TY - JOUR
T1 - Gene activation in plastids by the CRE site-specific recombinase
AU - Tungsuchat, Tarinee
AU - Kuroda, Hiroshi
AU - Narangajavana, Jarunya
AU - Maliga, Pal
N1 - Funding Information:
Acknowledgements This research was supported by grants from the NSF Eukaryotic Genetics Program MCB-0319958 and the USDA Biotechnology Risk Assessment Research Grant Program Award No. 2005-33120-16524 and a Rutgers F&A Special Research Grant. Tarinee Tungsuchat was the recipient of a Royal Golden Jubilee Ph.D. scholarship of the Thailand Research Fund.
PY - 2006/7
Y1 - 2006/7
N2 - We developed a novel system for gene activation in plastids that uses the CRE/loxP site-specific recombination system to create a translatable reading frame by excision of a blocking sequence. To test the system, we introduced an inactive gfp* gene into the tobacco plastid genome downstream of the selectable spectinomcyin resistance (aadA) marker gene. The aadA gene is the blocking sequence, and is flanked by directly oriented loxP sites for excision by the CRE. In the non-activated state, gfp* is transcribed from the aadA promoter, but the mRNA is not translated due to the lack of an AUG translation initiation codon. Green Fluorescent Protein (GFP) expression is activated by excision of the aadA coding segment to link up the gfp* coding region with the translation initiation codon of aadA. Tobacco plants that carry the inactive gfp* gene do not contain detectable levels of GFP. However, activation of gfp* resulted in GFP accumulation, proving the utility of CRE-induced protein expression in tobacco chloroplasts. The gene activation system described here will be useful to probe plastid gene function and for the production of recombinant proteins in chloroplasts.
AB - We developed a novel system for gene activation in plastids that uses the CRE/loxP site-specific recombination system to create a translatable reading frame by excision of a blocking sequence. To test the system, we introduced an inactive gfp* gene into the tobacco plastid genome downstream of the selectable spectinomcyin resistance (aadA) marker gene. The aadA gene is the blocking sequence, and is flanked by directly oriented loxP sites for excision by the CRE. In the non-activated state, gfp* is transcribed from the aadA promoter, but the mRNA is not translated due to the lack of an AUG translation initiation codon. Green Fluorescent Protein (GFP) expression is activated by excision of the aadA coding segment to link up the gfp* coding region with the translation initiation codon of aadA. Tobacco plants that carry the inactive gfp* gene do not contain detectable levels of GFP. However, activation of gfp* resulted in GFP accumulation, proving the utility of CRE-induced protein expression in tobacco chloroplasts. The gene activation system described here will be useful to probe plastid gene function and for the production of recombinant proteins in chloroplasts.
KW - CRE/loxP site-specific recombination
KW - Green fluorescent protein (GFP)
KW - Nicotiana tabacum
KW - Plastid gene activation
KW - Plastid transformation
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U2 - 10.1007/s11103-006-0044-5
DO - 10.1007/s11103-006-0044-5
M3 - Article
C2 - 16897486
AN - SCOPUS:33746708151
SN - 0167-4412
VL - 61
SP - 711
EP - 718
JO - Plant Molecular Biology
JF - Plant Molecular Biology
IS - 4-5
ER -