| Literature DB >> 31743597 |
Kim Le1, Christopher Tan1, Huong Le1, Jasmine Tat1, Ewelina Zasadzinska1, Jonathan Diep1, Ryan Zastrow1, Chun Chen1, Jennitte Stevens1.
Abstract
During biomanufacturing cell lines development, the generation and screening for single-cell derived subclones using methods that enable assurance of clonal derivation can be resource- and time-intensive. High-throughput miniaturization, automation, and analytic strategies are often employed to reduce such bottlenecks. The Beacon platform from Berkeley Lights offers a strategy to eliminate these limitations through culturing, manipulating, and characterizing cells on custom nanofluidic chips via software-controlled operations. However, explicit demonstration of this technology to provide high assurance of a single cell progenitor has not been reported. Here, a methodology that utilizes the Beacon instrument to ensure high levels of clonality is described. It is demonstrated that the Beacon platform can efficiently generate production cell lines with a superior clonality data package, detailed tracking, and minimal resources. A stringent in-process quality control strategy is established to enable rapid verification of clonal origin, and the workflow is validated using representative Chinese hamster ovary-derived cell lines stably expressing either green or red fluorescence protein. Under these conditions, a >99% assurance of clonal origin is achieved, which is comparable to existing imaging-coupled fluorescence-activated cell sorting seeding methods.Entities:
Keywords: Berkeley Lights; Chinese hamster ovary cells; cell line development; clonality assurance; digital cell culture
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Year: 2019 PMID: 31743597 DOI: 10.1002/biot.201900247
Source DB: PubMed Journal: Biotechnol J ISSN: 1860-6768 Impact factor: 4.677