Rapid development of stable transgene CHO cell lines by CRISPR/Cas9-mediated site-specific integration into C12orf35

Zhao, Menglin; Wang, Jiaxian; Luo, Manyu; Luo, Han; Zhao, Meiqi; Han, Lei; Zhang, Mengxiao; Yang, Hui; Xie, Yueqing; Jiang, Hua; Feng, Lei; Lu, Huili; Zhu, Jianwei

doi:10.1007/s00253-018-9021-6

Cited by 55 publications

(43 citation statements)

References 36 publications

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“…They found that C12orf35 locus (a telomeric region of chromosome 8) [ 34 ] was the most advantageous among these three genes. [ 35 ] T site of ywhae gene that we found in this study is the potential genome hotspot to construct cell lines for recombinant protein production. Further study will be needed for this information.…”

Section: Discussionmentioning

confidence: 87%

An Efficient Exogenous Gene Insertion Site in CHO Cells with High Transcription Level to Enhance AID‐Induced Mutation

Fan

Jiang

Ran

et al. 2020

Biotechnology Journal

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Antibodies have been extensively used for the purpose of scientific research, clinical diagnosis, and therapy. Combination of in vitro somatic hypermutation and mammalian cell surface display has been an efficient technology for antibody or other proteins optimization, in which the efficiency of activation-induced cytidine deaminase (AID) mutations in genes is one of the most important key factors. Gene transcriptional level has been found to be positively proportional to AID-induced mutation frequency. Thus, construction of the cell clone bearing a gene of interest (GOI) with high transcription level can increase AID-induced mutations. In this study, a retargetable gene cassette is inserted onto predetermined chromosome site (ywhae gene site) which is among the genes with the highest as well as stable transcription, and is found that one subsite is suitable to be retargeted for efficient protein display in Chinese hamster ovary (CHO) cells. The resultant cell clone (T31) has higher and more stable transcription/expression than CHO-puro clone which was previously established through the strategy of random insertion followed by a high-throughput selection. It also possesses a significantly higher mutation frequency to GOI than CHO-puro cells; thus, it is a better clone for the in vitro improvement of antibody affinity, and probably other properties.

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Section: Discussionmentioning

confidence: 87%

An Efficient Exogenous Gene Insertion Site in CHO Cells with High Transcription Level to Enhance AID‐Induced Mutation

Fan

Jiang

Ran

et al. 2020

Biotechnology Journal

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“…In prior works, the use of HDR-mediated SSI with linear donor DNA, sometimes referred to as homology-mediated end joining (HMEJ), was accomplished via nuclease-mediated cleavage and release of circular plasmids in vivo [21,37,50,51]. Nonetheless, we observed a 2.3fold improvement in SSI efficiency when using a PCR-amplified linear HDR donor compared with a plasmid HDR donor (both with similar homology arm lengths), which matches previously documented efficiency gains when comparing the two donor formats [21,50,51]. Together, our findings show the functionality of the reporter system and promote the use of linearized HDR donors to improve SSI efficiency relative to other DSB repair strategies.…”

Section: Comparison Of Repair Pathways For Ssi: Hdr Is Most Efficientmentioning

confidence: 99%

A Site‐Specific Integration Reporter System That Enables Rapid Evaluation of CRISPR/Cas9‐Mediated Genome Editing Strategies in CHO Cells

Hamaker

Lee

2020

Biotechnology Journal

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Abbreviations: bGHpA, bovine growth hormone polyadenylation signal; Cas9, CRISPRassociated protein 9; CHO, Chinese hamster ovary; CLD, cell line development; CRISPR, clustered regularly interspaced short palindromic repeats; DSB, double-strand break; eGFP, enhanced green fluorescent protein; FACS, fluorescence-activated cell sorting; gRNA, guide RNA; hCMV, human cytomegalovirus major immediate-early promoter; HDR, homologydirected repair; HMEJ, homology-mediated end joining; INDEL, insertion or deletion; KO, knockout; LP, landing pad; MMEJ, microhomology-mediated end joining; NHEJ, nonhomologous end joining; PAM, protospacer adjacent motif; PEST, sequence rich in proline,

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“…Direct silencing of the CMV promoter used for most transgenes, either by DNA-methylation or by changes in the histone modifications has also been shown [197][198][199][200]. These different strategies to silence the gene of interest are most likely due to the cell's drive to remove the stress of high productivity [201][202][203], by which ever means possible. Therefore, a frequent cause of loss of productivity is also the complete deletion of the recombinant genes from the genome [204,205].…”

Section: Maintaining Stabilitymentioning

confidence: 99%

Key Challenges in Designing CHO Chassis Platforms

et al. 2020

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Following the success of and the high demand for recombinant protein-based therapeutics during the last 25 years, the pharmaceutical industry has invested significantly in the development of novel treatments based on biologics. Mammalian cells are the major production systems for these complex biopharmaceuticals, with Chinese hamster ovary (CHO) cell lines as the most important players. Over the years, various engineering strategies and modeling approaches have been used to improve microbial production platforms, such as bacteria and yeasts, as well as to create pre-optimized chassis host strains. However, the complexity of mammalian cells curtailed the optimization of these host cells by metabolic engineering. Most of the improvements of titer and productivity were achieved by media optimization and large-scale screening of producer clones. The advances made in recent years now open the door to again consider the potential application of systems biology approaches and metabolic engineering also to CHO. The availability of a reference genome sequence, genome-scale metabolic models and the growing number of various “omics” datasets can help overcome the complexity of CHO cells and support design strategies to boost their production performance. Modular design approaches applied to engineer industrially relevant cell lines have evolved to reduce the time and effort needed for the generation of new producer cells and to allow the achievement of desired product titers and quality. Nevertheless, important steps to enable the design of a chassis platform similar to those in use in the microbial world are still missing. In this review, we highlight the importance of mammalian cellular platforms for the production of biopharmaceuticals and compare them to microbial platforms, with an emphasis on describing novel approaches and discussing still open questions that need to be resolved to reach the objective of designing enhanced modular chassis CHO cell lines.

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Rapid development of stable transgene CHO cell lines by CRISPR/Cas9-mediated site-specific integration into C12orf35

Cited by 55 publications

References 36 publications

An Efficient Exogenous Gene Insertion Site in CHO Cells with High Transcription Level to Enhance AID‐Induced Mutation

An Efficient Exogenous Gene Insertion Site in CHO Cells with High Transcription Level to Enhance AID‐Induced Mutation

A Site‐Specific Integration Reporter System That Enables Rapid Evaluation of CRISPR/Cas9‐Mediated Genome Editing Strategies in CHO Cells

Key Challenges in Designing CHO Chassis Platforms

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