AI Article Synopsis
- Glycoprotein therapeutics play a vital role in the biopharmaceutical industry, serving large patient populations and generating significant revenue, but their purification processes are complex and yield losses are common.
- The lack of a reliable affinity platform method complicates the development of effective chromatographic steps, and affinity tags can interfere with protein characteristics despite offering some solutions.
- This chapter introduces a novel approach using elastin-like polypeptide (ELP) and self-cleaving split inteins for the one-step purification of tagless glycoproteins, demonstrating its effectiveness with the highly purified anti-ErbB2 ML39 scFv from Expi293F cells.
Article Abstract
Glycoprotein therapeutics are currently used by large patient populations and generate significant revenue for the biopharmaceutical industry. These therapeutic proteins are currently purified at industrial scale using individualized processes involving multiple chromatographic steps. In the absence of a viable affinity platform method, the required chromatographic steps are difficult to develop and inevitably lead to significant yield losses. Further, during preclinical development, there is a need for reliable platform technologies capable of performing high-throughput screening for biologic candidates. Although affinity tags can provide a solution to some of these challenges, they require specific affinity resins, and the tag itself can interfere with the target protein characteristics. Fusion protein systems consisting of elastin-like polypeptide (ELP) and self-cleaving split inteins such as Npu DnaE can serve as potential non-chromatographic platform technologies for the single-step purification of tagless glycoproteins expressed in mammalian cells. In this chapter, we demonstrate the use of this technology to obtain highly purified anti-ErbB2 ML39 single-chain variable fragment (scFv) expressed from Expi293F suspension cells.
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| http://dx.doi.org/10.1007/978-1-0716-3362-5_13 | DOI Listing |
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