Peptide ligands for the universal purification of exosomes by affinity chromatography

IF 3.5 2区生物学 Q2 BIOTECHNOLOGY & APPLIED MICROBIOLOGY

Biotechnology and Bioengineering Pub Date : 2024-08-04 DOI:10.1002/bit.28821

Ryan E. Kilgore, Brandyn D. Moore, Sobhana A. Sripada, Wenning Chu, Shriarjun Shastry, Eduardo Barbieri, Shiqi Hu, Weihua Tian, Heidi Petersen, Mohammad Mohammadifar, Aryssa Simpson, Ashley Brown, Joseph Lavoie, Driss Elhanafi, Steffen Goletz, Ke Cheng, Michael A. Daniele, Stefano Menegatti

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引用次数: 0

Abstract

Exosomes are gaining prominence as vectors for drug delivery, vaccination, and regenerative medicine. Owing to their surface biochemistry, which reflects the parent cell membrane, these nanoscale biologics feature low immunogenicity, tunable tissue tropism, and the ability to carry a variety of payloads across biological barriers. The heterogeneity of exosomes' size and composition, however, makes their purification challenging. Traditional techniques, like ultracentrifugation and filtration, afford low product yield and purity, and jeopardizes particle integrity. Affinity chromatography represents an excellent avenue for exosome purification. Yet, current affinity media rely on antibody ligands whose selectivity grants high product purity, but mandates the customization of adsorbents for exosomes with different surface biochemistry while their binding strength imposes elution conditions that may harm product's activity. Addressing these issues, this study introduces the first peptide affinity ligands for the universal purification of exosomes from recombinant feedstocks. The peptides were designed to (1) possess promiscuous biorecognition of exosome markers, without binding process-related contaminants and (2) elute the product under conditions that safeguard product stability. Selected ligands SNGFKKHI and TAHFKKKH demonstrated the ability to capture of exosomes secreted by 14 cell sources and purified exosomes derived from HEK293, PC3, MM1, U87, and COLO1 cells with yields of up to 80% and up-to 50-fold reduction of host cell proteins (HCPs) upon eluting with pH gradient from 7.4 to 10.5, recommended for exosome stability. SNGFKKHI-Toyopearl resin was finally employed in a two-step purification process to isolate exosomes from HEK293 cell fluids, affording a yield of 68% and reducing the titer of HCPs to 68 ng/mL. The biomolecular and morphological features of the isolated exosomes were confirmed by analytical chromatography, Western blot analysis, transmission electron microscopy, nanoparticle tracking analysis.

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通过亲和层析法普遍纯化外泌体的肽配体。

作为药物输送、疫苗接种和再生医学的载体，外泌体的作用日益突出。由于外泌体的表面生物化学反映了母细胞膜，因此这些纳米级生物制剂具有免疫原性低、组织滋养性可调以及能够携带各种有效载荷穿越生物屏障等特点。然而，由于外泌体的大小和组成具有异质性，因此对其进行纯化具有挑战性。超速离心和过滤等传统技术的产物产量和纯度都很低，而且会危及颗粒的完整性。亲和色谱法是外泌体纯化的绝佳途径。然而，目前的亲和介质依赖于抗体配体，这种配体的选择性可获得高纯度的产品，但却要求针对不同表面生化性质的外泌体定制吸附剂，而其结合强度所带来的洗脱条件可能会损害产品的活性。为了解决这些问题，本研究首次推出了用于从重组原料中通用纯化外泌体的多肽亲和配体。这些肽的设计目的是：（1）对外泌体标记物具有杂乱的生物识别能力，不会结合与过程相关的污染物；（2）在保障产品稳定性的条件下洗脱产品。所选配体 SNGFKKHI 和 TAHFKKKH 证明能够捕获 14 种细胞来源分泌的外泌体，并纯化了来自 HEK293、PC3、MM1、U87 和 COLO1 细胞的外泌体。最后，SNGFKKHI-Toyopearl 树脂被用于两步纯化过程，从 HEK293 细胞液中分离出外泌体，产率达 68%，HCPs 的滴度降至 68 ng/mL。分析色谱、Western 印迹分析、透射电子显微镜和纳米粒子追踪分析证实了分离出的外泌体的生物分子和形态特征。

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来源期刊

Biotechnology and Bioengineering 工程技术-生物工程与应用微生物

CiteScore

7.90

自引率

5.30%

发文量

280

审稿时长

2.1 months

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