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To study the regulatory expression mechanism of soybean glycinin gene, Gy2, the 5` upstream region of the gene was searched for the presence of putative regulatory elements by nucleotide sequencing. It revealed various kinds of regulatory sequence ele...
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RISS 인기검색어
대두 원형질체와 형질전환된 담배에서의 대두 glycinin 유전자 Gy2 promoter 의 발현조절 기작 = Analysis of the Glycinin Gy2 Promoter Activity in Soybean Protoplasts and Transgenic Tobacco Plants
한글로보기https://www.riss.kr/link?id=A3211300
- 저자
- 발행기관
- 학술지명
- 권호사항
-
발행연도
1995
-
작성언어
-
-
KDC
500
-
등재정보
SCIE,KCI등재,SCOPUS
-
자료형태
학술저널
- 발행기관 URL
-
수록면
387-392(6쪽)
- 제공처
- 소장기관
-
0
상세조회 -
0
다운로드
부가정보
다국어 초록 (Multilingual Abstract)
To study the regulatory expression mechanism of soybean glycinin gene, Gy2, the 5` upstream region of the gene was searched for the presence of putative regulatory elements by nucleotide sequencing. It revealed various kinds of regulatory sequence elements commonly found in plant storage protein genes. There were canonical promoter sequences, TATA box (TATAAT) and AGGA box (GAAT) which are common in the 5` upstream region of the plant genes. The embryo factor binding sequence, RY repeat, CACA sequences, α-conglycinin enhancer-like sequences were also found. To delineate the function of these sequences, 5` upstream deletion mutants of Gy2 were prepared and fused to the α-glucuronidase (GUS) gene. Each chimeric construct was transferred into soybean protoplasts for transient assay, which led to the identification of the sequences between -281 and - 223, -170 and -122, of Gy2 promoter as negative regulatory elements, and the sequences between -223 and -170, -122 and -16 as positive regulatory elements. These results are consistent in transformed tobacco plants as well. The serially deleted promoter fragments fused to the GUS were transformed into Nicotiana tabacum by Agrobacterium tumefaciens using the binary vector system. GUS activity of Gy2 promoter deletion constructs was detected only in seeds but not in leaves with different levels of expression as in transient assay. These results suggest that the glycinin Gy2 promoter drives a tissue-specific expression in transgenic tobacco plants.
To study the regulatory expression mechanism of soybean glycinin gene, Gy2, the 5` upstream region of the gene was searched for the presence of putative regulatory elements by nucleotide sequencing. It revealed various kinds of regulatory sequence elements commonly found in plant storage protein genes. There were canonical promoter sequences, TATA box (TATAAT) and AGGA box (GAAT) which are common in the 5` upstream region of the plant genes. The embryo factor binding sequence, RY repeat, CACA sequences, α-conglycinin enhancer-like sequences were also found. To delineate the function of these sequences, 5` upstream deletion mutants of Gy2 were prepared and fused to the α-glucuronidase (GUS) gene. Each chimeric construct was transferred into soybean protoplasts for transient assay, which led to the identification of the sequences between -281 and - 223, -170 and -122, of Gy2 promoter as negative regulatory elements, and the sequences between -223 and -170, -122 and -16 as positive regulatory elements. These results are consistent in transformed tobacco plants as well. The serially deleted promoter fragments fused to the GUS were transformed into Nicotiana tabacum by Agrobacterium tumefaciens using the binary vector system. GUS activity of Gy2 promoter deletion constructs was detected only in seeds but not in leaves with different levels of expression as in transient assay. These results suggest that the glycinin Gy2 promoter drives a tissue-specific expression in transgenic tobacco plants.
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