首页> 美国卫生研究院文献>other >PREMELANOSOME AMYLOID-LIKE FIBRILS ARE COMPOSED OF ONLY GOLGI-PROCESSED FORMS OF PMEL17 THAT HAVE BEEN PROTEOLYTICALLY PROCESSED IN ENDOSOMES
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PREMELANOSOME AMYLOID-LIKE FIBRILS ARE COMPOSED OF ONLY GOLGI-PROCESSED FORMS OF PMEL17 THAT HAVE BEEN PROTEOLYTICALLY PROCESSED IN ENDOSOMES

机译:粒前类淀粉样原纤维仅由内含蛋白质组中经过蛋白化处理的PMEL17的高尔基加工形式组成

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摘要

Melanin pigments are synthesized within specialized organelles called melanosomes and polymerize on intralumenal fibrils that form within melanosome precursors. The fibrils consist of proteolytic fragments derived from Pmel17, a pigment cell-specific integral membrane protein. The intracellular pathways by which Pmel17 accesses melanosome precursors and the identity of the Pmel17 derivatives within fibrillar melanosomes have been a matter of debate. We show here that antibodies that detect Pmel17 within fibrillar melanosomes recognize only the lumenal products of proprotein convertase cleavage and not remaining products linked to the transmembrane domain. Moreover, antibodies to the N- and C-termini detect only Pmel17 isoforms present in early biosynthetic compartments, which constitute a large fraction of detectable steady state Pmel17 in cell lysates due to slow early biosynthetic transport and rapid consumption by fibril formation. Using an antibody to a lumenal epitope that is destroyed upon modification by O-linked oligosaccharides, we show that all post-endoplasmic reticulum Pmel17 isoforms are modified by Golgi-associated oligosaccharide transferases, and that only processed forms contribute to melanosome biogenesis. These data indicate that Pmel17 follows a single biosynthetic route from the endoplasmic reticulum through the Golgi complex and endosomes to melanosomes, and that only fragments encompassing previously described functional lumenal determinants are present within the fibrils. These data have important implications for the site and mechanism of fibril formation.
机译:黑色素色素是在称为黑色素体的特殊细胞器中合成的,并在黑色素体前体中形成的腔内原纤维上聚合。原纤维由衍生自Pmel17的蛋白水解片段组成,Pmel17是色素细胞特异性整合膜蛋白。 Pmel17进入黑素体前体的细胞内途径以及原纤维黑素体中Pmel17衍生物的身份一直是争论的话题。我们在这里显示检测纤丝黑色素体内的Pmel17的抗体仅识别前蛋白转化酶裂解的腔产物,而不识别连接跨膜结构域的剩余产物。而且,针对N末端和C末端的抗体仅检测到存在于早期生物合成区室中的Pmel17同工型,由于早期的生物合成运输缓慢和原纤维形成的快速消耗,其构成了细胞裂解物中可检测到的稳态Pmel17的很大一部分。使用抗被O-连接寡糖修饰后被破坏的管腔表位的抗体,我们显示了所有内质网Pmel17亚型都被高尔基相关的寡糖转移酶修饰,并且只有经过加工的形式才有助于黑素体的生物发生。这些数据表明Pmel17遵循从内质网穿过高尔基复合体和内体到黑素体的单一生物合成途径,并且在原纤维中仅存在包含先前描述的功能性内腔决定簇的片段。这些数据对原纤维形成的部位和机理具有重要意义。

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