Molecular characterization of cDNA encoding oxygen evolving enhancer protein 1 increased by salt treatment in the mangrove Bruguiera gymnorrhiza

Koichi Sugihara, Nobutaka Hanagata, Zvy Dubinsky, Sigeyuki Baba, Isao Karube

Research output: Contribution to journalArticlepeer-review

139 Scopus citations

Abstract

Young plants of the common Okinawa mangrove species Bruguiera gymnorrhiza were transferred from freshwater to a medium with seawater salt level (500 mM NaCl). Two-dimensional gel electrophoresis revealed in the leaf extract of the plant a 33 kDa protein with pI 5.2, whose quantity increased as a result of NaCl treatment. The N-terminal amino acids sequence of this protein had a significant homology with mature region of oxygen evolving enhancer protein 1 (OEE1) precursor. The cloning of OEE1 precursor cDNA fragment was carried out by means of reverse transcription-PCR (RT-PCR) using degenerated primers. Both 3'- and 5'-regions were isolated by rapid amplification of cDNA ends (RACE) method. The deduced amino acid sequence consisted of 322 amino acids and was 87% identical to that of Nicotiana tabacum. In B. gymnorrhiza, the predicted amino acid sequence of the mature protein starts at the residue number 85 of the open reading frame. The first 84-amino acid residues correspond to a typical transit sequence for the signal directing OEE1 to its appropriate compartment of chloroplast. The expression of OEE1 was analyzed together with other OEE subunits and D1 protein of photosystem II. The transcript levels of all the three OEEs were enhanced by NaCl treatment, but the significant increase of D1 protein was not observed.

Original languageEnglish
Pages (from-to)1279-1285
Number of pages7
JournalPlant and Cell Physiology
Volume41
Issue number11
DOIs
StatePublished - 2000

Bibliographical note

Funding Information:
We thank Dr. Yukiko Iwadate, Ms. Maina Yoshida and Minako Kaga, Mrs. Hitoshi Ito, Kentaro Saito, Tomohiro Togo and Kazuyuki Seki for their technical assistance. An Endowed Chair in Environmental Biotechnology funded by EBARA Corporation, Japan supported this work.

Keywords

  • Bruguiera gymnorrhiza
  • Molecular cloning
  • Oxygen evolving enhancer protein 1
  • Salt tolerance
  • Two-dimensional gel electrophoresis

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