Literature DB >> 12856162

Metabolic changes during cell growth inhibition by p27 overexpression.

A V Carvalhal1, I Marcelino, M J T Carrondo.   

Abstract

The overexpression of p27, a cyclin-dependent kinase (CDK) inhibitor, has been shown to effectively inhibit cell growth at the G1-phase of different cell lines, potentiating a valid genetic strategy for cell proliferation control. In order to characterize the energy requirements after p27 overexpression in CHO cells expressing SEAP (secreted form of the human alkaline phosphatase enzyme), key metabolic parameters were evaluated. Cell growth inhibition led to a significant increase in cell size concomitant with a 2-fold increase in cell protein content. The simultaneous increase of the intracellular proteolytic activity with protein content suggests higher protein synthesis. A general 2-fold increase in oxygen, glutamine and glucose consumption rates, coupled with an increase in lactate and ammonia production was observed. p27 overexpression led to a significant increase in the intracellular pool of AMP (8.5-fold), ADP (6-fold) and, more uncommonly, ATP (4.5-fold). Nevertheless, cells were able to maintain the equilibrium among the three adenine nucleotides since both the ATP/ADP ratio and the energy charge values remained similar to those observed with non-growth inhibited cells. This work shows that the observed 4-fold increase in SEAP specific productivity after cell growth inhibition by p27, occurred concomitantly with a higher expenditure of cell energy. This characterization of cell metabolism becomes important in demonstrating the applicability of growth inhibition systems.

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Year:  2003        PMID: 12856162     DOI: 10.1007/s00253-003-1385-5

Source DB:  PubMed          Journal:  Appl Microbiol Biotechnol        ISSN: 0175-7598            Impact factor:   4.813


  12 in total

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4.  Proliferation control strategies to improve productivity and survival during CHO based production culture : A summary of recent methods employed and the effects of proliferation control in product secreting CHO cell lines.

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Journal:  Cytotechnology       Date:  2007-03-01       Impact factor: 2.058

5.  Selection of chemically defined media for CHO cell fed-batch culture processes.

Authors:  Xiao Pan; Mathieu Streefland; Ciska Dalm; René H Wijffels; Dirk E Martens
Journal:  Cytotechnology       Date:  2016-11-29       Impact factor: 2.058

6.  High glucose and low specific cell growth but not mild hypothermia improve specific r-protein productivity in chemostat culture of CHO cells.

Authors:  Mauricio Vergara; Mauro Torres; Andrea Müller; Verónica Avello; Cristian Acevedo; Julio Berrios; Juan G Reyes; Norma A Valdez-Cruz; Claudia Altamirano
Journal:  PLoS One       Date:  2018-08-16       Impact factor: 3.240

7.  Metabolic characterization of a CHO cell size increase phase in fed-batch cultures.

Authors:  Xiao Pan; Ciska Dalm; René H Wijffels; Dirk E Martens
Journal:  Appl Microbiol Biotechnol       Date:  2017-09-26       Impact factor: 4.813

8.  Dynamic metabolic flux analysis using B-splines to study the effects of temperature shift on CHO cell metabolism.

Authors:  Verónica S Martínez; Maria Buchsteiner; Peter Gray; Lars K Nielsen; Lake-Ee Quek
Journal:  Metab Eng Commun       Date:  2015-06-19

9.  Decoupling Growth and Protein Production in CHO Cells: A Targeted Approach.

Authors:  James S Donaldson; Matthew P Dale; Susan J Rosser
Journal:  Front Bioeng Biotechnol       Date:  2021-06-02

10.  The relationship between mTOR signalling pathway and recombinant antibody productivity in CHO cell lines.

Authors:  Raihana Edros; Susan McDonnell; Mohamed Al-Rubeai
Journal:  BMC Biotechnol       Date:  2014-02-17       Impact factor: 2.563

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