EXPRESSION OF A BACTERIAL LYSINE DECARBOXYLASE GENE AND TRANSPORT OF THE PROTEIN INTO CHLOROPLASTS OF TRANSGENIC TOBACCO

被引：28

作者：

HERMINGHAUS, S

SCHREIER, PH

MCCARTHY, JEG

LANDSMANN, J

BOTTERMAN, J

BERLIN, J

机构：

[1] BIOL BUNDESANSTALT LAND & FORSTWIRTSCHAFT,INST BIOCHEM,MESSEWEG 11-12,W-3300 BRAUNSCHWEIG,GERMANY

[2] PLANT GENET SYST NV,GHENT,BELGIUM

[3] BAYER AG,INST BIOTECHNOL PF-E,W-5090 LEVERKUSEN,GERMANY

[4] GESELL BIOTECHNOL FORSCH GMBH,W-3300 BRAUNSCHWEIG,GERMANY

来源：

PLANT MOLECULAR BIOLOGY | 1991年 / 17卷 / 03期

关键词：

NICOTIANA-TABACUM; PLANT TRANSFORMATION; GENE EXPRESSION; BACTERIAL LYSINE DECARBOXYLASE; PROTEIN TRANSPORT; CHLOROPLASTS; CADAVERINE;

D O I：

10.1007/BF00040641

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

A possible approach for altering alkaloid biosynthesis in plants is the expression of genes encoding key enzymes of a pathway such as lysine decarboxylase (ldc) in transgenic plants. Two strategies were followed here: one focused on expression of the gene in the cytoplasm, the other on subsequent targeting of the protein to the chloroplasts. The ldcgene from Hafnia alvei was therefore (a) placed under the control of the 1' promoter of the bidirectional Tr promoter from Agrobacterium tumefaciens Ti- plasmid, and (b) cloned behind the rbcS promoter from potato fused to the coding region of the rbcS transit peptide. Both ldc constructs, introduced into Nicotiana tabacum with the aid of A. tumefaciens, were integrated into the plant genome and transcribed as shown by Southern and northern hybridization. However, LDC activity was only detectable in plants expressing mRNA under the control of the rbcS promoter directing the LDC fusion protein into chloroplasts with the aid of the transit peptide domain. In plants expressing the processed bacterial enzyme cadaverine levels increased from nearly zero to 0.3-1% of dry mass.

引用

页码：475 / 486

页数：12

共 46 条

[1] COPPER ENZYMES IN ISOLATED CHLOROPLASTS - POLYPHENOLOXIDASE IN BETA-VULGARIS [J].

ARNON, DI .

PLANT PHYSIOLOGY, 1949, 24 (01) :1-15

[2]

BEIER H, 1987, Z NATURFORSCH C, V42, P1307

[3]

BERLIN J, IN PRESS Z NATURFO C, V46

[4] CONSTRUCTION AND CHARACTERIZATION OF NEW CLONING VEHICLES .2. MULTIPURPOSE CLONING SYSTEM [J].

BOLIVAR, F ;

RODRIGUEZ, RL ;

GREENE, PJ ;

BETLACH, MC ;

HEYNEKER, HL ;

BOYER, HW ;

CROSA, JH ;

FALKOW, S .

GENE, 1977, 2 (02) :95-113

[5] SEPARATION AND CHARACTERIZATION OF INNER AND OUTER ENVELOPE MEMBRANES OF PEA-CHLOROPLASTS [J].

CLINE, K ;

ANDREWS, J ;

MERSEY, B ;

NEWCOMB, EH ;

KEEGSTRA, K .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1981, 78 (06) :3595-3599

[6]

Dellaporta S.L., 1983, PLANT MOL BIOL REP, V1, P19, DOI [10.1007/BF02712670, DOI 10.1007/BF02712670]

[7] MOLECULAR-CLONING OF OVERLAPPING SEGMENTS OF THE NOPALINE TI-PLASMID PTIC58 AS A MEANS TO RESTRICTION ENDONUCLEASE MAPPING [J].

DEPICKER, A ;

DEWILDE, M ;

DEVOS, G ;

DEVOS, R ;

VANMONTAGU, M ;

SCHELL, J .

PLASMID, 1980, 3 (02) :193-211

[8] BROAD HOST RANGE DNA CLONING SYSTEM FOR GRAM-NEGATIVE BACTERIA - CONSTRUCTION OF A GENE BANK OF RHIZOBIUM-MELILOTI [J].

DITTA, G ;

STANFIELD, S ;

CORBIN, D ;

HELINSKI, DR .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1980, 77 (12) :7347-7351

[9] CLONING AND CHARACTERIZATION OF A LYSINE DECARBOXYLASE GENE FROM HAFNIA-ALVEI [J].

FECKER, LF ;

BEIER, H ;

BERLIN, J .

MOLECULAR & GENERAL GENETICS, 1986, 203 (01) :177-184

[10]

FRITZ CC, IN PRESS P NATL ACAD

← 1 2 3 4 5 →