High‐efficiency affinity precipitation of multiple industrial mAbs and Fc‐fusion proteins from cell culture harvests using Z‐ELP‐E2 nanocages

Swartz, Andrew R.; Xu, Xuankuo; Traylor, Steven J.; Li, Zheng Jian; Chen, Wilfred

doi:10.1002/bit.26717

Cited by 14 publications

(16 citation statements)

References 25 publications

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“…The estimated HCP removal is 910-fold for the combination of the dewatering and washing steps, which is similar to, if not better than, the HCP reduction after a typical platform Protein A chromatography capture step. 11 The capacity of the bench-scale apparatus is 7.2 g mAb/day using the three membrane modules (one for dewatering and two for washing) each with 0.01 m 2 area. Expected buffer consumption is 0.9 L/g mAb.…”

Section: Transient Behaviormentioning

confidence: 99%

“…1,2 There is also growing interest in the use of precipitation for the initial purification (capture) of monoclonal antibody (mAb) products due to the significant increase in product titer that have been achieved over the past two decades. 3,4 mAbs have been successfully precipitated using cold ethanol and CaCl 2, 5 polyethylene glycol (PEG), 6 PEG and CaCl 2, 7 CaCl 2 and caprylic acid, 8 PEG and low pH 9 , zinc chloride (ZnCl 2 ) and PEG, 10 and elastin-like polypeptides (ELP) 11,12 among others.…”

Section: Introductionmentioning

confidence: 99%

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Enhanced filtration performance usingfeed‐and‐bleedconfiguration for purification of antibody precipitates

Zhao

Chen

Andini

et al. 2020

Biotechnology Progress

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Precipitation can be used for the initial purification of monoclonal antibodies (mAbs), with the soluble host cell proteins removed in the permeate by tangential flow microfiltration. The objective of this study was to examine the use of a feed-andbleed configuration to increase the effective conversion (ratio of permeate to feed flow rates) in the hollow fiber module to enable more effective washing of the precipitate. Experiments were performed using human serum Immunoglobulin G (IgG) precipitates formed with 10 mM zinc chloride and 7 wt% polyethylene glycol. The critical flux was evaluated as a function of the shear rate and IgG concentration, with the resulting correlation used to predict conditions that can achieve 90% conversion in a single pass with minimal fouling. Experimental data for both the start-up and steady-state performance are in good agreement with model calculations. These results were used to analyze the performance of an enhanced continuous precipitation-microfiltration process using the feed-and-bleed configuration for the initial capture / purification of a mAb product.

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Section: Transient Behaviormentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Enhanced filtration performance usingfeed‐and‐bleedconfiguration for purification of antibody precipitates

Zhao

Chen

Andini

et al. 2020

Biotechnology Progress

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“…Other technologies such as affinity precipitation and aqueous two‐phase systems (ATPS) have also been investigated as alternative downstream processing technologies to chromatographic purification. For example, affinity precipitation has been viewed as a cost‐effective and scalable alternative to affinity chromatography, but there are still some issues to overcome for this technology, such as co‐precipitation of contaminants and the use of harsh chemicals in affinity precipitation 16–19 . ATPS may be another attractive technology which performs multiple tasks for the extraction and purification of biological products using phase‐forming solvents 20–23 .…”

Section: Technologies For Legacy Process Improvementmentioning

confidence: 99%

Overcoming challenges of improving legacy biopharmaceutical processes

Gao¹,

Gervais²

2021

J of Chemical Tech & Biotech

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Continuous process improvement of biopharmaceutical processes is an expectation of the current regulatory environment (e.g. ICH Q8 and Q10), and extends to older products as well as new licences. Particularly in the case of older products, process changes are also often simply required to improve process efficiency, to facilitate easier manufacture and to update materials such as chromatography resins and filters that may become unavailable due to age. These older processes, or legacy processes, present unique challenges for process improvement. This paper discusses the challenges and strategies of implementing changes and new technologies for improving legacy manufacturing processes, and outlines the issues to be addressed during process redevelopment and validation, including product and process characterisation and particular regulatory constraints to ensure product profile and quality are maintained when making process changes. Case studies are presented, with a focus on adaptation of single‐use technologies for commercial biopharmaceutical processes. © 2021 Society of Chemical Industry (SCI).

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“…A peptide or biopolymer featuring a Protein A epitope is introduced to the cell culture and binds the desired mAb, subsequently inducing precipitation. Upon isolation and washing of the precipitate, the mAb can be released into solution by pH modulation, allowing further purification …”

Section: Introductionmentioning

confidence: 99%

“…Upon isolation and washing of the precipitate, the mAb can be released into solution by pH modulation, allowing further purification. 16,17 Other methods to overcome the challenges chromatin/DNA presents to Protein A chromatography involve modifying the operating conditions for Protein A chromatography itself. One strategy used chromatofocusing using a pH gradient through the Protein A column to reduce HCP coelution with the target mAb.…”

Section: Introductionmentioning

confidence: 99%

Enhancing Protein A performance in mAb processing: A method to reduce and rapidly evaluate host cell DNA levels during primary clarification

Koehler

Jokondo

Narayan

et al. 2019

Biotechnology Progress

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The use and impact of 3M™ Emphaze™ AEX Hybrid Purifier, a single‐use, fully synthetic chromatographic product, was explored to reduce host cell DNA (HC‐DNA) concentration during the primary clarification of a monoclonal antibody (mAb). An approximately 5‐log reduction in HC‐DNA was achieved at an Emphaze AEX Hybrid Purifier throughput of 200 L/m2. The appreciable reduction in HC‐DNA achieved during primary clarification enhanced Protein A chromatography performance, resulting in a sharper and narrower elution profile. In addition, a 24× improvement in host cell protein (HCP) removal and fewer impurities nonspecifically bound to the Protein A column were observed compared to those resulting from the use of depth filtration for clarification. The use of a rapid, qualitative acidification assay to facilitate HC‐DNA monitoring was also investigated. This assay involves the acidification‐induced precipitation of HC‐DNA, enabling the easy and rapid detection of DNA breakthrough across purification media such as Emphaze AEX Hybrid Purifier by means of turbidimetric and particle size measurements.

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High‐efficiency affinity precipitation of multiple industrial mAbs and Fc‐fusion proteins from cell culture harvests using Z‐ELP‐E2 nanocages

Cited by 14 publications

References 25 publications

Enhanced filtration performance usingfeed‐and‐bleedconfiguration for purification of antibody precipitates

Enhanced filtration performance usingfeed‐and‐bleedconfiguration for purification of antibody precipitates

Overcoming challenges of improving legacy biopharmaceutical processes

Enhancing Protein A performance in mAb processing: A method to reduce and rapidly evaluate host cell DNA levels during primary clarification

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