TY - JOUR
T1 - Chloroplast ribosome release factor 1 (AtcpRF1) is essential for chloroplast development
AU - Motohashi, Reiko
AU - Yamazaki, Takanori
AU - Myouga, Fumiyoshi
AU - Ito, Takuya
AU - Ito, Koichi
AU - Satou, Masakazu
AU - Kobayashi, Masatomo
AU - Nagata, Noriko
AU - Yoshida, Shigeo
AU - Nagashima, Akitomo
AU - Tanaka, Kan
AU - Takahashi, Seiji
AU - Shinozaki, Kazuo
N1 - Funding Information:
Acknowledgements We thank I. Furukawa and S. Kawamura of RIKEN for their skillful technical assistance; R. Yoshida and T. Amano for their helpful comments; F. Sato of Kyoto University and T. Nakano of RIKEN for the Rubisco L/S complex antibody; M. Ikeuchi of Tokyo University for the D1 antibody; and T. Masuda and K. Takamiya of Tokyo Institute of Technology for the LHCII antibody. This work was supported by a grant for Genome Research from RIKEN to K.S. and a Grant-in-Aid for Scientific Research and NISSAN Science foundation to R.M.
PY - 2007/7
Y1 - 2007/7
N2 - To study the functions of nuclear genes involved in chloroplast development, we systematically analyzed albino and pale green Arabidopsis thaliana mutants by use of the Activator/Dissociation (Ac/Ds) transposon tagging system. In this study, we focused on one of these albino mutants, designated apg3-1 (for a lbino or p ale g reen mutant 3). A gene encoding a ribosome release factor 1 (RF1) homologue was disrupted by the insertion of a Ds transposon into the APG3 gene; a T-DNA insertion into the same gene caused a similar phenotype (apg3-2). The APG3 gene (At3g62910) has 15 exons and encodes a protein (422-aa) with a transit peptide that functions in targeting the protein to chloroplasts. The amino acid sequence of APG3 showed 40.6% homology with an RF1 of Escherichia coli, and complementation analysis using the E. coli rf1 mutant revealed that APG3 functions as an RF1 in E. coli, although complementation was not successful in the RF2-deficient (rf2) mutants of E. coli. These results indicate that the APG3 protein is an orthologue of E. coli RF1, and is essential for chloroplast translation machinery; it was accordingly named AtcpRF1. Since the chloroplasts of apg3-1 plants contained few internal thylakoid membranes, and chloroplast proteins related to photosynthesis were not detected by immunoblot analysis, AtcpRF1 is thought to be essential for chloroplast development.
AB - To study the functions of nuclear genes involved in chloroplast development, we systematically analyzed albino and pale green Arabidopsis thaliana mutants by use of the Activator/Dissociation (Ac/Ds) transposon tagging system. In this study, we focused on one of these albino mutants, designated apg3-1 (for a lbino or p ale g reen mutant 3). A gene encoding a ribosome release factor 1 (RF1) homologue was disrupted by the insertion of a Ds transposon into the APG3 gene; a T-DNA insertion into the same gene caused a similar phenotype (apg3-2). The APG3 gene (At3g62910) has 15 exons and encodes a protein (422-aa) with a transit peptide that functions in targeting the protein to chloroplasts. The amino acid sequence of APG3 showed 40.6% homology with an RF1 of Escherichia coli, and complementation analysis using the E. coli rf1 mutant revealed that APG3 functions as an RF1 in E. coli, although complementation was not successful in the RF2-deficient (rf2) mutants of E. coli. These results indicate that the APG3 protein is an orthologue of E. coli RF1, and is essential for chloroplast translation machinery; it was accordingly named AtcpRF1. Since the chloroplasts of apg3-1 plants contained few internal thylakoid membranes, and chloroplast proteins related to photosynthesis were not detected by immunoblot analysis, AtcpRF1 is thought to be essential for chloroplast development.
KW - Albino mutant
KW - Chloroplast development
KW - Light regulation
KW - Translation
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U2 - 10.1007/s11103-007-9166-7
DO - 10.1007/s11103-007-9166-7
M3 - Article
C2 - 17450416
AN - SCOPUS:34250199736
SN - 0167-4412
VL - 64
SP - 481
EP - 497
JO - Plant Molecular Biology
JF - Plant Molecular Biology
IS - 5
ER -