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Cell Cycle Progression in Serum‐Free Cultures of Sf9 Insect Cells: Modulation by Conditioned Medium Factors and Implications for Proliferation and Productivity
Author(s) -
Doverskog Magnus,
Bertram Eva,
Ljunggren Jan,
Öhman Lars,
Sennerstam Roland,
Häggström Lena
Publication year - 2000
Publication title -
biotechnology progress
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.572
H-Index - 129
eISSN - 1520-6033
pISSN - 8756-7938
DOI - 10.1021/bp000108i
Subject(s) - sf9 , insect , microbiology and biotechnology , productivity , biology , cell culture , cell growth , cell cycle , cell , biochemistry , botany , genetics , gene , economics , spodoptera , recombinant dna , macroeconomics
Cell cycle progression was studied in serum‐free batch cultures of Spodoptera frugiperda (Sf9) insect cells, and the implications for proliferation and productivity were investigated. Cell cycle dynamics in KBM10 serum‐free medium was characterized by an accumulation of 50−70% of the cells in the G 2 /M phase of the cell cycle during the first 24 h after inoculation. Following the cell cycle arrest, the cell population was redistributed into G 1 and in particular into the S phase. Maximum rate of proliferation (μ N,max ) was reached 24−48 h after the release from cell cycle arrest, coinciding with a minimum distribution of cells in the G 2 /M phase. The following declining μ N could be explained by a slow increase in the G 2 /M cell population. However, at approximately 100 h, an abrupt increase in the amount of G 2 /M cells occurred. This switch occurred at about the same time point and cell density, irrespective of medium composition and maximum cell density. An octaploid population evolved from G 2 /M arrested cells, showing the occurrence of endoreplication in this cell line. In addition, conditioned medium factor(s) were found to increase μ N,max , decrease the time to reach μ N,max , and decrease the synchronization of cells in G 2 /M during the lag and growth phase. A conditioned medium factor appears to be a small peptide. On basis of these results we suggest that the observed cell cycle dynamics is the result of autoregulatory events occurring at key points during the course of a culture, and that entry into mitosis is the target for regulation. Infecting the Sf9 cells with recombinant baculovirus resulted in a linear increase in volumetric productivity of β‐galactosidase up to 68−75 h of culture. Beyond this point almost no product was formed. Medium renewal at the time of infection could only partly restore the lost hypertrophy and product yield of cultures infected after the transition point. The critical time of infection correlated to the time when the mean population cell volume had attained a minimum, and this occurred 24 h before the switch into the G 2 /M phase. We suggest that the cell density dependent decrease in productivity ultimately depends on the autoregulatory events leading to G 2 /M cell cycle arrest.

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