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Mannose 6 Dephosphorylation of Lysosomal Proteins Mediated by Acid Phosphatases Acp2 and Acp5

机译:酸性磷酸酶Acp2和Acp5介导的溶酶体蛋白的甘露糖6去磷酸化。

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摘要

Mannose 6-phosphate (Man6P) residues represent a recognition signal required for efficient receptor-dependent transport of soluble lysosomal proteins to lysosomes. Upon arrival, the proteins are rapidly dephosphorylated. We used mice deficient for the lysosomal acid phosphatase Acp2 or Acp5 or lacking both phosphatases (Acp2/Acp5−/−) to examine their role in dephosphorylation of Man6P-containing proteins. Two-dimensional (2D) Man6P immunoblot analyses of tyloxapol-purified lysosomal fractions revealed an important role of Acp5 acting in concert with Acp2 for complete dephosphorylation of lysosomal proteins. The most abundant lysosomal substrates of Acp2 and Acp5 were identified by Man6P affinity chromatography and mass spectrometry. Depending on the presence of Acp2 or Acp5, the isoelectric point of the lysosomal cholesterol-binding protein Npc2 ranged between 7.0 and 5.4 and may thus regulate its interaction with negatively charged lysosomal membranes at acidic pH. Correspondingly, unesterified cholesterol was found to accumulate in lysosomes of cultured hepatocytes of Acp2/Acp5−/− mice. The data demonstrate that dephosphorylation of Man6P-containing lysosomal proteins requires the concerted action of Acp2 and Acp5 and is needed for hydrolysis and removal of degradation products.
机译:6磷酸甘露糖(Man6P)残基代表有效的受体依赖性可溶性溶酶体蛋白向溶酶体的有效转运所需的识别信号。到达后,蛋白质迅速被去磷酸化。我们使用了缺乏溶酶体酸性磷酸酶Acp2或Acp5或缺乏两种磷酸酶(Acp2 / Acp5 -/-)的小鼠来检查它们在含Man6P蛋白质的去磷酸化中的作用。泰洛沙泊纯化的溶酶体级分的二维(2D)Man6P免疫印迹分析显示,Acp5与Acp2协同作用对于溶酶体蛋白的完全去磷酸化具有重要作用。通过Man6P亲和色谱法和质谱法鉴定了Acp2和Acp5的最丰富的溶酶体底物。取决于Acp2或Acp5的存在,溶酶体胆固醇结合蛋白Npc2的等电点范围为7.0至5.4,因此可以调节其与酸性pH下带负电荷的溶酶体膜的相互作用。相应地,发现未酯化的胆固醇积聚在Acp2 / Acp5 -/-小鼠培养的肝细胞的溶酶体中。数据表明,含Man6P的溶酶体蛋白的去磷酸化需要Acp2和Acp5的协同作用,并且是水解和去除降解产物所必需的。

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