neuroscience, University of Texas Southwestern Medical Center at Dallas, Dallas, Texas 75390, USA.
J Biol Chem. 2011 Aug 5;286(31):27447-53. doi: 10.1074/jbc.M111.243154. Epub 2011 Jun 17.
Notch is a transmembrane receptor that controls a diverse array of cellular processes including cell proliferation, differentiation, survival, and migration. The cellular outcome of Notch signaling is dependent on extracellular and intracellular signals, but the complexities of its regulation are not well understood. Canonical Notch signaling involves ligand association that triggers sequential and regulated proteolysis of Notch at several sites. Ligand-dependent proteolysis at the S2 site removes the bulk of the extracellular domain of Notch. Subsequent γ-secretase-mediated intramembrane proteolysis of the remaining membrane-tethered Notch fragment at the S3 site produces a nuclear-destined Notch intracellular domain (NICD). Here we show that following γ-secretase cleavage, Notch is proteolyzed at a novel S5 site. We have identified this S5 site to be eight amino acids downstream of the S3 site. Biochemical fractionation and purification resulted in the identification of the S5 site protease as the mitochondrial intermediate peptidase (MIPEP). Expression of the MIPEP-cleaved NICD (ΔNICD) results in a decrease in cell viability and mitochondria membrane potential. The sequential and regulated proteolysis by γ-secretase and MIPEP suggests a new means by which Notch function can be modulated.
Notch 是一种跨膜受体,控制着多种细胞过程,包括细胞增殖、分化、存活和迁移。Notch 信号的细胞结果取决于细胞外和细胞内信号,但它的调控复杂性还不是很清楚。经典的 Notch 信号涉及配体的结合,该结合触发 Notch 在几个位点的连续和调节性蛋白水解。配体依赖性的 S2 位点的蛋白水解去除了 Notch 胞外结构域的大部分。随后 γ-分泌酶介导的剩余膜结合 Notch 片段在 S3 位点的跨膜蛋白水解产生核定向 Notch 细胞内结构域 (NICD)。在这里,我们表明,在 γ-分泌酶切割之后,Notch 在一个新的 S5 位点被蛋白水解。我们已经确定了这个 S5 位点在 S3 位点下游八个氨基酸的位置。生化分级分离和纯化导致鉴定出 S5 位点蛋白酶为线粒体中间肽酶 (MIPEP)。表达 MIPEP 切割的 NICD (ΔNICD) 导致细胞活力和线粒体膜电位降低。γ-分泌酶和 MIPEP 的连续和调节性蛋白水解表明 Notch 功能可以被调节的一种新方法。
