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Collagen secretion screening in Drosophila supports a common secretory machinery and multiple Rab requirements

摘要Collagens are large secreted trimeric proteins making up most of the animal extracellular matrix.Secretion of collagen has been a focus of interest for cell biologists in recent years because collagen trimers are too large and rigid to fit into the COPII vesicles mediating transport from the endoplasmic reticulum (ER) to the Golgi.Collagen-specific mechanisms to create enlarged ER-to-Golgi transport carriers have been postulated,including cargo loading by conserved ER exit site (ERES) protein Tango1.Here,we report an RNAi screening for genes involved in collagen secretion in Drosophila.In this screening,we examined distribution of GFP-tagged Collagen Ⅳ in live animals and found 88 gene hits for which the knockdown produced intracellular accumulation of Collagen Ⅳ in the fat body,the main source of matrix proteins in the larva.Among these hits,only two affected collagen secretion specifically:PH4αEFB and Plod,encoding enzymes known to mediate posttranslational modification of collagen in the ER.Every other intracellular accumulation hit affected general secretion,consistent with the notion that secretion of collagen does not use a specific mode of vesicular transport,but the general secretory pathway.Included in our hits are many known players in the eukaryotic secretory machinery,like COPII and COPI components,SNAREs and Rab-GTPase regulators.Our further analysis of the involvement of Rab-GTPases in secretion shows that Rabl,Rab2 and RabX3,are all required at ERES,each of them differentially affecting ERES morphology.Abolishing activity of all three by Rep knockdown,in contrast,led to uncoupling of ERES and Golgi.We additionally present a characterization of a screening hit we named trabuco (tbc),encoding an ERES-localized TBC domain-containing Rab-GAP.Finally,we discuss the success of our screening in identifying secretory pathway genes in comparison to two previous secretion screenings in Drosophila S2 cells.

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作者单位 School of Life Sciences, Tsinghua University, Beijing 100084, China [1] School of Medicine, Tsinghua University, Beijing 100084, China [2]
栏目名称 Original Research
发布时间 2018-08-27
基金项目
We thank Hugo Bellen Fujian Zhang Thomas Lecuit Sally Horne-Badovinac the Bloomington Drosophila Stock Center,the Kyoto Stock Center,the Vienna Drosophila RNAi Center,the Tsinghua Fly Center,the Drosophila Genomics Research Center the Drosophila Carnegie Vector Collection for providing fly strains,antibodies and plasmids.We also thank Yiran Zang,Xingxin Liao,Huina Jia and Shuangchun Ma for technical assistance during the screening phase of this project.This research was funded by grants from the Natural Science Foundation of Tsinghua Initiative Program a 1000 Talents award,all to J.C.P.-P
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