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将灭活汉坦病毒感染细胞进行冷冻固定作为一种获得用于电子显微镜研究的高质量超微结构保存的方法。

Cryofixation of Inactivated Hantavirus-Infected Cells as a Method for Obtaining High-Quality Ultrastructural Preservation for Electron Microscopic Studies.

作者信息

Parvate Amar, Sengupta Ranjan, Williams Evan P, Xue Yi, Chu Yong-Kyu, Stahelin Robert V, Jonsson Colleen B

机构信息

Department of Biological Sciences, Purdue University, West Lafayette, IN, United States.

Medicinal Chemistry and Molecular Pharmacology and the Purdue Institute for Inflammation, Immunology and Infectious Disease, Purdue University, West Lafayette, IN, United States.

出版信息

Front Cell Infect Microbiol. 2020 Nov 6;10:580339. doi: 10.3389/fcimb.2020.580339. eCollection 2020.

Abstract

Hantaviruses rewire the host cell and induce extensive membrane rearrangements for their replication and the morphogenesis of the virion. Transmission electron microscopy (TEM) is a powerful technique for imaging these pathological membrane changes especially when combined with large volume electron tomography. Excellent preservation of membrane structure can be obtained when chemical fixation is combined with cryofixation via high pressure freezing making the samples amenable to serial-section tomographic reconstruction. Taking advantage of this, we have optimized a hybrid method that employs aldehyde fixation, a step that is essential for virus inactivation, followed by high-pressure freezing for ultrastructural study of Hantaan (HTN) and Andes (AND) virus infected Vero E6 cells. HTNV and ANDV are two species of the , from the Old and New World, respectively, and the causative agents of hemorrhagic fever with renal syndrome and hantavirus pulmonary syndrome in humans. We applied the method for the qualitative assessment of the perturbation of the endomembrane system induced by HTNV and ANDV in infected vs. mock-infected cells. Screening of serial-sections revealed consistency of membrane preservation across large volumes indicating potential of these samples for tomographic studies. Images revealed large-scale perturbations of the endomembrane system following HTNV-infection that included the dilation of the rough endoplasmic reticulum and fragmentation of the Golgi apparatus. Infected cells exhibited a tendency to accumulate large numbers of vacuoles that were especially apparent in ANDV. In summary, our hybrid method provides a path for the study of BSL-3 pathogens using cutting edge 3D-imaging technologies.

摘要

汉坦病毒重塑宿主细胞,并诱导广泛的膜重排以进行病毒复制和病毒粒子的形态发生。透射电子显微镜(TEM)是一种用于对这些病理性膜变化进行成像的强大技术,特别是与大体积电子断层扫描相结合时。当化学固定与通过高压冷冻的低温固定相结合时,可以获得出色的膜结构保存效果,使样品适合进行连续切片断层重建。利用这一点,我们优化了一种混合方法,该方法采用醛固定(这是病毒灭活必不可少的步骤),然后进行高压冷冻,用于对感染汉滩(HTN)病毒和安第斯(AND)病毒的Vero E6细胞进行超微结构研究。HTNV和ANDV分别是旧大陆和新大陆的两种汉坦病毒,是人类肾综合征出血热和汉坦病毒肺综合征的病原体。我们应用该方法对感染和未感染的细胞中HTNV和ANDV诱导的内膜系统扰动进行定性评估。连续切片的筛选显示,大量样本的膜保存具有一致性,表明这些样本具有进行断层扫描研究的潜力。图像显示,HTNV感染后内膜系统出现大规模扰动,包括粗面内质网扩张和高尔基体碎片化。感染的细胞表现出积累大量液泡的趋势,这在ANDV感染的细胞中尤为明显。总之,我们的混合方法为使用前沿的3D成像技术研究生物安全3级病原体提供了一条途径。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f2b3/7677528/8230d22a91bc/fcimb-10-580339-g0001.jpg

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