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Rapid and scalable purification of Escherichia coli active ribosomes using strong anion exchange spin columnsopen access

Authors
Yu, Ji HyunKim, HyegyungIyappan, KathirvelLee, JoongooYun, HyungdonKang, Taek Jin
Issue Date
Dec-2025
Publisher
한국생물공학회
Keywords
Anion exchange chromatography; Protein synthesis; Ribosome purification; Spin column
Citation
Biotechnology and Bioprocess Engineering, v.30, no.6, pp 1083 - 1092
Pages
10
Indexed
SCIE
SCOPUS
KCI
Journal Title
Biotechnology and Bioprocess Engineering
Volume
30
Number
6
Start Page
1083
End Page
1092
URI
https://scholarworks.dongguk.edu/handle/sw.dongguk/62255
DOI
10.1007/s12257-025-00246-2
ISSN
1226-8372
1976-3816
Abstract
Purification of active ribosomes is a prerequisite to studying ribosome functions. However, conventional purification methods such as ultracentrifugation, affinity tagging, and specialized chromatography present difficulties limiting their widespread use especially in laboratories with standard equipment. Here we describe a rapid and scalable method for purifying functionally active 70S ribosomes from Escherichia coli using strong anion exchange spin columns. Following optimization of buffer conditions for purification and precipitation steps for concentration, ribosomes can be prepared for cell-free protein synthesis in less than 1 h using only standard laboratory resources. The approach is successfully applied to both small- and large-scale samples, recovering ribosomes with translational activity up to 70% of commercial standards and protein/RNA compositions comparable to established protocols. This versatile technique streamlines ribosome purification, enabling efficient access for studies in structural biology, antibiotic screening, and translational regulation, especially where resources or sample volumes are constrained. © The Author(s), under exclusive licence to The Korean Society for Biotechnology and Bioengineering 2025.
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