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KPI 结构域控制 APP 二聚化、运输和加工的结构特征。

Structural features of the KPI domain control APP dimerization, trafficking, and processing.

机构信息

Institute of Neuroscience, Université Catholique de Louvain, Brussels, Belgium.

出版信息

FASEB J. 2012 Feb;26(2):855-67. doi: 10.1096/fj.11-190207. Epub 2011 Nov 15.

Abstract

The two major isoforms of human APP, APP695 and APP751, differ by the presence of a Kunitz-type protease inhibitor (KPI) domain in the extracellular region. APP processing and function is thought to be regulated by homodimerization. We used bimolecular fluorescence complementation (BiFC) to study dimerization of different APP isoforms and mutants. APP751 was found to form significantly more homodimers than APP695. Mutation of dimerization motifs in the TM domain did not affect fluorescence complementation, but native folding of KPI is critical for APP751 homodimerization. APP751 and APP695 dimers were mostly localized at steady state in the Golgi region, suggesting that most of the APP751 and 695 dimers are in the secretory pathway. Mutation of the KPI led to the retention of the APP homodimers in the endoplasmic reticulum. We finally showed that APP751 is more efficiently processed through the nonamyloidogenic pathway than APP695. These findings provide new insight on the particular role of KPI domain in APP dimerization. The correlation observed between dimerization, subcellular localization, and processing suggests that dimerization acts as an efficient regulator of APP trafficking in the secretory compartments that has major consequences on its processing.

摘要

人源 APP 的两种主要同工型 APP695 和 APP751,在细胞外区域的结构上存在一个 Kunitz 型蛋白酶抑制剂(KPI)结构域。APP 的加工和功能被认为是受同源二聚化调控的。我们使用双分子荧光互补(BiFC)来研究不同 APP 同工型和突变体的二聚化。结果发现 APP751 比 APP695 形成更多的同源二聚体。TM 结构域的二聚化基序突变不影响荧光互补,但 KPI 的天然折叠对 APP751 同源二聚化至关重要。APP751 和 APP695 二聚体在稳态时主要定位于高尔基区,这表明大多数 APP751 和 695 二聚体处于分泌途径中。KPI 突变导致 APP 同源二聚体在内质网中滞留。我们最终表明,APP751 通过非淀粉样蛋白生成途径比 APP695 更有效地被加工。这些发现为 KPI 结构域在 APP 二聚化中的特殊作用提供了新的见解。观察到的二聚化、亚细胞定位和加工之间的相关性表明,二聚化作为一种有效的 APP 运输调节剂,在分泌区室中发挥作用,对其加工有重大影响。

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