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来自寄生蜂的毒液囊泡有助于毒液蛋白进入宿主免疫细胞。

Venom vesicles from the parasitoid facilitate venom protein entry into host immune cells.

作者信息

Bretz Nicholas M, Lark Chris, Perkel Sarah, Jackson Rebecca, Driskell Jeremy D, Mobley James A, Mortimer Nathan T

机构信息

Department of Biochemistry & Biophysics, Oregon State University, Corvallis, OR, USA.

School of Biological Sciences, Illinois State University, Normal, IL, USA.

出版信息

bioRxiv. 2025 May 14:2025.05.08.652939. doi: 10.1101/2025.05.08.652939.

DOI:10.1101/2025.05.08.652939
PMID:40463271
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12132199/
Abstract

The parasitoid wasp infects larvae, laying an egg and injecting venom directly into the host body cavity. While infected hosts mount an immune response in an attempt to eliminate the parasitoid egg, parasitoid venom proteins act to inhibit these host immune responses and manipulate host physiology to ensure infection success. A key immune suppressive venom protein in is a venom-specific isoform of the SERCA (Sarco/endoplasmic reticulum Ca-ATPase) calcium pump. However, SERCA is a large hydrophobic protein, and the mechanism by which it and other venom proteins are transported into the host is not well understood. We used a variety of biophysical, biochemical, and cell biological approaches to assess the properties of venom. Electronic microscopy and nanoparticle tracking analysis revealed the presence of venom vesicles as a putative transport mechanism. We used tunable resistive pulse sensing (TRPS) to biophysically characterize these vesicles, and our TRPS data suggest venom is composed of multiple vesicle types that are distinguishable by size, zeta potential, and density. Finally, we fluorescently labeled venom vesicles to test for entry into host immune cells. We observed that these vesicles interact with immune cells membranes and are internalized into the cell. Our data support a model in which venom proteins, including SERCA, are packaged into an array of venom vesicles, and transported into host cells for immune suppression.

摘要

寄生蜂会感染幼虫,将卵产在宿主体腔内并直接注入毒液。虽然被感染的宿主会产生免疫反应以试图清除寄生蜂的卵,但寄生蜂毒液蛋白会抑制这些宿主免疫反应并操控宿主生理机能以确保感染成功。其中一种关键的免疫抑制毒液蛋白是肌浆网/内质网钙ATP酶(SERCA)钙泵的毒液特异性异构体。然而,SERCA是一种大型疏水蛋白,其以及其他毒液蛋白进入宿主的机制尚不清楚。我们使用了多种生物物理、生化和细胞生物学方法来评估毒液的特性。电子显微镜和纳米颗粒跟踪分析揭示了毒液囊泡的存在,这是一种假定的运输机制。我们使用可调电阻脉冲传感(TRPS)对这些囊泡进行生物物理表征,我们的TRPS数据表明毒液由多种囊泡类型组成,这些囊泡可通过大小、zeta电位和密度来区分。最后,我们用荧光标记毒液囊泡以测试其是否进入宿主免疫细胞。我们观察到这些囊泡与免疫细胞膜相互作用并被内化到细胞中。我们的数据支持这样一种模型,即包括SERCA在内的毒液蛋白被包装成一系列毒液囊泡,并被运输到宿主细胞中以实现免疫抑制。

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Venom vesicles from the parasitoid facilitate venom protein entry into host immune cells.来自寄生蜂的毒液囊泡有助于毒液蛋白进入宿主免疫细胞。
bioRxiv. 2025 May 14:2025.05.08.652939. doi: 10.1101/2025.05.08.652939.
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本文引用的文献

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The venom of Habrobracon hebetor induces alterations in host metabolism.平腹小蜂毒液能诱导宿主代谢发生改变。
J Exp Biol. 2024 Sep 1;227(17). doi: 10.1242/jeb.247694. Epub 2024 Sep 10.
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FlyBase: updates to the Drosophila genes and genomes database.FlyBase:果蝇基因和基因组数据库的更新。
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The lipid composition of extracellular vesicles: applications in diagnostics and therapeutic delivery.细胞外囊泡的脂质组成:在诊断和治疗递送中的应用。
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Parasitoid Wasps Can Manipulate Host Trehalase to the Benefit of Their Offspring.寄生蜂可以操纵宿主的海藻糖酶,以利于其后代。
Insects. 2022 Sep 13;13(9):833. doi: 10.3390/insects13090833.
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Hematopoietic plasticity mapped in and other insects.在 和其他昆虫中绘制造血可塑性图谱。
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ggVennDiagram: An Intuitive, Easy-to-Use, and Highly Customizable R Package to Generate Venn Diagram.ggVennDiagram:一个用于生成维恩图的直观、易用且高度可定制的R包。
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KEGG mapping tools for uncovering hidden features in biological data.KEGG 映射工具可用于揭示生物数据中的隐藏特征。
Protein Sci. 2022 Jan;31(1):47-53. doi: 10.1002/pro.4172. Epub 2021 Aug 26.
8
A parasitoid wasp of Drosophila employs preemptive and reactive strategies to deplete its host's blood cells.一种寄生蜂会采用先发制人和反应性策略来消耗其宿主的血细胞。
PLoS Pathog. 2021 May 28;17(5):e1009615. doi: 10.1371/journal.ppat.1009615. eCollection 2021 May.
9
New Lipophilic Fluorescent Dyes for Labeling Extracellular Vesicles: Characterization and Monitoring of Cellular Uptake.用于标记细胞外囊泡的新型亲脂性荧光染料:细胞摄取的表征与监测
Bioconjug Chem. 2021 Apr 21;32(4):680-684. doi: 10.1021/acs.bioconjchem.1c00068. Epub 2021 Mar 13.
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Measuring particle concentration of multimodal synthetic reference materials and extracellular vesicles with orthogonal techniques: Who is up to the challenge?用正交技术测量多模态合成参比材料和细胞外囊泡的颗粒浓度:谁能应对挑战?
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