CA1341419C - Process for the introduction of expressible genes into plant cell genomes and agrobacterium strains carrying hybrid ti plasmid vectors useful for this process - Google Patents
Process for the introduction of expressible genes into plant cell genomes and agrobacterium strains carrying hybrid ti plasmid vectors useful for this process Download PDFInfo
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Abstract
A process and vector compositions for the introduction of expressible genes into plant cell genomes by utilization of the vector properties of the Ti plasmids of Agrobacterium are described. Modified acceptor Ti plasmids are described which allow the introduction of any gene(s) of interest contained within an intermediate cloning vector carrying a region of homology with a corresponding region in the acceptor Ti plasmid. This introduction is achieved in Agrobacterium as a host by a single cross-over event which occurs within the two homologous DNA segments. The resulting hybrid Ti plasmids in Agrobacterium (vector compositions) can be used directly to infect plant cells, that can subsequently be screened for the expression of the product of the gene(s) of interest. From the transformed plant cells it is pos-sible to regenerate transformed fertile plants. This strategy is applicable to any of the plant transferable plasmids of Agrobacterium.
Description
PROCESS FOR THE INTRODUCTION OF EXPRESSIBLE GENES INTO PLANT
CELL GENOMES AND AGROBACTERIUM STRAINS CARRYING HYBRID TI
PLASMID VECTORS USEFUL FOR THIS PROCESS
Technical field of invention This invention relates to recombinant molecules, processes for their preparation, and processes for their introduction into plant cells and the plant cells or plants, respectively, containing foreign DNA sequences in their genome. More particularly, the invention relates to DNA sequences to be expressed in appropriate host plant cells. The recombinant DNA molecules contemplated are characterized by sequences that code for products, e.g. amino acids or polypeptides, useful for the growth of the plant or for improving its quality as nutrient, or for the production of valuable metabolites (e.g. alkaloids or steroid precursors).
In the description the following terms are used:
bom site : region of DNA where mob functions specifically interact and initiate autonomous DNA transfer.
Border seduence : DNA sequence which contains the ends of the T-DNA
Broad-host-range realicon : a DNA molecule capable of being transferred and maintained in many different host cells.
Callus tissue: a mass of unorganized and undifferentiated cells.
Clonin : the process of obtaining a population of organisms or DNA
or better:
sequences derived from one such organism or sequence by asexual reproduction.
the process of isolating a particular organism or part thereof, and the propagation of this subfraction as a homogenous population.
Cloninct vehicle : a plasmid, phage DNA or other DNA sequences which are able to replicate in a host cell, characterized by one or a small number of endonuclease recognition sites at which such DNA sequences may be cut in a determinable fashion without attendant loss of an essential X
__ 1 ~~+1 ~~
CELL GENOMES AND AGROBACTERIUM STRAINS CARRYING HYBRID TI
PLASMID VECTORS USEFUL FOR THIS PROCESS
Technical field of invention This invention relates to recombinant molecules, processes for their preparation, and processes for their introduction into plant cells and the plant cells or plants, respectively, containing foreign DNA sequences in their genome. More particularly, the invention relates to DNA sequences to be expressed in appropriate host plant cells. The recombinant DNA molecules contemplated are characterized by sequences that code for products, e.g. amino acids or polypeptides, useful for the growth of the plant or for improving its quality as nutrient, or for the production of valuable metabolites (e.g. alkaloids or steroid precursors).
In the description the following terms are used:
bom site : region of DNA where mob functions specifically interact and initiate autonomous DNA transfer.
Border seduence : DNA sequence which contains the ends of the T-DNA
Broad-host-range realicon : a DNA molecule capable of being transferred and maintained in many different host cells.
Callus tissue: a mass of unorganized and undifferentiated cells.
Clonin : the process of obtaining a population of organisms or DNA
or better:
sequences derived from one such organism or sequence by asexual reproduction.
the process of isolating a particular organism or part thereof, and the propagation of this subfraction as a homogenous population.
Cloninct vehicle : a plasmid, phage DNA or other DNA sequences which are able to replicate in a host cell, characterized by one or a small number of endonuclease recognition sites at which such DNA sequences may be cut in a determinable fashion without attendant loss of an essential X
__ 1 ~~+1 ~~
biological function of the DNA, e.g. , replication, production of coat proteins or loss of promoter or binding sites, and which contain a marker suitable for use in the identification of transformed cells, e.g., tetracycline resistance, or ampicillin resistance. A cloning vehicle is often called vector.
Coding seguence : DNA sequence which determines the amino acid sequence of a polypeptide.
Cointegrate : the structure resulting from a single cross-over event between two circular DNA molecules.
Complementation ' tm tans : process whereby a DNA molecule (replicon) which is not physically linked to another replicon can provide a diffusible substance which is missing and required by the other nonlinked replicon.
Coniuaation : the process whereby DNA is transferred from bacteria of one type to another type during cell-to-cell contact.
Crossing-over : the process of exchange of genetic material between homologous DNA sequences.
Deletion substitution : removal of one DNA sequence and its replacement by a different DNA sequence.
Differentiation : the process whereby descendents of a cell achieve and maintain specialization of structure and function.
DNA seguence or DNA segment : a linear array of nucleotides connected one to the other by phasphodiester bonds between the 3' and 5' carbons of adjacent pentoses.
Double cross-over : the process of resolution of a cointegrate structure into two circular DNA molecules. This process is used to exchange genetic information. One of the DNA circles has two regions of homology with the target DNA through which recombination can occur; these two regions bracket a nonhomologous DNA sequence which is to be exchanged with the target DNA. If this second cross-over occurs in the same region of DNA as the first, the original DNA circles will be generated. If this second cross-over occurs in the second homologous region, genetic exchange will have occurred between the two circles.
Expression : the process undergone by a structural gene to produce a polypeptide. It is a combination of transcription and translation.
Expression control seguence : a sequence of nucleotides that controls and regulates expression of structural genes when operatively linked to those genes.
F-tvaeplasmid : plasmid carrying the F (fertility) factor which allows the transfer of a copy of the plasmid to a host not carrying the F-factor.
Gene : a DNA sequence composed of two parts, ( 1 ) the coding sequence for the gene product, and (2) the sequences in the promoter region which control whether or not the gene will be expressed.
Genome : the entire DNA of a cell or a virus. It includes inter alia the structural genes coding for the polypeptide(s), as well as operator, promoter and ribosome binding and interaction sequences, including sequences such as the Shine-Dalgarno sequences.
Genotvae: the sum total of the genetic information contained in an organism.
Homologous recombination : recombination between two regions of DNA which contain homologous sequences.
I-type plasmid : a group of autotransferable plasmids of a different incompatibility group than F.
Incompatibility : Incapability of two DNA molecules of coexisting in the same cell in the absence of selective pressure.
Insertion : addition of a DNA sequence within the DNA sequence of another molecule.
Leader seguence : the region of an mRNA molecule extending from the 5' end to the beginning of the first structural gene; it also includes sites important to initiate translation of the coding sequence of the structural gene.
Meiosis : two successive divisions that reduce the starting number of 4 n chromosomes to 1 n in each of four product cells. This process is important in sexual reproduction.
X
Coding seguence : DNA sequence which determines the amino acid sequence of a polypeptide.
Cointegrate : the structure resulting from a single cross-over event between two circular DNA molecules.
Complementation ' tm tans : process whereby a DNA molecule (replicon) which is not physically linked to another replicon can provide a diffusible substance which is missing and required by the other nonlinked replicon.
Coniuaation : the process whereby DNA is transferred from bacteria of one type to another type during cell-to-cell contact.
Crossing-over : the process of exchange of genetic material between homologous DNA sequences.
Deletion substitution : removal of one DNA sequence and its replacement by a different DNA sequence.
Differentiation : the process whereby descendents of a cell achieve and maintain specialization of structure and function.
DNA seguence or DNA segment : a linear array of nucleotides connected one to the other by phasphodiester bonds between the 3' and 5' carbons of adjacent pentoses.
Double cross-over : the process of resolution of a cointegrate structure into two circular DNA molecules. This process is used to exchange genetic information. One of the DNA circles has two regions of homology with the target DNA through which recombination can occur; these two regions bracket a nonhomologous DNA sequence which is to be exchanged with the target DNA. If this second cross-over occurs in the same region of DNA as the first, the original DNA circles will be generated. If this second cross-over occurs in the second homologous region, genetic exchange will have occurred between the two circles.
Expression : the process undergone by a structural gene to produce a polypeptide. It is a combination of transcription and translation.
Expression control seguence : a sequence of nucleotides that controls and regulates expression of structural genes when operatively linked to those genes.
F-tvaeplasmid : plasmid carrying the F (fertility) factor which allows the transfer of a copy of the plasmid to a host not carrying the F-factor.
Gene : a DNA sequence composed of two parts, ( 1 ) the coding sequence for the gene product, and (2) the sequences in the promoter region which control whether or not the gene will be expressed.
Genome : the entire DNA of a cell or a virus. It includes inter alia the structural genes coding for the polypeptide(s), as well as operator, promoter and ribosome binding and interaction sequences, including sequences such as the Shine-Dalgarno sequences.
Genotvae: the sum total of the genetic information contained in an organism.
Homologous recombination : recombination between two regions of DNA which contain homologous sequences.
I-type plasmid : a group of autotransferable plasmids of a different incompatibility group than F.
Incompatibility : Incapability of two DNA molecules of coexisting in the same cell in the absence of selective pressure.
Insertion : addition of a DNA sequence within the DNA sequence of another molecule.
Leader seguence : the region of an mRNA molecule extending from the 5' end to the beginning of the first structural gene; it also includes sites important to initiate translation of the coding sequence of the structural gene.
Meiosis : two successive divisions that reduce the starting number of 4 n chromosomes to 1 n in each of four product cells. This process is important in sexual reproduction.
X
mob (mobilization functions) : a set of products which promote DNA transfer only in combination with tra functions. Mob can promote transfer of plasmids containing a bom site.
Mobilization : the process whereby one DNA molecule which is not able to transfer to another cell is helped to transfer by another DNA molecule.
Mobilization helper alasmid : a plasmid capable of providing diffusible products which another plasmid lacks for transfer to another host cell.
NoncoJuaative recombinant plasmid : a DNA molecule which is not capable of being transferred by itself from its host cell to another host cell during cell-to-cell contact. For transfer it will need further functions supplied by other DNA, e.g. by (a) helper plasmid(s).
Nucleotide : a monomeric unit of DNA or RNA consisting of a sugar moiety (pentose), a phosphate, and a nitrogenous heterocyclic base. The base is linked to the sugar moiety via a glycosidic bond (1' carbon of the pentose) and that combination of base and sugar is a nucleoside.
The base characterizes the nucleotide. The four DNA bases are adenine ("A"), guanine ("G") , cytosine ("C") , and thymine ("T"). The four RNA bases are A, G, C, and uracil ("U") .
Phenotyae : the observable characteristics of an individual resulting from the interaction between the genotype and the environment in which development occurs.
Plasmid : a nonchromosomal double-stranded DNA sequence comprising an intact "replicon" such that the plasmid is replicated in a host cell. When the piasmid is placed within a unicellular organism, the characteristics of that arganism are changed or transformed as a result of the DNA of the plasmid. For example, a plasmid carrying the gene for tetracycline resistance (TcR) transforms a cell previously sensitive to tetracycline into one which is resistant to it. A cell transformed by a plasmid is called "transformant".
Polyaeptide : a linear series of amino acids connected one to the other by peptide bonds between the a-amino and carboxy groups of adjacent amino acids.
Mobilization : the process whereby one DNA molecule which is not able to transfer to another cell is helped to transfer by another DNA molecule.
Mobilization helper alasmid : a plasmid capable of providing diffusible products which another plasmid lacks for transfer to another host cell.
NoncoJuaative recombinant plasmid : a DNA molecule which is not capable of being transferred by itself from its host cell to another host cell during cell-to-cell contact. For transfer it will need further functions supplied by other DNA, e.g. by (a) helper plasmid(s).
Nucleotide : a monomeric unit of DNA or RNA consisting of a sugar moiety (pentose), a phosphate, and a nitrogenous heterocyclic base. The base is linked to the sugar moiety via a glycosidic bond (1' carbon of the pentose) and that combination of base and sugar is a nucleoside.
The base characterizes the nucleotide. The four DNA bases are adenine ("A"), guanine ("G") , cytosine ("C") , and thymine ("T"). The four RNA bases are A, G, C, and uracil ("U") .
Phenotyae : the observable characteristics of an individual resulting from the interaction between the genotype and the environment in which development occurs.
Plasmid : a nonchromosomal double-stranded DNA sequence comprising an intact "replicon" such that the plasmid is replicated in a host cell. When the piasmid is placed within a unicellular organism, the characteristics of that arganism are changed or transformed as a result of the DNA of the plasmid. For example, a plasmid carrying the gene for tetracycline resistance (TcR) transforms a cell previously sensitive to tetracycline into one which is resistant to it. A cell transformed by a plasmid is called "transformant".
Polyaeptide : a linear series of amino acids connected one to the other by peptide bonds between the a-amino and carboxy groups of adjacent amino acids.
Promoter region : DNA sequences upstream to the start of the coding sequence which regulate transcription of the gene.
Promoter seauence : sequence at which RNA polymerase binds and promotes the faithful transcription of downstream sequences.
Recombinant DNA molecule or hybrid DNA: a hybrid DNA sequence comprising at least two nucleotide sequences, the first sequence not normally being found together in nature with the second.
Recombination: the creation of a new association of DNA molecules or parts of DNA
molecules.
Region of homology : a region of DNA which shares the same DNA sequence as that found in another region of DNA.
Realicon : a self-replicating genetic element possessing a site for the initiation of DNA replication and genes specifying the necessary functions for controlling replication.
Restriction fragiment : a DNA molecule resulting from double-stranded cleavage by an enzyme which recognizes a specific target DNA sequence.
RNA aolvmerase : enzyme which results in the transcription of DNA into RNA.
Selectable marker gene : a DNA sequence which, when expressed, gives that cell a growth advantage over cells which dg not contain that DNA sequence, when all cells are in growth medium which can distinguish the two types of cells. Commonly used selectable marker genes are those which encode resistance to antibiotics.
Single cross-over : the process of recombining two circular DNA molecules to form a cointegrate larger circle.
Structural Gene : a gene which codes for a polypeptide.
T-DNA : portion of the Ti plasmid as it is found stably integrated into the plant cell genome.
T-region : portion of the Ti plasmid which contains the DNA sequences which are transferred to the plant cell genome.
Ti plasmid : large plasmids found in strains of Agrobacterium tumefaciens containing the genetic information for tumor (crown gall) induction on susceptible plants.
Promoter seauence : sequence at which RNA polymerase binds and promotes the faithful transcription of downstream sequences.
Recombinant DNA molecule or hybrid DNA: a hybrid DNA sequence comprising at least two nucleotide sequences, the first sequence not normally being found together in nature with the second.
Recombination: the creation of a new association of DNA molecules or parts of DNA
molecules.
Region of homology : a region of DNA which shares the same DNA sequence as that found in another region of DNA.
Realicon : a self-replicating genetic element possessing a site for the initiation of DNA replication and genes specifying the necessary functions for controlling replication.
Restriction fragiment : a DNA molecule resulting from double-stranded cleavage by an enzyme which recognizes a specific target DNA sequence.
RNA aolvmerase : enzyme which results in the transcription of DNA into RNA.
Selectable marker gene : a DNA sequence which, when expressed, gives that cell a growth advantage over cells which dg not contain that DNA sequence, when all cells are in growth medium which can distinguish the two types of cells. Commonly used selectable marker genes are those which encode resistance to antibiotics.
Single cross-over : the process of recombining two circular DNA molecules to form a cointegrate larger circle.
Structural Gene : a gene which codes for a polypeptide.
T-DNA : portion of the Ti plasmid as it is found stably integrated into the plant cell genome.
T-region : portion of the Ti plasmid which contains the DNA sequences which are transferred to the plant cell genome.
Ti plasmid : large plasmids found in strains of Agrobacterium tumefaciens containing the genetic information for tumor (crown gall) induction on susceptible plants.
TL-DNA and TR-DNA : octopine crown gall tumor cells can contain two T-DNA
sequences, a left T-DNA, i.e. TL-DNA, and a right TR-DNA. TL-DNA
contains sequences also found in common with T-DNA of nopaline tumor cells whereas TR-DNA does not.
tr transfer functions, : both plasmid-encoded diffusible products and sites of action utilized during DNA transfer between cells, e.g. products required to make a bridge between two cells and the site at which DNA transfer is initiated.
Transcrietion : the process of producing mRNA from a structural gene or : the process involving base paring whereby the genetic information contained in DNA is used to order a complementary sequence of bases in an RNA chain.
Transformation : genetic modification induced by the incorporation of exogenous DNA into the DNA complement of a cell.
Translation : the process of producing a polypeptide from mRNA
or : the process whereby the genetic information present in an mRNA
molecule directs the order of specific amino acids during the synthesis of a polypeptide .
Undifferentiated pheno~e : a homologous appearance of cells in a tissue without any specialized parts.
Vector : a DNA molecule designed for transfer between different host cells .
~ 3t~1 41 9 Background Art The development of recombinant DNA techniques has made the genetic engineering of microorganisms a challenging prospect. These techniques might be extended to multicellular eukaryotes, if complete organisms could be regenerated from single somatic cells. The cells of some higher plants exhibit excellent regeneration capacities and, therefore, are good materials for the genetic engineering of higher organisms.
A major problem for the genetic engineering of plants is the availability of a system for the introduction of exogenous (foreign) DNA into the plant genome. Such a system is provided by the tumor-inducing (Ti) plasmids carried by the Gram-negative soil bacterium Agrobacterium tumefaciens. This organism has been shown to cause a neo-plastic transformation, called "crown gall", of wounded tissue of a very wide range of dicotyledonous plants. The proliferating neo-plasms synthesize novel, Ti-specified metabolites, called opines. The molecular basis of this transformation is the transfer and stable integration of a well-defined T-DNA (transferred DNA) fragment of the Ti plasmid in the plant cell genome. In other words, crown gall tumors contain in their chromosomal DNA a DNA segment called the T-DNA which is homologous to DNA sequences in the Ti plasmid used to induce the tumor line.
In all cases, this T-DNA corresponds to, and is colinear with, a continuous stretch of Ti plasmid DNA which is, therefore, called the T-region.
Ti plasmids are classified according to the type of opine synthesized in crown gall cells. Aarobacterium strains which induce the synthesis of nopaline [N-a-(1,3-dicarboxypropyl)-L-arginine] in crown gall cells are called nopaline strains, and strains which induce the synthesis of octopine [N-a-(N-1-carboxyethyl)-L-arginine]
are called octopine strains. These are the most commonly used Aarobacterium strains.
The use of T-DNA as a vector for plant genetic engineering was demonstrated in a model experiment in which the 14 kb bacterial transposon Tn7 was inserted in vivo x near the right border of the T-DNA from the Ti plasmid of the strain A4robacterium T37. Nopaline synthesis was eliminated in the tumors incited by agrobacteria carrying this Ti plasmid. Furthermore, Southern blotting hybridizations revealed that the entire Tn7 was present in the chromosomal DNA of these tumors as part of an otherwise normal T-DNA sequence (Hernalsteens et al., Nature 287 (1980), 654-656; Holsters et al., Mol. Gen. Genet. 185 (1982), 283-289). Thus, the introduction of this 14 kb DNA fragment into the 23 kb T-DNA has not altered the tatter's ability to be transferred to the plant cell genome.
The borders of the T-DNA from the Ti plasmid of the nopaline strain A4robacterium T37 have been very precisely determined. It is only a portion, roughly 23 kb, of the entire nopaline Ti plasmid. Furthermore, the borders of the T-DNA are known;
the nucleotide sequences which define the borders of the T-DNA have been determined and compared with the same region of the nopaline Ti plasmid (Zambryski et al.
, Science 209 (1980), 1385-1391; Zambryski et al., J. Mot. Appl. Genet. 1 (1982), 361-370). The borders of the T-region are most probably involved in the integration of the T-DNA into the plant cell genome.
Knowledge of the T-DNA sequences which define the borders of the transferred DNA is a basic requirement for the use of the Ti plasmid as a vector for DNA
transfer to plant cells. Thus, foreign DNA can be inserted within these borders to ensure its transfer to the plant cell genome. In addition, if one expects to utilize this system it is important that the transformed plant cells are normal rather than tumorous in their growth properties. To produce normal cells after T-DNA transfer requires knowledge of the functions encoded by the T-DNA itself. Thus, the T-region of the Ti plasmid has been subjected to intense genetic analysis to determine which regions are responsible for the tumor phenotype.
The T-DNA encodes functions which are responsible for the crown gall phenotype.
The genes have been localized to specific regions of the T-DNA (L-eemans et al., EMBO J. 1 (1982), 147-152; Willmitzer et al., EMBO J_. 1 {1982), 139-146). In general, there are at least 4 genes which control the undifferentiated phenotype of tumor callus tissue. Mutants in these genes can either lead to transformed tissues which appears shoot-like or root-like. The latter results are especially important if one hopes to transfer DNA to plants for expression in normal plant tissue rather than tumor tissue.
Recently, a mutant Ti plasmid was found to induce transformed shoots which were capable for regenerating into completely normal plants. These plants were fertile and even transmitted T-DNA specific sequences through meiosis, i.e. progeny plants still contained T-DNA specific sequences (Otten et al., Mol. Gen. Genet. 183 (1981 ), 209-213). However, the transformed plant tissue contained in its chromosomal DNA
a T-DNA which was very much reduced in size due to the generation of a large deletion which removed the region of the T-DNA controlling the tumor phenotype. It is not known whether the deletion occurred during the initial transformation event or as a subsequent event leading to shoot formation.
The Ti plasmids are large (200 kb) and many genes located at different sites on the Ti plasmid are involved in the transformation of plant cells. Therefore, it is not possible to construct a small Ti plasmid-derived cloning vector with unique endonuclease recognition sites at appropriate locations within the T-region, and possessing all functions essential for T-DNA transfer and stable incorporation into the plant cell genome. One known way to introduce a chosen DNA fragment into specific restriction enzyme cleavage sites of the T-region of a Ti plasmid has been to construct cloning plasmids which are able to replicate in Aprobacterium as well as in Escherichia coli, and which contain a chosen restriction fragment of the T-DNA.
Such cloning plasmids were denoted "intermediate vectors". Such intermediate vectors were used to analyze the functions encoded by the T-region (Leemans et al., J. Mol. Aaal. Genet. 1 (1981 ), 149-164).
Disclosure of the invention The present invention relates to a process for the introduction of expressible genes into plant cell genomes. It is one of the objects of the present invention to provide modified acceptor Ti plasmids which allow the introduction of any genes) of interest into these plasmids. The genes) of interest to be introduced is (are) contained within a novel intermediate cloning vector carrying a region of homology with a corresponding region in the acceptor Ti plasmid. The intermediate cloning vectors are a further object of this invention.
The introduction of the genes) of interest into the acceptor Ti plasmids is achieved by a single cross-over event which occurs within the two homologous DNA
segments of the acceptor Ti plasmid harbored in Agrobacterium and the intermediate cloning vector. The intermediate cloning vector is mobilized from Escherichia coli where it is propagated to Aarobacterium using helper plasmids. Such helper plasmids and their functions for mobilization are known (Finnegan et al., Mol. Gen. Genet. 185 (1982), 344-351).
The result of the single cross-over event in Aarobacterium is a hybrid Ti plasmid vector. Such hybrid Ti plasmid vectors are a further object of the invention The resulting hybrid plasmid vectors harbored in Agrobacterium (hereinafter called vector composition) can be used directly to infect plant cells which are subsequently screened for the expression of the product{s) of the gene{s) of interest. This process for preparing transformed plant cells by infection of plant cells with the vector composition, and the transformed plant cells, as well as plants generated therefrom are further objects of this invention. This strategy is applicable to any of the plant-transferable plasmids of Aarobacterium.
Description of drawings Fig. 1 illustrates one embodiment of an acceptor Ti plasmid of the invention which is the result of a deletion of the internal portion of the T-region, except for the border sequences (1 ) and (2). The border sequences are essential for the integration of the T-region into a plant cell genome. The region (3) between border sequences {1 ) and {2) is the DNA segment which will be transferred to the plant. The acceptor Ti plasmid contains a DNA segment (3) with a DNA
sequence which is homologous with at least a part of a DNA sequence in an intermediate cloning vector permitting integration of the intermediate cloning vector via a single cross-over event. The Ti plasmid region (4) codes for functions which are essential for the transfer by Agrobacterium of the T-region into plant cell genomes. This region has been designated as vir-region.
Fig. 2 illustrates an intermediate cloning vector of the invention to be inserted by a single cross-over event into the acceptor Ti plasmid of Fig. I. It contains a cloning vehicle DNA segment (3') with a DNA sequence which is homologous with a least part of the DNA segment (3) of the acceptor Ti plasmid permitting the desired single cross-over event. Moreover, the intermediate cloning vector contains a gene or group of genes (5) of interest having its natural promoter sequence. In general plant genes can be used in this construction as they are mare likely to be expressed. However, in principle any natural gene of interest can be inserted. The intermediate cloning vector may also contain a selectable marker gene (6). This gene should contain a promoter sequence which permits expression of the gene in plant cells. Plant cells containing this marker gene should have a selective growth advantage over cells without this ,, A. 4 gene; in this way plant cells which have been transformed by DNA containing this marker gene can be distinguished from untransformed plant cells .
Fig . 3 illustrates another embodiment of an intermediate cloning vector of the invention which is similar to the intermediate cloning vector of F'ig. 2, and is to be inserted by a single cross-over event into the acceptor Ti plasmid of Fig. 1. It contains the cloning vehicle DNA segment (3'), an exogen-ous promoter sequence (8) allowing regulated expression of the genes) of interest (7), and, if desired, a marker gene (6). . .
Fig. 4 schematically illustrates the construction of hybrid Ti plas-mid vectors of the invention from the acceptor Ti plasmid of F ig _ 1, and the intermediate cloning vectors of Figs 2 and 3 by a single cross-over event.
Fig. 5 outlines the steps involved in the genetic transfer of an in~errnedia~e cloning vector from E. coli to Aarobacterium containing «r acceptor Ti plasmid. 'The first step is the conjugation of the E. coll. strain (2) containing the inter-me4iate cloning vector to another E. coli strain (2) which cc:~tains ~wc helper plasmids far the later conjugation to Agrobacter ium. One helper plasmid contains DNA sequences irr_aortant for plasmid transfer (tra) and the other helper pl«smid c3ntains sequences which are important for the mobilization (mob). l~Vhen these helper plasmids are intro-duced by conjugation into E. call strain (1), the inter-mediate cloning vector contained therein will be capable of being transferred to other b~icterial strains. The tra and mob helper plasmids also contain antibiotic resistance mark-ers Abr2 and AbrJ which are different from those :found in -the intermediate cloning vector (Abr ). Thus, the pres-ence of all the plasmids can be monitored on selective media. A mobilizing strain (3) is obtained. This mobilizing strain (3) is conjugated to an A. tumefaciens strain (4) which contains the acceptor Ti plasmid of Fig. 1 followed by selection for antibiotic resistance markers) of the intermediate cloning vector. As the intermediate cloning vector cannot replicate in Agrobacterium, it can only be maintained if it has formed a cointegrate with the recipient acceptor Ti plasmid; this cointegrate structure in Aarobacterium (5) is the final hybrid Ti plasmid used to transfer DNA into plant cell genomes.
Fig. 6 illustrates the construction of a model acceptor Ti plasmid (A) which is analogous to that shown in Fig. 1. Here, a double cross-over event occurs between a Ti plasmid and another plasmid containing a DNA sequence which is to replace a portion of the original Ti plasmid. More specifically, the smaller plasmid contains the border sequences of the T-region (1; 2) in a cloning vehicle (3). A double cross-over results in the deletion of the internal portion T of the T-region and its replacement by the cloning vehicle. The acceptor Ti plasmid (A) obtained is capable of transferring DNA contained between the border sequences (1; 2) into plant cell genomes. The resulting transformed plant DNA will not produce tumoraus crown gall tissue as the genes controlling neoplastic growth are deleted in the Ti plasmid (A). Ti plasmid (A) is a very generalized acceptor Ti plasmid for any intermediate cloning vector with homology with cloning vehicle (3). The cloning vehicle (3) may be a conventional plasmid, such as pBR322 (or its derivatives).
Fig. 7 illustrates schematically the steps leading to the construction of an intermediate cloning vector in E. coli host cells. A gene of interest (5) bracketed by restriction endonuclease site R1 and a selectable marker gene (6) bracketed by .
restriction endonuclease site R2 are inserted into a cloning vehicle (3') containing single restriction sites for the en-zymes R1 and R2. All three molecules are digested with restriction enzymes R:i and/or ft~ and ligated together using DNA ligase to form the intermediate cloning vector. The cloning vehicle 3' mu:~t also contain additional DNA sequen-ces whi<:h code for antibiotic resistance (Abrl) to use as a selectable marker for bacterial genetics . The gene of inter-est (5) may be under the control of its natural promoter or of an exogenous promoter as outlizned in Figs. 2 and 3.
Fig . $ illustrates the ~ construction of another embodiment of an acceptor Ti plasmid (B) of the invention. Here, a double cross-over event occurs between a 'l"i plasrnid and a cloning - vehicle (3) which contains DNA sequences (9) and (10) which are homologoLes to Ti sequences just outside the border sequences (1) and (2) respectively. The double cross-over went results in the deletion of the entire 'T-re-gion T i.ncluying the border sequences (1) anal (2) and its replaceme~ i with the cloning vehicle (3) . Ti plasmid (B ) is an accep ~_or for intermediate cloning vectors which contain ti~!e gene ef interest c:lor~ed- bet:weEen the border sequen-ces (1) arid {2); (see Fig. 9).
Fig. ° illustrates an intermediate cloning vector of the invention to be inserted by a single cross-over event into the acceptor Ti plasmid i8) of Fig. $. It contains the border sequen-ces (1) and (2) which flank the genes) of interest (5). It also contains a cloning vehicle sequence (3' ) which is at least partially homologous to the cloning vehicle sequence - - (3) in the acceptor Ti plasmid (B) to allow homologous recombination between the two plasmids .
Fig. 10 schematically illustrat~a the construction of hybrid Ti plas-mid vectors of the invention from the acceptor Ti plasmid 1 ~~1 41 9 (B) of Fig. 8 and the corresponding intermediate cloning vector of Fig.
9. A single cross-over event introduces the intermediate cloning vector of Fig. 9 into the acceptor Ti plasmid (B) of Fig. 8.
The following figures 11 to 20 more specifically illustrate the invention.
Fig. 11 illustrates the insertion of the 5.2 kb HindIII fragment AcgB into pBR322 (see also Zambryski et al., Science 209 (1980), 1385-1391 ).
This fragment AcgB contains the right and left border regions of the nopaline Ti plasmid. This clone pAcgB is used in the construction of acceptor plasmid pGV3850, an "A-like" acceptor plasmid as shown in Fig: 6. it is obvious to those skilled in the art that a clone analogous to clone pAcgB can be obtained by using the cloned restriction fragments which contain the left and right border region of a wild-type Ti plasmid.
Fig. 12 illustrates the T-region of nopaline Ti plasmid pGV3839. The HindIII
restriction endonuclease sites are indicated as (H). Mutated HindIII
fragment 19 is indicated (19'). The acetylphosphotransferase gene providing kanamycin or neomycin resistance is indicated as aft and is located in the black box area. The borders of the T-region are indicated by arrows. The nopaline synthase gene is indicated by nos.
The numbers refer to the sizes of the restriction fragments according to Depicker et al., Plasmid 3 (1980), 193-211. The construction of the Ti plasmid pGV3838 can be taken from example 1, and the two references cited.
Fig. 13 illustrates the construction of acceptor Ti plasmid pGV3850. The plasmid pBR322-pAcgB (Fig. 11 ) is depicted in a linearized form. The pBR322 sequences are indicated by the cross-hatched area and the ampicillin resistance gene of pBR322 by ApR. Part of the T-region of pGV3839 which is shown in Fig. 12 is shown here; the HindIII
fragments (10) and (23) involved in homologous recombination with pAcgB and the apt gene are indicated. Double cross-over events lead to the construction of pGV3850 and another replicon containing the aft gene which is lost.
Fig. 14 illustrates schematically the construction of intermediate cloning vector pGV700 which is given in detail in example 2. The following abbreviations are used to indicate restriction endonuclease sites : B, BamHI; Bg, B,~r III; E, EcoRI; H, HindIII; S, SaII; Sm , Smal. The following abbreviations are used to indicate antibiotic resistance; Ap, ampicillin; Cm, chloramphenicol; Sm, streptomycin; Tc, tetracycline.
The numbers an the bottom of the figure which refer to TL-DNA
indicate the RNA transcripts of this region (Willmitzer et al., EMBO J. 1 (1982), 139-14fi).
Fig. 15 illustrates the structure of the intermediate cloning vector pGV750.
Its construction is described in example 2. The restriction endonuclease sites are indicated with their relative locations given in numbers as kilobase pairs (kb). Pstl sites are not indicated but there are 3 in the KmR/NmR region, and one in the Cb~ gene. The right and left borders are also indicated. The Bg-III/BamHI and HaaI/SmaI sites used in the construction of pGV750 are indicated but are not present in pGV750.
The shaded area corresponds to TL-DNA, the dark area to the KmR/
NmR region, the white area to contiguous Ti plasmid sequences, and the line to the cloning vehicle pBR325. Other abbreviations used are Ocs, octopine synthase; CmR, chloramphenicol resistance; CbR, carbenicillin (analogous to ampicillin) resistance, and KmR/NmR, kanamycin resistancelneomycin resistance.
Fig. 16 illustrates the construction of the intermediate vector pGV745 described in detail in example 3. pGV745 is used in the construction of V
4.
the acceptor plasmid pGV2260, a "B-like" acceptor plasmid shown in Figure 8. Restriction endonuclease sites are indicated as follows : B, BamHl; H, HindIII; R, EcoRI. The ampicillin resistance gene is indicated by ApR. The cross-hatched region indicates DNA
homologous to the left side of the T-DNA region of the octopine Ti plasmid and the white region indicates DNA homologous to the right side of the T-DNA region of the octopine Ti plasmid; the physical location and description of the starting plasmids pGV0219 and pGV0120 can be found in De Vos et al. , Plasmid 6 (1981), 249-253 .
Fig. 17 illustrates the construction of the acceptor plasmid pGV2260. The deletion substitution in pGV2217 is indicated as a black box containing the acetyl phosphotransferase gene (indicated aft) which provides resistance to neomycin and kanamycin. The intermediate vector pGV745 (Fig. 16) is depicted in linearized form; it has been opened at the Hindlll site of pGV745 shown in Fig. 16. The pBR322 sequence is indicated as a cross-hatched section and the ampicillin resistance gene by ApR. Double cross-over events lead to the construction of pGV2260 and the loss of the aft gene. Restriction endonuclease sites are indicated as follows : B, BamHL; H, HindIII; R, EcoRI.
Fig. 18 illustrates the construction of a plasmid pLGV2381 for the expression of genes downstream of the promoter of the nopaline synthase gene (nos). The 5' and 3' refer to the start and stop of transcription, and the ATG and TAA refer to the codons used to start and stop translation.
The heavy black line indicates the nos promoter region, and the white area indicates the nos coding region. ApR denotes ampicillin resistance, and KmR kanamycin resistance.
Fig. 19 illustrates the construction of the plasmid pAGV10 containing the complete octopine synthase (ocs) coding sequence and its insertion in plasmid pLGV2381 (see also Fig. 18) behind the nos promoter. The ix heavy black lines refer to the promoter regions and the white area to the ocs coding region . Other notations are as in Fig. 18.
Fig. 20 illustrates the nucleotide sequences around the promoter region of the nopaline synthase (nos) gene and the nucleotide sequences around the same region following fusion with the coding region of the octopine synthase gene. The point of fusion is indicated by an asterisk (*).
Several restriction endonuclease sites are indicated, BamHI, HindIII, and SacII. The 5' and 3' refer to the start and stop of transcription.
The ATG refers to the first codon used in translation and the TAA
refers to the stop codon used in translation. The large arrows indicate the coding regions of the nopaline gene in white and the octopine gene in stripes.
Detailed description of the invention Referring to Fig. 1, we have shown therein a simplified diagram of an acceptor Ti plasmid. This acceptor Ti plasmid contains the two border sequences (1; 2) or regions of the wild-type tumor-inducing (Ti) plasmid. The border sequences are essential for the integration of the T-region of Ti plasmids into a plant cell genome.
In other words, they are essential for the integration of any DNA sequence (3) or T-region into a plant cell genome located between these sequences.
The DNA sequence (3) of the acceptor Ti plasmid contains a DNA segment which is homologous with at least a part of a DNA sequence (3') of an intermediate cloning vector illustrated in Figs. 2 and 3. This homology is necessary for co-integration by a single cross-over event (homologous recombination) of the intermediate cloning vector with the acceptor Ti plasmid. The frequency of obtaining cointegrates is determined essentially by the length of the region of homology. In order to effect a homologous recombination event at a good frequency, regions of 1 to 4 kb are normally used (Leemans et al., J. Mol. Appl. Genet. 1 (1981 ), 149-164).
C.:- , Al '19S
Zo The acceptor Ti plasmid furthermore contains sequences (4) which are essential for the transfer by Aarobacterium of the T-region of the Ti plasmids into plant cell genomes.
The construction of such acceptor Ti plasmids and their cointegration with intermediate cloning vectors illustrated in Figs. 2 and 3 will be described later in connection with the discussion of Fig. 4.
In Figs. 2 and 3 we have shown simplified diagrams of intermediate cloning vectors for the cloning of any prokaryotic or eukaryotic genes) of interest to be expressed, i.e. transcribed under the control of a promoter and translated in plant cells. These intermediate cloning vectors contain a DNA segment (3') from a cloning vehicle containing with a DNA sequence which is homologous with at least a part of the DNA
segment (3) of the acceptor Ti plasmid thus permitting a single cross-over event.
Moreover, the intermediate cloning vectors contain at least one gene of interest (5;
7) which contains either its natural or an exogenous promoter sequence. The promoter sequence allows the expression of the inserted gene sequence(s). The use of an exogenous promoter sequence (tailored promoter) may be useful for directing the expression of the inserted genes) in a regulated fashion.
Examples of different types of regulation include the following : (i) tissue-specific expression, i.e. leaves, roots, stem, flowers; (ii) level of expression, i.e.
high or low;
and (iii) inducible expression, i.e. by temperature, light, or added chemical factors.
Examples of genes of interest for the intermediate cloning vectors are : DNA
fragments or sequences with the genetic information controlling the synthesis of products such as amino acids or sugars to modify the nutritive or growth potential of a plant; or products which provide protection against external pathogenic agents such as resistance to disease organisms or stressful environmental factors; or products which provide information on basic plant processes which are to be modified by genetic engineering techniques.
,:
Figures 2 and 3 each show intermediate cloning vectors which may contain selectable marker genes (6). Examples of selectable marker genes are those encoding resistance to antibiotics or toxic analogs (for example, amino acid analogs), or genes which can supply a defect in the recipient host cell.
Figure 4 illustrates the structures involved in the construction of hybrid Ti plasmid vectors and Figure 5 describes the actual conjugation steps involved in the isolation of Aarobacterium carrying the hybrid Ti plasmid vectors. Since the intermediate cloning vector is constructed in E. coli these steps are necessary to transfer the intermediate cloning vector to the acceptor Ti plasmid in Agrobacterium.
The known transfer process which was used to prepare modified Ti plasmids in which a portion of the T-region was replaced by an altered sequence involves many steps. Normally, most DNA recombinant manipulations are done in specially designed cloning vehicles such as pBR322 (Bolivar, Gene 2 (1977), 75-93).
However, these cloning vehicles cannot transfer on their own to Aarobacterium.
In the known process this problem is solved by a) replacing the pBR cloning vehicle sequence by another wide-host-range cloning vehicle, such as the mini-Sa plasmid (Leemans et al. , Gene 19 (1982), 361-364), capable of also replicating in Agrobacterium. The manipulations are effected in E. coli. An intermediate cloning vector is obtained.
b) Conjugation of the E. coli strain carrying the intermediate cloning vector containing the DNA of interest with another E. coli strain carrying a helper plasmid which cannot replicate in Aarobacterium but which can mediate transfer of itself and other DNAs to Aarobacterium.
c) Conjugation of E. coli obtained in step (b) with Aarobacterium containing a Ti plasmid. The helper plasmid is lost.
d) Since the intermediate cloning vector is capable of replicating and existing in Aqrobacterium as a separate replicon, the conjugants obtained in step (c) are a mixture of cells containing either the cointegrate between the intermediate cloning vector and the Ti plasmid or other cells containing the intermediate cloning vector and the Ti plasmid where no cointegration has occurred. In order to specifically isolate only the cointegrates, a second conjugation to another Aarobacterium strain without a Ti plasmid must be pertormed. This transfer is mediated by functions encoded by the Ti plasmid itself. Transfer of the intermediate cloning vector into the second Aqrobacterium strain is effected only in the form of a cointegrate with the Ti plasmid.
e) In order to obtain the final modified Ti plasmid with the desired replacement a second cross-over event is effected (Leemans et al., J. Mol. Aael. Genet. 1 (1981 ), 149-164).
The only other known method is essentially the same as outlined above, except that for step (d) another plasmid which is not compatible with the intermediate cloning vector is introduced into Aarobacterium: in this case, the cointegration (single cross-over event) can be selected for since all the intermediate cloning vectors which remain as independent replicons will be lost (Matzke ~t al., J. Mol. Appl.
Genet. 1 ( 1981 ), 39-49).
We describe a novel and much simplified method for the introduction of intermediate cloning vectors into acceptor Ti plasmids of Agrobacterium. Briefly, this method is based on the finding that helper plasmids of E_. coli allow transfer of many of the commonly used cloning plasmids (such as pBR322) dir_ ectly to A~qrobacterium.
Since none of these plasmids can replicate in Aarobacterium only those which can cointegrate with the acceptor Ti plasmid will be retained. In addition, we use this cointegrate in Aprobacterium as a vector composition directly for infection of plant cells. In this manner we have eliminated steps (d) and (e) described above which greatly increases the possibilities for using the acceptor Ti plasmids as vectors for DNA transfer to plant cell genomes by bath decreasing the time required for constructing modified hybrid Ti plasmids and increasing the flexibility of the possible constructions.
., Thus, as outlined in Figure 5, the introduction ofi the intermediate cloning vector into the acceptor Ti plasmid is accomplished in two steps. First, conjugation of E.
coli strain (1 ) carrying the intermediate cloning vector to another E. coli strain (2) carrying two plasmids which will help to mobilize the intermediate cloning vector to Agrobacterium. Typical and preferred examples of these helper plasmids are R64drd11 containing mob functions and pGJ28 containing tra functions (Finnegan et al., Mol. Gen. Genet. 185 (1982), 344-351 ). A bom site (Warren et al., Nature (1978), 259-261 ) on the cloning vehicle of the intermediate cloning vector is recognized by the functions encoded by the other two plasmids to allow transfer to occur. All plasmids should preferably contain antibiotic resistance markers to detect their presence. Secondly, the E. coli strain obtained, i.e. the mobilizing strain (3) carrying all three plasmids is conjugated to A4robacterium containing an acceptor Ti plasmid with a region of homology with the intermediate cloning vector. A
single cross-over event between the intermediate cloning vector and the acceptor Ti plasmid is detectable by selection for the antibiotic resistance marker of the intermediate cloning vector.
Figure 6 schematically illustrates the DNA molecules used to construct the acceptor Ti plasmid shown in Figure 1. We call this acceptor Ti plasmid (A) to distinguish it from the other acceptor Ti plasmid (B) (Fig. 8). The construction requires a double cross-over event between a Ti plasmid and another plasmid carrying the border sequences (1 ) and (2) in a cloning vehicle (3). As illustrated in the figure, the cloning vehicle sequence (3) lies between border sequence (1 ) on the left and (2) on the right; in order to show the correct polarity of the DNA strands, this can be drawn on a circle. However, to show the regions of homology used in the double cross-over event, this circle has been broken as indicated. This is an important subtlety to realize and it is also used in the construction of acceptor Ti plasmid (B) in Figure 8, i.e., if border sequences (1 ) and (2) were simply inserted within cloning vehicle sequence (3), a double cross-over event would produce a Ti plasmid with a deleted T-region but without the cloning vehicle sequence between the border sequences (1 ) -. and (2). As also shown here in Figure 6, the double cross-over event also produces 2~
a circular DNA molecule which contains the original T-region between border sequences (1 ) and (2); as this is not a replicon, it will be lost. Genetic selection for these events can be achieved by, for example, selecting for the loss of an antibiotic resistance marker contained within the T-region of the Ti plasmid and selecting for an antibiotic resistance marker contained within the cloning vehicle sequence (3).
Figure 7 schematically illustrates the construction of an intermediate cloning vector of Figs. 2 and 3. A gene of interest (5) and a selectable marker gene (5), each bracketed by a restriction endonuclease site R1 or R2, respectively, are inserted into a cloning vehicle sequence (3') which contains unique restriction sites for enzymes R1 and R2 by digestion and ligation of all molecules. The recombinant DNA
molecule obtained is used to transform E. coli host cells and transformants are selected for the antibiotic resistance marker (AbR' ) of the cloning vehicle sequence (3').
Figure 8 schematically illustrates the DNA molecules used to construct another embodiment of the invention, i.e. acceptor'Ti piasmid (B). Here a double cross-over event occurs between a Ti plasmid and a plasmid containing the cloning vehicle sequence (3) between the DNA sequences (9) and (10), which are located just outside the border sequences (1 ) and (2); in order to illustrate the homologous regions used in the cross-over event the small plasmid has been broken (as in Fig.
6). The product of the double cross-over event is acceptor Ti plasmid (B) and another circular DNA molecule which is lost containing the T-region from the original Ti plasmid plus the DNA sequences (2), (10), (9), and (1 ). Genetic selection can be achieved as described for Figure 6.
Figure 9 schematically illustrates an intermediate cloning vector to be used in combination with the acceptor Ti plasmid B of Figure 8. Here, the gene of interest (5) is inserted between the border sequences (1 ) and (2) which are contained in a cloning vehicle sequence (3').
Figure 10 schematically illustrates how a single cross-over event introduces the :~
intermediate cloning vector of Fig. 9 into the acceptor Ti plasmid (B). In this case, selection for the antibiotic resistance marker of the cloning vehicle sequence (3') of the intermediate cloning vector ensures that a hybrid Ti plasmid can be found which is the result of a cointegration between the two plasmids. A hybrid Ti plasmid is produced with the gene of interest contained within the border sequences (1 ) and (2). The hybrid plasmid thus constructed does not contain in its T-region a sequence which is a direct repeat (as for example the sequences (3) and (3') in hybrid Ti plasmid of Fig. 4, avoiding possible problems of instability of the hybrid vector or of the transformed DNA in the plant cell genome as a result of intramolecular recombination.
Unpublished results from our laboratory also indicate that for construction of the intermediate vector in Fig. 9, it is not essential to have both border sequences 1 and 2; it is sufficient but essential to have at least the right border sequence (2) (see Fig.
1 and Fig. 9), in order to obtain integration of the desired DNA sequence into the plant genome.
Knowledge of the restriction endonuclease maps of the Ti plasmids of Ag~robacterium, e.g. nopaline or octopine Ti plasmids (Depicker et al., Plasmid 3 (1980), 193-211; De Vos et al., Plasmid 6 (1981 ), 249-253), plus the knowledge of the restriction fragments which contain the T-DNA border regions (Zambryski et al., J. Mol. Appl. Genet. 1 (1982), 361-370; De Beuckeleer et al., Mol. Gen. Genet.
(1981 ), 283-288) enables now any investigator to construct acceptor Ti plasmids according to the process of this invention. The only additional skill required is the ability to perform conventional recombinant DNA techniques and basic bacterial genetic manipulations. The present invention is unique in that it specifically proposes the described acceptor Ti plasmids which have been shown to be effective for the construction of hybrid Ti plasmid vectors; furthermore these acceptor Ti plasmids are designed to form part of a process to introduce genes into the plant cell genome.
In order to further illustrate the disclosed acceptor Ti plasmids, intermediate cloning K
g .. . . , 2s vectors, hybrid Ti plasmid vectors and vector compositions, and to demonstrate the effectiveness of the vector compositions in providing transformed plant cells and plants showing expression of the foreign genes) integrated into the plant cell genome, the following examples are provided.
Example 1 Construction of acceptor Ti plasmid pGV3850 (type A) Starting strains and plasmids Agrobacterium tumefaciens (rifampicin-resistant strain C58C1, and chloramphenicol-erythromycin-resistant strain C58C1 derived from wild-type Aarobacterium) Ti plasmid = pGV3839 Plasmid of Fig. 11 = pAcgB
The Ti plasmid pGV3839 is constructed from a nopaline plasmid pTiC58tra°
(pGV3100; Holsters et al., Plasmid 3 (1980), 212-230). It contains a deletion substitution mutation near the centre of the T-region; the Smal fragment 24 internal to HindIII fragment 19 (Depicker et al., Plasmid 3 (1980), 193-211 ) has been substituted by a HindII fragment of pKC7 (Rao et al., Gene 7 (1979, 79-82) which contains the aft, (acetylghosphotransferase) gene of Tn5. This gene codes for resistance to the aminoglycosides neomycin and kanamycin. Figure 12 gives a restriction map of the T-region of pGV3839.
The plasmid pAcgB is an insert of AcgB in pBR322 which contains only the borders of the T-DNA (see Fig. 11 ). The borders are defined as the ends of the T-DNA
and these regions play a role in the stable integration of the T-DNA into the plant cell genome. The origin and analysis of this clone has been described in detail (Zambryski et al. , Science 209 (1980), 1385-1391 ). This clone was obtained by re-isolating portions of the T-DNA from transformed tobacco DNA. pAcgB contains the junction of two T-DNA copies which are arranged in tandem so that it contains the :>~
Cx 1 ~~1 41 9 left and right borders of the T-DNA. In addition, pAcgB contains the nopaline synthase gene since this genetic information maps very close to the right T-DNA
border. The plasmid pAcgB is used for the construction of an "A-like" acceptor Ti plasmid, pGV3850. Figure 6 outlines the structures involved and Figure 13 gives more precisely the regions of DNA involved in the double cross-over events leading to pGV3850.
The described plasmid pAcgB carries a ColEl-specific bom site in the pBR322 portion and can be mobilized from ~. coli to Aarabacterium by using the helper plasmids R64drdll and pGJ28. The plasmids R64drdll and pGJ28 contained in E.
coli are introduced into the E. coli strain carrying pAcgB by conjugation.
Transconjugants are selected as ampicillin-resistant (from the pBR322 sequences of pAcgB), streptomycin-resistant (from R64drdll) and kanamycin-resistant (from pGJ28) colonies.
The E. coli strain carrying all three plasmids is conjugated to A roq bacterium stain C58C1 which is rifampicin-resistant and which contains the Ti plasmid pGV3839.
The ampicillin-resistance of pBR322 is used to select for the first single cross-over event with the nopaline Ti plasmid. The only way that the ampicillin resistance can be stabilized in Aprobacterium is a cross-over event upon homologous recombination with pGV3839 through one of the homology regions near the T-region borders. By a second cross-over event through the other homology region, the central portion of the T-region of pGV3839 including the aft gene (kanamycin resistance) is replaced by the pBR322 sequences of the clone pAcgB. Second recombinants are thus ampicillin-resistant and kanamycin-sensitive . To increase the probability of isolating a second recombinant, the rifampicin-resistantAgrobacterium carrying the first recombinant (pAcgB::pGV3839) is conjugated with a second chloramphenicol/erythromycin-resistant Aarobacterium strain without a Ti plasmid. In this manner, a chloramphenicollerythromycin-resistant Agirobacterium pGV3850 can be obtained which is ampicillin-resistant and kanamycin-sensitive at a frequency of approximately one in 600 colonies.
~.
;~ ~a , 134~~119 Of course, there are other Ti plasmids which can be utilized to construct pGV3850-type acceptor Ti plasmids. Any Ti plasmid carrying a selectable marker gene near the centre of the T-region may be used as a recipient. Furthermore, a pAcgB-like plasmid may be constructed by inserting the T-region border fragments into pBR322 in such a way that the pBR322 sequences lie in-between the left border fragment and the right border fragment in the arientation left border fragment - pBR322 -right border fragment. For example, the left and right border fragments of the nopaline Ti plasmid are HindIII fragment 10 and 23, respectively (Depicker et al., Plasmid (1980), 193-211 ).
A single cross-over event will introduce an intermediate cloning vector containing any gene of interest which is inserted in pBR322 (or its derivatives) into the modified T-DNA region of pGV3850. The only requirement is that the DNA to be introduced contains an additional resistance marker gene to those already found in pBR322 to use as a means to select for the transfer of the intermediate cloning vector from E.
coli to Agrobacterium. This resistance market can be contained either within the pBR
sequences (such as CmR for pBR325 or KmR for pKC7) or within the DNA which is to be tested in the plant cell. In addition, in the acceptor Ti plasmid pGV3850 the ApR
gene pBR322 can be replaced by another resistance marker gene such as KmR; in this way even pBR322-containing intermediate cloning vectors which are ApR can be directly mobilized to this pGV3850-like acceptor Ti plasmid.
An added advantage of the pGV3850-type acceptor Ti plasmid is that it does not produce tumors in transformed plant cells. Cells which have been "transformed"
by pGV3850 can easily be screened from untransformed cells by assaying for the presence of nopaline as the shortened T-DNA region of pGV3850 still contains the gene encoding nopaline synthase. Of course, if the intermediate cloning vector which is cointegrated into the acceptor Ti plasmid pGV3850 contains a marker gene it can also be directly screened or selected for.
Besides insertion of defined intermediate cloning vectors containing a pBR322 sequence by a single cross-over event into the acceptor Ti plasmid pGV3850, this ~X
acceptor Ti plasmid can also be used as a recipient for cloned banks of DNA in pBR322 or its derivatives in a "shotgun"-type experiment. The total population of hybrid plasmid vectors in Aqrobacterium can be used to infect plant cells and is subsequently screened for expression of any selectable genes) of interest. For example, one can easily select for genes encoding amino acid synthesis by applying the total bank to plant cells which are deficient in the chosen amino acid.
The acceptor Ti plasmid pGV3850 has two phenotypic characteristics: (i) the inability to produce tumors, and (ii) the ability to synthesize nopaline if T-DNA
transfer occurs into the plant cell genome. Thus, several experiments are performed to check for these characteristics in various plant tissues infected with Agrobacterium containing pGV3850.
a) Tests with potato and carrot discs Inoculation of potato and carrot slices with the acceptor Ti plasmid pGV3850 results in the production of a small amount of callous tissue. This tissue is tested for the presence of nopaline and is found to be positive. It is interesting that this mutant is able to produce small callous tissue; however, it can only be obtained if the discs are grown in media containing low concentrations of both auxins and cytokinins.
b) Inoculation of whole plants with acceptor Ti plasmid pGV3850 Tobacco and petunia plantlets growing on sterile agar media (without hormones) are inoculated with pGV3850. A small amount of tissue growth can only be observed after several months (normally "wild-type" tumors are detected after two weeks.) This tissue doss not grow on hormone-free media but can be propagated further as sterile tissue culture on media containing both auxin and cytokinin. This tissue is also shown to be nopaline-positive.
c) Furthermore, since pGV3850 "transformed" cells are not tumor-like, these cells are capable of regenerating into normal plants which still contain in their genome the transferred DNA segment. Normal plants will be obtained by :~~.. ,~
culturing the transformed cells on conventional regeneration media (see also example 5).
To prove the usefulness of pGV3850 as an acceptor plasmid the following experiment is performed. An intermediate cloning vector containing oncogenic functions of the octopine T-DNA in pBR325 is recombined into A~,robacterium harboring pGV3850. The resulting hybrid Ti plasmid in Aarobacterium obtained by a single cross-over event is inoculated onto wounded tobacco plants. Tumor tissue develops after about two weeks. This is evidence that the tumor-inducing DNA
is reintroduced into pGV3850 and is expressed properly in transformed plant cells.
Example 2 Construction of intermediate cloning vectors pGV700 and pGV750 An overview of the constructions is represented schematically in figure 14.
HindIII
fragment 1, representing the right part of TL-DNA of the octopine Ti plasmid B6S3, and present in pGV0201 (De Vos et al. , Plasmid 6 (1981 ), 249-253), is inserted first in the HindIII site of the broad-host range vector pGV1122 (Leemans et al., Gene 19 (1982), 361-364). The recombinant plasmid pGV0201 contains the HindllIfragment 1 inserted in the unique HindIII site of the multicopy vector pBR322 (Bolivar et al., Gene 2 (1977), 95-113). pGV0201 and pGV1122 DNA is prepared as described by Betlach et al., Fed. Proc. 35 (1976), 2037-2043. Two pg of pGV0201 DNA are totally digested with 2 units of HindIII (all restriction enzymes are purchased from Boehringer Mannheim) for 1 hour at 37°C in a final volume of 20 N1. The incubation buffer is described by O'Farrell et al., Mol. Gen. Genet 179 (1980), 421-435.
Two Ng of pGV1122 DNA are totally digested with HindIII under the same conditions.
One tenth Ng of HindII1 digested pGV0201 is ligated to 0.05 Ng of HindIII-digested pGV1122 with 0.02 units of T4 ligase (Boehringer Mannheim) in a final volume of 20 øX
NI. Incubation buffer and conditions are as recommended by the manufacturer (Brochure "T4 ligase", Boehringer Mannheim, August 1980, #10.M.880.486).
Transformation of the ligation mixture into competent E. coli K514 hsr~ hsm' cells (Colson et al., Genetics 52 (1965), 1043-1050) is carried out as described by Dagert and Ehrlich, Gene 6 (1980), 23-28. Cells are plated on LB medium (Miller, Exaeriments in Molecular Genetics {1972), Cold Spring Harbor Laboratory, New York) supplemented with streptomycin (20 Ng/ml) and spectinomycin (50 pg/ml).
Transformants containing recombinant plasmids are screened for tetracycline sensitivity (10 Ng/ml), due to the insertionai inactivation of the gene coding for tetracycline resistance (Leemans et ~I. , Gene 19 (1982), 361-364).
Streptomycin-and spectinomycin-resistant and tetracycline-sensitive clones are physically characterized. Microscale DNA preparations are performed according to Klein et al.
(Plasmid 3 (1980), 88-91 ). The orientation of the HindIII fragment 1 in the HindIII
site of pGV1122 is determined by Sall digestion. Digestion (conditions according to O'Farrell et al., Mol. Gen. Genet. 179 (1980), 421-435) of recombinant plasmids gives 2 fragments after agarose gel electrophoresis. In the a-orientation there are fragments of 0.77 kb and 22.76 kb, whereas in the ~i-orientation there are fragments of 10.33 kb and 13.20 kb. A recombinant piasmid with the a-orientation is used in subsequent cloning and called pGV1168.
A B~c III-SaII fragment containing the left part of the TL-DNA (including the left border sequence) is introduced in pGV1168, cut with BgIII-SaII . This fragment is obtained from the recombinant plasmid pGV0153 (De Vos et al . , Plasmid 6 (1981 ), 249-253), containing BamHi fragment 8, from the T-region of pTiB6S3, inserted in the vector pBR322. pGV0153 and pGV1168 DNA is prepared according to Betlach et al. (Fed.
Proc. 35 (1976), 2037-2043). Ten Ng of pGV0153 DNA are completely digested with units of BgIII and 10 units of SaII for 1 hour at 37°C ire final volume of 100 NI. The digestion mixture is loaded on a preparative 0.8°~ agarose gel. The 2.14 kb BIgII-SaII fragment is recovered from this gel by electroelution as described by Allington et al., Anal. Biochim, 85 (1978), 188-196. Two pg of pGV1168 DNA are totally digested by 2 units of BgIII and 2 units Sali. One tenth pg of BgLII-SaII
fragment ,~.
1 341 ~+ 1 9 DNA is ligated to 0.02 pg of BgIIII-SaII-digested pGV1168 with 0.02 units of ligase in a final volume of 20 NI. The ligation mixture is transformed into competent E. coli K514 hsr hsm+ cells (Dagert and Erhlich, Gene 6 (1980) 23-28). Cells are plated on LB medium (Miller, Experiments in Molecular Genetics (1972), Cold Spring Harbor Laboratory, New York), supplemented with streptomycin (20 pg/ml) and spectinomycin (50 Ng/ml).
Microscale DNA preparations (Klein et al., Plasmid 3 (1980), 88-91 ) are performed from streptomycin- and spectinomycin-resistant transformants. Recombinant plasmids in which 2.14-kb-BgIII-SaII fragment is inserted in Bc~III-SaII-digested pGV1168 are identified by B~c III-SaII digestion, yielding 2 fragments of 2.14 kb and 21.82 kb. A plasmid with a digest pattern corresponding to these molecular weights (2.14 kb and 21.82 kb) is used for further cloning and called pGV1171. A 12.65-kb-fragment from pGV1171 contains the right and left TL-DNA border sequences (De Beuckeleer et al., in Proceedings IVth International Conference on Plant Pathogenic Bacteria, M. Ride (ed.) (1978), I.N.R.A., Angers, 115-126), as well as genes which permit oncogenic proliferation (Leemans et aL,EMBO J. (1982), 147-152). This HindIII fragment is inserted into the plasmid pBR325 (Bolivar, Gene 4 (1978), 136). pGV1171 and pBR325 are prepared according to Betlach et al., Fed. Proc.
(1976), 2037-2043). Two Ng of each DNA are totally digested with 2 units of HindIII
for 1 hour a 37°C (incubation buffer is described by O'Farrell et al., Mol. Gen. Genet.
179 (1980), 421-435). One tenth Ng of HindIII-digested pGV1171 is ligated to 0.05 Ng of pBR325, linearized with HindIII, with 0.02 units T4 DNA ligase.
Transformation of the ligation mixture in competent E. coli K514 hsr~ hsm+ is carried out as described by Dagert and Ehrlich, Gene 6 (1980), 23-28. Cells are plated on LB medium (Miller, Experiments in Molecular Genetics (1972), Cald Spring Harbor Laboratory, New York), supplemented with carbenicillin (100 Ng/ml). Carbenicillin-resistant clones are screened for sensitivity to tetracycline (10 Ng/ml), due to insertional inactivation of the gene coding for tetracycline resistance (Bolivar, Gene 4 (1978) 121-136).
Carbenicillin-resistant and tetracycline-sensitive clones are physically characterized by restriction enzyme digestion of DNA prepared from these clones by the ~- t o . i ~!Mv microscale technique (Klein et al., Plasmid 3 (1980), 88-91 ). BamHI digestion gives 4 DNA fragments : in the a-orientation fragments of 0.98 kb, 4.71 kb, 5.98 kb, and 7.02 kb are found whereas the (3-orientatian gives fragments of 0.98 kb, 4.71 kb, 1.71 kb, and 11.20 kb. A recombinant plasmid corresponding to the a-orientation is obtained, called pGV700, and used for further experiments.
pGV750 is derived from pGV700 by substituting a 2.81 kb BamHI-H~aI fragment coding for kanamycin resistance, for a 3.49-kb-BgIII-Smal fragment, encoding functions essential for oncogenicity, internal to the TI_,-region inserted in pGV700.
The BamHI-H~aI fragment encoding kanamycin resistance is obtained from ~: :TnS
(Berg et al., Proc. Natl. Acad. Sci. USA 72 (1975), 3628-3632). Preparation of a::TnS
is as described (Miller, Experiments in Molecular Genetics (1972), Cold Spring Harbor Laboratory, New York). pGV700 DNA is prepared according to Betlach et al.
(Fed. Proc. 35 (1976), 2037-2043). Two pg of pGV700 DNA are totally digested with 2 units of B~c II and 2 units Smal. Two Ngof A: :TnS DNA are totally digested with 2 units of BamHI and 2 units H .,~LaI. One pg of BamH1-Haa1 digested A: :TnS is ligated to 0.2 Ng BgIII-SmaI-digested pGV700 with 0.5 units of T4 DNA ligase in a final volume of 10 p1 (conditions are as recommended by the manufacturer). The ligation mixture is transformed in competent E. c~oli K514 hsr hsm+ cells (Dagert and Erhlich, Gene 6 (1980) 23-28). Cells are plated on I_B medium (Miller, Experiments in Molecular Genetics (1972), Cold Spring Harbor Laboratory, New York), supplemented with carbenicillin (100 Nglml) and kanamycin (25 Ng/ml) . CbRand KmR clones are physically characterized by restriction enzyme analysis of DNA
prepared according to the micro-scale technique (Klein et ai., Plasmid 3 (1980), 88-91 ). BgIII/BamHI double digests of this DNA gives 3 fragments of 3.94 kb, 5.89 kb, and 8.09 kb, whereas HindII1 digests yields 3 fragments of 2.68 kb, 5.99 kb, and 9.25 kb. A plasmid showing these digestion patterns is called pGV750 and is illustrated schematically in Figure 17 pGV700 and pGV750 are two different intermediate cloning vectors which contain the left and right border sequences of TL-DNA of the octopine Ti plasmid pTiB6S3;
~ 3~1 41 9 in addition, the internal T-region is deleted to different extents in each of the two plasmids. pGV700 contains a shortened T-region with genetic information for octopine synthase (transcript 3), and 3 other products, 4, 6a, and 6b (see Willmitzer et al., EMBO J. 1 (1982), 139-146, for a description of T-region products).
The combination of these three products (4, 6a, 6b) will cause shoot formation in transformed plants. pGV750 contains even less of the T-region, i.e. only the octopine synthase gene. The information for products 4, 6a, and 6b has been substituted by the antibiotic resistance marker gene encoding kanamycin (neomycin) resistance.
pGV700 arid pGV750 are examples of intermediate cloning vectors which can be used with acceptor Ti plasmids of the B-type (see Fig. 8 and example 3 below);
these vectors are partially analogous to the one shown in Fig. 9 except that they do not contain a gene of interest. A gene of interest can be easily inserted into these vectors as they contain single restriction endonuclease sites for cloning within their modified T-regions (see Figs. 14 and 15).
Example 3 Construction of acceptor Ti plasmid pGV2260 (type B) Starting strains and plasmids Aarobacterium tumefaciens (rifampicin-resistant strain C58C1 and erythromycin-chloramphenicol-resistant strain C58C1, derived from wild-type Agrobacterium) Ti plasmid = pGV2217 Intermediate vector (Fig. 16) = pGV745 The construction of the Ti plasmid pGV2217 has been described in detail (Leemans et al. , EMBO J. 1 {1982), 147-152). It contains a deletion substitution mutation of the entire TL-region of the octopine Ti plasmid : the BamHI fragments 8, 30b, 28, 17a and the left 3.76 kb BamHI-EcoRI fragment of the BamHI fragment 2 (De Vos et al. , '~ r r -'~,.
~~141 9 Piasmid 6 (1981 ), 249-253) have been substituted by an EcoRI-BamHI fragment of pKC7 (Rao & Rogers, Gene 7 (1979), 79-82) which contains the a~,t. (acetyl phosphotransferase) gene of Tn5. This gene codes for resistance to the aminoglycosides, neomycin and kanamycin.
The construction of the intermediate vector pGV745 is represented schematically in Fig. 16 and is described as follows. The recombinant plasmid pGV713 was derived from the octopine Ti plasmid subclone pGV0219 (De Vos et al., Plasmid 6 (1981 ), 249-253), containing HindIII fragments 14, 18c, 22e and 38c in a-orientation.
pGV0219 DNA was digested to completion with BamHI and subsequently ligated under conditions which favour self ligation of the plasmid (final concentration of DNA
in ligation mixture < INg DNAImI). Transformants were selected for ampicillin resistance, and physically characterized by restriction enzyme digestion. A
clone, which no longer contains the 6.5 kb BamHI fragment present in pGV0219, was isolated and called pGV713. This clone pGV713 was r~sed in subsequent cloning (see below). The recombinant plasmid pGV738 was derived from pGV0120 (De Vos et al., Plasmid 6 (1981 ), 249-253), containing BamHI fragment 2. pGV0120 DNA
was digested with EcoRI and self-ligated (as above for the construction of pGV713).
Transformants were selected for ampicillin resistance and analyzed by restriction enzyme digestion. A clone in which EcoRI fragments 20, 12, and a 2.95 kb EcoRI
fragment containing part of EcoRI fragment 19a and part of pBR322 were deleted, was used in further cloning and called pGV738. This plasmid still contains a 5.65 kb EcoRI-BamHI fragment from the right part of BamHI fragment 2 (De Vos et al., Plasmid 6 (1981 ), 249-253).
Next, pGV713 DNA was digested with HindITI and BamHI, and the digest was applied onto a preparative agarose gei. After electrophoresis the 2.30 kb HindIII-BamHI fragment, contained within pGV713, was purified by electroelution (as described by Allington et al., Anal. Biochem. 85 (1975), 188-196). This fragment was figated to pGV738, digested to completion with HindIII and BamHI. After transformation, ampicillin-resistant clones were physically characterized by 1 ~~+1 41 9 restriction enzyme digestion. For example, EcoRl-BamHI digestion should give 2 fragments of respectively 3.98 kb (= vector part) and 7.95 kb (= insert part).
A
recombinant plasmid with these characteristics was called pGV745 and used as intermediate vector for the construction of the acceptor Ti plasmid pGV2260.
The plasmid pGV745 contains a ColEl-specific bom site in the pBR322 portion and can be mobilized from E. coli to Ac~robacterium by using the helper plasmids R64drd11 and pGJ28, as described in example 1 (construction of the acceptor Ti plasmid pGV3850).
pGV745 was mobilized to Agrobacterium strain C58C1 which is rifampicin-resistant and contains the Ti plasmid pGV2217. The first cross-over event was selected by using the ampicillin resistance of pBR322 in the same way as described in example 1 (the construction of the acceptor Ti plasmid pGV3850) . By a second cross-over event the deletion substitution mutation present in pGV2217 is replaced by the pBR322 sequences of the plasmid pGV745. Second recombinants were picked-up by directly screening the ampicillin-resistant transconjugants, which resulted from cointegration of pGV745 with pGV2217, for the loss of kanamycin resistance. In this way, a rifampicin Aarobacterium strain C58C1, containing pGV2260 (ampicillin-resistant, kanamycin-sensitive), was obtained.
This Ti plasmid pGV2260 will be used as an acceptor plasmid (type B) for intermediate cloning vectors of the pGV700- or pGV750-type. These are composed of (i) a DNA fragment carrying the ampicillin resistance gene, the origin of replication and the bom site of pBR322 ; (ii) a DNA fragment containing the left and right border sequences of the TL-DNA, and an additional resistance marker to those already present on pBR322, which will enable the genetic selection for the transfer of the intermediate cloning vector from ~. coli to Ag~robacterium as well as for its cointegration in the acceptor Ti plasmid pGV2260.
For example, we have been able to show that Aprobacterium carrying a cointegrate between pGV2260 and pGV700 is capable of transferring the expected DNA
y~: ..'~""' sequences (those contained between the T-DNA borders) to plant cell genome.
The transformed plant cells exhibit the expected phenotype i.e. tumors which produce shoots, given that pGV700 contains the genetic information for three products (4, 6a, 6b; see Willmitzer et al., EMBO J. 1 (1982), 139-146). In this mannerwe have shown that an acceptor Ti plasmid of the B-type is capable of transferring DNA to plant cells when used as a cointegrate with an intermediate cloning vector of the type illustrated in Fig. 9 and given in example 2.
Example 4 Construction of an intermediate cloning vector containing a gene to be expressed in plants Until the present invention, insertion of whole genes into more or less random positions within the T-region of Ti plasmids has not resulted in expression of the foreign sequence following transfer to the plant genome. According to the process of this invention, the coding region of (any) foreign genes) of interest can be linked to transcriptional initiation and termination signals which are known to be functional in the plant cell. The usefulness of this approach is demonstrated according to the present invention by experiments involving the DNA sequences encoding the nopaline synthase gene. The entire sequence of this gene and the exact start and stop of transcription are known (Depicker et al., J. Mol. Appl. Genet. 1 (1982), 561-574). According to the present invention, the protein-coding region of any foreign gene can be inserted adjacent to the nos promoter. As an example of a foreign gene sequence, the coding region of the octopine synthase gene (De Greve et al., J.
Mol.
Appl. Genet. 1 (982), 499-512) is inserted adjacent to the nos promoter. This construction is mobilized into an acceptor Ti plasmid and used to infect plants. The resulting tumor tissue is assayed for the presence of octopine, and is found to be positive.
The construction of the intermediate cloning vector containing the chimeric nopaline promoter : octopine synthase structural gene is shown and described in figures 18 to i _ w 38 ~ 3~+~ 41 9 20.
Briefly, the restriction fragment HindlII-23 containing the nos gene is engineered in vitro to remove most of the nos coding sequence, and retain the nos promoter adjacent to the restriction endonuclease site BamHI (Fig. 18). Ten Ng of pGV0422 (a pBR322 derivative carrying the HindlIl-23 fragment which contains the complete nos gene; Depicker et al. , Plasmid (1980), 193-211 ) are digested with Sau3A and the 350 by fragment carrying the nos promoter is isolated from a preparative 5%
polyacrylamide gel. The promoter fragment is ligated to Bg~III -cut pKC7 (Rao et al., Gene 7 (1979), 79-82) previously treated with bacterial alkaline phosphatase (BAP) to remove 5'-terminal phosphate groups. Twenty pg of the resulting plasmid (pLGVl3) are digested with B~c III and treated with 7 units of the Ba131 exonuclease (Biolabs, New England) for 4 -10 minutes in 400 NI of 12 mM MgC1 Z, 12 mM
CaC12, 0.6 M NaCI, I mM EDTA, and 20 mM Tris-HCI, pH 8.0, at 30°C. During this time approximately 20 - 50 by of DNA are removed. The Ba131-treated molecules are digested with BamHI, and incubated with the Klenow fragment of DNA polymerase and all four deoxynucleoside triphosphates {at 10 mM each) to fill in the ends.
Plasmids are screened for a regenerated BamHI site derived from the ligation of a filled-in BamHI end and the end of the Ba131 deletion. The sizes of the BamHI-SacII
fragment of several candidates are estimated in a 6°~ urea-polyacrylamide gel, and the nucleotide sequences of the candidates with sizes ranging between 200 -nucleotides are determined. The clone pLGV81 containing the SaCII-BamHI
fragment of 203 by carrying the promoter is used to substitute the SacII-BamHI
fragment in the nos gene in pGV0422; the final promoter vector is called pLGV2381.
All the recombinant plasmids are selected by transformation of the E_. coli strain HB101.
The plasmid vector containing the engineered nos promoter is digested with BamHI
and the coding sequence for oc which is contained on a BamHI fragment is inserted into this site. The ocs coding sequence is also engineered in vitro to be bracketed by the BamHI restriction endonuclease site as described in Fig. 19. Ten pg of BamHI
fragment 17a of the octopine Ti plasmid B6S3 (De Vos et al., Plasmid 6 (1981 ), 249-253), are digested with BamHI and Smal, the fragment containing the ocs-coding sequence isolated from a 1 % agarose gel, and ligated to the large BamHI-PvuII
fragment of pBR322; 20 Ng of the resulting plasmid, pAGV828, is digested with BamHI, treated with the exonuclease Ba131 as described in Figure 18, subsequently digested with HindIII, and the ends are filled-in and self-ligated. The sizes of the Ba131 deletions are estimated in a 6% polyacrylamide gel. The nucleotide sequences of several candidates are determined, and a candidate having only 7 by remaining of the 5'-untranslated leader sequence is chosen for further work (pOCS~). In order to bracket the ocs sequence with BamHI sites, the CIaI-RsaI
fragment is filled-in and subcloned into the BaII site of pLC236 (Remaut et al. , Gene 15 (1981 ), 81-93). The resulting plasmid pAGV40 is digested with BamHI, the fragment carrying the ocs sequence isolated by electraelution from a preparative 1 agarose gel, and ligated to pLGV2381 previously cut with BamHI, and treated with BAP (bacterial alkaline phosphatase). The insertion of the ocs sequence in pLGV2381 is obtained in both orientations (pN0-1 and pN0-2).
The nucleotide sequences showing the exact junction point in the nos:ocs fusion are shown in Fig. 20.
Further, the plasmid vector containing the engineered nos promoter is used to insert DNA from the plasmid R67 which encodes the enzyme dihydrofolate reductase. The coding sequence containing the dihydrofolate reductase gene is contained on a BamHI fragment as described (O'Hare et al. , Proc. Natl. Acad. Sci. USA 78 ( 1981 ), 1527-1531 ), and thus is easily inserted into the nos promoter vector containing the BamHI site adjacent to the promoter region as described above. This gene is an example of a selectable marker gene (see for example Figs 2, 3, 4, 5, and 7) since when expressed it provides resistance to the antibiotic methotrexate. When this intermediate cloning vector is mobilized into an Aprobacterium containing a wild-type nopaline acceptor Ti plasmid, a single cross-over event occurs and a hybrid Ti-plasmid vector is obtained. The vector composition is used to infect plants.
The W
i 1~414i9 a0 resulting tumor tissue is found to be capable of sustained growth in the presence of 0.5 Ng/ml methotrexate.
The construction of the intermediate cloning vectors containing the ocs and dihydrofolate reductase coding regions behind the nos promoter described above, and their transfer and expression in transformed plant cells following cointegration with the Ti plasmid of Agrobacterium provides evidence that foreign genes can be transferred and expressed in plant cells according to the processes of this invention.
example 5 Isolation of plant cells and plants containing the desired genes) inserted in their chromosomes We have obtained plant cells and whole plants transformed with non-oncogenic acceptor Ti plasmid derivatives (e.g. pGV3850) using any of the following three methods:
(1 ) inoculation in vivo of whole plants followed by subsequent culture in vitro on media which allow the regeneration of shoots;
(2) coinfection in vivo of whole plants in the presence of other Agrobacteria strains which directly induce shoots at the wound site;
(3) cocultivation in vitro of single plant cell protoplasts.
We will describe each of these methods below.
The first method is based on a modification of methods normally used to obtain infection of whole plant tissues with wild-type Aprobacterium strains which results in the production of crown gall tissues. Since pGV385(7 is a non tumor-producing (nononcogenic) A~4robacterium derivative, no tumorous growth is observed at the infected site. However, if the infected tissue is removed and propagated in tissue culture, transformed tissues can easily be obtained. After an initial culture period (simply to increase the mass of the tissue) the wound site tissue is grown under ..
conditions which allow shoots to form. Both untransformed and pGV3850-transformed cells will produce shoots. The transformed shoots can easily be distinguished by a simple assay for the presence of nopaline.
We have obtained pGV3850- transformed calli and shoots derived from decapitated tobacco plantlets of Nicotiana tabacum Wisconsin 38 using the following protocol (all manipulations are done under sterile conditions in a laminar flow hood) .
(1 ) Use 6-week old tobacco seedlings grown in small jars (10 cm diameter x 10 cm height) on solid Murashige & Skoog (MS) medium (Murashige and Skoog, Phvsiol. Plant. 15 (1962) 473-497) containing 0.8% agar.
(2) Remove youngest top leaves with a scalpel and discard.
(3) Inoculate wound surface with a spatula or toothpick containing Aprobacterium derived from a fresh plate culture grown under selective conditions (e.g. for the rifampicin-resistant, ampicillin resistant Aqrobacterium strain containing Ti plasmid pGV3850, YEB medium containing 100 pg/ml rifampicin and 100 Ng/ml carbenicillin are used; YEB medium : 5 g/1 Bacto beef extract, 1 g/1 Bacto yeast extract, 5 g/1 peptone, 5 g/1 sucrose, 2 x 10-3 M MgS04, pH 7.2, and 15 g/1 agar). Inoculate at least 8 plantlets for each pGV3850 construction.
(4) Incubate 2 weeks; there should be little or no response at the site of inoculation; sometimes very tiny calli appear.
(5) Remove a thin section less than 1 mm thick from the wound surface.
Incubate this section of the wounded surface on a plate containing Linsmaier and Skoog (LS) agar medium (Linsmaier and Skoog, P_hvsiol. Plant. 18 (1965) 100-127) with auxins and cytokinins (1 mgl1 NAA, 0.2 mg/l BAP) and 1 sucrose.
(6) After about 6 weeks callus should be large enough, about 5 mm diameter at least, to test a portion for the presence of nopaline. Not all wound calli produce nopaline; approximately ane in four plants produce a nopaline-positive wound callus.
(7) Transfer nopaline-positive calli to agar plates containing regeneration " ~ medium : LS medium as above + 1 % sucrose and 1 mg/1 BAP cytokinin.
A
-, ~ 3~~ 4~ 9 (8) Good-sized shoots (1 cm high) appear after about 4-6 weeks. Transfer the shoots to fresh agar plates containing LS medium + 1 °!o sucrose without hormones to allow further growth and root formation.
sequences, a left T-DNA, i.e. TL-DNA, and a right TR-DNA. TL-DNA
contains sequences also found in common with T-DNA of nopaline tumor cells whereas TR-DNA does not.
tr transfer functions, : both plasmid-encoded diffusible products and sites of action utilized during DNA transfer between cells, e.g. products required to make a bridge between two cells and the site at which DNA transfer is initiated.
Transcrietion : the process of producing mRNA from a structural gene or : the process involving base paring whereby the genetic information contained in DNA is used to order a complementary sequence of bases in an RNA chain.
Transformation : genetic modification induced by the incorporation of exogenous DNA into the DNA complement of a cell.
Translation : the process of producing a polypeptide from mRNA
or : the process whereby the genetic information present in an mRNA
molecule directs the order of specific amino acids during the synthesis of a polypeptide .
Undifferentiated pheno~e : a homologous appearance of cells in a tissue without any specialized parts.
Vector : a DNA molecule designed for transfer between different host cells .
~ 3t~1 41 9 Background Art The development of recombinant DNA techniques has made the genetic engineering of microorganisms a challenging prospect. These techniques might be extended to multicellular eukaryotes, if complete organisms could be regenerated from single somatic cells. The cells of some higher plants exhibit excellent regeneration capacities and, therefore, are good materials for the genetic engineering of higher organisms.
A major problem for the genetic engineering of plants is the availability of a system for the introduction of exogenous (foreign) DNA into the plant genome. Such a system is provided by the tumor-inducing (Ti) plasmids carried by the Gram-negative soil bacterium Agrobacterium tumefaciens. This organism has been shown to cause a neo-plastic transformation, called "crown gall", of wounded tissue of a very wide range of dicotyledonous plants. The proliferating neo-plasms synthesize novel, Ti-specified metabolites, called opines. The molecular basis of this transformation is the transfer and stable integration of a well-defined T-DNA (transferred DNA) fragment of the Ti plasmid in the plant cell genome. In other words, crown gall tumors contain in their chromosomal DNA a DNA segment called the T-DNA which is homologous to DNA sequences in the Ti plasmid used to induce the tumor line.
In all cases, this T-DNA corresponds to, and is colinear with, a continuous stretch of Ti plasmid DNA which is, therefore, called the T-region.
Ti plasmids are classified according to the type of opine synthesized in crown gall cells. Aarobacterium strains which induce the synthesis of nopaline [N-a-(1,3-dicarboxypropyl)-L-arginine] in crown gall cells are called nopaline strains, and strains which induce the synthesis of octopine [N-a-(N-1-carboxyethyl)-L-arginine]
are called octopine strains. These are the most commonly used Aarobacterium strains.
The use of T-DNA as a vector for plant genetic engineering was demonstrated in a model experiment in which the 14 kb bacterial transposon Tn7 was inserted in vivo x near the right border of the T-DNA from the Ti plasmid of the strain A4robacterium T37. Nopaline synthesis was eliminated in the tumors incited by agrobacteria carrying this Ti plasmid. Furthermore, Southern blotting hybridizations revealed that the entire Tn7 was present in the chromosomal DNA of these tumors as part of an otherwise normal T-DNA sequence (Hernalsteens et al., Nature 287 (1980), 654-656; Holsters et al., Mol. Gen. Genet. 185 (1982), 283-289). Thus, the introduction of this 14 kb DNA fragment into the 23 kb T-DNA has not altered the tatter's ability to be transferred to the plant cell genome.
The borders of the T-DNA from the Ti plasmid of the nopaline strain A4robacterium T37 have been very precisely determined. It is only a portion, roughly 23 kb, of the entire nopaline Ti plasmid. Furthermore, the borders of the T-DNA are known;
the nucleotide sequences which define the borders of the T-DNA have been determined and compared with the same region of the nopaline Ti plasmid (Zambryski et al.
, Science 209 (1980), 1385-1391; Zambryski et al., J. Mot. Appl. Genet. 1 (1982), 361-370). The borders of the T-region are most probably involved in the integration of the T-DNA into the plant cell genome.
Knowledge of the T-DNA sequences which define the borders of the transferred DNA is a basic requirement for the use of the Ti plasmid as a vector for DNA
transfer to plant cells. Thus, foreign DNA can be inserted within these borders to ensure its transfer to the plant cell genome. In addition, if one expects to utilize this system it is important that the transformed plant cells are normal rather than tumorous in their growth properties. To produce normal cells after T-DNA transfer requires knowledge of the functions encoded by the T-DNA itself. Thus, the T-region of the Ti plasmid has been subjected to intense genetic analysis to determine which regions are responsible for the tumor phenotype.
The T-DNA encodes functions which are responsible for the crown gall phenotype.
The genes have been localized to specific regions of the T-DNA (L-eemans et al., EMBO J. 1 (1982), 147-152; Willmitzer et al., EMBO J_. 1 {1982), 139-146). In general, there are at least 4 genes which control the undifferentiated phenotype of tumor callus tissue. Mutants in these genes can either lead to transformed tissues which appears shoot-like or root-like. The latter results are especially important if one hopes to transfer DNA to plants for expression in normal plant tissue rather than tumor tissue.
Recently, a mutant Ti plasmid was found to induce transformed shoots which were capable for regenerating into completely normal plants. These plants were fertile and even transmitted T-DNA specific sequences through meiosis, i.e. progeny plants still contained T-DNA specific sequences (Otten et al., Mol. Gen. Genet. 183 (1981 ), 209-213). However, the transformed plant tissue contained in its chromosomal DNA
a T-DNA which was very much reduced in size due to the generation of a large deletion which removed the region of the T-DNA controlling the tumor phenotype. It is not known whether the deletion occurred during the initial transformation event or as a subsequent event leading to shoot formation.
The Ti plasmids are large (200 kb) and many genes located at different sites on the Ti plasmid are involved in the transformation of plant cells. Therefore, it is not possible to construct a small Ti plasmid-derived cloning vector with unique endonuclease recognition sites at appropriate locations within the T-region, and possessing all functions essential for T-DNA transfer and stable incorporation into the plant cell genome. One known way to introduce a chosen DNA fragment into specific restriction enzyme cleavage sites of the T-region of a Ti plasmid has been to construct cloning plasmids which are able to replicate in Aprobacterium as well as in Escherichia coli, and which contain a chosen restriction fragment of the T-DNA.
Such cloning plasmids were denoted "intermediate vectors". Such intermediate vectors were used to analyze the functions encoded by the T-region (Leemans et al., J. Mol. Aaal. Genet. 1 (1981 ), 149-164).
Disclosure of the invention The present invention relates to a process for the introduction of expressible genes into plant cell genomes. It is one of the objects of the present invention to provide modified acceptor Ti plasmids which allow the introduction of any genes) of interest into these plasmids. The genes) of interest to be introduced is (are) contained within a novel intermediate cloning vector carrying a region of homology with a corresponding region in the acceptor Ti plasmid. The intermediate cloning vectors are a further object of this invention.
The introduction of the genes) of interest into the acceptor Ti plasmids is achieved by a single cross-over event which occurs within the two homologous DNA
segments of the acceptor Ti plasmid harbored in Agrobacterium and the intermediate cloning vector. The intermediate cloning vector is mobilized from Escherichia coli where it is propagated to Aarobacterium using helper plasmids. Such helper plasmids and their functions for mobilization are known (Finnegan et al., Mol. Gen. Genet. 185 (1982), 344-351).
The result of the single cross-over event in Aarobacterium is a hybrid Ti plasmid vector. Such hybrid Ti plasmid vectors are a further object of the invention The resulting hybrid plasmid vectors harbored in Agrobacterium (hereinafter called vector composition) can be used directly to infect plant cells which are subsequently screened for the expression of the product{s) of the gene{s) of interest. This process for preparing transformed plant cells by infection of plant cells with the vector composition, and the transformed plant cells, as well as plants generated therefrom are further objects of this invention. This strategy is applicable to any of the plant-transferable plasmids of Aarobacterium.
Description of drawings Fig. 1 illustrates one embodiment of an acceptor Ti plasmid of the invention which is the result of a deletion of the internal portion of the T-region, except for the border sequences (1 ) and (2). The border sequences are essential for the integration of the T-region into a plant cell genome. The region (3) between border sequences {1 ) and {2) is the DNA segment which will be transferred to the plant. The acceptor Ti plasmid contains a DNA segment (3) with a DNA
sequence which is homologous with at least a part of a DNA sequence in an intermediate cloning vector permitting integration of the intermediate cloning vector via a single cross-over event. The Ti plasmid region (4) codes for functions which are essential for the transfer by Agrobacterium of the T-region into plant cell genomes. This region has been designated as vir-region.
Fig. 2 illustrates an intermediate cloning vector of the invention to be inserted by a single cross-over event into the acceptor Ti plasmid of Fig. I. It contains a cloning vehicle DNA segment (3') with a DNA sequence which is homologous with a least part of the DNA segment (3) of the acceptor Ti plasmid permitting the desired single cross-over event. Moreover, the intermediate cloning vector contains a gene or group of genes (5) of interest having its natural promoter sequence. In general plant genes can be used in this construction as they are mare likely to be expressed. However, in principle any natural gene of interest can be inserted. The intermediate cloning vector may also contain a selectable marker gene (6). This gene should contain a promoter sequence which permits expression of the gene in plant cells. Plant cells containing this marker gene should have a selective growth advantage over cells without this ,, A. 4 gene; in this way plant cells which have been transformed by DNA containing this marker gene can be distinguished from untransformed plant cells .
Fig . 3 illustrates another embodiment of an intermediate cloning vector of the invention which is similar to the intermediate cloning vector of F'ig. 2, and is to be inserted by a single cross-over event into the acceptor Ti plasmid of Fig. 1. It contains the cloning vehicle DNA segment (3'), an exogen-ous promoter sequence (8) allowing regulated expression of the genes) of interest (7), and, if desired, a marker gene (6). . .
Fig. 4 schematically illustrates the construction of hybrid Ti plas-mid vectors of the invention from the acceptor Ti plasmid of F ig _ 1, and the intermediate cloning vectors of Figs 2 and 3 by a single cross-over event.
Fig. 5 outlines the steps involved in the genetic transfer of an in~errnedia~e cloning vector from E. coli to Aarobacterium containing «r acceptor Ti plasmid. 'The first step is the conjugation of the E. coll. strain (2) containing the inter-me4iate cloning vector to another E. coli strain (2) which cc:~tains ~wc helper plasmids far the later conjugation to Agrobacter ium. One helper plasmid contains DNA sequences irr_aortant for plasmid transfer (tra) and the other helper pl«smid c3ntains sequences which are important for the mobilization (mob). l~Vhen these helper plasmids are intro-duced by conjugation into E. call strain (1), the inter-mediate cloning vector contained therein will be capable of being transferred to other b~icterial strains. The tra and mob helper plasmids also contain antibiotic resistance mark-ers Abr2 and AbrJ which are different from those :found in -the intermediate cloning vector (Abr ). Thus, the pres-ence of all the plasmids can be monitored on selective media. A mobilizing strain (3) is obtained. This mobilizing strain (3) is conjugated to an A. tumefaciens strain (4) which contains the acceptor Ti plasmid of Fig. 1 followed by selection for antibiotic resistance markers) of the intermediate cloning vector. As the intermediate cloning vector cannot replicate in Agrobacterium, it can only be maintained if it has formed a cointegrate with the recipient acceptor Ti plasmid; this cointegrate structure in Aarobacterium (5) is the final hybrid Ti plasmid used to transfer DNA into plant cell genomes.
Fig. 6 illustrates the construction of a model acceptor Ti plasmid (A) which is analogous to that shown in Fig. 1. Here, a double cross-over event occurs between a Ti plasmid and another plasmid containing a DNA sequence which is to replace a portion of the original Ti plasmid. More specifically, the smaller plasmid contains the border sequences of the T-region (1; 2) in a cloning vehicle (3). A double cross-over results in the deletion of the internal portion T of the T-region and its replacement by the cloning vehicle. The acceptor Ti plasmid (A) obtained is capable of transferring DNA contained between the border sequences (1; 2) into plant cell genomes. The resulting transformed plant DNA will not produce tumoraus crown gall tissue as the genes controlling neoplastic growth are deleted in the Ti plasmid (A). Ti plasmid (A) is a very generalized acceptor Ti plasmid for any intermediate cloning vector with homology with cloning vehicle (3). The cloning vehicle (3) may be a conventional plasmid, such as pBR322 (or its derivatives).
Fig. 7 illustrates schematically the steps leading to the construction of an intermediate cloning vector in E. coli host cells. A gene of interest (5) bracketed by restriction endonuclease site R1 and a selectable marker gene (6) bracketed by .
restriction endonuclease site R2 are inserted into a cloning vehicle (3') containing single restriction sites for the en-zymes R1 and R2. All three molecules are digested with restriction enzymes R:i and/or ft~ and ligated together using DNA ligase to form the intermediate cloning vector. The cloning vehicle 3' mu:~t also contain additional DNA sequen-ces whi<:h code for antibiotic resistance (Abrl) to use as a selectable marker for bacterial genetics . The gene of inter-est (5) may be under the control of its natural promoter or of an exogenous promoter as outlizned in Figs. 2 and 3.
Fig . $ illustrates the ~ construction of another embodiment of an acceptor Ti plasmid (B) of the invention. Here, a double cross-over event occurs between a 'l"i plasrnid and a cloning - vehicle (3) which contains DNA sequences (9) and (10) which are homologoLes to Ti sequences just outside the border sequences (1) and (2) respectively. The double cross-over went results in the deletion of the entire 'T-re-gion T i.ncluying the border sequences (1) anal (2) and its replaceme~ i with the cloning vehicle (3) . Ti plasmid (B ) is an accep ~_or for intermediate cloning vectors which contain ti~!e gene ef interest c:lor~ed- bet:weEen the border sequen-ces (1) arid {2); (see Fig. 9).
Fig. ° illustrates an intermediate cloning vector of the invention to be inserted by a single cross-over event into the acceptor Ti plasmid i8) of Fig. $. It contains the border sequen-ces (1) and (2) which flank the genes) of interest (5). It also contains a cloning vehicle sequence (3' ) which is at least partially homologous to the cloning vehicle sequence - - (3) in the acceptor Ti plasmid (B) to allow homologous recombination between the two plasmids .
Fig. 10 schematically illustrat~a the construction of hybrid Ti plas-mid vectors of the invention from the acceptor Ti plasmid 1 ~~1 41 9 (B) of Fig. 8 and the corresponding intermediate cloning vector of Fig.
9. A single cross-over event introduces the intermediate cloning vector of Fig. 9 into the acceptor Ti plasmid (B) of Fig. 8.
The following figures 11 to 20 more specifically illustrate the invention.
Fig. 11 illustrates the insertion of the 5.2 kb HindIII fragment AcgB into pBR322 (see also Zambryski et al., Science 209 (1980), 1385-1391 ).
This fragment AcgB contains the right and left border regions of the nopaline Ti plasmid. This clone pAcgB is used in the construction of acceptor plasmid pGV3850, an "A-like" acceptor plasmid as shown in Fig: 6. it is obvious to those skilled in the art that a clone analogous to clone pAcgB can be obtained by using the cloned restriction fragments which contain the left and right border region of a wild-type Ti plasmid.
Fig. 12 illustrates the T-region of nopaline Ti plasmid pGV3839. The HindIII
restriction endonuclease sites are indicated as (H). Mutated HindIII
fragment 19 is indicated (19'). The acetylphosphotransferase gene providing kanamycin or neomycin resistance is indicated as aft and is located in the black box area. The borders of the T-region are indicated by arrows. The nopaline synthase gene is indicated by nos.
The numbers refer to the sizes of the restriction fragments according to Depicker et al., Plasmid 3 (1980), 193-211. The construction of the Ti plasmid pGV3838 can be taken from example 1, and the two references cited.
Fig. 13 illustrates the construction of acceptor Ti plasmid pGV3850. The plasmid pBR322-pAcgB (Fig. 11 ) is depicted in a linearized form. The pBR322 sequences are indicated by the cross-hatched area and the ampicillin resistance gene of pBR322 by ApR. Part of the T-region of pGV3839 which is shown in Fig. 12 is shown here; the HindIII
fragments (10) and (23) involved in homologous recombination with pAcgB and the apt gene are indicated. Double cross-over events lead to the construction of pGV3850 and another replicon containing the aft gene which is lost.
Fig. 14 illustrates schematically the construction of intermediate cloning vector pGV700 which is given in detail in example 2. The following abbreviations are used to indicate restriction endonuclease sites : B, BamHI; Bg, B,~r III; E, EcoRI; H, HindIII; S, SaII; Sm , Smal. The following abbreviations are used to indicate antibiotic resistance; Ap, ampicillin; Cm, chloramphenicol; Sm, streptomycin; Tc, tetracycline.
The numbers an the bottom of the figure which refer to TL-DNA
indicate the RNA transcripts of this region (Willmitzer et al., EMBO J. 1 (1982), 139-14fi).
Fig. 15 illustrates the structure of the intermediate cloning vector pGV750.
Its construction is described in example 2. The restriction endonuclease sites are indicated with their relative locations given in numbers as kilobase pairs (kb). Pstl sites are not indicated but there are 3 in the KmR/NmR region, and one in the Cb~ gene. The right and left borders are also indicated. The Bg-III/BamHI and HaaI/SmaI sites used in the construction of pGV750 are indicated but are not present in pGV750.
The shaded area corresponds to TL-DNA, the dark area to the KmR/
NmR region, the white area to contiguous Ti plasmid sequences, and the line to the cloning vehicle pBR325. Other abbreviations used are Ocs, octopine synthase; CmR, chloramphenicol resistance; CbR, carbenicillin (analogous to ampicillin) resistance, and KmR/NmR, kanamycin resistancelneomycin resistance.
Fig. 16 illustrates the construction of the intermediate vector pGV745 described in detail in example 3. pGV745 is used in the construction of V
4.
the acceptor plasmid pGV2260, a "B-like" acceptor plasmid shown in Figure 8. Restriction endonuclease sites are indicated as follows : B, BamHl; H, HindIII; R, EcoRI. The ampicillin resistance gene is indicated by ApR. The cross-hatched region indicates DNA
homologous to the left side of the T-DNA region of the octopine Ti plasmid and the white region indicates DNA homologous to the right side of the T-DNA region of the octopine Ti plasmid; the physical location and description of the starting plasmids pGV0219 and pGV0120 can be found in De Vos et al. , Plasmid 6 (1981), 249-253 .
Fig. 17 illustrates the construction of the acceptor plasmid pGV2260. The deletion substitution in pGV2217 is indicated as a black box containing the acetyl phosphotransferase gene (indicated aft) which provides resistance to neomycin and kanamycin. The intermediate vector pGV745 (Fig. 16) is depicted in linearized form; it has been opened at the Hindlll site of pGV745 shown in Fig. 16. The pBR322 sequence is indicated as a cross-hatched section and the ampicillin resistance gene by ApR. Double cross-over events lead to the construction of pGV2260 and the loss of the aft gene. Restriction endonuclease sites are indicated as follows : B, BamHL; H, HindIII; R, EcoRI.
Fig. 18 illustrates the construction of a plasmid pLGV2381 for the expression of genes downstream of the promoter of the nopaline synthase gene (nos). The 5' and 3' refer to the start and stop of transcription, and the ATG and TAA refer to the codons used to start and stop translation.
The heavy black line indicates the nos promoter region, and the white area indicates the nos coding region. ApR denotes ampicillin resistance, and KmR kanamycin resistance.
Fig. 19 illustrates the construction of the plasmid pAGV10 containing the complete octopine synthase (ocs) coding sequence and its insertion in plasmid pLGV2381 (see also Fig. 18) behind the nos promoter. The ix heavy black lines refer to the promoter regions and the white area to the ocs coding region . Other notations are as in Fig. 18.
Fig. 20 illustrates the nucleotide sequences around the promoter region of the nopaline synthase (nos) gene and the nucleotide sequences around the same region following fusion with the coding region of the octopine synthase gene. The point of fusion is indicated by an asterisk (*).
Several restriction endonuclease sites are indicated, BamHI, HindIII, and SacII. The 5' and 3' refer to the start and stop of transcription.
The ATG refers to the first codon used in translation and the TAA
refers to the stop codon used in translation. The large arrows indicate the coding regions of the nopaline gene in white and the octopine gene in stripes.
Detailed description of the invention Referring to Fig. 1, we have shown therein a simplified diagram of an acceptor Ti plasmid. This acceptor Ti plasmid contains the two border sequences (1; 2) or regions of the wild-type tumor-inducing (Ti) plasmid. The border sequences are essential for the integration of the T-region of Ti plasmids into a plant cell genome.
In other words, they are essential for the integration of any DNA sequence (3) or T-region into a plant cell genome located between these sequences.
The DNA sequence (3) of the acceptor Ti plasmid contains a DNA segment which is homologous with at least a part of a DNA sequence (3') of an intermediate cloning vector illustrated in Figs. 2 and 3. This homology is necessary for co-integration by a single cross-over event (homologous recombination) of the intermediate cloning vector with the acceptor Ti plasmid. The frequency of obtaining cointegrates is determined essentially by the length of the region of homology. In order to effect a homologous recombination event at a good frequency, regions of 1 to 4 kb are normally used (Leemans et al., J. Mol. Appl. Genet. 1 (1981 ), 149-164).
C.:- , Al '19S
Zo The acceptor Ti plasmid furthermore contains sequences (4) which are essential for the transfer by Aarobacterium of the T-region of the Ti plasmids into plant cell genomes.
The construction of such acceptor Ti plasmids and their cointegration with intermediate cloning vectors illustrated in Figs. 2 and 3 will be described later in connection with the discussion of Fig. 4.
In Figs. 2 and 3 we have shown simplified diagrams of intermediate cloning vectors for the cloning of any prokaryotic or eukaryotic genes) of interest to be expressed, i.e. transcribed under the control of a promoter and translated in plant cells. These intermediate cloning vectors contain a DNA segment (3') from a cloning vehicle containing with a DNA sequence which is homologous with at least a part of the DNA
segment (3) of the acceptor Ti plasmid thus permitting a single cross-over event.
Moreover, the intermediate cloning vectors contain at least one gene of interest (5;
7) which contains either its natural or an exogenous promoter sequence. The promoter sequence allows the expression of the inserted gene sequence(s). The use of an exogenous promoter sequence (tailored promoter) may be useful for directing the expression of the inserted genes) in a regulated fashion.
Examples of different types of regulation include the following : (i) tissue-specific expression, i.e. leaves, roots, stem, flowers; (ii) level of expression, i.e.
high or low;
and (iii) inducible expression, i.e. by temperature, light, or added chemical factors.
Examples of genes of interest for the intermediate cloning vectors are : DNA
fragments or sequences with the genetic information controlling the synthesis of products such as amino acids or sugars to modify the nutritive or growth potential of a plant; or products which provide protection against external pathogenic agents such as resistance to disease organisms or stressful environmental factors; or products which provide information on basic plant processes which are to be modified by genetic engineering techniques.
,:
Figures 2 and 3 each show intermediate cloning vectors which may contain selectable marker genes (6). Examples of selectable marker genes are those encoding resistance to antibiotics or toxic analogs (for example, amino acid analogs), or genes which can supply a defect in the recipient host cell.
Figure 4 illustrates the structures involved in the construction of hybrid Ti plasmid vectors and Figure 5 describes the actual conjugation steps involved in the isolation of Aarobacterium carrying the hybrid Ti plasmid vectors. Since the intermediate cloning vector is constructed in E. coli these steps are necessary to transfer the intermediate cloning vector to the acceptor Ti plasmid in Agrobacterium.
The known transfer process which was used to prepare modified Ti plasmids in which a portion of the T-region was replaced by an altered sequence involves many steps. Normally, most DNA recombinant manipulations are done in specially designed cloning vehicles such as pBR322 (Bolivar, Gene 2 (1977), 75-93).
However, these cloning vehicles cannot transfer on their own to Aarobacterium.
In the known process this problem is solved by a) replacing the pBR cloning vehicle sequence by another wide-host-range cloning vehicle, such as the mini-Sa plasmid (Leemans et al. , Gene 19 (1982), 361-364), capable of also replicating in Agrobacterium. The manipulations are effected in E. coli. An intermediate cloning vector is obtained.
b) Conjugation of the E. coli strain carrying the intermediate cloning vector containing the DNA of interest with another E. coli strain carrying a helper plasmid which cannot replicate in Aarobacterium but which can mediate transfer of itself and other DNAs to Aarobacterium.
c) Conjugation of E. coli obtained in step (b) with Aarobacterium containing a Ti plasmid. The helper plasmid is lost.
d) Since the intermediate cloning vector is capable of replicating and existing in Aqrobacterium as a separate replicon, the conjugants obtained in step (c) are a mixture of cells containing either the cointegrate between the intermediate cloning vector and the Ti plasmid or other cells containing the intermediate cloning vector and the Ti plasmid where no cointegration has occurred. In order to specifically isolate only the cointegrates, a second conjugation to another Aarobacterium strain without a Ti plasmid must be pertormed. This transfer is mediated by functions encoded by the Ti plasmid itself. Transfer of the intermediate cloning vector into the second Aqrobacterium strain is effected only in the form of a cointegrate with the Ti plasmid.
e) In order to obtain the final modified Ti plasmid with the desired replacement a second cross-over event is effected (Leemans et al., J. Mol. Aael. Genet. 1 (1981 ), 149-164).
The only other known method is essentially the same as outlined above, except that for step (d) another plasmid which is not compatible with the intermediate cloning vector is introduced into Aarobacterium: in this case, the cointegration (single cross-over event) can be selected for since all the intermediate cloning vectors which remain as independent replicons will be lost (Matzke ~t al., J. Mol. Appl.
Genet. 1 ( 1981 ), 39-49).
We describe a novel and much simplified method for the introduction of intermediate cloning vectors into acceptor Ti plasmids of Agrobacterium. Briefly, this method is based on the finding that helper plasmids of E_. coli allow transfer of many of the commonly used cloning plasmids (such as pBR322) dir_ ectly to A~qrobacterium.
Since none of these plasmids can replicate in Aarobacterium only those which can cointegrate with the acceptor Ti plasmid will be retained. In addition, we use this cointegrate in Aprobacterium as a vector composition directly for infection of plant cells. In this manner we have eliminated steps (d) and (e) described above which greatly increases the possibilities for using the acceptor Ti plasmids as vectors for DNA transfer to plant cell genomes by bath decreasing the time required for constructing modified hybrid Ti plasmids and increasing the flexibility of the possible constructions.
., Thus, as outlined in Figure 5, the introduction ofi the intermediate cloning vector into the acceptor Ti plasmid is accomplished in two steps. First, conjugation of E.
coli strain (1 ) carrying the intermediate cloning vector to another E. coli strain (2) carrying two plasmids which will help to mobilize the intermediate cloning vector to Agrobacterium. Typical and preferred examples of these helper plasmids are R64drd11 containing mob functions and pGJ28 containing tra functions (Finnegan et al., Mol. Gen. Genet. 185 (1982), 344-351 ). A bom site (Warren et al., Nature (1978), 259-261 ) on the cloning vehicle of the intermediate cloning vector is recognized by the functions encoded by the other two plasmids to allow transfer to occur. All plasmids should preferably contain antibiotic resistance markers to detect their presence. Secondly, the E. coli strain obtained, i.e. the mobilizing strain (3) carrying all three plasmids is conjugated to A4robacterium containing an acceptor Ti plasmid with a region of homology with the intermediate cloning vector. A
single cross-over event between the intermediate cloning vector and the acceptor Ti plasmid is detectable by selection for the antibiotic resistance marker of the intermediate cloning vector.
Figure 6 schematically illustrates the DNA molecules used to construct the acceptor Ti plasmid shown in Figure 1. We call this acceptor Ti plasmid (A) to distinguish it from the other acceptor Ti plasmid (B) (Fig. 8). The construction requires a double cross-over event between a Ti plasmid and another plasmid carrying the border sequences (1 ) and (2) in a cloning vehicle (3). As illustrated in the figure, the cloning vehicle sequence (3) lies between border sequence (1 ) on the left and (2) on the right; in order to show the correct polarity of the DNA strands, this can be drawn on a circle. However, to show the regions of homology used in the double cross-over event, this circle has been broken as indicated. This is an important subtlety to realize and it is also used in the construction of acceptor Ti plasmid (B) in Figure 8, i.e., if border sequences (1 ) and (2) were simply inserted within cloning vehicle sequence (3), a double cross-over event would produce a Ti plasmid with a deleted T-region but without the cloning vehicle sequence between the border sequences (1 ) -. and (2). As also shown here in Figure 6, the double cross-over event also produces 2~
a circular DNA molecule which contains the original T-region between border sequences (1 ) and (2); as this is not a replicon, it will be lost. Genetic selection for these events can be achieved by, for example, selecting for the loss of an antibiotic resistance marker contained within the T-region of the Ti plasmid and selecting for an antibiotic resistance marker contained within the cloning vehicle sequence (3).
Figure 7 schematically illustrates the construction of an intermediate cloning vector of Figs. 2 and 3. A gene of interest (5) and a selectable marker gene (5), each bracketed by a restriction endonuclease site R1 or R2, respectively, are inserted into a cloning vehicle sequence (3') which contains unique restriction sites for enzymes R1 and R2 by digestion and ligation of all molecules. The recombinant DNA
molecule obtained is used to transform E. coli host cells and transformants are selected for the antibiotic resistance marker (AbR' ) of the cloning vehicle sequence (3').
Figure 8 schematically illustrates the DNA molecules used to construct another embodiment of the invention, i.e. acceptor'Ti piasmid (B). Here a double cross-over event occurs between a Ti plasmid and a plasmid containing the cloning vehicle sequence (3) between the DNA sequences (9) and (10), which are located just outside the border sequences (1 ) and (2); in order to illustrate the homologous regions used in the cross-over event the small plasmid has been broken (as in Fig.
6). The product of the double cross-over event is acceptor Ti plasmid (B) and another circular DNA molecule which is lost containing the T-region from the original Ti plasmid plus the DNA sequences (2), (10), (9), and (1 ). Genetic selection can be achieved as described for Figure 6.
Figure 9 schematically illustrates an intermediate cloning vector to be used in combination with the acceptor Ti plasmid B of Figure 8. Here, the gene of interest (5) is inserted between the border sequences (1 ) and (2) which are contained in a cloning vehicle sequence (3').
Figure 10 schematically illustrates how a single cross-over event introduces the :~
intermediate cloning vector of Fig. 9 into the acceptor Ti plasmid (B). In this case, selection for the antibiotic resistance marker of the cloning vehicle sequence (3') of the intermediate cloning vector ensures that a hybrid Ti plasmid can be found which is the result of a cointegration between the two plasmids. A hybrid Ti plasmid is produced with the gene of interest contained within the border sequences (1 ) and (2). The hybrid plasmid thus constructed does not contain in its T-region a sequence which is a direct repeat (as for example the sequences (3) and (3') in hybrid Ti plasmid of Fig. 4, avoiding possible problems of instability of the hybrid vector or of the transformed DNA in the plant cell genome as a result of intramolecular recombination.
Unpublished results from our laboratory also indicate that for construction of the intermediate vector in Fig. 9, it is not essential to have both border sequences 1 and 2; it is sufficient but essential to have at least the right border sequence (2) (see Fig.
1 and Fig. 9), in order to obtain integration of the desired DNA sequence into the plant genome.
Knowledge of the restriction endonuclease maps of the Ti plasmids of Ag~robacterium, e.g. nopaline or octopine Ti plasmids (Depicker et al., Plasmid 3 (1980), 193-211; De Vos et al., Plasmid 6 (1981 ), 249-253), plus the knowledge of the restriction fragments which contain the T-DNA border regions (Zambryski et al., J. Mol. Appl. Genet. 1 (1982), 361-370; De Beuckeleer et al., Mol. Gen. Genet.
(1981 ), 283-288) enables now any investigator to construct acceptor Ti plasmids according to the process of this invention. The only additional skill required is the ability to perform conventional recombinant DNA techniques and basic bacterial genetic manipulations. The present invention is unique in that it specifically proposes the described acceptor Ti plasmids which have been shown to be effective for the construction of hybrid Ti plasmid vectors; furthermore these acceptor Ti plasmids are designed to form part of a process to introduce genes into the plant cell genome.
In order to further illustrate the disclosed acceptor Ti plasmids, intermediate cloning K
g .. . . , 2s vectors, hybrid Ti plasmid vectors and vector compositions, and to demonstrate the effectiveness of the vector compositions in providing transformed plant cells and plants showing expression of the foreign genes) integrated into the plant cell genome, the following examples are provided.
Example 1 Construction of acceptor Ti plasmid pGV3850 (type A) Starting strains and plasmids Agrobacterium tumefaciens (rifampicin-resistant strain C58C1, and chloramphenicol-erythromycin-resistant strain C58C1 derived from wild-type Aarobacterium) Ti plasmid = pGV3839 Plasmid of Fig. 11 = pAcgB
The Ti plasmid pGV3839 is constructed from a nopaline plasmid pTiC58tra°
(pGV3100; Holsters et al., Plasmid 3 (1980), 212-230). It contains a deletion substitution mutation near the centre of the T-region; the Smal fragment 24 internal to HindIII fragment 19 (Depicker et al., Plasmid 3 (1980), 193-211 ) has been substituted by a HindII fragment of pKC7 (Rao et al., Gene 7 (1979, 79-82) which contains the aft, (acetylghosphotransferase) gene of Tn5. This gene codes for resistance to the aminoglycosides neomycin and kanamycin. Figure 12 gives a restriction map of the T-region of pGV3839.
The plasmid pAcgB is an insert of AcgB in pBR322 which contains only the borders of the T-DNA (see Fig. 11 ). The borders are defined as the ends of the T-DNA
and these regions play a role in the stable integration of the T-DNA into the plant cell genome. The origin and analysis of this clone has been described in detail (Zambryski et al. , Science 209 (1980), 1385-1391 ). This clone was obtained by re-isolating portions of the T-DNA from transformed tobacco DNA. pAcgB contains the junction of two T-DNA copies which are arranged in tandem so that it contains the :>~
Cx 1 ~~1 41 9 left and right borders of the T-DNA. In addition, pAcgB contains the nopaline synthase gene since this genetic information maps very close to the right T-DNA
border. The plasmid pAcgB is used for the construction of an "A-like" acceptor Ti plasmid, pGV3850. Figure 6 outlines the structures involved and Figure 13 gives more precisely the regions of DNA involved in the double cross-over events leading to pGV3850.
The described plasmid pAcgB carries a ColEl-specific bom site in the pBR322 portion and can be mobilized from ~. coli to Aarabacterium by using the helper plasmids R64drdll and pGJ28. The plasmids R64drdll and pGJ28 contained in E.
coli are introduced into the E. coli strain carrying pAcgB by conjugation.
Transconjugants are selected as ampicillin-resistant (from the pBR322 sequences of pAcgB), streptomycin-resistant (from R64drdll) and kanamycin-resistant (from pGJ28) colonies.
The E. coli strain carrying all three plasmids is conjugated to A roq bacterium stain C58C1 which is rifampicin-resistant and which contains the Ti plasmid pGV3839.
The ampicillin-resistance of pBR322 is used to select for the first single cross-over event with the nopaline Ti plasmid. The only way that the ampicillin resistance can be stabilized in Aprobacterium is a cross-over event upon homologous recombination with pGV3839 through one of the homology regions near the T-region borders. By a second cross-over event through the other homology region, the central portion of the T-region of pGV3839 including the aft gene (kanamycin resistance) is replaced by the pBR322 sequences of the clone pAcgB. Second recombinants are thus ampicillin-resistant and kanamycin-sensitive . To increase the probability of isolating a second recombinant, the rifampicin-resistantAgrobacterium carrying the first recombinant (pAcgB::pGV3839) is conjugated with a second chloramphenicol/erythromycin-resistant Aarobacterium strain without a Ti plasmid. In this manner, a chloramphenicollerythromycin-resistant Agirobacterium pGV3850 can be obtained which is ampicillin-resistant and kanamycin-sensitive at a frequency of approximately one in 600 colonies.
~.
;~ ~a , 134~~119 Of course, there are other Ti plasmids which can be utilized to construct pGV3850-type acceptor Ti plasmids. Any Ti plasmid carrying a selectable marker gene near the centre of the T-region may be used as a recipient. Furthermore, a pAcgB-like plasmid may be constructed by inserting the T-region border fragments into pBR322 in such a way that the pBR322 sequences lie in-between the left border fragment and the right border fragment in the arientation left border fragment - pBR322 -right border fragment. For example, the left and right border fragments of the nopaline Ti plasmid are HindIII fragment 10 and 23, respectively (Depicker et al., Plasmid (1980), 193-211 ).
A single cross-over event will introduce an intermediate cloning vector containing any gene of interest which is inserted in pBR322 (or its derivatives) into the modified T-DNA region of pGV3850. The only requirement is that the DNA to be introduced contains an additional resistance marker gene to those already found in pBR322 to use as a means to select for the transfer of the intermediate cloning vector from E.
coli to Agrobacterium. This resistance market can be contained either within the pBR
sequences (such as CmR for pBR325 or KmR for pKC7) or within the DNA which is to be tested in the plant cell. In addition, in the acceptor Ti plasmid pGV3850 the ApR
gene pBR322 can be replaced by another resistance marker gene such as KmR; in this way even pBR322-containing intermediate cloning vectors which are ApR can be directly mobilized to this pGV3850-like acceptor Ti plasmid.
An added advantage of the pGV3850-type acceptor Ti plasmid is that it does not produce tumors in transformed plant cells. Cells which have been "transformed"
by pGV3850 can easily be screened from untransformed cells by assaying for the presence of nopaline as the shortened T-DNA region of pGV3850 still contains the gene encoding nopaline synthase. Of course, if the intermediate cloning vector which is cointegrated into the acceptor Ti plasmid pGV3850 contains a marker gene it can also be directly screened or selected for.
Besides insertion of defined intermediate cloning vectors containing a pBR322 sequence by a single cross-over event into the acceptor Ti plasmid pGV3850, this ~X
acceptor Ti plasmid can also be used as a recipient for cloned banks of DNA in pBR322 or its derivatives in a "shotgun"-type experiment. The total population of hybrid plasmid vectors in Aqrobacterium can be used to infect plant cells and is subsequently screened for expression of any selectable genes) of interest. For example, one can easily select for genes encoding amino acid synthesis by applying the total bank to plant cells which are deficient in the chosen amino acid.
The acceptor Ti plasmid pGV3850 has two phenotypic characteristics: (i) the inability to produce tumors, and (ii) the ability to synthesize nopaline if T-DNA
transfer occurs into the plant cell genome. Thus, several experiments are performed to check for these characteristics in various plant tissues infected with Agrobacterium containing pGV3850.
a) Tests with potato and carrot discs Inoculation of potato and carrot slices with the acceptor Ti plasmid pGV3850 results in the production of a small amount of callous tissue. This tissue is tested for the presence of nopaline and is found to be positive. It is interesting that this mutant is able to produce small callous tissue; however, it can only be obtained if the discs are grown in media containing low concentrations of both auxins and cytokinins.
b) Inoculation of whole plants with acceptor Ti plasmid pGV3850 Tobacco and petunia plantlets growing on sterile agar media (without hormones) are inoculated with pGV3850. A small amount of tissue growth can only be observed after several months (normally "wild-type" tumors are detected after two weeks.) This tissue doss not grow on hormone-free media but can be propagated further as sterile tissue culture on media containing both auxin and cytokinin. This tissue is also shown to be nopaline-positive.
c) Furthermore, since pGV3850 "transformed" cells are not tumor-like, these cells are capable of regenerating into normal plants which still contain in their genome the transferred DNA segment. Normal plants will be obtained by :~~.. ,~
culturing the transformed cells on conventional regeneration media (see also example 5).
To prove the usefulness of pGV3850 as an acceptor plasmid the following experiment is performed. An intermediate cloning vector containing oncogenic functions of the octopine T-DNA in pBR325 is recombined into A~,robacterium harboring pGV3850. The resulting hybrid Ti plasmid in Aarobacterium obtained by a single cross-over event is inoculated onto wounded tobacco plants. Tumor tissue develops after about two weeks. This is evidence that the tumor-inducing DNA
is reintroduced into pGV3850 and is expressed properly in transformed plant cells.
Example 2 Construction of intermediate cloning vectors pGV700 and pGV750 An overview of the constructions is represented schematically in figure 14.
HindIII
fragment 1, representing the right part of TL-DNA of the octopine Ti plasmid B6S3, and present in pGV0201 (De Vos et al. , Plasmid 6 (1981 ), 249-253), is inserted first in the HindIII site of the broad-host range vector pGV1122 (Leemans et al., Gene 19 (1982), 361-364). The recombinant plasmid pGV0201 contains the HindllIfragment 1 inserted in the unique HindIII site of the multicopy vector pBR322 (Bolivar et al., Gene 2 (1977), 95-113). pGV0201 and pGV1122 DNA is prepared as described by Betlach et al., Fed. Proc. 35 (1976), 2037-2043. Two pg of pGV0201 DNA are totally digested with 2 units of HindIII (all restriction enzymes are purchased from Boehringer Mannheim) for 1 hour at 37°C in a final volume of 20 N1. The incubation buffer is described by O'Farrell et al., Mol. Gen. Genet 179 (1980), 421-435.
Two Ng of pGV1122 DNA are totally digested with HindIII under the same conditions.
One tenth Ng of HindII1 digested pGV0201 is ligated to 0.05 Ng of HindIII-digested pGV1122 with 0.02 units of T4 ligase (Boehringer Mannheim) in a final volume of 20 øX
NI. Incubation buffer and conditions are as recommended by the manufacturer (Brochure "T4 ligase", Boehringer Mannheim, August 1980, #10.M.880.486).
Transformation of the ligation mixture into competent E. coli K514 hsr~ hsm' cells (Colson et al., Genetics 52 (1965), 1043-1050) is carried out as described by Dagert and Ehrlich, Gene 6 (1980), 23-28. Cells are plated on LB medium (Miller, Exaeriments in Molecular Genetics {1972), Cold Spring Harbor Laboratory, New York) supplemented with streptomycin (20 Ng/ml) and spectinomycin (50 pg/ml).
Transformants containing recombinant plasmids are screened for tetracycline sensitivity (10 Ng/ml), due to the insertionai inactivation of the gene coding for tetracycline resistance (Leemans et ~I. , Gene 19 (1982), 361-364).
Streptomycin-and spectinomycin-resistant and tetracycline-sensitive clones are physically characterized. Microscale DNA preparations are performed according to Klein et al.
(Plasmid 3 (1980), 88-91 ). The orientation of the HindIII fragment 1 in the HindIII
site of pGV1122 is determined by Sall digestion. Digestion (conditions according to O'Farrell et al., Mol. Gen. Genet. 179 (1980), 421-435) of recombinant plasmids gives 2 fragments after agarose gel electrophoresis. In the a-orientation there are fragments of 0.77 kb and 22.76 kb, whereas in the ~i-orientation there are fragments of 10.33 kb and 13.20 kb. A recombinant piasmid with the a-orientation is used in subsequent cloning and called pGV1168.
A B~c III-SaII fragment containing the left part of the TL-DNA (including the left border sequence) is introduced in pGV1168, cut with BgIII-SaII . This fragment is obtained from the recombinant plasmid pGV0153 (De Vos et al . , Plasmid 6 (1981 ), 249-253), containing BamHi fragment 8, from the T-region of pTiB6S3, inserted in the vector pBR322. pGV0153 and pGV1168 DNA is prepared according to Betlach et al. (Fed.
Proc. 35 (1976), 2037-2043). Ten Ng of pGV0153 DNA are completely digested with units of BgIII and 10 units of SaII for 1 hour at 37°C ire final volume of 100 NI. The digestion mixture is loaded on a preparative 0.8°~ agarose gel. The 2.14 kb BIgII-SaII fragment is recovered from this gel by electroelution as described by Allington et al., Anal. Biochim, 85 (1978), 188-196. Two pg of pGV1168 DNA are totally digested by 2 units of BgIII and 2 units Sali. One tenth pg of BgLII-SaII
fragment ,~.
1 341 ~+ 1 9 DNA is ligated to 0.02 pg of BgIIII-SaII-digested pGV1168 with 0.02 units of ligase in a final volume of 20 NI. The ligation mixture is transformed into competent E. coli K514 hsr hsm+ cells (Dagert and Erhlich, Gene 6 (1980) 23-28). Cells are plated on LB medium (Miller, Experiments in Molecular Genetics (1972), Cold Spring Harbor Laboratory, New York), supplemented with streptomycin (20 pg/ml) and spectinomycin (50 Ng/ml).
Microscale DNA preparations (Klein et al., Plasmid 3 (1980), 88-91 ) are performed from streptomycin- and spectinomycin-resistant transformants. Recombinant plasmids in which 2.14-kb-BgIII-SaII fragment is inserted in Bc~III-SaII-digested pGV1168 are identified by B~c III-SaII digestion, yielding 2 fragments of 2.14 kb and 21.82 kb. A plasmid with a digest pattern corresponding to these molecular weights (2.14 kb and 21.82 kb) is used for further cloning and called pGV1171. A 12.65-kb-fragment from pGV1171 contains the right and left TL-DNA border sequences (De Beuckeleer et al., in Proceedings IVth International Conference on Plant Pathogenic Bacteria, M. Ride (ed.) (1978), I.N.R.A., Angers, 115-126), as well as genes which permit oncogenic proliferation (Leemans et aL,EMBO J. (1982), 147-152). This HindIII fragment is inserted into the plasmid pBR325 (Bolivar, Gene 4 (1978), 136). pGV1171 and pBR325 are prepared according to Betlach et al., Fed. Proc.
(1976), 2037-2043). Two Ng of each DNA are totally digested with 2 units of HindIII
for 1 hour a 37°C (incubation buffer is described by O'Farrell et al., Mol. Gen. Genet.
179 (1980), 421-435). One tenth Ng of HindIII-digested pGV1171 is ligated to 0.05 Ng of pBR325, linearized with HindIII, with 0.02 units T4 DNA ligase.
Transformation of the ligation mixture in competent E. coli K514 hsr~ hsm+ is carried out as described by Dagert and Ehrlich, Gene 6 (1980), 23-28. Cells are plated on LB medium (Miller, Experiments in Molecular Genetics (1972), Cald Spring Harbor Laboratory, New York), supplemented with carbenicillin (100 Ng/ml). Carbenicillin-resistant clones are screened for sensitivity to tetracycline (10 Ng/ml), due to insertional inactivation of the gene coding for tetracycline resistance (Bolivar, Gene 4 (1978) 121-136).
Carbenicillin-resistant and tetracycline-sensitive clones are physically characterized by restriction enzyme digestion of DNA prepared from these clones by the ~- t o . i ~!Mv microscale technique (Klein et al., Plasmid 3 (1980), 88-91 ). BamHI digestion gives 4 DNA fragments : in the a-orientation fragments of 0.98 kb, 4.71 kb, 5.98 kb, and 7.02 kb are found whereas the (3-orientatian gives fragments of 0.98 kb, 4.71 kb, 1.71 kb, and 11.20 kb. A recombinant plasmid corresponding to the a-orientation is obtained, called pGV700, and used for further experiments.
pGV750 is derived from pGV700 by substituting a 2.81 kb BamHI-H~aI fragment coding for kanamycin resistance, for a 3.49-kb-BgIII-Smal fragment, encoding functions essential for oncogenicity, internal to the TI_,-region inserted in pGV700.
The BamHI-H~aI fragment encoding kanamycin resistance is obtained from ~: :TnS
(Berg et al., Proc. Natl. Acad. Sci. USA 72 (1975), 3628-3632). Preparation of a::TnS
is as described (Miller, Experiments in Molecular Genetics (1972), Cold Spring Harbor Laboratory, New York). pGV700 DNA is prepared according to Betlach et al.
(Fed. Proc. 35 (1976), 2037-2043). Two pg of pGV700 DNA are totally digested with 2 units of B~c II and 2 units Smal. Two Ngof A: :TnS DNA are totally digested with 2 units of BamHI and 2 units H .,~LaI. One pg of BamH1-Haa1 digested A: :TnS is ligated to 0.2 Ng BgIII-SmaI-digested pGV700 with 0.5 units of T4 DNA ligase in a final volume of 10 p1 (conditions are as recommended by the manufacturer). The ligation mixture is transformed in competent E. c~oli K514 hsr hsm+ cells (Dagert and Erhlich, Gene 6 (1980) 23-28). Cells are plated on I_B medium (Miller, Experiments in Molecular Genetics (1972), Cold Spring Harbor Laboratory, New York), supplemented with carbenicillin (100 Nglml) and kanamycin (25 Ng/ml) . CbRand KmR clones are physically characterized by restriction enzyme analysis of DNA
prepared according to the micro-scale technique (Klein et ai., Plasmid 3 (1980), 88-91 ). BgIII/BamHI double digests of this DNA gives 3 fragments of 3.94 kb, 5.89 kb, and 8.09 kb, whereas HindII1 digests yields 3 fragments of 2.68 kb, 5.99 kb, and 9.25 kb. A plasmid showing these digestion patterns is called pGV750 and is illustrated schematically in Figure 17 pGV700 and pGV750 are two different intermediate cloning vectors which contain the left and right border sequences of TL-DNA of the octopine Ti plasmid pTiB6S3;
~ 3~1 41 9 in addition, the internal T-region is deleted to different extents in each of the two plasmids. pGV700 contains a shortened T-region with genetic information for octopine synthase (transcript 3), and 3 other products, 4, 6a, and 6b (see Willmitzer et al., EMBO J. 1 (1982), 139-146, for a description of T-region products).
The combination of these three products (4, 6a, 6b) will cause shoot formation in transformed plants. pGV750 contains even less of the T-region, i.e. only the octopine synthase gene. The information for products 4, 6a, and 6b has been substituted by the antibiotic resistance marker gene encoding kanamycin (neomycin) resistance.
pGV700 arid pGV750 are examples of intermediate cloning vectors which can be used with acceptor Ti plasmids of the B-type (see Fig. 8 and example 3 below);
these vectors are partially analogous to the one shown in Fig. 9 except that they do not contain a gene of interest. A gene of interest can be easily inserted into these vectors as they contain single restriction endonuclease sites for cloning within their modified T-regions (see Figs. 14 and 15).
Example 3 Construction of acceptor Ti plasmid pGV2260 (type B) Starting strains and plasmids Aarobacterium tumefaciens (rifampicin-resistant strain C58C1 and erythromycin-chloramphenicol-resistant strain C58C1, derived from wild-type Agrobacterium) Ti plasmid = pGV2217 Intermediate vector (Fig. 16) = pGV745 The construction of the Ti plasmid pGV2217 has been described in detail (Leemans et al. , EMBO J. 1 {1982), 147-152). It contains a deletion substitution mutation of the entire TL-region of the octopine Ti plasmid : the BamHI fragments 8, 30b, 28, 17a and the left 3.76 kb BamHI-EcoRI fragment of the BamHI fragment 2 (De Vos et al. , '~ r r -'~,.
~~141 9 Piasmid 6 (1981 ), 249-253) have been substituted by an EcoRI-BamHI fragment of pKC7 (Rao & Rogers, Gene 7 (1979), 79-82) which contains the a~,t. (acetyl phosphotransferase) gene of Tn5. This gene codes for resistance to the aminoglycosides, neomycin and kanamycin.
The construction of the intermediate vector pGV745 is represented schematically in Fig. 16 and is described as follows. The recombinant plasmid pGV713 was derived from the octopine Ti plasmid subclone pGV0219 (De Vos et al., Plasmid 6 (1981 ), 249-253), containing HindIII fragments 14, 18c, 22e and 38c in a-orientation.
pGV0219 DNA was digested to completion with BamHI and subsequently ligated under conditions which favour self ligation of the plasmid (final concentration of DNA
in ligation mixture < INg DNAImI). Transformants were selected for ampicillin resistance, and physically characterized by restriction enzyme digestion. A
clone, which no longer contains the 6.5 kb BamHI fragment present in pGV0219, was isolated and called pGV713. This clone pGV713 was r~sed in subsequent cloning (see below). The recombinant plasmid pGV738 was derived from pGV0120 (De Vos et al., Plasmid 6 (1981 ), 249-253), containing BamHI fragment 2. pGV0120 DNA
was digested with EcoRI and self-ligated (as above for the construction of pGV713).
Transformants were selected for ampicillin resistance and analyzed by restriction enzyme digestion. A clone in which EcoRI fragments 20, 12, and a 2.95 kb EcoRI
fragment containing part of EcoRI fragment 19a and part of pBR322 were deleted, was used in further cloning and called pGV738. This plasmid still contains a 5.65 kb EcoRI-BamHI fragment from the right part of BamHI fragment 2 (De Vos et al., Plasmid 6 (1981 ), 249-253).
Next, pGV713 DNA was digested with HindITI and BamHI, and the digest was applied onto a preparative agarose gei. After electrophoresis the 2.30 kb HindIII-BamHI fragment, contained within pGV713, was purified by electroelution (as described by Allington et al., Anal. Biochem. 85 (1975), 188-196). This fragment was figated to pGV738, digested to completion with HindIII and BamHI. After transformation, ampicillin-resistant clones were physically characterized by 1 ~~+1 41 9 restriction enzyme digestion. For example, EcoRl-BamHI digestion should give 2 fragments of respectively 3.98 kb (= vector part) and 7.95 kb (= insert part).
A
recombinant plasmid with these characteristics was called pGV745 and used as intermediate vector for the construction of the acceptor Ti plasmid pGV2260.
The plasmid pGV745 contains a ColEl-specific bom site in the pBR322 portion and can be mobilized from E. coli to Ac~robacterium by using the helper plasmids R64drd11 and pGJ28, as described in example 1 (construction of the acceptor Ti plasmid pGV3850).
pGV745 was mobilized to Agrobacterium strain C58C1 which is rifampicin-resistant and contains the Ti plasmid pGV2217. The first cross-over event was selected by using the ampicillin resistance of pBR322 in the same way as described in example 1 (the construction of the acceptor Ti plasmid pGV3850) . By a second cross-over event the deletion substitution mutation present in pGV2217 is replaced by the pBR322 sequences of the plasmid pGV745. Second recombinants were picked-up by directly screening the ampicillin-resistant transconjugants, which resulted from cointegration of pGV745 with pGV2217, for the loss of kanamycin resistance. In this way, a rifampicin Aarobacterium strain C58C1, containing pGV2260 (ampicillin-resistant, kanamycin-sensitive), was obtained.
This Ti plasmid pGV2260 will be used as an acceptor plasmid (type B) for intermediate cloning vectors of the pGV700- or pGV750-type. These are composed of (i) a DNA fragment carrying the ampicillin resistance gene, the origin of replication and the bom site of pBR322 ; (ii) a DNA fragment containing the left and right border sequences of the TL-DNA, and an additional resistance marker to those already present on pBR322, which will enable the genetic selection for the transfer of the intermediate cloning vector from ~. coli to Ag~robacterium as well as for its cointegration in the acceptor Ti plasmid pGV2260.
For example, we have been able to show that Aprobacterium carrying a cointegrate between pGV2260 and pGV700 is capable of transferring the expected DNA
y~: ..'~""' sequences (those contained between the T-DNA borders) to plant cell genome.
The transformed plant cells exhibit the expected phenotype i.e. tumors which produce shoots, given that pGV700 contains the genetic information for three products (4, 6a, 6b; see Willmitzer et al., EMBO J. 1 (1982), 139-146). In this mannerwe have shown that an acceptor Ti plasmid of the B-type is capable of transferring DNA to plant cells when used as a cointegrate with an intermediate cloning vector of the type illustrated in Fig. 9 and given in example 2.
Example 4 Construction of an intermediate cloning vector containing a gene to be expressed in plants Until the present invention, insertion of whole genes into more or less random positions within the T-region of Ti plasmids has not resulted in expression of the foreign sequence following transfer to the plant genome. According to the process of this invention, the coding region of (any) foreign genes) of interest can be linked to transcriptional initiation and termination signals which are known to be functional in the plant cell. The usefulness of this approach is demonstrated according to the present invention by experiments involving the DNA sequences encoding the nopaline synthase gene. The entire sequence of this gene and the exact start and stop of transcription are known (Depicker et al., J. Mol. Appl. Genet. 1 (1982), 561-574). According to the present invention, the protein-coding region of any foreign gene can be inserted adjacent to the nos promoter. As an example of a foreign gene sequence, the coding region of the octopine synthase gene (De Greve et al., J.
Mol.
Appl. Genet. 1 (982), 499-512) is inserted adjacent to the nos promoter. This construction is mobilized into an acceptor Ti plasmid and used to infect plants. The resulting tumor tissue is assayed for the presence of octopine, and is found to be positive.
The construction of the intermediate cloning vector containing the chimeric nopaline promoter : octopine synthase structural gene is shown and described in figures 18 to i _ w 38 ~ 3~+~ 41 9 20.
Briefly, the restriction fragment HindlII-23 containing the nos gene is engineered in vitro to remove most of the nos coding sequence, and retain the nos promoter adjacent to the restriction endonuclease site BamHI (Fig. 18). Ten Ng of pGV0422 (a pBR322 derivative carrying the HindlIl-23 fragment which contains the complete nos gene; Depicker et al. , Plasmid (1980), 193-211 ) are digested with Sau3A and the 350 by fragment carrying the nos promoter is isolated from a preparative 5%
polyacrylamide gel. The promoter fragment is ligated to Bg~III -cut pKC7 (Rao et al., Gene 7 (1979), 79-82) previously treated with bacterial alkaline phosphatase (BAP) to remove 5'-terminal phosphate groups. Twenty pg of the resulting plasmid (pLGVl3) are digested with B~c III and treated with 7 units of the Ba131 exonuclease (Biolabs, New England) for 4 -10 minutes in 400 NI of 12 mM MgC1 Z, 12 mM
CaC12, 0.6 M NaCI, I mM EDTA, and 20 mM Tris-HCI, pH 8.0, at 30°C. During this time approximately 20 - 50 by of DNA are removed. The Ba131-treated molecules are digested with BamHI, and incubated with the Klenow fragment of DNA polymerase and all four deoxynucleoside triphosphates {at 10 mM each) to fill in the ends.
Plasmids are screened for a regenerated BamHI site derived from the ligation of a filled-in BamHI end and the end of the Ba131 deletion. The sizes of the BamHI-SacII
fragment of several candidates are estimated in a 6°~ urea-polyacrylamide gel, and the nucleotide sequences of the candidates with sizes ranging between 200 -nucleotides are determined. The clone pLGV81 containing the SaCII-BamHI
fragment of 203 by carrying the promoter is used to substitute the SacII-BamHI
fragment in the nos gene in pGV0422; the final promoter vector is called pLGV2381.
All the recombinant plasmids are selected by transformation of the E_. coli strain HB101.
The plasmid vector containing the engineered nos promoter is digested with BamHI
and the coding sequence for oc which is contained on a BamHI fragment is inserted into this site. The ocs coding sequence is also engineered in vitro to be bracketed by the BamHI restriction endonuclease site as described in Fig. 19. Ten pg of BamHI
fragment 17a of the octopine Ti plasmid B6S3 (De Vos et al., Plasmid 6 (1981 ), 249-253), are digested with BamHI and Smal, the fragment containing the ocs-coding sequence isolated from a 1 % agarose gel, and ligated to the large BamHI-PvuII
fragment of pBR322; 20 Ng of the resulting plasmid, pAGV828, is digested with BamHI, treated with the exonuclease Ba131 as described in Figure 18, subsequently digested with HindIII, and the ends are filled-in and self-ligated. The sizes of the Ba131 deletions are estimated in a 6% polyacrylamide gel. The nucleotide sequences of several candidates are determined, and a candidate having only 7 by remaining of the 5'-untranslated leader sequence is chosen for further work (pOCS~). In order to bracket the ocs sequence with BamHI sites, the CIaI-RsaI
fragment is filled-in and subcloned into the BaII site of pLC236 (Remaut et al. , Gene 15 (1981 ), 81-93). The resulting plasmid pAGV40 is digested with BamHI, the fragment carrying the ocs sequence isolated by electraelution from a preparative 1 agarose gel, and ligated to pLGV2381 previously cut with BamHI, and treated with BAP (bacterial alkaline phosphatase). The insertion of the ocs sequence in pLGV2381 is obtained in both orientations (pN0-1 and pN0-2).
The nucleotide sequences showing the exact junction point in the nos:ocs fusion are shown in Fig. 20.
Further, the plasmid vector containing the engineered nos promoter is used to insert DNA from the plasmid R67 which encodes the enzyme dihydrofolate reductase. The coding sequence containing the dihydrofolate reductase gene is contained on a BamHI fragment as described (O'Hare et al. , Proc. Natl. Acad. Sci. USA 78 ( 1981 ), 1527-1531 ), and thus is easily inserted into the nos promoter vector containing the BamHI site adjacent to the promoter region as described above. This gene is an example of a selectable marker gene (see for example Figs 2, 3, 4, 5, and 7) since when expressed it provides resistance to the antibiotic methotrexate. When this intermediate cloning vector is mobilized into an Aprobacterium containing a wild-type nopaline acceptor Ti plasmid, a single cross-over event occurs and a hybrid Ti-plasmid vector is obtained. The vector composition is used to infect plants.
The W
i 1~414i9 a0 resulting tumor tissue is found to be capable of sustained growth in the presence of 0.5 Ng/ml methotrexate.
The construction of the intermediate cloning vectors containing the ocs and dihydrofolate reductase coding regions behind the nos promoter described above, and their transfer and expression in transformed plant cells following cointegration with the Ti plasmid of Agrobacterium provides evidence that foreign genes can be transferred and expressed in plant cells according to the processes of this invention.
example 5 Isolation of plant cells and plants containing the desired genes) inserted in their chromosomes We have obtained plant cells and whole plants transformed with non-oncogenic acceptor Ti plasmid derivatives (e.g. pGV3850) using any of the following three methods:
(1 ) inoculation in vivo of whole plants followed by subsequent culture in vitro on media which allow the regeneration of shoots;
(2) coinfection in vivo of whole plants in the presence of other Agrobacteria strains which directly induce shoots at the wound site;
(3) cocultivation in vitro of single plant cell protoplasts.
We will describe each of these methods below.
The first method is based on a modification of methods normally used to obtain infection of whole plant tissues with wild-type Aprobacterium strains which results in the production of crown gall tissues. Since pGV385(7 is a non tumor-producing (nononcogenic) A~4robacterium derivative, no tumorous growth is observed at the infected site. However, if the infected tissue is removed and propagated in tissue culture, transformed tissues can easily be obtained. After an initial culture period (simply to increase the mass of the tissue) the wound site tissue is grown under ..
conditions which allow shoots to form. Both untransformed and pGV3850-transformed cells will produce shoots. The transformed shoots can easily be distinguished by a simple assay for the presence of nopaline.
We have obtained pGV3850- transformed calli and shoots derived from decapitated tobacco plantlets of Nicotiana tabacum Wisconsin 38 using the following protocol (all manipulations are done under sterile conditions in a laminar flow hood) .
(1 ) Use 6-week old tobacco seedlings grown in small jars (10 cm diameter x 10 cm height) on solid Murashige & Skoog (MS) medium (Murashige and Skoog, Phvsiol. Plant. 15 (1962) 473-497) containing 0.8% agar.
(2) Remove youngest top leaves with a scalpel and discard.
(3) Inoculate wound surface with a spatula or toothpick containing Aprobacterium derived from a fresh plate culture grown under selective conditions (e.g. for the rifampicin-resistant, ampicillin resistant Aqrobacterium strain containing Ti plasmid pGV3850, YEB medium containing 100 pg/ml rifampicin and 100 Ng/ml carbenicillin are used; YEB medium : 5 g/1 Bacto beef extract, 1 g/1 Bacto yeast extract, 5 g/1 peptone, 5 g/1 sucrose, 2 x 10-3 M MgS04, pH 7.2, and 15 g/1 agar). Inoculate at least 8 plantlets for each pGV3850 construction.
(4) Incubate 2 weeks; there should be little or no response at the site of inoculation; sometimes very tiny calli appear.
(5) Remove a thin section less than 1 mm thick from the wound surface.
Incubate this section of the wounded surface on a plate containing Linsmaier and Skoog (LS) agar medium (Linsmaier and Skoog, P_hvsiol. Plant. 18 (1965) 100-127) with auxins and cytokinins (1 mgl1 NAA, 0.2 mg/l BAP) and 1 sucrose.
(6) After about 6 weeks callus should be large enough, about 5 mm diameter at least, to test a portion for the presence of nopaline. Not all wound calli produce nopaline; approximately ane in four plants produce a nopaline-positive wound callus.
(7) Transfer nopaline-positive calli to agar plates containing regeneration " ~ medium : LS medium as above + 1 % sucrose and 1 mg/1 BAP cytokinin.
A
-, ~ 3~~ 4~ 9 (8) Good-sized shoots (1 cm high) appear after about 4-6 weeks. Transfer the shoots to fresh agar plates containing LS medium + 1 °!o sucrose without hormones to allow further growth and root formation.
(9) Let shoots grow 1 or 2 weeks such that a portion (one or two small leaves) can be removed to test for the presence of nopaline.
(10) Transfer nopaline-positive shoots to larger vessels (10 cm jars as above containing MS medium as in (1 ) to grow further.
N.B. All plant culture media far infected tissues contain 500 Ng/ml of the antibiotic cefotaxime (Claforan~, Hoechst) as a selection against A~arobacterium containing pGV3850. This drug works well to prevent growth of all A-.ac irobacteria (including those which are carbenicillin-resistant).
Another method to obtain transformed and shooting tissues has been recently developed in our laboratory. This method is based on the observation that certain mutant Ti plasmid strains of Aqrobacterium induce crown gall tumors which produce shoots. Such shoot-inducing (shi) mutants map to a particular region of the T-DNA
(transferred DNA segment) of the Ti plasmids of A. tumefaciens (Leemans et al., EMBO J. 1 (1982) 147-152; Joos et al., Cell ~2 (1983) 1057-10fi7). Often the induced shoots are composed of completely normal untransformed cells. Thus, we tried to inoculate plants with a mixture of two different Aorobacteria, one carrying an octopine Ti plasmid shooter mutant and the other carrying pGV3850. In this manner, there is a good chance that the octopine shooter mutation can induce shoots which have been transformed with pGV3850. We have inoculated plants with Agrobacterium containing Ti plasmid pGV3850 and an octopine shoot inducing Ti plasmid in a 5:1 ratio. In this way we have obtained pGV3850-transformed shoots;
these shoots are easily screened by assaying for the presence of nopaline.
This method avoids the need for any elaborate tissue culture methods. The nopaline-positive shoots are transferred to media containing simple salts and sugar with any growth-regulating hormones to allow further growth. After the shoots have reached a sufficient size they can easily be transferred to soil for propagation. This coinfection procedure should be particularly useful for transforming plant species which are not ~;
. ~."r 1 readily amenable to tissue culture. Thus, a whole range of agronomically and economically important plants, such as legumes, medicinal plants, and ornamentals will be able to be engineered by Aarobacterium.
The third procedure allows the isolation of Nicotiana tabacum protoplasts and the selection of hormone-independent T-DNA-transformed cell clones after co-cultivation of the protoplast-derived cells with oncogenic Ac~obacterium strains. An analogous technique can be used for the selection of transformed cells when other dominant selective markers are used, such as antibiotic resistance genes constructed in such a way as to be expressed in higher plant cells (see example 3).
In this case, however, the conditions for selection have to be optimized in each case (concentration of the selective agent, time between transformatian and selection, concentration of the protoplast-derived cells or cell colonies in the selective medium). If no selection for the transformed cells is possible, e.g. because avirulent T-DNA mutants are used, such as e.g. pGV3850 or pGV2217 (Leemans et al., EMBO J. 1 (1982), 147-152), it is possible to cultivate the cells after genetic transformation on auxin- and cytokinin-containing medium (e.g. Murashige and Skoog medium (Murashige and Skoog, P_ hysiol. Plant 15 (1962), 473-497) with 2 mg/litre NAA (a-naphthalene acetic acid) and 0.3 mg/litre kinetin), and to identify the transformed colonies by their opine content. In this way, after electrophoretic analysis for agropine and mannopine synthesis (method see t_eemans et al., J.
Mol.
Appl. Genet. 1 (1981 ), 149-164) about 660 colonies can be found, obtained after infection with pGV2217, a Nicotiana tabacum SRI cell line which synthesizes the TR-encoded opine mannopine (N2-(1-mannityl)-glutamine). Numerous shoots are formed after incubation of callus pieces of this cell line on regeneration medium (Murashige and Skoog medium with BAP (6-benzylaminopurine) (1 mg/litre) as the sole plant growth regulator). All 20 shoots analyzed are still able to synthesize mannopine.
After transfer onto hormone-free Murashige and Skoog medium, the shoots grow as morphologically normal tobacco plants still containing mannopine.
The protoplast isolation and transformation described here for N. tabacum can also 1 3~1 41 9 be used for N. plumbaginifolia.
2. Experimental procedures 2.1. Shoot culture conditions Nicotiana tabacum shoot cultures are maintained in 250 ml glass jars on hormone-free Murashige and Skoog medium (Murashige and Skoog, Physiol.
Plant 15 (1962), 473-497) under sterile conditions in a culture room (16 hour day, 1500 lux white fluorescent light ("ACEC LF 58 W/2 4300°K
Economy"), 24°C, 70% relative humidity). Five week old shoot cultures are used for protoplast isolation.
2.2. Protoplast isolation Aseptic techniques are used far all steps in protoplast isolation and culture.
The protoplasts are isolated by a mixed enzyme procedure. All leaves, except for very young leaves smaller than 2 cm, can be used for protoplast isolation.
The leaves are cut in strips, about 2 - 3 mm wide, with a sharp scalpel knife.
Two to three grams of leaf material is incubated 18 hours at 24°C in 50 ml enzyme mixture in the dark without agitation. The enzyme mixture consists of 0.5% cellulose Onozuka* R-10 and 0.2% macerozyme Onozuka R-10 in hormone-free K3 medium (Nagy and Malign, Z. Pflanzenphvsiol. 78 (1976), 453-455). The mixture is filter-sterilized through a 0.22 Nm pore membrane, and can be stored for at least 6 months at -20°C without notable loss of activity.
2.3. Protoplast culture After 18 hours incubation the mixture is agitated gently in order to release the protoplasts. The mixture is subsequently filtered through a 50 Nm sieve, and the filtrate is transferred to 10 ml centrifuge tubes. After centrifugation for 6 minutes at 60 - 80 g in a swinging bucket rotor the protoplasts form a dark ;, t a,y /rp.
*trade mark 45 ~ 3 4 ~ 4 ~ 9 green floating band. The liquid underlying the protoplasts, and the debris which forms the pellet, are removed using a capillary tube connected to a peristaltic pump. The protoplasts are pooled in one tube and washed 2 times with culture medium. The culture medium is the K3 medium (Nagy and Maliga, Z. Pflanzenahysial. 78 (1976), 453-455) with NAA (0.1 mg/litre) and kinetin (0.2 mg/litre) as growth regulators. The medium is adjusted to pH 5.6 and sterilized through 0.22 Nm filter membrane. After the second wash, the protoplasts are counted using a Thoma hemacytometer (obtained from "Assistant", F.R.G.) , and resuspended in culture medium at a final density of 105 protoplasts/ml. The protoplasts are cultured in a volume of 10 ml per 9 cm diameter tissue culture quality petri dish. The dishes are sealed with Parafilm~ and incubated for 24 hours in the dark, and thereafter in dim light (500 - 1000 lux) at 24°C.
2.4. Transformation by co-cultivation The protoplast cultures are infected 5 days after isolation. Agrobacterium cultures are grown for 18 hours in liquid LB medium (Miller, Experiments in Molecular Genetics (1972). Cold Spring Harbor Laboratory, New York), and resuspended in K3 culture medium at a density of 2 x 109 cells/ml. Fifty NI of this suspension is added to the plant protoplast cultures and after sealing with Parafilm~, the cultures are incubated under the same conditions as described under 2.3. After 48 hours the cultures are transferred to 10 ml centrifuge tubes and centrifuged in a swinging bucket rotor at 60 - 80 g for 6 minutes.
The floating band and pellet are pooled and resuspended in 10 ml of K3 medium (Nagy and Maliga, Z. Pflanzen~~h~~ol. 78 (1976), 453-455) supplemented with an antibiotic (carbenicillin 1000 Ng/ml or cefotaxime 500 N9/ml).
After two weeks of incubation, the protoplast-derived micro-calli are centrifuged and resuspended in K3 medium (Nagy and Maliga, Z.
. Pflanzenahysiol. 78 (1976), 453-455) with the same growth regulator and antibiotic concentrations as before, but 0.3 M sucrose instead of 0.4 M. The cell density in this medium is adjusted to about 2 5 x 103 micro-calli per ml.
After two more weeks of incubation under the same conditions the calli are transferred to K3 medium with the same antibiotic concentrations as before, but with reduced sucrose (0.2 M) and growth regulators (NAA 0.01 mg/litre and kinetin 0.02 mg/litre). After two or three more weeks of incubation, the putative transformants can be recognized by their light green and compact aspect, and better growth. These colonies are then transferred to hormone-free Linsmaier and Skoog medium (Linsmaier and Skoog, P, hysiol. Plant. 18 (1965), 100-127) solified with 0.6% agar and containing reduced antibiotic concentrations (carbenicillin 500 pg/ml or cefotaxime 250 Ng/ml).
Opine tests can be done on the putative transformants which grow on this hormone-free medium when they reach 3 - 4 mm in diameter. Half of each colony is used for the detection of octopine and nopaline (Aerts et al., Plant Sci. Lett. 17 (1979), 43-50) or agropine and mannopine (Leemans et al., J.
Mol. Appl. Genet. 1 (1981 ), 149-164). This test allows to confirm the transformed nature of the colonies selected on hormone-free medium.
Afterwards, the selected colonies can be cultured on antibiotic-free medium.
2.5. Co-cultivation without selection on hormone-free media When selection for transformed cells is not possible (e.g. because avirulent T-DNA mutants are used) or is not required because a dominant selectable marker such as an antibiotics resistance gene is present in the T-DNA, the treatment of the protoplast-derived cells can be simplified (the hormone reduction steps are no longer necessary). The protoplasts are treated as described previously until the infection step. Forty-eight hours after addition of the bacteria the protoplast-derived cells are centrifuged (6 minutes, 60-80 g), and resuspended in medium AG (Caboche, Planta 149 (1980), 7-18) which is able to support cell growth at very low density. The cells are counted using a Fuchs-Rosenthal counting chamber (obtained from "Assistant", F. R .
G.), and resuspended at the density required for subsequent work. If the colonies must be manipulated individually for opine tests, plating at low cell density (100 protoplast-derived cells and cell colonies per ml) gives large cell colonies after one month of incubation. If drug selection for the transformed cells is possible, the cells are incubated at a higher density (103 -104/ml), and the selective agent used is added to the medium in a concentration and at a time which has to be optimized for each type of selection.
2.6. Regeneration of whole plant from callous tissue Normal plants are easily obtained from callous tissue (for example either derived from protoplast transformation or from whole plant inoculation (see 2.7). The callous tissue is grown an Murashige and Skoog medium containing 1 mg/ml BAP; this medium induces shoot formation after 1 - 2 months. These shoots can be transferred to medium without hormones so that roots form and a complete plant is produced.
2.7. Tumor induction on tobacco seedlings Tobacco seeds (e.g. cultivar Wisconsin 38) are surface sterilized by treatment with 70% denaturated ethanoI/Ha0 for 2 minutes; followed by 10%
commercial bleach and 0.1 % sodium docecyl sulfate (SDS); further rinsed 5 time with sterile H20.
The sterile seeds are sown in large (25 mm wide) test tubes containing the salts of Murashige and Skoog medium solidified with 0.7% agar and covered with polycarbonate tops. Then the tubes are incubated in culture room (12,000 lux, 16 hours light/8 hours dark; 70% relative humidity; 24°C).
After4 - 6 weeks the plants are ready to use. They remain optimal for at least another month.
Plantlets should be at least 3 cm high and have four or more leaves . The plants are then decapitated transversally through the youngest internode with a new sterile scalpel blade; the upper part of the plant removed from the tube, and bacteria from an agar plate culture applied on the wound surtace with a flamed microspatula.
Tumors appear after 2 weeks for the wild-type and after a longer time for some of the attenuated mutant strains. This method is used inoculate tobacco (Nicotiana tabacum), Nicotiana plumbaainifolia and Petunia h_ybrida.
4~ 1 ~~1 41 9 Concluding remarks The present invention offers for the first time the possibility to transform plants with Aprobacterium harboring a hybrid Ti plasmid vector which lacks the oncogenic functions of the T-region of wild-type Ti plasmids. Since the influence of the oncogenic functions of the T-region on the transfer of DNA from the Ti plasmid to plant cells was not known, it is surprising that nevertheless transfer of the modified T-region containing (a) genes) of interest to plant cells occurs. There is cointegration and stable maintenance of this transferred DNA in the plant cell genome. Furthermore, expression of chosen genes) of interest can be achieved provided the genes) either contain - or are constructed to contain - suitable promoter sequences. The concept of effecting a single cross-over event between an intermediate cloning vector containing the chosen genes) of interest with an especially designed acceptor Ti plasmid greatly simplifies the construction of any hybrid Ti plasmid vector useful for the transformation of plant cells. The especially designed acceptor Ti plasmids contain the DNA segment of a conventional cloning vehicle such that any genes) of interest (which has been inserted into the same or a related cloning vehicle as part of an intermediate cloning vector) can form a cointegrate by a single cross-over event. The two segments of the cloning vehicles) provide the necessary regions of homology for recombination.
Microorganisms and intermediate cloning vectors, acceptor Ti plasmids and hybrid plasmid vectors prepared by the processes of this invention are exemplified by cultures deposited in the German Collection of Microorganisms (DSM), Gottingen, on December 21 st, 1983, and identified there as (1) intermediate vector plasmid pAcgB in Escherichia coli K12 HB101;
(2) Aprobacterium tumefaciens C58C1 rifampicin-resistant strain carrying carbenicillin-resistant acceptor Ti plasmid pGV3850;
(3) intermediate vector plasmid pGV700 in Escherichia coli K12 strain K514 (thr leu thi lac hsdR);
(4) intermediate vector plasmid pGV750 in Escherichia coli K12 strain K514 (as ~- , above in (3));
(5) Aprobacterium tumefaciens C58C1 rifampicin-resistant strain carrying carbenicillin-resistant acceptor Ti plasmid pGV2260;
(6) intermediate vector plasmid pN0-1 carrying the octopine synthase coding region under the control of the nopaline promoter, in Escherichia coli K12 HB101;
(7) strain used in mobilization of intermediate vectors to A rg obacterium =
carrying mobilizing plasmids pGJ28 and R64drdll (Van Haute et al., EMBO J.
2 (1983), 411-418); GJ23 is Escherichia coli K12, JC2926, a recA derivative of AB1157 (Howard-Flanders et al. , Genetics 49 (1964), 237-246).
These cultures were assigned accession numbers 2792. (1 ), 2798 (2), 2796 (3), 2797. (4), 2799 (5), 2833 (6), and .2793. (7), respectively.
While we have hereinbefore presented a number of embodiments of this invention, it is apparent that our basic constructions can be altered to provide other embodiments which utilize the processes and compositions of this invention.
.~ ~,~
N.B. All plant culture media far infected tissues contain 500 Ng/ml of the antibiotic cefotaxime (Claforan~, Hoechst) as a selection against A~arobacterium containing pGV3850. This drug works well to prevent growth of all A-.ac irobacteria (including those which are carbenicillin-resistant).
Another method to obtain transformed and shooting tissues has been recently developed in our laboratory. This method is based on the observation that certain mutant Ti plasmid strains of Aqrobacterium induce crown gall tumors which produce shoots. Such shoot-inducing (shi) mutants map to a particular region of the T-DNA
(transferred DNA segment) of the Ti plasmids of A. tumefaciens (Leemans et al., EMBO J. 1 (1982) 147-152; Joos et al., Cell ~2 (1983) 1057-10fi7). Often the induced shoots are composed of completely normal untransformed cells. Thus, we tried to inoculate plants with a mixture of two different Aorobacteria, one carrying an octopine Ti plasmid shooter mutant and the other carrying pGV3850. In this manner, there is a good chance that the octopine shooter mutation can induce shoots which have been transformed with pGV3850. We have inoculated plants with Agrobacterium containing Ti plasmid pGV3850 and an octopine shoot inducing Ti plasmid in a 5:1 ratio. In this way we have obtained pGV3850-transformed shoots;
these shoots are easily screened by assaying for the presence of nopaline.
This method avoids the need for any elaborate tissue culture methods. The nopaline-positive shoots are transferred to media containing simple salts and sugar with any growth-regulating hormones to allow further growth. After the shoots have reached a sufficient size they can easily be transferred to soil for propagation. This coinfection procedure should be particularly useful for transforming plant species which are not ~;
. ~."r 1 readily amenable to tissue culture. Thus, a whole range of agronomically and economically important plants, such as legumes, medicinal plants, and ornamentals will be able to be engineered by Aarobacterium.
The third procedure allows the isolation of Nicotiana tabacum protoplasts and the selection of hormone-independent T-DNA-transformed cell clones after co-cultivation of the protoplast-derived cells with oncogenic Ac~obacterium strains. An analogous technique can be used for the selection of transformed cells when other dominant selective markers are used, such as antibiotic resistance genes constructed in such a way as to be expressed in higher plant cells (see example 3).
In this case, however, the conditions for selection have to be optimized in each case (concentration of the selective agent, time between transformatian and selection, concentration of the protoplast-derived cells or cell colonies in the selective medium). If no selection for the transformed cells is possible, e.g. because avirulent T-DNA mutants are used, such as e.g. pGV3850 or pGV2217 (Leemans et al., EMBO J. 1 (1982), 147-152), it is possible to cultivate the cells after genetic transformation on auxin- and cytokinin-containing medium (e.g. Murashige and Skoog medium (Murashige and Skoog, P_ hysiol. Plant 15 (1962), 473-497) with 2 mg/litre NAA (a-naphthalene acetic acid) and 0.3 mg/litre kinetin), and to identify the transformed colonies by their opine content. In this way, after electrophoretic analysis for agropine and mannopine synthesis (method see t_eemans et al., J.
Mol.
Appl. Genet. 1 (1981 ), 149-164) about 660 colonies can be found, obtained after infection with pGV2217, a Nicotiana tabacum SRI cell line which synthesizes the TR-encoded opine mannopine (N2-(1-mannityl)-glutamine). Numerous shoots are formed after incubation of callus pieces of this cell line on regeneration medium (Murashige and Skoog medium with BAP (6-benzylaminopurine) (1 mg/litre) as the sole plant growth regulator). All 20 shoots analyzed are still able to synthesize mannopine.
After transfer onto hormone-free Murashige and Skoog medium, the shoots grow as morphologically normal tobacco plants still containing mannopine.
The protoplast isolation and transformation described here for N. tabacum can also 1 3~1 41 9 be used for N. plumbaginifolia.
2. Experimental procedures 2.1. Shoot culture conditions Nicotiana tabacum shoot cultures are maintained in 250 ml glass jars on hormone-free Murashige and Skoog medium (Murashige and Skoog, Physiol.
Plant 15 (1962), 473-497) under sterile conditions in a culture room (16 hour day, 1500 lux white fluorescent light ("ACEC LF 58 W/2 4300°K
Economy"), 24°C, 70% relative humidity). Five week old shoot cultures are used for protoplast isolation.
2.2. Protoplast isolation Aseptic techniques are used far all steps in protoplast isolation and culture.
The protoplasts are isolated by a mixed enzyme procedure. All leaves, except for very young leaves smaller than 2 cm, can be used for protoplast isolation.
The leaves are cut in strips, about 2 - 3 mm wide, with a sharp scalpel knife.
Two to three grams of leaf material is incubated 18 hours at 24°C in 50 ml enzyme mixture in the dark without agitation. The enzyme mixture consists of 0.5% cellulose Onozuka* R-10 and 0.2% macerozyme Onozuka R-10 in hormone-free K3 medium (Nagy and Malign, Z. Pflanzenphvsiol. 78 (1976), 453-455). The mixture is filter-sterilized through a 0.22 Nm pore membrane, and can be stored for at least 6 months at -20°C without notable loss of activity.
2.3. Protoplast culture After 18 hours incubation the mixture is agitated gently in order to release the protoplasts. The mixture is subsequently filtered through a 50 Nm sieve, and the filtrate is transferred to 10 ml centrifuge tubes. After centrifugation for 6 minutes at 60 - 80 g in a swinging bucket rotor the protoplasts form a dark ;, t a,y /rp.
*trade mark 45 ~ 3 4 ~ 4 ~ 9 green floating band. The liquid underlying the protoplasts, and the debris which forms the pellet, are removed using a capillary tube connected to a peristaltic pump. The protoplasts are pooled in one tube and washed 2 times with culture medium. The culture medium is the K3 medium (Nagy and Maliga, Z. Pflanzenahysial. 78 (1976), 453-455) with NAA (0.1 mg/litre) and kinetin (0.2 mg/litre) as growth regulators. The medium is adjusted to pH 5.6 and sterilized through 0.22 Nm filter membrane. After the second wash, the protoplasts are counted using a Thoma hemacytometer (obtained from "Assistant", F.R.G.) , and resuspended in culture medium at a final density of 105 protoplasts/ml. The protoplasts are cultured in a volume of 10 ml per 9 cm diameter tissue culture quality petri dish. The dishes are sealed with Parafilm~ and incubated for 24 hours in the dark, and thereafter in dim light (500 - 1000 lux) at 24°C.
2.4. Transformation by co-cultivation The protoplast cultures are infected 5 days after isolation. Agrobacterium cultures are grown for 18 hours in liquid LB medium (Miller, Experiments in Molecular Genetics (1972). Cold Spring Harbor Laboratory, New York), and resuspended in K3 culture medium at a density of 2 x 109 cells/ml. Fifty NI of this suspension is added to the plant protoplast cultures and after sealing with Parafilm~, the cultures are incubated under the same conditions as described under 2.3. After 48 hours the cultures are transferred to 10 ml centrifuge tubes and centrifuged in a swinging bucket rotor at 60 - 80 g for 6 minutes.
The floating band and pellet are pooled and resuspended in 10 ml of K3 medium (Nagy and Maliga, Z. Pflanzen~~h~~ol. 78 (1976), 453-455) supplemented with an antibiotic (carbenicillin 1000 Ng/ml or cefotaxime 500 N9/ml).
After two weeks of incubation, the protoplast-derived micro-calli are centrifuged and resuspended in K3 medium (Nagy and Maliga, Z.
. Pflanzenahysiol. 78 (1976), 453-455) with the same growth regulator and antibiotic concentrations as before, but 0.3 M sucrose instead of 0.4 M. The cell density in this medium is adjusted to about 2 5 x 103 micro-calli per ml.
After two more weeks of incubation under the same conditions the calli are transferred to K3 medium with the same antibiotic concentrations as before, but with reduced sucrose (0.2 M) and growth regulators (NAA 0.01 mg/litre and kinetin 0.02 mg/litre). After two or three more weeks of incubation, the putative transformants can be recognized by their light green and compact aspect, and better growth. These colonies are then transferred to hormone-free Linsmaier and Skoog medium (Linsmaier and Skoog, P, hysiol. Plant. 18 (1965), 100-127) solified with 0.6% agar and containing reduced antibiotic concentrations (carbenicillin 500 pg/ml or cefotaxime 250 Ng/ml).
Opine tests can be done on the putative transformants which grow on this hormone-free medium when they reach 3 - 4 mm in diameter. Half of each colony is used for the detection of octopine and nopaline (Aerts et al., Plant Sci. Lett. 17 (1979), 43-50) or agropine and mannopine (Leemans et al., J.
Mol. Appl. Genet. 1 (1981 ), 149-164). This test allows to confirm the transformed nature of the colonies selected on hormone-free medium.
Afterwards, the selected colonies can be cultured on antibiotic-free medium.
2.5. Co-cultivation without selection on hormone-free media When selection for transformed cells is not possible (e.g. because avirulent T-DNA mutants are used) or is not required because a dominant selectable marker such as an antibiotics resistance gene is present in the T-DNA, the treatment of the protoplast-derived cells can be simplified (the hormone reduction steps are no longer necessary). The protoplasts are treated as described previously until the infection step. Forty-eight hours after addition of the bacteria the protoplast-derived cells are centrifuged (6 minutes, 60-80 g), and resuspended in medium AG (Caboche, Planta 149 (1980), 7-18) which is able to support cell growth at very low density. The cells are counted using a Fuchs-Rosenthal counting chamber (obtained from "Assistant", F. R .
G.), and resuspended at the density required for subsequent work. If the colonies must be manipulated individually for opine tests, plating at low cell density (100 protoplast-derived cells and cell colonies per ml) gives large cell colonies after one month of incubation. If drug selection for the transformed cells is possible, the cells are incubated at a higher density (103 -104/ml), and the selective agent used is added to the medium in a concentration and at a time which has to be optimized for each type of selection.
2.6. Regeneration of whole plant from callous tissue Normal plants are easily obtained from callous tissue (for example either derived from protoplast transformation or from whole plant inoculation (see 2.7). The callous tissue is grown an Murashige and Skoog medium containing 1 mg/ml BAP; this medium induces shoot formation after 1 - 2 months. These shoots can be transferred to medium without hormones so that roots form and a complete plant is produced.
2.7. Tumor induction on tobacco seedlings Tobacco seeds (e.g. cultivar Wisconsin 38) are surface sterilized by treatment with 70% denaturated ethanoI/Ha0 for 2 minutes; followed by 10%
commercial bleach and 0.1 % sodium docecyl sulfate (SDS); further rinsed 5 time with sterile H20.
The sterile seeds are sown in large (25 mm wide) test tubes containing the salts of Murashige and Skoog medium solidified with 0.7% agar and covered with polycarbonate tops. Then the tubes are incubated in culture room (12,000 lux, 16 hours light/8 hours dark; 70% relative humidity; 24°C).
After4 - 6 weeks the plants are ready to use. They remain optimal for at least another month.
Plantlets should be at least 3 cm high and have four or more leaves . The plants are then decapitated transversally through the youngest internode with a new sterile scalpel blade; the upper part of the plant removed from the tube, and bacteria from an agar plate culture applied on the wound surtace with a flamed microspatula.
Tumors appear after 2 weeks for the wild-type and after a longer time for some of the attenuated mutant strains. This method is used inoculate tobacco (Nicotiana tabacum), Nicotiana plumbaainifolia and Petunia h_ybrida.
4~ 1 ~~1 41 9 Concluding remarks The present invention offers for the first time the possibility to transform plants with Aprobacterium harboring a hybrid Ti plasmid vector which lacks the oncogenic functions of the T-region of wild-type Ti plasmids. Since the influence of the oncogenic functions of the T-region on the transfer of DNA from the Ti plasmid to plant cells was not known, it is surprising that nevertheless transfer of the modified T-region containing (a) genes) of interest to plant cells occurs. There is cointegration and stable maintenance of this transferred DNA in the plant cell genome. Furthermore, expression of chosen genes) of interest can be achieved provided the genes) either contain - or are constructed to contain - suitable promoter sequences. The concept of effecting a single cross-over event between an intermediate cloning vector containing the chosen genes) of interest with an especially designed acceptor Ti plasmid greatly simplifies the construction of any hybrid Ti plasmid vector useful for the transformation of plant cells. The especially designed acceptor Ti plasmids contain the DNA segment of a conventional cloning vehicle such that any genes) of interest (which has been inserted into the same or a related cloning vehicle as part of an intermediate cloning vector) can form a cointegrate by a single cross-over event. The two segments of the cloning vehicles) provide the necessary regions of homology for recombination.
Microorganisms and intermediate cloning vectors, acceptor Ti plasmids and hybrid plasmid vectors prepared by the processes of this invention are exemplified by cultures deposited in the German Collection of Microorganisms (DSM), Gottingen, on December 21 st, 1983, and identified there as (1) intermediate vector plasmid pAcgB in Escherichia coli K12 HB101;
(2) Aprobacterium tumefaciens C58C1 rifampicin-resistant strain carrying carbenicillin-resistant acceptor Ti plasmid pGV3850;
(3) intermediate vector plasmid pGV700 in Escherichia coli K12 strain K514 (thr leu thi lac hsdR);
(4) intermediate vector plasmid pGV750 in Escherichia coli K12 strain K514 (as ~- , above in (3));
(5) Aprobacterium tumefaciens C58C1 rifampicin-resistant strain carrying carbenicillin-resistant acceptor Ti plasmid pGV2260;
(6) intermediate vector plasmid pN0-1 carrying the octopine synthase coding region under the control of the nopaline promoter, in Escherichia coli K12 HB101;
(7) strain used in mobilization of intermediate vectors to A rg obacterium =
carrying mobilizing plasmids pGJ28 and R64drdll (Van Haute et al., EMBO J.
2 (1983), 411-418); GJ23 is Escherichia coli K12, JC2926, a recA derivative of AB1157 (Howard-Flanders et al. , Genetics 49 (1964), 237-246).
These cultures were assigned accession numbers 2792. (1 ), 2798 (2), 2796 (3), 2797. (4), 2799 (5), 2833 (6), and .2793. (7), respectively.
While we have hereinbefore presented a number of embodiments of this invention, it is apparent that our basic constructions can be altered to provide other embodiments which utilize the processes and compositions of this invention.
.~ ~,~
Claims (16)
1. A vector combination comprising:
(i) an acceptor Ti plasmid which does not contain T-DNA genes that control neoplastic growth and is incapable of inducing tumours in plants, said Ti plasmid comprising:
(a) the two border sequences of the T
region of a wild-type Ti plasmid;
(b) a DNA sequence derived from a cloning vehicle, located between the two border sequences; and (c) a DNA segment of a wild-type Ti plasmid containing DNA sequences essential for the transfer by Agrobacterium of the T-region of wild-type Ti plasmids into plant cell genomes: and (ii) an intermediate cloning vector, comprising:
(a) at least one gene of interest under the control of a promoter capable of directing gene expression in plants;
and (b) a cloning vehicle segment containing a DNA sequence which is homologous with the DNA sequence (i)(b) in said acceptor Ti plasmid, permitting a single cross-over event.
(i) an acceptor Ti plasmid which does not contain T-DNA genes that control neoplastic growth and is incapable of inducing tumours in plants, said Ti plasmid comprising:
(a) the two border sequences of the T
region of a wild-type Ti plasmid;
(b) a DNA sequence derived from a cloning vehicle, located between the two border sequences; and (c) a DNA segment of a wild-type Ti plasmid containing DNA sequences essential for the transfer by Agrobacterium of the T-region of wild-type Ti plasmids into plant cell genomes: and (ii) an intermediate cloning vector, comprising:
(a) at least one gene of interest under the control of a promoter capable of directing gene expression in plants;
and (b) a cloning vehicle segment containing a DNA sequence which is homologous with the DNA sequence (i)(b) in said acceptor Ti plasmid, permitting a single cross-over event.
2. The vector combination according to claim 1, wherein the acceptor Ti plasmid is substantially free of internal T-DNA sequences of a wild-type Ti plasmid.
3. The vector combination according to claim 1 or 2, characterized in that the intermediate cloning vector additionally contains at least one selectable marker gene, adjacent to the gene of interest.
4 . The vector combination according to claim 1 or 2, wherein the gene of interest contained in the intermediate cloning vector is under the control of its natural promoter.
5 . The vector combination according to claim 1 or 2 , wherein the gene of interest contained in the intermediate cloning vector is under the control of a promoter which is exogenous with respect to the gene of interest.
6. A vector combination comprising:
(i) an acceptor Ti plasmid, which is incapable of inducing tumours in plants being free of border sequences and internal T-DNA
sequences of a wild-type Ti plasmid, said acceptor Ti plasmid comprising:
(a) a DNA segment of a wild-type Ti plasmid without the T-region and without the two border sequences of the T-region;
and (b) a DNA sequence derived from a cloning vehicle; and (ii) an intermediate cloning vector, comprising:
(a) a cloning vehicle segment containing the two border sequences of the T
region of a wild-type Ti plasmid and a DNA sequence located outside of said two border sequences which is homologous with the DNA sequence (i) (b) in said acceptor Ti plasmid permitting a single cross-over event wherein the region between said border sequences does not contain T-DNA genes that control neoplastic growth; and (b) at least one gene of interest under the control of a promoter capable of directing gene expression in plants located between the two border sequences in a manner allowing its integration into the plant genome.
(i) an acceptor Ti plasmid, which is incapable of inducing tumours in plants being free of border sequences and internal T-DNA
sequences of a wild-type Ti plasmid, said acceptor Ti plasmid comprising:
(a) a DNA segment of a wild-type Ti plasmid without the T-region and without the two border sequences of the T-region;
and (b) a DNA sequence derived from a cloning vehicle; and (ii) an intermediate cloning vector, comprising:
(a) a cloning vehicle segment containing the two border sequences of the T
region of a wild-type Ti plasmid and a DNA sequence located outside of said two border sequences which is homologous with the DNA sequence (i) (b) in said acceptor Ti plasmid permitting a single cross-over event wherein the region between said border sequences does not contain T-DNA genes that control neoplastic growth; and (b) at least one gene of interest under the control of a promoter capable of directing gene expression in plants located between the two border sequences in a manner allowing its integration into the plant genome.
7. The vector combination of claim 6, wherein the region between the two border sequences in the intermediate cloning vector is substantially free of internal T-DNA sequences of a wild-type Ti plasmid.
8. The vector combination of claim 6 or 7 in which the acceptor Ti plasmid is pGV2260, DSM 2799.
9. The vector combination of claim 6 or 7 in which the intermediate cloning vector contains additionally at least one selectable marker gene adjacent to the gene of interest.
10. The vector combination of claim 5 or 7 in which the intermediate cloning vector is further characterized in that the gene of interest is under the control of its natural promoter.
11. The vector combination of claim 6 or 7 in which the intermediate cloning vector is further characterized in that the gene of interest is under they control of a promoter which is exogenous with respect to the gene of interest.
12. The vector combination of claim 6 or 7 in which the intermediate cloning vector is pGV750, DSM
2797.
2797.
13. The acceptor Ti plasmid pGV2260, DSM 2799.
14. The intermediate cloning vector pGV750, DSM 2797.
15. A process far the preparation of a hybrid Ti plasmid which comprise producing a vector combination according to any one of claims 1 to 5 in an Agrobacterium by mobilizing the intermediate cloning vector in the presence of helper plasmids to an Agrobacterium containing the acceptor Ti plasmid and allowing a cointegration to proceed between the intermediate cloning vector and the acceptor Ti plasmid by a single cross-over event.
16. A process far the preparation of a hybrid Ti plasmid which comprises producing a vector combination according to any one of claims 6 to 12 in an Agrobacterium by mobilizing the intermediate cloning vector in the presence of helper plasmids to an Agrobacterium containing the acceptor Ti plasmid and allowing a cointegration to proceed between the intermediate cloning vector and the acceptor Ti plasmid by a single cross-over event.
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DE (3) | DE3382838T2 (en) |
DK (1) | DK173104B1 (en) |
IL (1) | IL70610A (en) |
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ATE282692T1 (en) * | 1983-01-13 | 2004-12-15 | Max Planck Gesellschaft | NON-ONCOGENIC TI-PLASMID VECTOR SYSTEM AND RECOMBINANT DNA MOLECULES USABLE FOR INTRODUCING EXPRESSABLE GENES INTO PLANT GENOMS |
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WO1984002919A1 (en) * | 1983-01-17 | 1984-08-02 | Monsanto Co | Plasmids for transforming plant cells |
JPS60500795A (en) * | 1983-01-17 | 1985-05-30 | モンサント カンパニ− | genetically transformed plants |
NL8300699A (en) * | 1983-02-24 | 1984-09-17 | Univ Leiden | METHOD FOR BUILDING FOREIGN DNA INTO THE NAME OF DIABIC LOBAL PLANTS; METHOD FOR PRODUCING AGROBACTERIUM TUMEFACIENS BACTERIEN; STABLE COINTEGRATE PLASMIDS; PLANTS AND PLANT CELLS WITH CHANGED GENETIC PROPERTIES; PROCESS FOR PREPARING CHEMICAL AND / OR PHARMACEUTICAL PRODUCTS. |
NZ207766A (en) * | 1983-04-15 | 1987-03-06 | Lubrizol Genetics Inc | Plant structural gene expression |
NZ209338A (en) * | 1983-09-14 | 1988-02-12 | Lubrizol Genetics Inc | Plasmid for the transformation of a plant cell |
US4658082A (en) * | 1984-07-25 | 1987-04-14 | Atlantic Richfield Company | Method for producing intact plants containing foreign DNA |
BR8600161A (en) * | 1985-01-18 | 1986-09-23 | Plant Genetic Systems Nv | CHEMICAL GENE, HYBRID, INTERMEDIATE PLASMIDIO VECTORS, PROCESS TO CONTROL INSECTS IN AGRICULTURE OR HORTICULTURE, INSECTICIDE COMPOSITION, PROCESS TO TRANSFORM PLANT CELLS TO EXPRESS A PLANTINIDE TOXIN, PRODUCED BY CULTURES, UNITED BY BACILLA |
US5180873A (en) * | 1985-04-16 | 1993-01-19 | Dna Plant Technology Corporation | Transformation of plants to introduce closely linked markers |
EP0267159A3 (en) * | 1986-11-07 | 1990-05-02 | Ciba-Geigy Ag | Process for the genetic modification of monocotyledonous plants |
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EP2123751A4 (en) | 2007-01-25 | 2010-06-02 | Kyowa Hakko Kirin Co Ltd | Novel peptide |
US8383381B2 (en) | 2007-09-27 | 2013-02-26 | Shjonogi & Co., Ltd. | Method for producing hydroxylated adaivjantane using cytochrome P450 |
WO2009054435A1 (en) | 2007-10-24 | 2009-04-30 | Otsuka Chemical Co., Ltd. | Polypeptide having enhanced effector function |
JP5662149B2 (en) | 2008-08-13 | 2015-01-28 | 協和発酵キリン株式会社 | Genetically modified protein S composition |
US8304249B2 (en) | 2008-10-09 | 2012-11-06 | Kyowa Medex Co., Ltd. | Fructosyl peptide oxidase |
KR101913440B1 (en) | 2010-03-02 | 2018-10-30 | 교와 핫꼬 기린 가부시키가이샤 | Modified antibody composition |
WO2011118739A1 (en) | 2010-03-26 | 2011-09-29 | 協和発酵キリン株式会社 | Novel antibody having modification site introduced therein, and antibody fragment |
JP5058332B2 (en) | 2010-07-14 | 2012-10-24 | 住友ゴム工業株式会社 | Isoprene oligomer, polyisoprene, and production methods thereof, rubber composition, and pneumatic tire |
EP3020810B1 (en) | 2013-07-09 | 2019-04-10 | Kyowa Medex Co., Ltd. | Glycated hexapeptide oxidase and use thereof |
JP6448194B2 (en) | 2014-01-20 | 2019-01-09 | 住友ゴム工業株式会社 | By introducing a gene encoding cis-prenyltransferase and a gene encoding NogoBreceptor into the host, the transformant in which the cis-prenyltransferase and NogoBreceptor were expressed in the host, and the transformant were used. Method for producing polyisoprenoid |
JP6557990B2 (en) | 2015-02-23 | 2019-08-14 | 住友ゴム工業株式会社 | Vector containing gene encoding specific promoter and specific protein, transformed plant introduced with the vector, and method for improving polyisoprenoid production by introducing the vector into the plant |
JP6557989B2 (en) | 2015-02-23 | 2019-08-14 | 住友ゴム工業株式会社 | Vector containing gene encoding specific promoter and specific protein, transformed plant introduced with the vector, and method for improving polyisoprenoid production by introducing the vector into the plant |
JP6719174B2 (en) | 2015-02-23 | 2020-07-08 | 住友ゴム工業株式会社 | A vector containing a specific promoter and a gene encoding a specific protein, a transformed plant into which the vector is introduced, and a method for improving the production amount of polyisoprenoid by introducing the vector into the plant |
JP6579640B2 (en) | 2017-01-10 | 2019-09-25 | 国立大学法人山口大学 | Anti-GPC3 antibody |
JP2020195326A (en) | 2019-06-03 | 2020-12-10 | 住友ゴム工業株式会社 | Method of producing natural rubber, transgenic plant, method of producing pneumatic tire, and method of producing rubber product |
JP6923166B2 (en) | 2019-07-16 | 2021-08-18 | 住友ゴム工業株式会社 | Fusion protein, substance manufacturing method, vector, transformed cell, pneumatic tire manufacturing method and rubber product manufacturing method |
JP2021080204A (en) | 2019-11-19 | 2021-05-27 | 住友ゴム工業株式会社 | Fusion proteins, methods for producing substance, vectors, transformed cells, methods for manufacturing pneumatic tires, and methods for manufacturing rubber products |
WO2021177074A1 (en) | 2020-03-05 | 2021-09-10 | 住友ゴム工業株式会社 | Method for producing polyisoprenoid, vector, transformed plant, method for producing pneumatic tire, and method for producing rubber product |
JP2023040705A (en) | 2021-09-10 | 2023-03-23 | 住友ゴム工業株式会社 | Method for producing trans-polyisoprenoid, vector, transgenic organism, method for producing pneumatic tire, and method for producing rubber product |
JP2023127869A (en) | 2022-03-02 | 2023-09-14 | 住友ゴム工業株式会社 | Mutant cis-prenyltransferase (cpt) family protein, method for producing polyisoprenoid, vector, transgenic plant, method for producing pneumatic tire, and method for producing rubber product |
JP2023127868A (en) | 2022-03-02 | 2023-09-14 | 住友ゴム工業株式会社 | Mutant cis-prenyltransferase (cpt) family protein, method for producing polyisoprenoid, vector, transgenic plant, method for producing pneumatic tire, and method for producing rubber product |
JP2023127870A (en) | 2022-03-02 | 2023-09-14 | 住友ゴム工業株式会社 | Mutant cis-prenyltransferase (cpt) family protein, method for producing polyisoprenoid, vector, transgenic plant, method for producing pneumatic tire, and method for producing rubber product |
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AT373279B (en) * | 1977-11-08 | 1984-01-10 | Genentech Inc | METHOD FOR PRODUCING A RECOMBINATION CLONING SUPPORT |
JPS595512A (en) * | 1982-06-30 | 1984-01-12 | 松下電工株式会社 | Contact material |
ATE282692T1 (en) * | 1983-01-13 | 2004-12-15 | Max Planck Gesellschaft | NON-ONCOGENIC TI-PLASMID VECTOR SYSTEM AND RECOMBINANT DNA MOLECULES USABLE FOR INTRODUCING EXPRESSABLE GENES INTO PLANT GENOMS |
JPS62129585A (en) * | 1985-11-29 | 1987-06-11 | Kyocera Corp | Pump operation device |
-
1983
- 1983-12-22 AT AT89102441T patent/ATE282692T1/en not_active IP Right Cessation
- 1983-12-22 AT AT88105808T patent/ATE255162T1/en not_active IP Right Cessation
- 1983-12-22 DE DE3382838T patent/DE3382838T2/en not_active Expired - Lifetime
- 1983-12-22 DE DE8383112985T patent/DE3381568D1/en not_active Expired - Lifetime
- 1983-12-22 DE DE3382839T patent/DE3382839D1/en not_active Expired - Lifetime
-
1984
- 1984-01-03 IL IL70610A patent/IL70610A/en not_active IP Right Cessation
- 1984-01-11 CA CA004451015A patent/CA1341524C/en not_active Expired - Lifetime
- 1984-01-11 CA CA000617136A patent/CA1341419C/en not_active Expired - Lifetime
- 1984-01-12 DK DK198400136A patent/DK173104B1/en not_active IP Right Cessation
- 1984-01-13 JP JP59005512A patent/JPS59140885A/en active Granted
- 1984-01-13 AU AU23274/84A patent/AU546542B2/en not_active Expired
-
1987
- 1987-05-25 JP JP62129585A patent/JP2769539B2/en not_active Expired - Lifetime
-
1988
- 1988-04-25 JP JP63103749A patent/JP2726267B2/en not_active Expired - Fee Related
-
1990
- 1990-09-05 JP JP2236922A patent/JPH03108478A/en active Pending
-
1992
- 1992-09-30 JP JP4261509A patent/JPH06105629A/en active Pending
-
2000
- 2000-06-21 JP JP2000186437A patent/JP2001029092A/en active Pending
Also Published As
Publication number | Publication date |
---|---|
DK13684A (en) | 1984-07-14 |
DE3382838D1 (en) | 2004-01-08 |
IL70610A (en) | 1992-08-18 |
CA1341524C (en) | 2007-04-03 |
JPH06105629A (en) | 1994-04-19 |
JP2726267B2 (en) | 1998-03-11 |
JPS63283587A (en) | 1988-11-21 |
ATE255162T1 (en) | 2003-12-15 |
JPS59140885A (en) | 1984-08-13 |
DK173104B1 (en) | 2000-01-17 |
JPH0258917B2 (en) | 1990-12-11 |
AU546542B2 (en) | 1985-09-05 |
DE3382838T2 (en) | 2004-04-15 |
DE3381568D1 (en) | 1990-06-21 |
JP2001029092A (en) | 2001-02-06 |
AU2327484A (en) | 1984-07-19 |
DE3382839D1 (en) | 2004-12-23 |
DK13684D0 (en) | 1984-01-12 |
JPS6339587A (en) | 1988-02-20 |
ATE282692T1 (en) | 2004-12-15 |
JPH03108478A (en) | 1991-05-08 |
JP2769539B2 (en) | 1998-06-25 |
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