Improved production of recombinant human antithrombin III in Chinese hamster ovary cells by ATF4 overexpression

Ohya, Takeshi; Hayashi, Tetsuji; Kiyama, Eriko; Nishii, Hiroko; Miki, Hajime; Kobayashi, Kaoru; Honda, Kohsuke; Ômasa, Takeshi; Ohtake, Hisao

doi:10.1002/bit.21758

Cited by 89 publications

(67 citation statements)

References 28 publications

(39 reference statements)

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“…Induction of GADD34 in HP can potentially reverse translational attenuation leading to increase in product titres and productivity. Corroborating this hypothesis is a recent study (Ohya et al 2008), where overexpression of ATF4 and GADD34 led to increase in productivity of thrombopoietin. Similarly, increase in XBP1 S levels indicates activation of Ire1a pathway.…”

Section: Dynamics Of Uprmentioning

confidence: 83%

“…This compares well with other studies on cell engineering of various chaperones and UPR pathway genes. For example, over-expression of GADD34, specific productivity of AT-III increased from 15 to 30 pg/cell/day (Ohya et al 2008). Similarly, over-expression of PDI in CHO cells increased productivity to about 22 pg/cell/day (Borth et al 2005).…”

Section: Discussionmentioning

confidence: 97%

“…The fraction of XBP1 S to XBP1 T mRNA increases slightly from day 3 to day 4, indicating further activation of the pathway. Presence of XBP1s has been observed in other recombinant CHO cell lines as well (Tigges and Fussenegger 2006;Ohya et al 2008). The presence of high levels of XBP1 S in an unstressed cell is a possible reason for the ineffectiveness of XBP1 overexpression on productivity (Ku et al 2008).…”

Section: Dynamics Of Ire1a Signaling Branch Of Upr Pathwaymentioning

confidence: 95%

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Dynamics of unfolded protein response in recombinant CHO cells

Prashad

Mehra

2014

Cytotechnology

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Genes in the protein secretion pathway have been targeted to increase productivity of monoclonal antibodies in Chinese hamster ovary cells. The results have been highly variable depending on the cell type and the relative amount of recombinant and target proteins. This paper presents a comprehensive study encompassing major components of the protein processing pathway in the endoplasmic reticulum (ER) to elucidate its role in recombinant cells. mRNA profiles of all major ER chaperones and unfolded protein response (UPR) pathway genes are measured at a series of time points in a high-producing cell line under the dynamic environment of a batch culture. An initial increase in IgG heavy chain mRNA levels correlates with an increase in productivity. We observe a parallel increase in the expression levels of majority of chaperones. The chaperone levels continue to increase until the end of the batch culture. In contrast, calreticulin and ERO1-L alpha, two of the lowest expressed genes exhibit transient time profiles, with peak induction on day 3. In response to increased ER stress, both the GCN2/PKR-like ER kinase and inositol-requiring enzyme-1alpha (Ire1a) signalling branch of the UPR are upregulated. Interestingly, spliced X-Box binding protein 1 (XBP1s) transcription factor from Ire1a pathway is detected from the beginning of the batch culture. Comparison with the expression levels in a low producer, show much lower induction at the end of the exponential growth phase. Thus, the unfolded protein response strongly correlates with the magnitude and timing of stress in the course of the batch culture.

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Section: Dynamics Of Uprmentioning

confidence: 83%

Section: Discussionmentioning

confidence: 97%

Section: Dynamics Of Ire1a Signaling Branch Of Upr Pathwaymentioning

confidence: 95%

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Dynamics of unfolded protein response in recombinant CHO cells

Prashad

Mehra

2014

Cytotechnology

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“…Expression of an humanized anti-CD154 antibody in CHO DG44 cells was only modestly enhanced by individual or combined overexpression of the cytosolic ATF6 fragment, XBP-1, or a fragment of eIF2a carrying the S51A point mutation (Ailor and Reff 2005). Expression of human antithrombin III or granulocyte-macrophage colonystimulating factor in CHO DXB11 cells was not enhanced by spliced XBP-1 (Ohya et al 2007). XBP-1 was spliced in antithrombin III expressing CHO DXB11 cells even before introduction of spliced XBP-1 cDNA (Ohya et al 2007).…”

Section: Engineering Of the Uprmentioning

confidence: 89%

Engineering of chaperone systems and of the unfolded protein response

Khan

Schröder

2008

Cytotechnology

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“…Indeed, yeast cells producing a GPCR were found to exhibit the hallmarks of a constitutively-active UPR [36]. In mammalian cells, activation of UPR-like responses has been shown to significantly improve recombinant protein production [37][38][39]. Similarly, in yeast overexpression of the genes encoding the Kar2 and PDI chaperones both reduced the UPR and increased heterologous protein production [40].…”

Section: An Up-regulated Unfolded Protein Responsementioning

confidence: 99%

Mapping the yeast host cell response to recombinant membrane protein production: Relieving the biological bottlenecks

Ashe

Bill

2011

Biotechnology Journal

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Membrane proteins are targeted by over 50 % of marketed pharmaceuticals, and as most membrane proteins are not naturally abundant, they must be produced recombinantly for the structural biology that is a pre-requisite to structure-based drug design. Unfortunately, obtaining high yields of functional, recombinant membrane proteins remains a major bottleneck in contemporary bioscience. Trial-and-error optimisation studies have not (and cannot) reveal mechanistic details of the biology of recombinant protein production, highlighting the need for defined and rational optimisation strategies based upon experimental observation. To this end, we have published a transcriptome and subsequent genetic analysis that has identified genes implicated in high-yielding yeast cell factories. These results have highlighted a role for alterations to a cell's protein synthetic capacity in the production of high yielding cells: paradoxically, reduced protein synthesis favors higher yields of recombinant membrane protein. These results highlight a potential bottleneck at the protein folding or translocation stage of protein production.

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Improved production of recombinant human antithrombin III in Chinese hamster ovary cells by ATF4 overexpression

Cited by 89 publications

References 28 publications

Dynamics of unfolded protein response in recombinant CHO cells

Dynamics of unfolded protein response in recombinant CHO cells

Engineering of chaperone systems and of the unfolded protein response

Mapping the yeast host cell response to recombinant membrane protein production: Relieving the biological bottlenecks

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