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Metalloprotease ADAM10 Is Required for Notch1 Site 2 Cleavage

机译:Notch1位点2切割需要金属蛋白酶ADAM10

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摘要

Notch signaling is controlled by ligand binding, which unfolds a negative control region to induce proteolytic cleavage of the receptor. First, a membrane-proximal cleavage is executed by a metalloprotease, removing the extracellular domain. This allows γ-secretase to execute a second cleavage within the Notch transmembrane domain, which releases the intracellular domain to enter the nucleus. Here we show that the ADAM10 metalloprotease Kuzbanian, but not ADAM17/tumor necrosis factor α-converting enzyme, plays an essential role in executing ligand-induced extracellular cleavage at site 2 (S2) in cells and localizes this step to the plasma membrane. Importantly, genetic or pharmacological inhibition of metalloproteases still allowed extracellular cleavage of Notch, indicating the presence of unknown proteases with the ability to cleave at S2. Gain of function mutations identified in human cancers and in model organisms that map to the negative control region alleviate the requirement for ligand binding for extracellular cleavage to occur. Because cancer-causing Notch1 mutations also depend on (rate-limiting) S2 proteolysis, the identity of these alternative proteases has important implications for understanding Notch activation in normal and cancer cells.
机译:Notch信号传导受配体结合控制,配体结合会展开阴性对照区域以诱导受体的蛋白水解切割。首先,通过金属蛋白酶执行膜近端切割,去除细胞外结构域。这允许γ-分泌酶在Notch跨膜结构域内进行第二次切割,从而释放细胞内结构域进入细胞核。在这里,我们显示ADAM10金属蛋白酶Kuzbanian,而不是ADAM17 /肿瘤坏死因子α转化酶,在细胞中第2位(S2)处执行配体诱导的细胞外裂解中起重要作用,并将这一步骤定位于质膜。重要的是,金属蛋白酶的遗传或药理抑制作用仍然允许Notch的细胞外裂解,表明存在具有在S2裂解的能力的未知蛋白酶。在人类癌症和映射到阴性对照区域的模型生物中鉴定到的功能突变的获得,减轻了配体结合发生细胞外切割的需求。由于致癌的Notch1突变也依赖于(限速)S2蛋白水解,因此这些替代蛋白酶的身份对于理解正常细胞和癌细胞中的Notch活化具有重要意义。

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