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内质网货物受体SURF4促进促红细胞生成素的高效分泌。

The Endoplasmic Reticulum Cargo Receptor SURF4 Facilitates Efficient Erythropoietin Secretion.

作者信息

Lin Zesen, King Richard, Tang Vi, Myers Greggory, Balbin-Cuesta Ginette, Friedman Ann, McGee Beth, Desch Karl, Ozel Ayse Bilge, Siemieniak David, Reddy Pavan, Emmer Brian, Khoriaty Rami

机构信息

Department of Pharmacology, University of Michigan, Ann Arbor, Michigan, USA.

Department of Internal Medicine, University of Michigan, Ann Arbor, Michigan, USA.

出版信息

Mol Cell Biol. 2020 Nov 6;40(23). doi: 10.1128/MCB.00180-20.

Abstract

Erythropoietin (EPO) stimulates erythroid differentiation and maturation. Though the transcriptional regulation of EPO has been well studied, the molecular determinants of EPO secretion remain unknown. Here, we generated a HEK293T reporter cell line that provides a quantifiable and selectable readout of intracellular EPO levels and performed a genome-scale CRISPR screen that identified SURF4 as an important mediator of EPO secretion. Targeting with multiple independent single guide RNAs (sgRNAs) resulted in intracellular accumulation and extracellular depletion of EPO. Both of these phenotypes were rescued by expression of cDNA. Additionally, we found that disruption of SURF4 resulted in accumulation of EPO in the endoplasmic reticulum (ER) compartment and that SURF4 and EPO physically interact. Furthermore, SURF4 disruption in Hep3B cells also caused a defect in the secretion of endogenous EPO under conditions mimicking hypoxia, ruling out an artifact of heterologous overexpression. This work demonstrates that SURF4 functions as an ER cargo receptor that mediates the efficient secretion of EPO. Our findings also suggest that modulating SURF4 may be an effective treatment for disorders of erythropoiesis that are driven by aberrant EPO levels. Finally, we show that SURF4 overexpression results in increased secretion of EPO, suggesting a new strategy for more efficient production of recombinant EPO.

摘要

促红细胞生成素(EPO)刺激红细胞分化和成熟。尽管对EPO的转录调控已有深入研究,但EPO分泌的分子决定因素仍不清楚。在此,我们构建了一种HEK293T报告细胞系,它能提供细胞内EPO水平的可量化和可选择读数,并进行了全基因组规模的CRISPR筛选,确定SURF4是EPO分泌的重要介质。用多个独立的单向导RNA(sgRNA)靶向导致EPO在细胞内积累和细胞外耗竭。这两种表型都通过cDNA的表达得到挽救。此外,我们发现SURF4的破坏导致EPO在内质网(ER)区室中积累,且SURF4与EPO存在物理相互作用。此外,在模拟缺氧条件下,Hep3B细胞中SURF4的破坏也导致内源性EPO分泌缺陷,排除了异源过表达的假象。这项工作表明SURF4作为一种ER货物受体,介导EPO的有效分泌。我们的发现还表明,调节SURF4可能是治疗由异常EPO水平驱动的红细胞生成障碍的有效方法。最后,我们表明SURF4过表达导致EPO分泌增加,这为更高效生产重组EPO提出了一种新策略。

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