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Isolation of cDNA for Pea Phytochrome Using an Expression Vector |
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| Authors: | Tomizawa, Ken-ichi Komeda, Yoshibumi Sato, Naoki Nagatani, Akira lino, Tetsuo Furuya, Masaki |
| Affiliation: | 1Department of Biology, Faculty of Science, University of Tokyo Hongo, Tokyo 113, Japan 2Molecular Genetics Research Laboratory, University of Tokyo Hongo, Tokyo 113, Japan 3Division of Biological Regulation, National Institute for Basic Biology 38 Nishigonaka, Myodaijicho, Okazaki, Aichi 444, Japan |
| Abstract: | Partially purified phytochrome mRNA was obtained from etiolatedpea epicotyls by polyribosome immunoprecipitation or by sizefractionation of total poly(A)+RNA, and used for the synthesisof double-stranded complementary DNA (cDNA). cDNA librarieswere constructed using an Escherichia coli expression vector,pUC9, and screened for phytochrome cDNA by colony immunologicalassay. Nine colonies were found to produce a 27 kDa polypeptidethat was reactive to both polyclonal and monoclonal antipeaphytochrome antibodies. The plasmids from these colonies containedcDNA inserts of 1.2 or 2.0 kbp. Hybridization-arrest translationassay verified that the cDNA clones contained a sequence codingfor phytochrome polypeptide. RNA blot hybridization analysisindicated that the cDNA hybridized to a 4.1 kb poly(A)+RNA indark-grown pea. (Received March 22, 1986; Accepted June 13, 1986) |
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