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Routing of Hansenula polymorpha alcohol oxidase: An alternative peroxisomal protein-sorting machinery

机译:多形汉逊酵母乙醇氧化酶的路线:一种过氧化物酶体蛋白分选机制

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Import of Hansenula polymorpha alcohol oxidase (AO) into peroxisomes is dependent on the PTS1 receptor, HpPex5p. The PTS1 of AO (-LARF) is sufficient to direct reporter proteins to peroxisomes. To study AO sorting in more detail, strains producing mutant AO proteins were constructed. AO containing a mutation in the FAD binding fold was mislocalized to the cytosol. This indicates that the PTS1 of AO is not sufficient for import of AO. AO protein in which the PTS1 was destroyed (-LARA) was normally sorted to peroxisomes. Moreover, C-terminal deletions of up to 16 amino acids did not significantly affect AO import, indicating that the PTS1 was not necessary for targeting. Consistent with these observations we found that AO import occurred independent from the C-terminal TPR-domain of HpPex5p, known to bind PTS1 peptides. Synthesis of the N-terminal domain (amino acids 1-272) of HpPex5p in pex5 cells restored AO import, whereas other PTS1 proteins were mislocalized to the cytosol. These data indicate that AO is imported via a novel HpPex5p-dependent protein translocation pathway, which does not require the PTS1 of AO and the C-terminal TPR domains of HpPex5p, but involves FAD binding and the N-terminus of HpPex5p. [References: 46]
机译:汉逊酵母多形汉斯醇氧化酶(AO)的导入过氧化物酶体取决于PTS1受体HpPex5p。 AO的PTS1(-LARF)足以将报告蛋白引导至过氧化物酶体。为了更详细地研究AO分选,构建了产生突变AO蛋白的菌株。 FAD结合折叠中包含突变的AO错位到细胞质中。这表明AO的PTS1不足以导入AO。通常将其中PTS1被破坏的AO蛋白(-LARA)分类为过氧化物酶体。此外,最多16个氨基酸的C末端缺失不会显着影响AO的导入,这表明PTS1并不是靶向的必要条件。与这些观察结果一致,我们发现AO的导入独立于已知与PTS1肽结合的HpPex5p的C端TPR域。在pex5细胞中HpPex5p的N末端结构域(氨基酸1-272)的合成恢复了AO的导入,而其他PTS1蛋白则错位到了细胞质中。这些数据表明,AO是通过一种新型的HpPex5p依赖性蛋白转运途径导入的,该途径不需要AO的PTS1和HpPex5p的C端TPR结构域,但涉及FAD结合和HpPex5p的N末端。 [参考:46]

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