Production of a self-activating CBM-factor X fusion protein in a stable transformed Sf9 insect cell line using high cell density perfusion culture

Gorenflo, Volker M.; Pfeifer, Tom; Lesnicki, Gary; Kwan, Emily; Grigliatti, Thomas A.; Kilburn, Douglas G.; Piret, James M.

doi:10.1007/s10616-005-0703-4

Cited by 12 publications

(12 citation statements)

References 31 publications

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“…A detailed review of the acoustic settler has been published by Shirgaonkar et al (2004). 6 cells/mL and 40 Â 10 6 cells/mL have been reported using the acoustic settler (Zhang et al 1998;Gorenflo et al 2004) and Gorenflo obtained 10 Â 10 6 CHO cells/mL in 100 L scale (Gorenflo et al 2002). An improvement of the technology was brought by installing an air-driven system able to suck the cell broth into the settler chamber and to back flush the cells into the bioreactor, avoiding the use of a peristaltic pump and enabling to empty the chamber completely (Gorenflo et al 2003).…”

Section: Acoustic Settlermentioning

confidence: 99%

Perfusion Processes

Chotteau

2014

Cell Engineering

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The interest for perfusion is increasing nowadays. This new focus has emerged from a synergy of a demand for disposable equipment and the availability of robust cell separation device, as well as the need for higher flexibility and lower investment cost. The cell separation devices mostly used today are based on filtration, i.e. alternating flow filtration, tangential flow filtration, spin-filter, or acceleration/gravity, i.e. inclined settler, centrifuge, acoustic settler. This paper gives an introduction to the basic concepts of perfusion and its practical implementation. It reviews the actual cell separation devices and describes the approaches used in the field to develop and optimize the perfusion processes.

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Section: Acoustic Settlermentioning

confidence: 99%

Perfusion Processes

Chotteau

2014

Cell Engineering

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“…Perfusion culture has been frequently studied and often involves the use of pumps to recirculate the cells. Pump damage was found to reduce the viability of a variety of animal cell types, including insect (Merten, 2000;Gorenflo et al, 2004), hybridoma (LaPorte et al, 1996) and CHO cells (Kim et al, 2008). Yet, in perfusion culture, the rate of pumping is far lower than here, circulation rates being about 1 to 10 bioreactor volumes/day (Merten, 2000;Kim et al, 2008) compared to ~ 100 to ~ 200 per day here.…”

Section: An Overall Perspective From Both Studiesmentioning

confidence: 99%

Scale-down studies for assessing the impact of different stress parameters on growth and product quality during animal cell culture

Nienow

Scott

Hewitt

et al. 2013

Chemical Engineering Research and Design

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“…In the case of stably transformed insect cells, baculovirus infection is no longer necessary for expression of the recombinant protein. The hypothesis is that in the cases of stably transformed insect cells the potential of the high cell density culture methods such as fed batch and perfusion (Gorenflo et al, 2004) can be fully realized. High cell density culture methods which can result in significant increases in cell densities increase the potential for bioprocess intensification (Griffiths, 1990) resulting in a subsequent increase in the volumetric productivity without increasing the size of the reactor, and a concurrent decrease in the requirements for liquid handling and overall downstream unit operations (Chisti and Moo-Young, 1996;Smith et al, 1991).…”

Section: Introductionmentioning

confidence: 99%

“…Earlier workers have described perfusion culture methods for recombinant protein expression using Sf-9-BEVS (Jäger, 1996;Zhang et al, 1998); the system however, is better suited for cells which express a secreted protein in a stable continuous manner, allowing the product to be harvested for prolonged periods of time. Gorenflo et al (2004) studied the expression of a recombinant protein saCBMFX in stably transformed Sf-9 insect cells in the perfusion system and reported that the protein produced had a higher activity than that expressed in a mammalian expression system. Stably transformed Drosophila S2 cells have also been used for the expression of several human proteins including erythropoietin, interleukin-2 (hIL-2), and human transferrin (hTF).…”

Section: Introductionmentioning

confidence: 99%

High cell density fed batch and perfusion processes for stable non‐viral expression of secreted alkaline phosphatase (SEAP) using insect cells: Comparison to a batch Sf‐9‐BEV system

Jardin

Montes

Lanthier

et al. 2006

Biotech & Bioengineering

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The development of insect cells expressing recombinant proteins in a stable continuous manner is an attractive alternative to the BEV system for recombinant protein production. High cell density fed batch and continuous perfusion processes can be designed to maximize the productivity of stably transformed cells. A cell line (Sf-9SEAP) expressing high levels of the reporter protein SEAP stably was obtained by lipid-mediated transfection of Sf-9 insect cells and further selection and screening. The expression of the Sf-9SEAP cells was compared with the BEVS system. It was observed that, the yield obtained in BEVS was similar to the batch Sf-9SEAP at 8 and 7 IU/mL, respectively. The productivity of this foreign gene product with the stable cells was enhanced by bioprocess intensification employing the fed-batch and perfusion modes of culture to increase the cell density in culture. The fed batch process yielded a maximum cell density of 28 x 10(6) cells/mL and 12 IU/mL of SEAP. Further improvements in the productivity could be made using the perfusion process, which demonstrated a stable production rate for extended periods of time. The process was maintained for 43 days, with a steady-state cell density of 17-20 x 10(6) cells/mL and 7 IU/mL SEAP. The total yield obtained in the perfusion process (394 IU) was approximately 22 and 8 times higher than that obtained in a batch (17.6 IU) and fed batch (46.1 IU) process, respectively.

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Production of a self-activating CBM-factor X fusion protein in a stable transformed Sf9 insect cell line using high cell density perfusion culture

Cited by 12 publications

References 31 publications

Perfusion Processes

Perfusion Processes

Scale-down studies for assessing the impact of different stress parameters on growth and product quality during animal cell culture

High cell density fed batch and perfusion processes for stable non‐viral expression of secreted alkaline phosphatase (SEAP) using insect cells: Comparison to a batch Sf‐9‐BEV system

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