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表面活性蛋白C前体蛋白向远端加工区室的顺行运输需要PPDY介导的与Nedd4泛素连接酶的结合。

Anterograde transport of surfactant protein C proprotein to distal processing compartments requires PPDY-mediated association with Nedd4 ubiquitin ligases.

作者信息

Kotorashvili Adam, Russo Scott J, Mulugeta Surafel, Guttentag Susan, Beers Michael F

机构信息

From the Surfactant Biology Laboratories, Department of Medicine, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104.

Division of Neonatology, Department of Pediatrics, Children's Hospital of Philadelphia, Philadelphia, Pennsylvania 19104.

出版信息

J Biol Chem. 2009 Jun 12;284(24):16667-16678. doi: 10.1074/jbc.M109.002816. Epub 2009 Apr 14.

DOI:10.1074/jbc.M109.002816
PMID:19366705
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2713532/
Abstract

Biosynthesis of surfactant protein C (SP-C) by alveolar type 2 cells requires proteolytic processing of a 21-kDa propeptide (proSP-C21) in post-Golgi compartments to yield a 3.7-kDa mature form. Scanning alanine mutagenesis, binding assays, and co-immunoprecipitation were used to characterize the proSP-C targeting domain. Delivery of proSP-C21 to distal processing organelles is dependent upon the NH2-terminal cytoplasmic SP-C propeptide, which contains a conserved PPDY motif. In A549 cells, transfection of EGFP/proSP-C21 constructs containing polyalanine substitution for Glu11-Thr18, 13PPDY16, or 14P,16Y produced endoplasmic reticulum retention of the fusion proteins. Protein-protein interactions of proSP-C with known WW domains were screened using a solid-phase array that revealed binding of the proSP-C NH2 terminus to several WW domains found in the Nedd4 family of E3 ligases. Specificity of the interaction was confirmed by co-immunoprecipitation of proSP-C and Nedd4 or Nedd4-2 in epithelial cell lines. By Western blotting and reverse transcription-PCR, both forms were detected in primary human type 2 cells. Knockdown of Nedd4-2 by small interference RNA transfection of cultured human type 2 cells blocked processing of 35S-labeled proSP-C21. Mutagenesis of potential acceptor sites for ubiquitination in the cytosolic domain of proSP-C (Lys6, Lys34, or both) failed to inhibit trafficking of EGFP/proSP-C21. These results indicate that PPDY-mediated interaction with Nedd4 E3-ligases is required for trafficking of proSP-C. We speculate that the Nedd4/proSP-C tandem is part of a larger protein complex containing a ubiquitinated component that further directs its transport.

摘要

肺泡Ⅱ型细胞合成表面活性蛋白C(SP-C)需要在高尔基体后区室对21 kDa的前体肽(proSP-C21)进行蛋白水解加工,以产生3.7 kDa的成熟形式。采用扫描丙氨酸诱变、结合试验和免疫共沉淀来表征proSP-C靶向结构域。proSP-C21向远端加工细胞器的转运取决于NH2末端细胞质SP-C前体肽,其包含一个保守的PPDY基序。在A549细胞中,转染含有将Glu11-Thr18、13PPDY16或14P、16Y替换为聚丙氨酸的EGFP/proSP-C21构建体导致融合蛋白在内质网中滞留。使用固相阵列筛选proSP-C与已知WW结构域的蛋白质-蛋白质相互作用,结果显示proSP-C的NH2末端与E3连接酶Nedd4家族中发现的几个WW结构域结合。通过上皮细胞系中proSP-C与Nedd4或Nedd4-2的免疫共沉淀证实了相互作用的特异性。通过蛋白质印迹和逆转录PCR,在原代人Ⅱ型细胞中检测到了这两种形式。通过对培养的人Ⅱ型细胞进行小干扰RNA转染敲低Nedd4-2可阻断35S标记的proSP-C21的加工。对proSP-C胞质结构域中潜在泛素化受体位点(Lys6、Lys34或两者)进行诱变未能抑制EGFP/proSP-C21的转运。这些结果表明,proSP-C的转运需要PPDY介导的与Nedd4 E3连接酶的相互作用。我们推测Nedd4/proSP-C串联体是一个更大的蛋白质复合物的一部分,该复合物包含一个泛素化成分,进一步指导其运输。

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