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THE PLANT CELL, Vol 2, Issue 2 95-106, Copyright © 1990 by American Society of Plant Biologists


RESEARCH ARTICLES

Analysis of Stress-Induced or Salicylic Acid-Induced Expression of the Pathogenesis-Related 1a Protein Gene in Transgenic Tobacco

M. Ohshima, H. Itoh, M. Matsuoka, T. Murakami and Y. Ohashi
National Institute of Agrobiological Resources, Tsukuba Science City, Tsukuba, Ibaraki 305, Japan

The cis-acting elements for regulating gene expression of the tobacco pathogenesis-related 1a protein gene were analyzed in transgenic plants. The 5[prime]-flanking 2.4-kilobase fragment from the pathogenesis-related 1a protein gene was joined to the bacterial [beta]-glucuronidase gene and introduced into tobacco cells by Agrobacterium-mediated gene transfer. Promoter activity was monitored by quantitative and histochemical assay of [beta]-glucuronidase activity in leaves of regenerated transgenic plants. The level of [beta]-glucuronidase activity was clearly increased by treatment with salicylic acid, by cutting stress, and by local lesion formation caused by tobacco mosaic virus infection. Cytochemical studies of the induced [beta]-glucuronidase activity revealed tissue-specific and developmentally regulated expression of the pathogenesis-related 1a gene after stress or chemical treatment and after pathogen attack. To identify the cis-acting element more precisely, a series of 5[prime]-deleted chimeric genes was constructed and transformed into tobacco plants. Transgenic plants with a 0.3-kilobase fragment of the 5[prime]-flanking region of the pathogenesis-related 1a gene had the same qualitative response as those with the 2.4-kilobase fragment upon treatment with salicylic acid or infection with TMV. Thus, the 0.3-kilobase DNA sequence fragment was sufficient to allow the regulated expression of the pathogenesis-related 1a gene.


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