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纳米颗粒二次离子质谱法分析细胞外囊泡。

Nanoprojectile Secondary Ion Mass Spectrometry for Analysis of Extracellular Vesicles.

机构信息

Department of Chemistry, Texas A&M University, College Station, Texas 77843, United States.

Department of Physiology and Biomedical Engineering, Mayo Clinic, 200 1st Street SW St-11-14, Rochester, Minnesota 55905, United States.

出版信息

Anal Chem. 2021 May 25;93(20):7481-7490. doi: 10.1021/acs.analchem.1c00689. Epub 2021 May 14.

Abstract

We describe a technique based on secondary ion mass spectrometry with nanoprojectiles (NP-SIMS) for determining the protein content of extracellular vesicles, EVs, via tagged antibodies. The technique uses individual gold nanoprojectiles (e.g., Au and Au), separated in time and space, to bombard a surface. For each projectile impact (10-20 nm in diameter), the co-emitted molecules are mass analyzed and recorded as an individual mass spectrum. Examining these individual mass spectra for co-localized species allows for nanoscale mass spectrometry to be performed. The high lateral resolution of this technique is well suited for analyzing nano-objects. SIMS is generally limited to analyzing small molecules (below ∼1500 Da); therefore, we evaluated three molecules (eosin, erythrosine, and BHHTEGST) as prospective mass spectrometry tags. We tested these on a model surface comprising a mixture of all three tags conjugated to antibodies and found that NP-SIMS could detect all three tags from a single projectile impact. Applying the method, we tagged two surface proteins common in urinary EVs, CD63 and CD81, with anti-CD63-erythrosine and anti-CD81-BHHTEGST. We found that NP-SIMS could determine the relative abundance of the two proteins and required only a few hundred or thousand EVs in the analysis region to detect the presence of the tagged antibodies.

摘要

我们描述了一种基于带有纳米射弹的次级离子质谱(NP-SIMS)的技术,用于通过标记抗体来确定细胞外囊泡(EVs)的蛋白质含量。该技术使用单个金纳米射弹(例如 Au 和 Au),在时间和空间上分开,来轰击表面。对于每个射弹撞击(直径为 10-20nm),共发射的分子被质量分析并记录为单个质谱。检查这些共定位物质的单个质谱允许进行纳米级质谱分析。该技术的高横向分辨率非常适合分析纳米物体。SIMS 通常限于分析小分子(低于约 1500Da);因此,我们评估了三种分子(曙红、赤藓红和 BHHTEGST)作为潜在的质谱标记物。我们在一个模型表面上测试了这三种标记物,该表面由三种标记物与抗体共轭的混合物组成,发现 NP-SIMS 可以从单个射弹撞击中检测到所有三种标记物。应用该方法,我们用抗 CD63-赤藓红和抗 CD81-BHHTEGST 标记了两种常见于尿液 EVs 的表面蛋白 CD63 和 CD81。我们发现 NP-SIMS 可以确定这两种蛋白质的相对丰度,并且只需要在分析区域中有几百或几千个 EV 就可以检测到标记抗体的存在。

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