Abstract
BackgroundThere are a growing number of reports on the sub-physiological temperature culturing of mammalian cells for increased recombinant protein yields. However, the effect varies and the reasons for the enhancement are not fully elucidated. Expression of cold-inducible RNA-binding protein (cirp, also called cirbp or hnRNP A18) is known to be induced in response to mild, but not severe, hypothermia in mammalian cells. To clarify the molecular mechanism underlying the induction and to exploit this to improve the productivity of recombinant proteins, we tried to identify the regulatory sequence(s) in the 5′ flanking region of the mouse cirp gene.ResultsBy transiently transfecting HEK293 cells with plasmids expressing chloramphenicol acetyltransferase as a reporter, we found that the cirp 5′ flanking region octanucleotide 5′-TCCCCGCC-3′ is a mild-cold responsive element (MCRE). When 3 copies of MCRE were placed upstream of the CMV promoter and used in transient transfection, reporter gene expression was increased 3- to 7-fold at 32°C relative to 37°C in various cell lines including HEK293, U-2 OS, NIH/3T3, BALB/3T3 and CHO-K1 cells. In stable transfectants, MCRE also enhanced the reporter gene expression at 32°C, although more copy numbers of MCRE were necessary. Sp1 transcription factor bound to MCRE in vitro. Immunohistochemistry and chromatin immunoprecipitation assays demonstrated that more Sp1, but not Sp3, was localized in the nucleus to bind to the cirp regulatory region containing MCRE at 32°C than 37°C. Overexpression of Sp1 protein increased the expression of endogenous Cirp as well as a reporter gene driven by the 5′ flanking region of the cirp gene, and down-regulation of Sp1 had the opposite effect. Mutations within the MCRE sequence in the 5′ flanking region abolished the effects of Sp1 on the reporter gene expression both at 37°C and 32°C.ConclusionsCold-induced, as well as constitutive, expression of cirp is dependent, at least partly, on MCRE and Sp1. The present novel enhancer permits conditional high-level gene expression at moderately low culture temperatures and could be utilized to increase the yield of recombinant proteins in mammalian cells.
Highlights
There are a growing number of reports on the sub-physiological temperature culturing of mammalian cells for increased recombinant protein yields
We have found that Specificity protein 1 (Sp1) binds to the identified mild-cold responsive element (MCRE) sequence, and that downregulation of Sp1 expression suppresses the induction of cirp gene expression at 32°C
Identification of the cis-regulatory element that enhances gene expression at 32°C To analyze the transcriptional regulation of cirp expression, we isolated an approximately 10 kb-long 50 genomic fragment upstream of the transcription start site
Summary
There are a growing number of reports on the sub-physiological temperature culturing of mammalian cells for increased recombinant protein yields. Expression of cold-inducible RNA-binding protein (cirp, called cirbp or hnRNP A18) is known to be induced in response to mild, but not severe, hypothermia in mammalian cells. To clarify the molecular mechanism underlying the induction and to exploit this to improve the productivity of recombinant proteins, we tried to identify the regulatory sequence(s) in the 50 flanking region of the mouse cirp gene. Cold-inducible RNA-binding protein (Cirp, called Cirbp or hnRNP A18) is the first cold shock protein identified in mammals [1,2]. Expression of Cirp is induced in response to mild, but not severe, hypothermia. The mechanism(s) underlying the induction of cold shock proteins by mild hypothermia has not yet been fully elucidated
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