AU2005312023A1 - Stress tolerance in plants through selective inhibition of trehalose-6-phosphate phosphatase - Google Patents

Description

WO 2006/060376 PCT/US2005/043097 STRESS TOLERANCE IN PLANTS THROUGH SELECTIVE INHIBITION OF TREHALOSE-6-PHOSPHATE PHOSPHATASE 5 FIELD OF THE INVENTION The present invention encompasses the stress-responsive expression of a nucleic acid sequence capable of down-regulating trehalose-6-phosphate phosphatase activity for the purpose of increasing yield and/or improving abiotic stress tolerance of plants. 10 BACKGROUND OF THE INVENTION Abiotic stress can affect plant development in different ways depending on the timing, severity, and duration of the stress. Maize plants are, for example, relatively drought tolerant, 15 and can withstand moderate to severe drought in the early and late stages of the growing season. However, maize is quite susceptible to water stress during a 10-14 day period around flowering. Non-irrigated maize grown in the U.S. Corn Belt typically experiences water stress in late summer during flowering. This stress usually manifests itself in the form of reduced kernel set due to ovule/embryo abortion. In the simplest terms, when roots are Z0 experiencing osmotic stress, they produce abscisic acid (ABA) which is translocated throughout the plant. In the leaf, this triggers closure of the stomata, thus reducing water loss through transpiration. Unfortunately, this also limits gas exchange and consequently photosynthesis is reduced. Without sucrose from photosynthesis, the developing ovule or embryo rapidly depletes its starch reserve and aborts. Z5 The trehalose pathway in plants is shown in Figure 1. The pathway is positioned to demonstrate similarity to sucrose synthesis via sucrose-6-phosphate synthase (8) and sucrose 6-phosphate phosphatase (9). Trehalose synthesis is catalyzed by trehalose-6-phosphate synthase (T6PS) (10), yielding trehalose-6-phosphate (T6P) and trehalose-6-phosphate phosphatase (T6PP) (11), yielding trehalose. Trehalase (12) cleaves trehalose into two 30 glucose molecules. These enzymes are well characterized in microbes and were thought to occur in only a few plants, such as the dessication tolerant Myrothanmnus flabellifolia, because measurable trehalose accumulates when they dry down (reviewed in MUiller et al., 1995). Many crops do not accumulate detectable trehalose, therefore most researchers believed they lacked the ability to make it. Furthermore, exogenously applied trehalose can 35 be toxic to plant tissues (Veluthambi et al., 1981). The E. coli genes encoding T6PS and Page 1 WO 2006/060376 PCT/US2005/043097 T6PP were cloned in the early 1990's (Kaasen et al., 1992), and formed the basis for early work to use genetic engineering to improve plant tolerance to water stress (Holmstrom et al., 1996; Goddijn et al., 1997). This early plant genetic engineering work was based on evidence obtained with 5 microorganisms. It is well established that trehalose improves desiccation tolerance of microorganisms and macromolecules (Weimken, 1990). These experiments provided a direct correlation between trehalose levels and desiccation tolerance. Many groups attempted to genetically engineer trehalose synthesis in plants (Rontein et al., 2002). Much of their work is aimed to increase trehalose levels (Hoekema et al., 1999). A number of inventions used the E. 0 coli or yeast trehalose synthesis genes. In summary, engineered plants produced only small amounts of trehalose despite increasing the plant's capacity to make trehalose by as much as ten-fold (Londesborough et al., 2000). Further investigation showed the low trehalose accumulation in transgenics was due, in part, to endogenous trehalase activity (Goddijn et al., 1997). Other workers believed that 5 sucrose and starch synthesis limited the plant's capacity to make trehalose (Hoekema et al., 1999). More recent publications disclosed methods to improve trehalose accumulation in transgenic plants by inhibiting trehalase (Goddijn et al., 2003), expressing an E. coli T6PS T6PP fusion protein (Garg et al., 2002; Jang et al., 2003) and expressing the E. coli trehalose synthesis gene in plastids (Lebel et al., 2004). Some groups achieved improved trehalose 20 accumulation and, most reported small improvements in drought tolerance even though overall growth defects were observed in the transgenic plants. Advances in genome information and complementation work in yeast identified plant genes encoding functional T6PS, T6PP and trehalase (Vogel et al., 1998; Blizquez et al., 1998; Aescherbacher et al., 1999; Mtiller et al., 2001; Vogel et al., 2001). Trehalose pathway 25 genes are expressed at low levels, but expression has been detected in all tissues examined. Sequence data from several plant species indicate the presence of trehalose metabolism genes (Leyman et al., 2001; Wingler, 2002; Eastmond and Graham, 2003; Eastmond et al., 2003). In most plant genetic engineering studies the trehalose pathway enzymes, or genes designed to influence a trehalose pathway enzyme activity (for example, an antisense RNA 30 construct), are targeted to the cytosol (Holmstrom et al., 1996; Goddijn et al., 1997; Romero et al., 1997; Pilon-Smits et al., 1998; Garg et al., 2002; Jang et al., 2003). Despite their enormous increase--or change in--synthetic capacity, the experiments do little to influence trehalose or trehalose-6-phosphate in these plants. In fact, tobacco and potato plants Page 2 WO 2006/060376 PCT/US2005/043097 expressing the E. coli T6PS and T6PP genes tend to suffer pleotropic growth defects (Goddijn et al., 1997). Thus, there is a need to develop stress tolerant plants that do not also exhibit growth defects. 5 SUMMARY The present invention relates to transgenic plants comprising a polypeptide encoding a nucleic acid that targets an endogenous T6PP gene, wherein the isolated DNA molecule is under the control of a promoter that is stress-inducible in vegetative tissue. The nucleic acid 0 may also be developmentally expressed in maturing kernels. Stress induced expression of the nucleic acid of the invention increases the availability of carbon to developing florets/kernels when plants are under stress conditions, such as a water deficit. The polypeptide of the present invention transformed into a plant thereby permits more photosynthate to be directed to the developing ovules/embryos resulting in stabilized yield in growing environments that 5 are subject to periodic stress. The present invention further includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, the isolated DNA sequence is operatively linked to a promoter that is stress induced in vegetative tissue, wherein the nucleic acid is capable of down-regulating a T6PP gene. 0 The present invention includes a method of increasing the starch content in the kernel of a plant comprising the steps of transforming a plant cell with a DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP; generating a plant from the plant cell; inducing expression of the 25 nucleic acid in the vegetative tissue of the plant when the plant is subjected to stress conditions during its reproductive stage; and increasing starch content in the kernel compared to the starch content in the kernel of an isogenic plant not containing the DNA molecule when the transgenic plant and the isogenic plant are grown under substantially the same stress conditions. 30 The present invention further includes a double stranded short interfering nucleic acid (siRNA) molecule that down regulates expression of a T6PP gene in the vegetative tissue of a plant, wherein said siRNA molecule comprises at least about 21 base pairs. Page 3 WO 2006/060376 PCT/US2005/043097 The present invention encompasses a double stranded siRNA molecule that down regulates expression of a T6PP gene, wherein a first strand of the double stranded siRNA molecule comprises a nucleotide sequence substantially similar to the nucleotide sequence of a T6PP gene or a portion thereof and, wherein a second strand of the double-stranded siRNA 5 molecule comprises a nucleotide sequence that is complementary to the sequence of the first strand. The invention also includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating 0 a T6PP gene. The invention includes an isolated DNA molecule comprising a polynucleotide wherein said polynucleotide is depicted by SEQ ID. NO 6. The invention includes an isolated DNA molecule comprising a polynucleotide, wherein said nucleotide sequence comprises at least about 21 consecutive base pairs of SEQ 15 IDNO. 6. The invention includes an isolated DNA molecule comprising polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP gene, and wherein said polynucleotide is placed in a sense or antisense orientation 20 relative to said promoter. The invention also includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP gene, wherein said promoter is derived from the 5' region of a Rabl 17 gene and 25 exhibits promoter activity in plants. The invention also includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP gene, wherein said promoter is derived from the 5' region of a Rab 17 gene and 30 exhibits promoter activity in plants and further comprises a 3' region derived from a Rabl7 gene and exhibits terminator activity in plants. The invention further includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a Page 4 WO 2006/060376 PCT/US2005/043097 promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP gene, wherein said promoter comprises about 100-1649 contiguous nucleotides of DNA, wherein said contiguous nucleotides of DNA have from 85% to 100% identity to about 100 to 1649 contiguous nucleotides of DNA having the sequence of SEQ ID 5 NO. 42. The invention further includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid wherein said nucleic acid is capable of forming into a double stranded RNA. The invention further includes an isolated DNA molecule comprising a 0 polynucleotide encoding a nucleic acid wherein said nucleic acid comprises co-suppressor RNA. The invention further includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid wherein said nucleic acid comprises catalytic RNA. The invention further includes an isolated DNA molecule comprising a 15 polynucleotide encoding a nucleic acid wherein said nucleic acid sequence is capable of forming into a triplex nucleic acid. The invention further includes an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of 20 down-regulating a T6PP gene, wherein said promoter is also expressed in seed tissue. The invention also includes a plant cell having an isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP gene, and also includes a transgenic plant derived from said plant 25 cell. The invention further includes an isolated DNA molecule wherein said DNA molecule is depicted by SEQ ID NO. 8 or SEQ. ID. NO. 18. DESCRIPTION OF THE FIGURES 30 Fig. 1 is a schematic representation of the primary sugar metabolism pathways in a typical plant cell. The various sugar and activated sugar pools associated with starch and sucrose synthesis are shown. A permanent block in trehalose synthesis has been shown in the art to be lethal. However, the present invention recognizes that a conditional block in the Page 5 WO 2006/060376 PCT/US2005/043097 pathway from T-6-P to trehalose using a stress-inducible promoter to express T6PP-RNAi in vegetative tissue, redirects flux to sucrose or starch synthesis in a stress-inducible or developmental pattern. Fig. 2 is a schematic representation showing how the maize T6PP 1 cDNA sequences 5 were assembled. In section (A), the cDNAs were identified by TBLASTN queries of maize EST and cDNA databases and assembled in Sequencher. The strands 1, 2, and 3 shown at the bottom of section A show the plus (+) open reading frames. Strand 1 (ZmT6PP-1) contains the largest continuous open reading frame and is highlighted. Section (B) depicts the ZmT6PP-1 protein sequence. o10 Figs. 3A and 3B show the alignment of T6PP protein sequences. The Arabidopsis AtT6PPA and AtT6PPB sequences are aligned with the rice and maize homologs OsT6PP-1, OsT6PP-2, ZmT6PP-1, ZmT6PP-2, ZmT6PP-3. The alignment also includes ZmT6PP-target. The alignment was performed using AlignX within Vector NTI (Version 7.1). Fig. 4A shows the phylogenetic relationship of the maize, rice and Arabidopsis T6PP .5 proteins. Fig. 4B shows a similarity and divergence table illustrating similarity of each protein to the others along the horizontal axis and divergence of each protein from the others along the vertical axis. Similarity values are above and divergence values are below the '100' figure in each column. 10 Fig. 5 is a bar chart showing the expression profile of the OsT6PP-1 gene in various tissues. Relative expression above 100 is considered significant. The expression profile is consistent with the known expression of the Arabidopsis AtT6PP-A gene. Fig. 6 is a diagram showing sequence alignment of the maize ESTs (GenBank Accession Nos. BE510187, AW171812, AW081181, AI855276, BE453688 and AI941695). 5 ZmT6PP clone sequence data are denoted by t3.rev.91331.abi and tl.rev.91323.abl. Also identified are the primers used to clone the ZmT6PP-1 cDNA fragment and to construct the ZmT6PP-dsRNA cassette. Fig. 7 is a map of the maize T6PP-1 cDNA fragment in the pCR 4 TOPO vector, referred to as pCR4-TOPO-ZmT6PP-NS. 0 Fig. 8 is a map of the pNOV3210 expression cassette. Fig. 9 is a map of the pNOV3232 expression cassette. Fig. 10 is a map of the pRabl7-T6PP-RNAi construct. The complete Rabl7 expression cassette can be mobilized as a KpnI fragment. Page 6 WO 2006/060376 PCT/US2005/043097 Fig. 11A is a map of an Agrobacteriumn tumefaciens binary vector, pNOV2117, that contains the phosphmannose isomerase (cPMI-01) plant selectable marker within its T-DNA borders. Fig. 11B is a map of an Agrobacterium tumefaciens Rabl7-T6PP-RNAi expression 5 cassette cloned in pNOV2117. Fig. 12 illustrates kernel set yield data from a greenhouse experiment. Plants representing each genotype were subjected to well-watered (WW) or salt-stressed (SS) conditions during the two-week period around flowering. Azygotes (WT) and hemizygotes (TPP) were then scored for kernel set. Data are the means, n=3-5. 0 Fig. 13 illustrates kernel set yield data from a second greenhouse experiment. Plants representing each genotype were subjected to well-watered (WW) or salt-stressed (SS) conditions during the two-week period around flowering. Azygotes (WT) and hemizygotes (TPP) were then scored for kernel set. Data are the means, n=14-20. Fig. 14 illustrates kernel set yield data for Rabl7-T6PP-RNAi Event 78A18B in the 5 field. Ears from each plant in the field were harvested and shelled. The kernels counted and weighed. The means for hemizygous and azygous plants were calculated. The asterisk indicates a statistically significant difference between azygous and hemizygous plants. Fig. 15 illustrates yield data for Rabl7-T6PP-RNAi Event 81A10B progeny in the field. Ears from each plant in the field were harvested and shelled. The kernels counted and 20 weighed. The means for hemizygous and azygous plants were calculated. The asterisk indicates a statistically significant difference between azygous and hemizygous plants. Figs. 16A and 16B illustrate the alignment of the conserved T6PP cDNA sequence from several plant species. The alignment also includes T6PP-RNAi sequence. The alignment was perfonnrmed using AlignX within Vector NTI (Version 7.1). 25 Fig. 17 shows the phylogenetic relationship of conserved T6PP cDNA sequence from several plant species. The table illustrates percent similarity of each sequence to the others along the horizontal axis. The analysis was performed using AlignX within Vector NTI (Version 7.1). DETAILED DESCRIPTION OF THE INVENTION 30 The trehalose pathway represents a level of flux control through central sugar metabolism. Several studies identified control mechanisms that regulate enzymes in the metabolic network shown in Figure 1. The data are by no means exhaustive. However, given the ubiquity of the trehalose pathway and pathway gene expression in plants (Wingler, 2002), Page 7 WO 2006/060376 PCT/US2005/043097 and the lethality of a knockout at the pathway's entry point (Eastmond et al., 2002) the present invention recognizes that the trehalose pathway probably functions as a checkpoint to help regulate glucose-1-phosphate (g-1-P), glucose-6-phosphate (g-6-P) and fructose-6 phosphate (f-6-P) pool size in the cytosol. In situations where the capacity to generate these 5 molecules exceeds capacity to utilize them, the trehalose pathway acts as a "spill way" to quickly inactivate g-6-P and uridine diphosphate glucose (UDP-g) and recycle the glucose moiety. In this capacity the pathway sets up an apparent futile cycle that needlessly consumes energy, by converting substrates to products and later converts those products back to the original substrates. This assertion is not without precedence in plant biochemical networks 0 (Rontein et al., 2002b; Ronocha et al., 2001). Such control mechanisms are worth the slight, but necessary, energy expenditure because of their greater role in maintaining the stability of the system. Thus, the present invention further recognizes that the trehalose pathway provides a rapid, probably low-capacity, control mechanism to stabilize cytosolic hexose phosphate pools. 5 The trehalose pathway is poised to compete with other metabolic processes--such as starch synthesis, sucrose synthesis and glycolysis--for g-6-p and UDP-g. The present invention takes into account that engineering plants to express a heterologous protein(s), such as T6PP or T6PS, that may not be subject to endogenous regulation, using strong constitutive promoters pulls activated sugars out of central carbon metabolism. This wastes considerable Z0 energy and retards growth. Therefore, the composition and method of the present invention includes using promoters that are drought-inducible in vegetative tissue, that may also developmentally expressed in maturing kernels, operably linked to a nucleic acid molecule that when expressed in a plant cell, inhibits expression of the endogenous T6PP gene or the products thereof. By doing so, sugars are directed to synthesis of starch and sucrose for their 25 availability to developing kernels when plants are subject to.enviromnental stress. The present invention uses genetic engineering to decrease or eliminate, via down regulation, the expression of maize endogenous T6PP genes. There are numerous methods known to those skilled in the art for modifying expression of endogenous genes. Post transcriptional gene silencing (PTGS), triplex-forming nucleic acid, ribozymes, inactive 30 protein subunits and single-stranded monoclonal antibodies can all be used to eliminate or repress gene expression, as discussed in more detail below. In diverse eukaryotes, including plants, double stranded RNA (dsRNA) triggers destruction of any RNA sharing sequence with the double stranded RNA molecule Page 8 WO 2006/060376 PCT/US2005/043097 (Hutvigner and Zamore, 2002). It begins by the conversion of dsRNA into short 21-23 nucleotide fragments by the multi-domain RNAse III enzyme, Dicer (Lee et al., 2004; Pham et al., 2004). These small interfering RNAs (siRNAs) direct the degradation of target RNAs complementary to the siRNA sequence (Elbashir et al., 2001). In addition Dicer also cleaves 5 roughly 70 nt precursor stem-loop RNA structures into single-stranded 21-23 nt RNAs known as microRNAs (miRNAs) (Grishok et al., 2001; Reinhart et al., 2002). This is the basis for RNA interference (RNAi) technology that is used to suppress the expression of endogenous and heterologous genes in a sequence specific manner (Fire et al., 1998; Carthew, 2001; Elbashir et al., 2001). A RNAi suppressing construct can be designed in a 0 number of ways, for example, transcription of a inverted repeat which can form a long hair pin molecule, inverted repeats separated by a spacer sequence that could be an unrelated sequence such as GUS or an intron sequence. The present invention also contemplates transcription of sense- and antisense-RNA strands by opposing promoters, or cotranscription of sense and antisense genes. .5 Antisense RNA technology can be also be used to down-regulate expression of a specific endogenous gene. This is a down-regulation approach used to modify a desired plant enzyme level or activity. Antisense RNA results in down-regulation at the RNA translational level. Down-regulation by antisense RNA, as described by Shewmaker et al. (1992) has been shown effective with a variety of plant genes (Rothstein et al., 1987; Smith et al., 1988; van 20 der Krol et al., 1988; Bird et al., 1991; Bartley et al., 1992; Gray et al., 1992; Knutzon et al., 1992; Shimada et al., 1993; Kull, et al., 1995; Slabas and Elborough, 2000). In the nucleus, antisense RNA may directly interfere with transcription or form duplexes with the heterogeneous nuclear RNA (hnRNA). Alternatively, in the cytoplasm, antisense RNA may form a double-stranded molecule with the complimentary mRNA and prevent the translation 25 of mRNA into protein. Co-suppression, as described by Seymour et al., (1993) is another approach applicable for down-regulation of plant gene expression. Co-suppressor RNA, in contrast to anti-sense RNA, is in the same orientation as the RNA transcribed from the target gene, i.e., the "sense" orientation. It has been used extensively to produce transgenic plants having modified gene 30 expression levels (Napoli et al., 1990; Brusslan et al., 1993; Vaucheret et al., 1995; Jorgensen et al., 1996). The mechanism of co-suppression is thought to be caused by the production of antisense RNA by read-through transcription from distal promoters located on the opposite strand of the chromosomal DNA (Grierson et al. 1991). It's now understood that there are Page 9 WO 2006/060376 PCT/US2005/043097 common features associated with all forms of RNA-mediated gene silencing (Matzke et al., 2002; Tijsterman et al., 2002). Another down regulation approach involves the use of ribozyme technology (Atkins et al., 1995; De-Feyter et al., 1996). Ribozyme technology, like antisense methodologies, also 5 works at the RNA translational level and involves making catalytic RNA molecules that bind to, and cleave the mRNA of interest. Ribozymes have recently been demonstrated as an effective method for the down-regulation of plant proteins (Waterhouse and Wang, 2002) and control of plant pathogens (Atkins et al., 2002). A further down-regulation method includes use of co-suppressor or 'sense' nucleic 0 acids and dsRNAs. Nucleic acid sequences can be constructed which will bind to duplex nucleic acid either in the gene or the DNA:RNA complex of transcription, to form a stable triple helix-containing or triplex nucleic acid to inhibit transcription and/or expression of the target gene (Frank-Kamenetskii and Mirkin, 1995). Such nucleic acid sequences are constructed using the base-pairing rules of triple helix formation and the nucleotide sequence 5 of the gene or mRNA of interest. These nucleic acid sequences can block target gene-type activity in a number of ways, including prevention of transcription of the gene or by binding to mRNA as it is transcribed by the gene. A dominant-negative genetic approach can also be used to down-regulate specific types of enzymes. The presence of a dominant trait, i.e. the expression of a transgene, results 20 in a reduction of enzyme activity or reduced production of the enzymatic end-product. Some enzymes are complexes of two or more protein subunits. Such an enzyme's activity relies on the proper assembly of these subunits to form functional enzyme. Expression of a non functional subunit that can interact with the other subunit(s) can produce a non-functional enzyme and hence reduce enzymatic activity. The non-functional aspect may be in respect to, 25 but not limited to, subunit interaction, substrate binding or enzyme catalysis, for example. Another approach to down-regulate proteins in plants relies on the use of monoclonal antibodies (MAb) and/or functional fragments thereof, such as single chain antibodies (SCAb) that specifically recognize and bind transit peptides (Sukhapinda et al., 2004). As a result, steady-state levels of corresponding passenger proteins can be reduced. The above 30 described technologies and other technologies known to those skilled in the art for down regulating genes may be used in the present invention. The present invention includes down-regulating the endogenous maize T6PP gene by constructing a chimeric polynucleotide comprising a promoter that is drought-inducible in Page 10 WO 2006/060376 PCT/US2005/043097 vegetative tissue operatively linked to a nucleic acid, wherein when expressed in a plant cell the nucleic acid, or a portion thereof, is capable of reducing the expression of an endogenous T6PP gene of a plant cell. In one embodiment of the invention, the promoter is drought inducible in vegetative tissue. In another embodiment of the invention, the promoter is 5 derived from the 5' region of a Rabl7 gene. The invention encompasses the polypeptide also having a terminator sequence derived from the 3' region of the Rab 17 gene. When a recombinant promoter is used, the promoter can also be selected to cause expression of T6PP-RNAi in a manner that is different than how the ZmT6PP-1 protein is expressed by the plant in its native state. For example, the promoter may have no effect on O10 the level at which the ZmT6PP-1 protein is expressed, express the T6PP-RNAi without being induced by an environmental stress and/or express the T6PP-RNAi in response to a different form or degree of environmental stress than would otherwise be needed to induce expression of the Zm-T6PP-1 protein. The present invention recognizes that strong constitutive promoters should not be used to cause decreased levels of ZmT6PP-1 gene expression. 15 Examples of such strong constitutive promoters include, but are not limited to, the nopaline synthase (NOS) and octopine synthase (OCS) promoters (Jones et al., 1992), the cauliflower mosaic virus (CaMV) 19S and 35S promoters (Odell et al., 1985) or the enhanced CaMV 35S promoters (Kay et al., 1987). Constitutively down-regulating the trehalose pathway is known to cause pleotropic growth defects. Specific down-regulation of T6PP to direct photosynthate 20 to starch and sucrose in select cells is desirable. A tissue specific promoter could be used to alter ZmT6PP-1 gene expression in tissues that are highly sensitive to stress. Examples tissue-specific promoters include, but are not limited to, seed-specific promoters for the B. napus napin gene (Kridl and Knauf, 1995), the soybean 7S promoter (Fujiwara and Beachy, 1994), the Arabidopsis 12S globulin Z5 (cruciferin) promoter (Pang et al., 1988), the maize 27 kD zein promoter (Ueda et al., 1992) and the rice glutelin 1 promoter (Goto et al., 1999), fruit active promoters such as the E8 promoter from tomatoes (Mehta et al., 2002), tuber-specific promoters such as the patatin promoter (Kuehn et al., 2003), and the promoter for the small subunit of ribulose-1,5-bis phosphate carboxylase (ssRUBISCO) whose expression is activated in photosynthetic tissues 30 such as leaves (Laporte et al., 2001). Alternatively, a promoter could be used to induce the expression of the T6PP-RNAi gene only at a proper time, such as prior to a drought that occurs at or around the time of flowering, thereby improving the reproductive capability of the crop and increasing the Page 11 WO 2006/060376 PCT/US2005/043097 productivity of the land. This may be accomplished by applying an exogenous inducer by a grower whenever desired (Chua and Aoyama, 2000; Caddock et al., 2003). Similarly, a promoter can be used which turns on at a dehydration condition that is wetter than the dehydration condition at which the plant normally exhibits dehydration tolerance. This would 5 enable the level at which a plant responds to dehydration to be altered. Promoters which are known or are found to cause inducible transcription of the DNA into mRNA in plant cells can be used in the present invention. Such promoters may be obtained from a variety of sources such as plant and inducible microbial sources, and may be activated by a variety of exogenous stimuli, such as cold, heat, dehydration, pathogenesis and 0 chemical treatment. The particular promoter selected is preferably capable of causing sufficient expression of the T6PP-RNAi to enhance plant tolerance to environmental stress conditions such as water deficit. Examples of promoters which may be used include, but are not limited to, the promoter for the DRE (C-repeat) binding protein gene dreb2a (Liu et al., 1998) that is activated by dehydration and high-salt stress; the promoter for delta 1-pyrroline 5 5-carboxylate synthetase (P5CS) whose expression is induced by dehydration, high salt and treatment with the plant hormone abscisic acid (ABA) (Yoshiba et al., 1995; Zhang et al., 1997); the promoter for the rd22 gene from Arabidopsis whose transcription is induced by salt stress, water deficit and endogenous ABA (Yamaguchi-Shinozaki and Shinozaki, 1993a); the promoter for the rd29b gene (Yamaguchi-Shinizaki and Shinozaki, 1993b) whose !0 expression is induced by desiccation, salt stress and exogenous ABA treatment (Ishitani et al., 1998); the promoter for the rabl8 gene, or other dehydrins, from Arabidopsis whose transcripts accumulate in plants exposed to water deficit or exogenous ABA treatment (Nylander et al., 2001); the maize Rabl7 promoter that is drought-inducible in vegetative tissue and developmentally expressed in maturing kernels (Vilardell et al., 1991); and the 25 promoter for the pathogenesis-related protein la (PR-la) gene whose expression is induced by pathogenesis organisms or by chemicals such as salicylic acid and polyacrylic acid (Uknes et al., 1993). It should be noted that the promoters described above may be further modified to alter their expression characteristics. For example, the drought/ABA inducible promoter for the 30 rabl 8 gene may be incorporated into seed-specific promoters such that the rab18 promoter is drought/ABA inducible only in developing seeds. Similarly, any number of chimeric promoters can be created by ligating a DNA fragment sufficient to confer environmental stress inducibility from the promoters described above to constitute promoters with other Page 12 WO 2006/060376 PCT/US2005/043097 specificities such as tissue-specific promoters, developmentally regulated promoters, light regulated promoters, hormone-responsive promoters, etc. This should result in the creation of chimeric promoters capable of being used to cause expression of the T6PP-RNAi gene in any plant tissue or combination of plant tissues. Expression can also be made to occur either at a 5 specific time during a plant's life cycle or throughout the plant's life cycle. In one embodiment, the promoter of the instant invention modulates ZmT6PP-1 expression in plants experiencing various abiotic or environmental stresses, including cold, heat, dehydration, and/or salt stress that directly affect plant water relations. These promoters come from genes, and the like, that include, but are not limited to, the CBF/DREB family of 10 transcription factors shown to be induced by cold, salt, and dehydration stress (Jaglo-Ottosen et al., 1998); the maize Rabl7 promoter that is drought-inducible in vegetative tissue and developmentally expressed in maturing kernels (Vilardell et al., 1991); the LP3 water-deficit induced gene (Wang et al., 2002); the Arabidopsis CIPK3 gene that is responsive to ABA and stress conditions, including cold, high salt, wounding, and drought (Kim et al., 2003); the 15 barley (Hordeum vulgare) HVA22 gene that is induced dehydration, salinity, extreme temperatures, and ABA (Brands and Ho, 2002); the betaine aldehyde dehydrogenase (AcBADH) gene from the halophyte Atriplex centralasiatica Iljin that is induced by drought, salinity, cold stress and ABA (Yin et al., 2002); and the wheat Esi47 gene which is induced by salt stress and ABA (Shen et al., 2001). Expression of endogenous or exogenous -0 nucleotides under the direction of a stress-induced promoter may result in maintenance of a desirable plant phenotype under adverse environmental conditions such as water deficit. Expression cassettes containing the above promoters can function with a transcriptional terminator. In many cases the nopaline synthase (NOS) terminator performs this function. Many skilled in the art consider this terminator adequate for most applications 15 (Lessard et al., 2002). However, there are exceptions. In some cases expression cassette. performance improves when the NOS terminator is replaced with a similar sequence derived from the same gene the promoter is based on (No et al., 2000; Nuccio and Thomas, 2000; Moreno-Fonseca and Covarrubias, 2001). These exceptions often arise when use of the NOS terminus yields unsatisfactory results. The role gene terminator sequences play in overall .0 regulation is not fully understood. Those who recognize this potential and require faithful reproduction of an endogenous gene expression pattern will replace the NOS terminator with similar sequence derived from the gene used to produce the promoter. Likewise, those skilled Page 13 WO 2006/060376 PCT/US2005/043097 in the art may also choose a gene terminator derived from a gene other than that used for the promoter in order to construct an expression cassette with the desired regulatory properties. Stress-induced yield reduction in maize is most pronounced when plants experience stress approximately during the two-week period prior to anthesis and during the first week of 5 anthesis. This corresponds to the V12-V18 period of maize development (Ritchie et al., 1997). During this time the ear is formed, and the number and arrangement of ear spikelets is determined (Kiesselbach, 1999). Ovules, the kernel progenitors, develop within spikelets and are very susceptible to stress (Zinselmeier et al., 1995a), such as drought. One study showed a correlation between ovule starch depletion and the propensity to abort (Zinselmeier et al., 10 1999). Other work suggested ovary abortion can be reversed by increasing carbohydrate flux to ovules during periods of stress (Zinselmeier et al., 1995b). The present invention is directed to genetic engineering solutions to reduce environmental stress related yield loss in maize by increasing carbohydrate flux to developing kernels when such kernels are developing during periods of environmental stress, by using a promoter that is drought 15 inducible in vegetative tissue and that may also be developmentally expressed in maturing kernels. Examples of suitable plants for which stress tolerance may be induced according to the methods of the present invention and which may be transformed with the expression cassettes of the invention include monocotyledonous and dicotyledonous plants such as field Z0 crops, cereals, fruit and vegetables such as: canola, sunflower, tobacco, sugarbeet, cotton soya, maize, wheat, barley, rice, sorghum, tomatoes, mangoes, peaches, apples, pears, strawberries, bananas, melons, potatoes, carrots, lettuce, cabbage and onion. Example 1: Identification and acquisition of the ZmTPP1 gene The first vascular plant trehalose-6-phosphate phosphatase genes were cloned from :5 Arabidopsis thaliana by complementation of a yeast tps2 deletion mutant (Vogel et al. 1998). The genes designated AtTPPA and AtTPPB (GenBank accessions AF007778 and AF007779) were shown at that time to have trehalose-6-phosphate phosphatase activity. The AtTPPA and AtTTPB protein sequences were used in TBLASTN queries of maize and rice sequence databases. Sequence alignments organized the hits into individual genes. Fig. 2A, is a cartoon 0 depicting the alignment that defines ZmT6PP-1. Three maize and two rice T6PP homologs were identified. The cDNA sequences corresponding to the predicted protein sequence for each gene--ZmT6PP-1, -2 and -3 and OsT6PP-1 and -2-- are depicted by SEQ. ID NOS. 1, 2, 3, 4 and 5, respectively. These T6PPs are shown in global alignment the Arabidopsis T6PPs Page 14 WO 2006/060376 PCT/US2005/043097 in Figure 3. The relationship between each protein to the others is further analyzed using a phylogenetic tree (Fig. 4A) and a similarity/divergence table (Fig. 4B). Results suggest that ZmT6PP-1 is the likely maize homolog of AtTPPA and ZmT6PP-2 is the likely maize homolog of AtTPPB. The ZmT6PP-1 gene was targeted for inactivation because the EST 5 data show it is expressed in a pattern consistent with AtT6PPA. However, the EST data are limited due to unequal tissue representation among the maize EST libraries. To compensate, the OsT6PP-1 cDNA sequence was used to query Expression Profiling data. The results, in Figure 5, show the OsT6PP-1 is expressed at a relatively low level in most tissues, which agrees with the data for AtT6PPA (Vogel et al., 1998). 0 A partial ZmT6PP-1 cDNA (SEQ ID NO. 13) was amplified from a maize mixed tissue cDNA library in two steps (Fig. 6). The library was cloned in the NotI and SalI restriction sites of the Invitrogen vector pCMVSPORT6. A first fragment referred to as T6PP1 was produced in a 50 pL reaction mixture consisting of 1 pL maize cDNA library, 200 pM dNTPs (dATP, dCTP, dGTP, TTP), 1 pL 20 pM oligonucleotide primer ZmTPP-lb 5 (5'-TTCTCCCTATCTATGTTGGAG-3') (SEQ ID NO. 19), 1 ptL 20 pM oligonucleotide primer ZmTPP-2 (5'-CGCAACACAGTGAAACACTAGAAGG-3') (SEQ ID NO. 20), 1 p1L 10X Expand High Fidelity buffer and 1 pL Expand High Fidelity polymerase (Roche Diagnostics, Cat. No. 1 759 078). The thermocycling program was 94oC for 2 minutes followed by 40 cycles of (94oC for 15 seconds, 58oC for 30 seconds, 68oC for 1.0 minute) 0 followed by 68oC for 5.0 minutes. A second fragment, referred to as T6PP2 (SEQ ID NO. 14), was produced in a 50 p1L reaction mixture consisting of 1 tL maize cDNA library, 200 pM dNTPs, 1 pL 20 pM oligonucleotide primer ZmTPP-2r (5'-CCTTCTAGTGTTTCACTGTGTTGCG-3') (SEQ ID NO. 21), 1 pL 20 pM oligonucleotide primer psport-forward (5' 25 GCCAGTGCCTAGCTTATAATACG-3') (SEQ ID NO. 22), 1 pL 10X Expand High Fidelity buffer and 1 pL Expand High Fidelity polymerase (Roche Diagnostics, Cat. No. 1 759 078). The thermocycling program was 94oC for 2 minutes followed by 40 cycles of (94oC for 15 seconds, 58oC for 30 seconds, 68oC for 1.0 minute) followed by 68 0 C for 5.0 minutes. 30 The T6PP1 and T6PP2 fragments were joined using the splicing by overlap extension PCR method. The 50 pL reaction mixture consisted of 2 pL T6PP1 reaction mix, 2 p1L T6PP2 reaction mix, 200 pM dNTPs, 1 pL 20 pM oligonucleotide primer ZmTPP-lb, 1 p1L Page 15 WO 2006/060376 PCT/US2005/043097 20 pM oligonucleotide primer psport-forward, 1 ptL 10X Expand High Fidelity buffer and 1 ptL Expand High Fidelity polymerase (Roche Diagnostics, Cat. No. 1 759 078). The thermocycling program was 5 cycles of (94oC for 30 seconds, 68oC for 1.0 minute) followed by 35 cycles of (94oC for 30 seconds, 58oC for 30 seconds, 68oC for 1.0 minute) followed by 5 68oC for 7.0 minutes. Cloned the 0.8 kb DNA product, encoding the ZmT6PP-1 fragment, with the TOPO TA cloning kit for sequencing (Invitrogen, Cat. No. K4575-01). 2.0 p L of the reaction mix was transformed into 50 pL Topl0 competent cells (Invitrogen, Cat. No. C4040-03). The pCR-4-TOPO-ZmT6PP-NS recombinants containing the ZmT6PP-1 fragment were identified by digesting 5 pL pCR-4-TOPO-ZmT6PP-NS miniprep DNA 10 (prepared using the QIAprep Spin Miniprep procedure from Qiagen, Cat. No. 27106) with EcoRI (New England Biolabs) in a 20 [tL reaction containing 2 pg BSA and 2 pL 10X EcoRI restriction endonuclease buffer (New England Biolabs). The reaction was incubated at 37oC for 2 hours then pCR-4-TOPO-ZmT6PP-NS (EcoRI) products were resolved on 1% TAE agarose. The pCR-4-TOPO-ZmT6PP-NS clones were sequenced using the ABI PRISM dye 15 terminator cycle sequencing kit (Perkin Elmer). The pCR-4-TOPO-ZmT6PP-NS map is shown in Fig. 7. Example 2: Construction of the Rabl7 Expression Cassette An expression cassette based on the maize Rab 17 gene was discovered to be drought Z0 inducible (Vilardell et al., 1990) in vegetative tissue and developmentally expressed in maturing seeds (Vilardell et al., 1991). One embodiment of the present invention is to provide a nucleic acid construct that comprises a promoter that is drought inducible in vegetative tissue operatively linked to a nucleic acid molecule, wherein when expressed in a plant cell the nucleic acid molecule is capable of reducing the expression of an endogenous T6PP gene 5 of a plant cell. The invention includes a nucleic acid construct having a promoter derived from the 5' region of a Rab 17 gene and that exhibits promoter activity in plants. The invention also includes the nucleic acid construct comprising all or part of a nucleic acid sequence encoding T6PP-RNAi, wherein the Rabl7 promoter drives the T6PP 0 RNAi expression cassette to create a conditional block in the trehalose pathway. The T6PP RNAi expression cassette of the invention re-directs carbohydrate to sucrose or starch synthesis in reproductive tissue and in vegetative tissue during periods of water deficit. Page 16 WO 2006/060376 PCT/US2005/043097 The nucleic acid construct of the invention further includes both the 5' and 3'-regions derived from the maize Rabl 17 gene, wherein the regions exhibit promoter and terminator activity in plants, respectively. In one embodiment of the invention, both the 5' and 3' regions were used in the nucleic acid construct to assure that the transgene expression mimics 5 maize Rabl7 expression. To begin, cDNA sequence was gathered, aligned and annotated. The published gDNA sequence (GenBank Accession No. X159940) was used to query public and proprietary databases. The Rabl7 cDNA sequence was broken into exons and aligned with Rabl7 gDNA to provide the requisite annotation and map the translation start and stop codons onto the gDNA. 10 The ZmRabl7 promoter was amplified from maize gDNA in a 50 pL reaction mixture consisting of 100 ng maize gDNA, 200 gM dNTPs, 1 pL 20 pM oligonucleotide primer 000426A (5'-GGTACCAAGCTTAATTCGCCCTTATAAACT-3') (SEQ ID NO. 33), 1 iL 20 pM oligonucleotide primer 000426B (5' ACTGCAGTTAGATCTAGTCTTCGTGCTTGTGT-3') (SEQ ID NO. 24), 1 p.L 10X 5 Expand High Fidelity buffer and 1 p.L Expand High Fidelity polymerase. The thermocycling program was 94oC for 2 minutes followed by 40 cycles of (94oC for 15 seconds, 58oC for 30 seconds, 68oC for 2.0 minutes) followed by 68 0 C for 5.0 minutes. The 0.6 kb DNA product encoding the ZmRabl7 promoter was cloned with the TOPO TA cloning kit for sequencing following manufactures' instructions. 2.0 pL of the reaction mix was transformed into 50 pL .0 Topl0 competent cells following manufactures' instructions. pCR-4-TOPO-pZmRabl7 recombinants containing the ZmRabl7 promoter were identified by digesting 5 gL pCR-4 TOPO-pZmRabl7 miniprep DNA with EcoRI in a 20 ptL reaction containing 2 ig BSA and 2 gL 10X EcoRI restriction endonuclease buffer. The reaction was incubated at 37oC for 2 hours then pCR-4-TOPO-pZmRabl7 (EcoRI) products were resolved on 1% TAE agarose. 5 The pCR-4-TOPO-pZmRabl7 clones were sequenced using the ABI PRISM dye terminator cycle sequencing kit. The pCR-4-TOPO-pZmnRab 17 sequence is given as SEQ ID NO. 11. The ZmRabl7 terminator was amplified from maize gDNA in a 50 pL reaction mixture consisting of 100 ng maize gDNA, 200 ptM dNTPs, 1 pL 20 p.M oligonucleotide primer 000426C (5'-ACTGCAGTACGTGGCTGTGCTGTG-3') (SEQ ID NO. 25), 1 pL 20 0 p.M oligonucleotide primer 000426D (5'-CGGTACCAATTGCATGCGTCTAATCA-3') (SEQ ID NO. 26), 1 p.L 10X Expand High Fidelity buffer and 1 p.L Expand High Fidelity polymerase. The thermocycling program was 94oC for 2 minutes followed by 40 cycles of Page 17 WO 2006/060376 PCT/US2005/043097 (94oC for 15 seconds, 58 0 C for 30 seconds, 68 0 C for 2.0 minutes) followed by 68 0 C for 5.0 minutes. The 0.6 kb DNA product encoding the ZmRabl7 terminus was cloned with the TOPO TA cloning kit. 2.0 [tL of the reaction mix was transformed into 50 p L Top10 competent cells. pCR-4-TOPO-tZmRabl7 recombinants containing the ZmRabl7 terminator 5 were identified by digesting 5 ptL pCR-4-TOPO-tZmRabl7 miniprep DNA with EcoRI in a 20 p L reaction containing 2 tg BSA and 2 pL 10X EcoRI restriction endonuclease buffer. The reaction was incubated at 37oC for 2 hours then pCR-4-TOPO-tZmRabl7 (EcoRI) products were resolved on 1% TAE agarose. The pCR-4-TOPO-tZmRabl7 clones were then sequenced. The pCR-4-TOPO-tZmRabl7 sequence is given as SEQ ID NO. 12. 0 pZmRabl7 and tZmRabl7 were amplified from pCR-4-TOPO-pZmniRabl7 and pCR 4-TOPO-tZmRabl7, respectively, as described above. The PCR products were purified with the MinElute PCR purification kit (Qiagen, Cat. No. 28004), digested in 50 p L reactions containing 5 [tg BSA, 5 pL 10X restriction endonuclease buffer 1, 2.5 p L KpnI and 2.5 p L PstI (New England Biolabs). The reactions were incubated at 37oC for more than 6 hours, 15 then at 70oC for 20 minutes. The 0.5 kb pRAB17 (KpnI/PstI) and 0.7 kb tZmRabl7 (Kpnl/PstI) DNA were resolved on 1.0% TAE agarose and the bands were excised. The DNA and extracted and recovered using the QIAquick Gel extraction kit (Qiagen, Cat. No.28704). Each fragment was eluted in 40 ptL ddH20. 40 ptL of pRAB17 (KpnI/PstI) was ligated to 40 p L tZmRabl7 (KpnI/PstI) in a 100 20 p L reaction containing 10 pL 10X T4 DNA ligase buffer (New England Biolabs) and 10 p L T4 DNA ligase (400 Units/tL- New England Biolabs). The ligation reaction was incubated more than 8 hours at 16oC. The ligation was precipitated with 20 pg glycogen, 0.3 M

CH

2 COONa (pH 5.2) and 2.5 volumes ethanol at -20oC for more than 2 hours. The ligation products were recovered by micro centrifugation, washed with 70% ethanol, dried under 25 vacuum and resuspended in 14 ptL ddH 2 0. The ligation products were digested in a 20 pL reaction containing 2 [tg BSA, 2 tL 10X restriction endonuclease buffer 1 and 2 jtL KpnI. The reaction was incubated at 37oC for more than 6 hours, then at 70oC for 20 minutes. The resolved DNA was digested on 1.0% TAE agarose and excised the 1.3 kb pZmnRabl7-tZmRabl7 (KpnI) band. The pZmRabl7 30 tZmRabl 17 (KpnI) DNA was extracted and recovered it using the QIAquick Gel extraction kit (Qiagen, Cat. No.28704). The recovered pZmRabl7-tZmRabl7 (KpnI) DNA was precipitated with 20 pig glycogen, 0.3 M CH 2 COONa (pH 5.2) and 2.5 volumes ethanol at Page 18 WO 2006/060376 PCT/US2005/043097 20oC for more than 2 hours. The pZmRabl7-tZmRabl7 (KpnI) DNA was recovered by micro centrifugation, washed with 70% ethanol, dried under vacuum and resuspended in 5 pL ddH 2 0. 2 pg of pBluescript II (KS-)--aka pBS--DNA (QIAprep Spin Miniprep procedure 5 from Qiagen, Cat. No. 27106) was digested in a 20 p L reaction containing 2 jtg BSA, 2 pL 10X restriction endonuclease buffer 1 and 2 pL KpnI. Incubated the reaction at 37oC for more than 6 hours, then at 70 0 C for 20 minutes. 1 pL 10X restriction endonuclease buffer 1, 1 p L 1 Unit/[iL calf-intestinal alkaline phosphatase and 8 pL ddH 2 0 were then added to the reaction and incubated at 37oC for 30 minutes. The pBS (KpnI/CIP) DNA was resolved on 1.0% TAE 0 agarose and the 3.0 kb pBS (KpnI/CIP) band was excised. The pBS (KpnI/CIP) DNA was recovered and precipitated with 20 pg glycogen, 0.3 M CH 2 COONa (pH 5.2) and 2.5 volumes ethanol at -20oC for more than 2 hours. The pBS (KpnI/CIP) DNA was recovered by micro centrifugation, washed with 70% ethanol, dried under vacuum and resuspended in 5 pL ddH 2 0. 15 4.0 pL ofpZmniRabl7-tZmRabl7 (KpnI) was ligated to 4.0 ptL pBS (KpnI/CIP) in a 10 pL reaction containing 1 pL 10X T4 DNA ligase buffer and 1 pL T4 DNA ligase (400 Units/pL) and incubated more than 8 hours at 16'C. 5.0 pL of ligation mix was transformed into 50 ptL Top10 competent cells. pBS-pZmRabl7/tZmRabl7 recombinants were verified by digesting 2 ptL pBS-pZmnRabl7/tZmRabl7 miniprep DNA with 1.0 ptL KpnI in 10 ptL 20 reactions containing 1 ptg BSA and 1 ptL 10X restriction endonuclease buffer 1. The reactions were incubated at 37oC for 2 hours then pBS-pZmRabl7/tZmRab17 (KpnI) DNA was resolved on 1% TAE agarose. The pBS-pZmRabl7/tZmRabl7 clones were then sequenced. The pBS-pZmRabl7/tZmRabl7 sequence was designated as pNOV3010 (SEQ ID NO. 17). The pNOV3010 map is shown in Fig. 8. 25 pNOV3010 lacks flexibility to clone genes of interest. Additional restriction sites were added at the pZmnRabl7/tZmRabl7 junction to increase flexibility by ligating a synthetic adapter to the vector. The adapter (Synthetic Adaptor I) was made by combining 40 ptL of 50 [tM oligonucleotide 000809A (5'-PGATCGGCGCGCCTGTTAATTAATTGC GGCCGC-3') (SEQ ID NO. 27), 40 ptL of 50 jtM oligonucleotide 000809B (5' 30 PGATCGCGGCCGCAATTAATTAACAGGCGCGCC-3') (SEQ ID NO. 28)--where P is a 5'-phosphate group--in a 100 tL mixture that is 25 mM in Tris-HC1 (pH 8.0) and 10 mM in Page 19 WO 2006/060376 PCT/US2005/043097 MgCl 2 . The mixture was boiled for 5 minutes, removed from heat and naturally cooled to room temperature (about 60 minutes). This yields a 20 jiM Synthetic Adaptor I solution. pNOV3010 was prepared by digesting 14 pL of miniprep pNOV3010 DNA with 2 jIL BglII in a 20 jiL reaction containing 2 jig BSA and 2 jL 10X restriction endonuclease buffer 5 3. The reaction was incubated at 37oC for 6 hours, then at 70oC for 20 minutes. 1 jtL 10X of the restriction endonuclease buffer 3, 1 jtL 1 Unit/jtL calf-intestinal alkaline phosphatase (CIP-New England Biolabs) and 8 jL ddH 2 0 was added to the reaction and then incubated at 37oC for 30 minutes. pNOV3010 (BglII/CIP) digestion products were resolved on 1% TAE agarose, the pNOV3010 (BglII/CIP) DNA band was extracted and recovered. The 0 pNOV3010 (BglII/CIP) DNA was then precipitated with 20 jtg glycogen, 0.3 M CH 2 COONa (pH 5.2) and 2.5 volumes ethanol at -20 0 C for more than 2 hours. pNOV3010 (BglII/CIP) DNA was recovered by micro centrifugation, washed with 70% ethanol, dried under vacuum and resuspended in 5 jtL ddH20. 4.5 jtL Synthetic Adaptor I was ligated to 2.5 jtL pNOV3010 (BglIl/CIP) in a 10 pL .5 reaction containing 1 jiL 10X T4 DNA ligase buffer (New England Biolabs) and 1 jtL T4 DNA ligase (400 U/jtL- New England Biolabs) and incubated more than 8 hours at 16oC. 4 jtL of ligation was transformed into 50 jtL XL-1 supercompetent cells (Stratagene, Cat. No. 200236). The recombinants were verified by digesting 5 jiL miniprep DNA in a 20 jtL reaction containing 2 jtg BSA, 2 jtL 10X restriction endonuclease buffer 4 and 1 jiL AscI. 20 The products were resolved on 1.0% TAE agarose. The finished clone was designated as pNOV3232 (SEQ ID NO. 7). The map for pNOV3232 is shown in Fig. 9. Example 3: Construction of the T6PP-RNAi Expression Cassette The primers used to produce the T6PP-RNAi gene are shown in Fig. 6. Two PCR 25 fragments were produced from pCR-4-TOPO-ZmT6PP-NS template (Fig. 7). Fragment 1 (SEQ ID NO. 15) contains a portion of the CMVpSPORT6 vector that functions as the loop in the T6PP-RNAi gene product. High-fidelity PCR was used to amplify Fragment 1 from pCR-4-TOPO-ZmT6PP-1 in a 50 jtL reaction mixture consisting of 1 jtL pCR-4-TOPO ZmT6PP-NS miniprep DNA, 200 jtM dNTPs, 20 jtM oligonucleotide primer 001L (5' 30 ATAGGCGCGCCATGTTGGAGATGACAGAACAGATC-3') (SEQ ID NO. 38), 20 jiM oligonucleotide primer 002R (5'-ATACCGCGGGGACTGTCCTGCAGGTTTAAACG-3') (SEQ ID NO. 39), 5 jtL 10X cloned Pfu buffer and 2.5 Units of Pfuturbo DNA polymerase Page 20 WO 2006/060376 PCT/US2005/043097 (Stratagene, Cat. No. 600252) in a final volume of 50 qL. The thermocycling program was 95oC for 30 seconds then 40 cycles of (95oC for 10 seconds, 65oC for 60 seconds, 72 0 C for 2 minutes) then 72oC for 10 minutes. The Fragment 1 DNA product was recovered and the DNA was ethanol precipitated with glycogen carrier. The Fragment 1 DNA was recovered by 5 micro centrifugation, washed with 70% ethanol, dried under vacuum and resuspended in 14 pL ddH20. Fragment 2 is given as SEQ ID NO. 16. High-fidelity PCR was used to amplify Fragment 2 from pCR-4-TOPO-ZmT6PP-NS in a 50 pL reaction mixture consisting of 1 pL pCR-4-TOPO-ZmT6PP-NS miniprep DNA, 200 [tM dNTPs, 20 pM oligonucleotide primer 0 003L (5'-GCGTTAATTAAATGTTGGAGATGACAGAACAGATC-3') (SEQ ID NO. 40), 20 tM oligonucleotide primer 004R (5' ATACCGCGGCGCAACACAGTGAAACACTAGAAGG-3') (SEQ ID NO. 41), 5 [LL 10X cloned Pfu buffer and 2.5 Units of Pfuturbo DNA polymerase in a final volume of 50 pL. The thermocycling program was 95oC for 30 seconds then 40 cycles of (95oC for 10 seconds, 5 65oC for 60 seconds, 72oC for 2 minutes) then 72oC for 10 minutes. The Fragment 2 DNA product was recovered and the DNA was ethanol precipitated with glycogen carrier. The Fragment 2 DNA was recovered by micro centrifugation, washed with 70% ethanol, dried under vacuum and resuspended in 14 ptL ddH 2 0. Fragment 1 and Fragment 2 DNA were digested, separately, in a 20 tL reaction 0 mixtures containing 2 ptg BSA, 2 tL 10X restriction endonuclease buffer and 2 pL SacII. The digests were incubated at 37oC for 2 hours. The enzyme was inactivated by incubation for 15 minutes at 65oC. 4.0 ptL of Fragment 1 (SacII) DNA was ligated to 4.0 pL Fragment 2 (SacII) DNA in a 10 pL ligation mixture containing 1 pL 10X T4 DNA ligase buffer and 1 pL T4 DNA ligase (400 Units/ptL), which was incubated more than 24 hours at 16oC. The 25 enzyme was inactivated by incubation for 15 minutes at 65oC. This yielded the T6PP-RNAi gene (SEQ ID NO. 6). The T6PP-RNAi gene was digested in a 20 ptL reaction mixture containing 2 pg BSA, 2 tL 10OX restriction endonuclease buffer, 1 [tL PacI and 1 tL AscI. The digest was incubated at 37 0 C for 2 hours. The ZmRabl7 expression cassette plasmid, pNOV3232 (Fig. 9) (SEQ ID 30 NO. 7), was digested in a 20 piL reaction mixture containing 2 [tg BSA, 2 ptL 10X restriction endonuclease buffer, 1 L PacI and 1 pL AscI. Resolved the T6PP-RNAi gene (AscI/PacI) and pNOV3232 (AscI/PacI) digestion products on 1% TAE agarose, extracted the 1136 bp Page 21 WO 2006/060376 PCT/US2005/043097 T6PP-RNAi gene (AscI/PacI) and 4262 bp pNOV3232 (Ascl/PacI) DNA bands and recovered the DNAs. The recovered DNAs were precipitated with 20 ptg glycogen, 0.3 M

CH

2 COONa (pH 5.2) and 2.5 volumes ethanol at -20'C for more than 2 hours. The DNAs were recovered by micro centrifugation, washed with 70% ethanol, dried under vacuum and 5 resuspended each in 5 pL ddH20. 4.0 pL of the T6PP-RNAi gene (AscI/PacI) was ligated to 4.0 [L pNOV3232 (Ascl/PacI) in a 10 gL reaction containing 1 pL 10X T4 DNA ligase buffer and 1 pL T4 DNA ligase (400 Units/pL) and incubated more than 8 hours at 16oC. 5.0 tL of the ligation mix was transformed into 50 pL Topl0 competent cells. pRabl7-T6PP-RNAi recombinants 0 were verified by digesting 2 LL pRabl7-T6PP-RNAi miniprep DNA with 1.0 4L KpnI in 10 [tL reactions containing 1 pg BSA and 1 tL 10X restriction endonuclease buffer 1. The reactions were incubated at 37oC for 2 hours then the pRabl7-T6PP-RNAi (KpnI) DNA was resolved on 1% TAE agarose. The pRabl7-T6PP-RNAi DNA sequence was verified and the construct designated SEQ ID NO. 8. The pRabl7-T6PP-RNAi expression cassette map is .5 shown in Fig. 10. Example 4: Construction of a modified Rabl7-T6PP-RNAi expression cassette To improve trait performance the maize Rabl7 promoter sequence was modified to incorporate the complete Rabl7 5'-UTR, the first intron from the maize Rabl7 gene and 20 about 15 nucleotides of the second maize Rabl7 exon. This modified 5'-regulatory sequence of the invention was designed to replace the Rabl 17 promoter in pNOV3240. Specific changes made in the Rabl7 5'-regulatory sequence (Seq Id. No. 7) to construct the modified promoter are: (1) The 'G' at nucleotide 604 was changed to 'C', (2) The 'A' at nucleotide 665 was changed to 'T', (3) The 'A' at nucleotide 718 was changed to 'T', (4) The 'A' at nucleotide 748 25 was changed to 'T' and (5) The 'G' at nucleotide 783 was changed to 'C'. Finally, to facilitate recombinant DNA procedures, the PacI and AscI restriction endonuclease sites were added after the '...TCGGAGGAC' nucleotides ofRabl7 exon 2. The maize Rabl7 5'-regulatory sequence was amplified from gDNA using high fidelity PCR. A 50 tL reaction mixture contains 100 ng maize gDNA (Cv. 6N615), 200 jIM 30 dNTPs, 1 pL 20 pM prRabl7-F3 (5'-TCAAAACTATAGTATTTTAAAATTGC-3') (SEQ ID NO. 29), 1 iL 20 [tM prRabl7-R3 (5'-GTCCTCCGACTTAAACACG-3') (SEQ ID NO. 30), 5 pL 10X Expand High Fidelity buffer and 1 ptL Expand High Fidelity polymerase. The Page 22 WO 2006/060376 PCT/US2005/043097 thermocycling program is 95 0 C for 2 minutes followed by 40 cycles of (94oC for 15 seconds, 68 0 C for 7.5 minutes) followed by 68oC for 10 minutes. The Rabl7 5'-regulatory sequence was cloned with the TOPO XL PCR cloning kit. pCR-XL-TOPO-Rabl7-gDNA recombinants were identified by digesting 5 tL pCR-XL-TOPO-Rabl7-gDNA miniprep 5 DNA in 20 p L reactions containing 2 [tg BSA and 2 pL 10X EcoRI restriction endonuclease buffer. The reactions were incubated at 37oC for 2 hours and the pCR-XL-TOPO-Rabl7 gDNA (EcoRI) products are resolved on 1% TAE agarose. The pCR-XL-TOPO-Rabl7 gDNA clone was then sequenced. The modified Rab17 promoter required several sequence changes. First, potential 0 translation initiation codons were eliminated. First, potential translation initiation codons were eliminated using the Stratagene QuikChange Multi Site-Directed Mutagenesis Kit (Cat. No. 200513). The primers that were used to make the changes are: RabATG1 (5'-CGTGCAAGCATCATCGAGTACGGTCAGCAG-3')(SEQ ID NO. 31), RabATG2 (5'-CGCCACGGGCCTTGTCGACCAGTACG-3') (SEQ ID NO. 32), 5 RabATG3 (5'-GCACCGGCGGCTTGAGGCACGGCA-3') (SEQ ID NO. 33), RabATG4 (5'-CCACCGGCGGCTTGGGCCAGCTGG-3') (SEQ ID NO. 34), and RabATG5 (5'-GGCGCTGGCATCGGTGGCGGGCAG-3') (SEQ ID NO. 35). High-fidelity PCR was used to attach restriction endonuclease sites to the modified Rabl7 promoter. The 50 jtL reaction mixture contained 1 pL pCR-XL-TOPO-Rab17-gDNA 20 mini-prep DNA, 300 [tM dNTPs, 1 ptL 20 pM AscI-Rabl7 (5'

TTAATTAAGGCGCGCCTTCAAAACTATAGTATTTAAAATTGC-

3 ') (SEQ ID NO. 36), 1 pL 20 IM Rabl7-Paci-Asc-3 (5'

TTGGCGCGCCTTAATTAAGTCCTCCGACTTAAACAC-

3 ') (SEQ ID NO. 37), 5 p[L 10X Proofstart High Fidelity buffer, 10 pL Q solution and 2 pL Proofstart High Fidelity 25 polymerase. The thermocycling program was 95oC for 5 minutes followed by 45 cycles of (94oC for 30 seconds, 50oC for 1 minute, 72oC for 4 minutes) followed by 72oC for 15 minutes. The PCR product was purified and digested in 50 p1L reactions containing 5 jig BSA, 5 jiL 10X restriction endonuclease buffer 4 and 5.0 jiL AscI. The reaction was incubated at 37 0 C for more than 6 hours, then at 70 0 C for 20 minutes. The 1.0 kb pRab17 30 mod (AscI) was resolved on 1.0% TAE agarose and the band was excised. The DNA was extracted and recovered. The recovered pRabl7-mod (AscI) DNA was ethanol precipitated with glycogen carrier. The pRabl7-mod (AscI) DNA fragment was recovered by micro Page 23 WO 2006/060376 PCT/US2005/043097 centrifugation, washed with 70% ethanol, dried under vacuum and resuspended in 5 4pL ddH 2 0. 2 pg of pNOV3240 miniprep DNA was digested in a 20 4L reaction mixture containing 2 4g BSA, 2 [tL 10X restriction endonuclease buffer 4 and 2 4L AscI. The 5 reaction mixture was incubated at 37 0 C for more than 6 hours, then at 70 0 C for 20 minutes. Then 1 pL restriction endonuclease buffer 4, 1 tL 1 Unit/jtL calf-intestinal alkaline phosphatase and 8 [tL ddH 2 0 were added to the reaction mixture and incubated at 37oC for 30 minutes. The pNOV3240 (AscI/CIP) DNA was resolved on 1.0% TAE agarose and the 11 kb pNOV3240 (Ascl/CIP) band was excised. The pNOV3240 (Ascl/CIP) DNA was extracted 0 and recovered. The recovered pNOV3240 (Ascl/CIP) DNA was ethanol precipitated with glycogen carrier. The pNOV3240 (AscI/CIP) DNA was recovered by micro centrifugation, washed with 70% ethanol, and dried under vacuum and resuspended in 5 jtL ddH 2 0. 4.0 p.L pRabl7-mod (AscI) was ligated to 4.0 gL pNOV3240 (AscI/CIP) in a 10 ptL ligation mixture containing 1 jtL 10X T4 DNA ligase buffer and 1 IL T4 DNA ligase (400 5 Units/tL). The ligation mixture was incubated for more than 8 hours at 16'C. 5.0 [IL of ligation mixture was transformed into 50 ptL Top10 competent cells. The modified pNOV3240 recombinants were verified by digesting 2 pL modified-pNOV3240 miniprep DNA with 1 ptL SalI in 10 pL reactions containing 1 ptg BSA and 1 [tL of the appropriate 10X restriction endonuclease buffer. Digests were incubated at 37 0 C for 2 hours then 20 resolved on 1% TAE agarose. The positive modified-pNOV3240 recombinants were sequenced. The nucleotide sequence of the modified Rabl7-T6PP-RNAi expression cassette is depicted in SEQ ID NO. 18. Example 5: Construction of the Binary Agrobacterium tumefaciens Plasmid 25 2 pg ofpNOV2117 (Fig. 11A) was digested in a 20 ptL reaction containing 2 ptg BSA, 2 pL 10X restriction endonuclease buffer 1 and 2 pL KpnI. The reaction was incubated at 37oC for more than 6 hours, then at 70oC for 20 minutes. 1 ptL 10X restriction endonuclease buffer 1, 1 ptL 1 Unit/pL calf-intestinal alkaline phosphatase (CIP) and 8 pL ddH 2 0 was then added and incubated at 37oC for 30 minutes. 2 ptg pRabl7-T6PP-RNAi miniprep DNA was 30 digested in a 20 pL reaction containing 2 ptg BSA, 2 pL 10X restriction endonuclease buffer 1 and 2 tL KpnI. The reaction was incubated at 37 0 C for more than 6 hours. Page 24 WO 2006/060376 PCT/US2005/043097 The digested plasmid DNAs, pNOV2117 (KpnI/CIP) and pRabl7-T6PP-RNAi (KpnI), were resolved on 1.0% TAE agarose and the 9.2 kb pNOV2117 (KpnI/CIP) and the 2.5 kb pRabl7-T6PP-RNAi (KpnI) DNA bands were excised. The pNOV2117 (KpnI/CIP) and pRabl7-T6PP-RNAi (KpnI) DNAs were extracted and then precipitated with 20 ig 5 glycogen, 0.3 M CH 2 COONa (pH 5.2) and 2.5 volumes ethanol at -20 0 C for more than 2 hours. The pNOV2117 (KpnI/CIP) and pRabl7-T6PP-RNAi (KpnI) DNA fragments were recovered by micro centrifugation, washed with 70% ethanol, dried under vacuum and resuspended each in 5 [L ddH 2 0. 4.0 pL pNOV2117 (KpnI/CIP) was ligated to 4.0 pL pRabl7-T6PP-RNAi (KpnI) in a 0 10 pL reaction containing 1 pL 10X T4 DNA ligase buffer and 1 pL T4 DNA ligase (400 U/tL) and incubated more than 8 hours at 16oC. 5.0 pL of ligation mix was transformed into 50 ptL Top10 competent cells. pNOV2117-pRabl7-T6PP-RNAi recombinants were identified by digesting 7.5 pL pNOV2117-pRabl7-T6PP-RNAi miniprep DNA with 1.0 p.L KpnI in 10 pL reactions containing 1 tg BSA and 1 pL 10X restriction endonuclease buffer 1. The .5 reactions were incubated at 37 0 C for 2 hours and then pNOV2117-pRabl7-T6PP-RNAi (KpnI) DNA products were resolved on 1% TAE agarose. The pNOV2117-pRabl7-T6PP RNAi junction sequence was verified and it was designated as pNOV3240. Its map is shown in Fig. 1 B. 20 Example 6: Maize Transformation Numerous transformation vectors available for plant transformation are known to those of ordinary skill in the plant transformation arts, and the genes pertinent to this invention can be used in conjunction with any such vectors. The selection of vector depends upon the preferred transformation technique and the target species for transformation. For 25 certain target species, different antibiotic or herbicide selection markers are preferred. Selection markers used routinely in transformation include the nptII gene, which confers resistance to kanamycin and related antibiotics (Vieira and Messing, 1982; Bevan et al., 1983), the bar gene, which confers resistance to the herbicide phosphinothricin (White et al., 1990; Spencer et al., 1990), the hph gene, which confers resistance to the antibiotic 30 hygromycin (Blochlinger and Diggelmann, 1984), the manA gene, which allows for positive selection in the presence of mannose (Miles and Guest, 1984; Bojsen et al., 1998), and the Page 25 WO 2006/060376 PCT/US2005/043097 dhfr gene, which confers resistance to methotrexate (Bourouis and Bruno,1983), and the EPSPS gene, which confers resistance to glyphosate (Shah et al., 1990; 1993). Many vectors are available for transformation using Agrobacterium tumefaciens. These typically carry at least one T-DNA border sequence and include vectors such as 5 pBIN19 (Bevan, 1984). Typical vectors suitable for Agrobacterium transformation include the binary vectors pCIB200 and pCIB2001, as well as the binary vector pCIBO10 and hygromycin selection derivatives thereof. (See, for example, Ligon et al., 1997). Other vectors are available for non-Agrobacterium tumefaciens transformation. Transformation without the use of Agrobacterium tumefaciens circumvents the requirement for T-DNA 0 sequences in the chosen transformation vector and consequently vectors lacking these sequences are utilized in addition to vectors such as the ones described above which contain T-DNA sequences. Transformation techniques that do not rely on Agrobacterium include transformation via particle bombardment, protoplast uptake (e.g. PEG and electroporation) and microinjection. The choice of vector depends largely on the preferred selection for the 5 species being transformed. Typical vectors suitable for non-Agrobacterium transformation include pCIB3064, pSOGl9, and pSOG35. (See, for example, Ligon et al., 1997). Once the DNA sequence of interest is cloned into an expression system, it is transformed into a plant cell. Methods for transformation and regeneration of plants are well known in the art. For example, Ti plasmid vectors have been utilized for the delivery of 0 foreign DNA, as well as direct DNA uptake, liposomes, electroporation, microinjection, and microprojectiles. In addition, bacteria from the genus Agrobacterium can be utilized to transform plant cells. Transformation techniques for dicotyledons are well known in the art and include Agrobacterium-based techniques and techniques that do not require Agrobacterium. Non 5 Agrobacterium techniques involve the uptake of exogenous genetic material directly by protoplasts or cells. This is accomplished by PEG- or electroporation-mediated uptake, particle bombardment-mediated delivery, or microinjection. In each case the transformed cells are regenerated to whole plants using standard techniques known in the art. Transformation of most monocotyledon species has now also become routine. 0 Preferred techniques include direct gene transfer into protoplasts using PEG or electroporation techniques, particle bombardment into callus tissue, as well as Agrobacterium-mediated transformation. Page 26 WO 2006/060376 PCT/US2005/043097 Plants from transformation events are grown, propagated and bred to yield progeny with the desired trait, and seeds are obtained with the desired trait, using processes well known in the art Once a nucleic acid sequence of the invention has been cloned into an expression 5 system, it is transformed into a plant cell. The receptor and target expression cassettes of the present invention can be introduced into the plant cell in a number of art-recognized ways. Methods for regeneration of plants are also well known in the art. For example, Ti plasmid vectors have been utilized for the delivery of foreign DNA, as well as direct DNA uptake via electroporation, microinjection, and microprojectiles. In addition, bacteria from the genus 0 Agrobacterium can be utilized to transform plant cells. Below are descriptions of representative techniques for transforming both dicotyledonous and monocotyledonous plants, as well as a representative plastid transformation technique. Transformation techniques for dicotyledons are well known in the art and include Agrobacterium-based techniques and techniques that do not require Agrobacterium. Non 5 Agrobacterium techniques involve the uptake of exogenous genetic material directly by protoplasts or cells. This can be accomplished by PEG- or electroporation-mediated uptake, particle bombardment-mediated delivery, or microinjection. Examples of these techniques are described (Paszkowski et al., 1984; Potrykus et al., 1985; Reich et al., 1986; Klein et al., 1987). In each case the transformed cells are regenerated to whole plants using standard .0 techniques known in the art. Agrobacterium-mediated transformation is a preferred technique for transformation of dicotyledons because of its high efficiency of transformation and its broad utility with many different species. Agrobacterium transformation typically involves the transfer of the binary vector carrying the foreign DNA of interest (e.g. pCIB200 or pCIB2001) to an appropriate 15 Agrobacterium strain. This may depend on the complement of Vir genes carried by the host Agrobacterium strain either on a co-resident Ti plasmid or on the chromosome (e.g. strain CIB542 for pCIB200 and pCIB2001 (Uknes et al., 1993)). The transfer of the recombinant binary vector to Agrobacterium is accomplished by a triparental mating procedure using E. coli carrying the recombinant binary vector, a helper E. coli strain which carries a plasmid 30 such as pRK2013 and which is able to mobilize the recombinant binary vector to the target Agrobacterium strain. Alternatively, the recombinant binary vector can be transferred to Agrobacterium by DNA transformation (H6fgen and Willmitzer, 1988). Page 27 WO 2006/060376 PCT/US2005/043097 Transformation of the target plant species by recombinant Agrobacterium usually involves co-cultivation of the Agrobacterium with explants from the plant to be transformed and follows protocols well known in the art. Transformed tissue is regenerated on selection medium containing the antibiotic, herbicide or other compound that the selectable marker, 5 present between the binary plasmid T-DNA borders, is designed to provide resistance. Another approach to transforming plant cells with a gene involves propelling inert or biologically active particles at plant tissues and cells. This technique is disclosed in Sanford et al. (1990; 1991; 1992). Generally, this procedure involves propelling inert or biologically active particles at the cells under conditions effective to penetrate the outer surface of the cell 10 and afford incorporation within the interior thereof. When inert particles are utilized, the vector can be introduced into the cell by coating the particles with the vector containing the desired gene. Alternatively, the target cell can be surrounded by the vector so that the vector is carried into the cell by the wake of the particle. Biologically active particles (e.g., dried yeast cells, dried bacterium or a bacteriophage, each containing DNA sought to be 15 introduced) can also be propelled into plant cell tissue. Transformation of most monocotyledon species has now also become routine. Preferred techniques include direct gene transfer into protoplasts using PEG or electroporation techniques, and particle bombardment into callus tissue. Transformations can be undertaken with a single DNA species or multiple DNA species (i.e. co-transformation) 20 and both these techniques are suitable for use with this invention. Co-transformation may have the advantage of avoiding complete vector construction and of generating transgenic plants with unlinked loci for the gene of interest and the selectable marker, enabling the removal of the selectable marker in subsequent generations, should this be regarded desirable. However, a disadvantage of the use of co-transformation is the less than 100% frequency 25 with which separate DNA species are integrated into the genome (Schocher et al., 1986). Several U.S. Patents describe techniques for the preparation of callus and protoplasts from an elite inbred line of maize, transformation of protoplasts using PEG or electroporation, and the regeneration of maize plants from transformed protoplasts (Tomes et al., 1999; Dudits et al., 2001; Koziel et al., 2002). Gordon-Kamm et al. (1990) and Fromm et 30 al. (1990) have published techniques for transformation of A188-derived maize lines using particle bombardment. Furthermore, Koziel et al. (1993, 2002) describe techniques for the transformation of elite inbred lines of maize by particle bombardment. This technique utilizes Page 28 WO 2006/060376 PCT/US2005/043097 immature maize embryos of 1.5-2.5 mm length excised from a maize ear 14-15 days after pollination and a PDS-1000He Biolistics device for bombardment. Transformation of rice can also be undertaken by direct gene transfer techniques utilizing protoplasts or particle bombardment. Protoplast-mediated transformation has been 5 described for Japonica-types and Indica-types (Zhang et al., 1988; Shimamoto et al., 1989; Datta et al., 1990). Both types are also routinely transformable using particle bombardment (Christou et al., 1991). Furthermore, Gobel and Nakakido (1993) describe techniques for the transformation of rice via electroporation. Horn et al. (1989) describe techniques for the generation, transformation and 0 regeneration of Pooideae protoplasts. These techniques allow the transformation of Dactylis and wheat. Furthermore, wheat transformation has been described by Vasil et al. (1992) using particle bombardment into cells of type C long-term regenerable callus, and also by Vasil et al. (1993) and Weeks et al. (1993) using particle bombardment of immature embryos and immature embryo-derived callus. A preferred technique for wheat transformation, however, 5 involves the transformation of wheat by particle bombardment of immature embryos and includes either a high sucrose or a high maltose step prior to gene delivery. Prior to bombardment, 0.75-1.0 millimeter embryos are plated onto MS medium with 3% sucrose (Murashige and Skoog, 1962) and 3 mg/L 2,4-D for induction of somatic embryos, which proceeds in the dark. On the chosen day of bombardment, embryos are removed from the :0 induction medium and placed onto the osmoticum (induction medium with sucrose or maltose added at the desired concentration, typically 15%). Embryos plasmolyze for 2-3 hours, then they are bombarded. Although not critical, each target plate usually contains twenty embryos. An appropriate gene-carrying plasmid (such as pCIB3064 or pSG35) is precipitated '5 onto micrometer size gold particles using standard procedures. Each plate of embryos is shot with the DuPont Biolistics® helium device using a burst pressure of ~1000 psi using a standard 80 mesh screen. After bombardment, the embryos (still on osmoticum) are placed back into the dark to recover for about 24 hours. Then embryos are removed from the osmoticum and placed back onto induction medium where they stay for about a month before 0 regeneration. Embryo explants with developing embryogenic callus are then transferred to regeneration medium (MS + 1 mg/L NAA, 5 mg/L GA), and further containing the appropriate selection agent (10 mg/L basta in the case of pCIB3064 and 2 mg/L methotrexate in the case of pSOG35). After approximately one month, developed shoots are transferred to Page 29 WO 2006/060376 PCT/US2005/043097 larger sterile containers known as "GA7s" which contain half-strength MS, 2% sucrose, and the same concentration of selection agent. Transformation of monocotyledons using Agrobacterium has also been described (See, Hiei and Komari, 1994; 1997; and Negrotto et al., 2000) incorporated herein by 5 reference. The plasmid, pNOV3240, was introduced in Agrobacterium tumefaciens using electroporation. Transformed Agrobacterium cells were used to transfer the Rabl7-T6PP RNAi expression cassette into the maize (Al 88xHiII) genome. The T-DNA enables positive identification of transformants via regeneration on media containing mannose. Sixty-three 10 events were generated. Of these, Taqman analysis identified 15 events with a single copy of the transgene and no beyond border sequence. When possible, TO plants were self-pollinated; otherwise they were pollinated with JHAFO31. Example 7: Greenhouse Growth Conditions 15 Corn seed is sown into 2.5 SVD pots (Classic 600, ~ 2 gallon nursery containers) in Universal mix (Sungrow Horticulture, Pine Bluff, AR). Universal mix is 45% Peat moss, 45% bark , 5% perlite, 5% vermiculite. Environmental conditions for greenhouse maize cultivation is typically 16 hour days (average light intensity 600 imol m-2s- 2 ), day time temperature of 80-86 0 F, night time temperature 70-76 0 F and relative humidity greater than 20 50%. Plants are placed on 2" platforms to avoid contact with the greenhouse floor. Plants are hand watered until daily irrigation is required, then they are placed on irrigation drip. The irrigation schedule is 4 minutes every other day. Plants were routinely treated with insecticides to control pests. 25 Example 8: Evaluation of Transgenic Maize Expressing Rabl7-T6PP-RNAi in the Greenhouse The greenhouse evaluation is a controlled water-stress experiment that quantifies ovule viability in water-stressed and unstressed plants. Data from unstressed plants represent the genotype's potential to set seed under ideal conditions. Data from water-stressed plants 30 quantify kernel abortion that results from drought at the time of flowering. The results of these experiments can be predictive of field performance. We used this tool to select transgenic events for field evaluations. Page 30 WO 2006/060376 PCT/US2005/043097 Seed from selfed plants were sown as above. Taqman analysis was used to divide the progeny hemizygous (containing Rabl7-T6PP-RNAi) and azygous (lost the Rabl7-T6PP RNAi) groups. Seedlings were transferred to 600 pots, above, and maintained using standard greenhouse procedures until they reached the V6 growth stage (Ritchie et al., 1997). All 5 plants were treated with the systemic pesticide, Marathon, to reduce susceptibility to pests. Water stress was gradually imposed, using salt as the osmoticum (Nuccio et al. 1998). The salt consisted of sodium chloride/calcium chloride at a 10:1 molar ratio, delivered in 0.5X Hoagland's Solution, to prevent sodium-induced disruption of potassium uptake. Salt concentration in the irrigant was increased from 50 mM to 100 mM to 150 mM every three 10 days to give plants time to adjust to the salt. Plants were maintained on 150 mM salt solution through the flowering period, typically two weeks, after which pots were thoroughly flushed with water and plants were returned to normal irrigation. This protocol typically reduced kernel set by 40-60%, compared to control plants that received no salt. Each plant's ability to adjust to the imposed water stress was measured by sampling .5 the first fully expanded leaf, at its mid-point, for solute potential. Three 3/4 inch circular leaf punches were collected and analyzed for leaf-sap solute potential using a dewpoint vapor pressure osmometer. Plants were sampled three days after the 150 mM salt treatment between 10:00-11:00 AM. The leaf sap solute potentials were compared to soil solute potentials to determine how well the plant adjusted to the water stress. Typically plants did not differ in 0 their adjustment to the imposed water stress. Typically 15-20 seed per transgenic event were sown to give 7-10 individual azygotes and 7-10 individual hemizygotes. Plants were arranged in a complete, randomized block design consisting of three replicates per treatment. Developing ears were covered with pollination bags before silk emergence. Pollen shed and silk emergence dates were recorded '5 and individual ears were hand pollinated 2-3 times with donor pollen on successive days. Pollination bags were removed after completing all pollinations. Ears were harvested 30 days after pollinations, and dried for 4 days to 15% moisture content. Ears were shelled and the kernels were counted and weighed. 0 Example 9: Greenhouse Experiment 1 Eight Rabl7-T6PP-RNAi events were studied for their ability to set seed under water stress. Twenty-four T1 seed from each event (a selfed TO parent) were germinated. Taqman analysis was used to establish zygosity in each seedling. Homozygotes were set aside for seed Page 31 WO 2006/060376 PCT/US2005/043097 bulking. Hemizygotes and azygotes were analyzed using the greenhouse water stress protocol, above (Example 8). In this experiment non-transformed A188 plants served as the benchmark. The kernel set data, summarized in Figure 12, show that each event is unique. The water stress protocol was somewhat severe in that the benchmark A188 plants suffered 5 more than 70% reduction in kernel set. In general the presence of the transgene improves kernel set in water stressed plants, the average improvement across all transgenic events was 39%. In particular, in Event 81A10B, hemizygotes had more than double the kernel set of corresponding azygotes. Also, water-stressed hemizygotes from Event 78A18B set six times more kernels than azygotes. The data indicate the Rabl7-T6PP-RNAi expression cassette 0 improves kernel set in maize. Example 10: Greenhouse Experiment 2 Two Rabl7-T6PP-RNAi events, 78A18B(13) and 81AlOB(10) were studied for their ability to set seed under water stress. Ninety-six T2 seed from each event (a selfed Tl parent) 5 were germinated. Taqman analysis was used to establish zygosity in each seedling. Hemizygotes and azygotes were analyzed using the greenhouse water stress protocol, above (Example 8). In this experiment 81A10lB(10) azygotes served as the benchmark. The water stress protocol was effective in that the benchmark 81AlOB(10) azygotes suffered about a 45% reduction in kernel set. In general the presence of the transgene may reduce kernel set in 10 well-watered plants. However, the transgene either has little effect on, or slightly improves kernel set in water-stressed plants. Example 11: Evaluation of Transgenic Maize Expressing Rabl7-T6PP-RNAi in the Field The field evaluations were conducted to test transgene performance under conditions 25 typically used by growers. The general field criteria were four-row plots, 17.5 feet long separated by 2-3 foot alleys with about 40 plants per row. The outer rows were planted with azygotes and the inner rows were planted with segregating transgenics. The field was divided into a well-watered treatment block and a water-stressed treatment block, and drip irrigation was used to water the fields. Each block had a dedicated irrigation manifold. To maintain 30 uniformity the most remote plot was less than 100 feet from the irrigation manifold. There were 3 plots per Event per treatment (a total of six per Event). Event plots were planted at a different distance from the irrigation manifold in a randomized complete block design. Well watered and water-stress treatment blocks were separated by 16 rows (50 ft). Page 32 WO 2006/060376 PCT/US2005/043097 T1 homozygous seed from Event 78A18B and Event 81AO10B were back-crossed twice with JHAF031, and the 1:1 segregating seed were planted in the summer of 2003 in Hawaii. The planting site has well drained sandy soil and typically gets less than 3" of rainfall during the summer. Taqman analysis of seedlings was performed to establish the 5 presence of the transgene. In this way, azygotes and hemizygotes were randomly dispersed in each plot. The well-watered block was irrigated optimally throughout the experiment. The water-stress block was watered optimally until plants reached approximately V6, at which time water was withheld. Plants were returned to optimal irrigation after 90% silk emergence. 10 The amount of water applied to the field and rainfall were recorded. After plants transitioned to reproductive development, pollen shed and silk emergence dates were recorded for each plant. Plant response to water deficit was also recorded by monitoring appearance of physiological stress symptoms such as leaf greying and curling, and sampling leaf tissue to measure solute potential. Each plant's ability to adjust to the imposed water .5 stress was measured by sampling the first fully expanded leaf, at its mid-point, for solute potential. Three 3/4 inch circular leaf punches were collected and analyzed for leaf-sap solute potential using a dewpoint vapor pressure osmometer. Plants in the water-stressed block were sampled during the period of maximum stress. Plants in the well-watered block were sampled a few days after the water-stressed block. Sampling took place between 8:00-10:00 AM. The 0 leaf sap solute potentials for plants within each plot were compared to establish field uniformity. Ears from each plant were harvested and shelled. Kernels were counted and weighed. The data from hemizygous individuals were compared to azygous individuals to gauge the transgene's effect on kernel set. Results for the two Rabl7-T6PP-RNAi events are 5 summarized in Figures 14 and 15. On average, the water-stress reduced kernel set in azygous A78A18B (Fig. 14) individuals by 47 %, whereas the hemizygous individuals suffered only a 30% yield reduction under the same conditions. Figure 15 shows the A81A10lB hemizygous individuals suffered a slightly greater drought-induced yield reduction than the corresponding azygotes (30% vs. 25%, respectively). However, this yield reduction is significantly offset by 0 the more than 10% yield enhancement afforded by the transgene. Results from this field experiment demonstrate the effectiveness of the Rabl7-T6PP-RNAi transgene in stabilizing kernel set in drought stressed maize. Page 33 WO 2006/060376 PCT/US2005/043097 Example 12: Application of the Rabl7-T6PP-RNAi to other plant species The gene silencing activity of a double-stranded RNA is sequence specific. Studies in plant, insect, nematode, mammalian and other eukaryotic systems indicate that a homologous 21-23 base sequence is sufficient to cause gene silencing (Waterhouse and Helliwell, 2003; 5 McManus and Sharp, 2002). The length requirement of 21 bases is a lower limit and there is evidence that mismatches can be tolerated (McManus and Sharp, 2002). With this in mind, it's clear that more effective RNA-mediated gene silencing is achieved with longer templates (Thomas et al., 2001). Furthermore gene regulatory sequence does function in a predictable way across species boundaries (See, for example, Nuccio and Thomas, 2000). 0 The transgenic constructs of the present invention can be used to reduce expression of T6PP in other plants species. Cross-species efficacy was established by querying public and proprietary cDNA databases to identify T6PP encoding sequences in other plant species. The "hits" were aligned and used to generate contigs as described in Fig. 2. T6PP homologues from sorghum, barley, wheat, sugar cane and rye were identified. The sequence fragments .5 from each gene corresponding to the T6PP-RNAi fragment were compared by alignment (Fig. 16) and similarity (Fig. 17). For comparison ZmT6PP-1 amino acids 334-393, in Fig. 3, are encoded by nucleotides 1-180 of the ZmT6PP-1 cDNA shown in Fig. 16. The results demonstrate there the transgenic construct of the present invention will function to silence T6PP in other crop species. This shows the construct can be used to 20 improve environmental stress tolerance in not only maize, but also other important cereal crops. Page 34 WO 2006/060376 PCT/US2005/043097 References Aeschbacher, R.A., MUiller, J., Boller, T., Wiemken, A. (1999). Purification of the trehalase GMTRE1 from Soybean nodules and cloning of its cDNA. GMTRE1 is expressed at a low 5 level in multiple tissues. Plant Physiol. 119, 489-495. Atkins, D., Young, M., Uzzell, S., Kelly, L., Fillatti, J., Gerlach, W.L. (1995). 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Plant Physiol. 121, 25-25. 5 Page 45

Claims (1)

100-1649 contiguous nucleotides of DNA, wherein said contiguous nucleotides of DNA have from 85% to 100% identity to about 100 to 1649 contiguous nucleotides of DNA having the sequence of SEQ ID NO. 42. 12) The DNA molecule according to claim 1, wherein said nucleic acid is capable of 0 forming into a double stranded RNA. 13) The polynucleotide according to claim 1, wherein said nucleic acid comprises co suppressor RNA. 14) The DNA molecule according to claim 1, wherein said nucleic acid comprises catalytic RNA. Page 46 WO 2006/060376 PCT/US2005/043097 15) The DNA molecule according to claim 1, wherein said nucleic acid is capable of forming into a triplex nucleic acid. 16) The DNA molecule according to claim 1 wherein said promoter is also expressed in seed tissue. 5 17) A plant cell comprising the DNA molecule according to claim 1. 18) A transgenic plant, or a part thereof, comprising the plant cell according to claim 17. 19) The plant cell according to claim 17, wherein said nucleotide sequence of claim 1 comprises at least about 21 consecutive base pairs of SEQ ID NO. 6. 20) The transgenic plant, or part thereof, according to claim 18, wherein said 0 polynucleotide of claim 1 comprises at least about 21 consecutive base pairs of SEQ IDNO. 6. 21) The transgenic plant according to claim 1, wherein said plant is a monocot plant. 22) The transgenic plant according to claim 1, wherein said plant is a barley, rice, maize, wheat, sorghum, sugar cane or rye. 5 23) The transgenic plant according to claim 1, wherein said plant is a maize plant. 24) The DNA molecule according to claim 1, wherein said nucleic acid is expressed in seed tissue. 25) The DNA molecule according to claim 1, wherein said DNA molecule is depicted by SEQ ID NO. 8 or SEQ. ID. NO. 18. 10 26) The DNA molecule according to claim 1, wherein said promoter is also developmentally expressed in kernels of said transgenic plant. 27) An isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue and encoding a TPP protein or antibody capable of down-regulating 25 a TPP gene. 28) The isolated DNA molecule according to claim 27, wherein said promoter is expressed in seed tissue. 29) An isolated DNA molecule comprising a polynucleotide encoding an RNAi, said polynucleotide is operatively linked to a promoter that is drought induced in 30 vegetative tissue, wherein when said RNAi is capable of down-regulating the expression of a T6PP gene. 30) The DNA molecule according to claim 29, wherein said polynucleotide is depicted by SEQ ID. NO 6. Page 47 WO 2006/060376 PCT/US2005/043097 31) The DNA molecule according to claim 30, wherein said polynucleotide comprises at least about 21 consecutive base pairs of SEQ ID NO. 6. 32) The DNA molecule according to claim 31, wherein said polynucleotide is a complement to said 21 consecutive base pairs. 5 33) The DNA molecule according to claim 29, wherein said promoter is derived from the 5' region of a Rab 17 gene and exhibits promoter activity in plants. 34) The DNA molecule according to claim 29, wherein said DNA molecule comprises a 3' region derived from a Rabl7 gene and exhibits terminator activity in plants. 35) The DNA molecule according to claim 29, wherein said promoter comprises about 0 100-1649 contiguous nucleotides of DNA, wherein said contiguous nucleotides of DNA have from 85% to 100% identity to about 100 to 1649 contiguous nucleotides of DNA having the sequence of SEQ ID NO. 42. 36) A plant cell comprising the DNA molecule according to claim 29. 37) A transgenic plant, or a part thereof, comprising the plant cell according to claim 36. 5 38) The plant cell according to claim 36, wherein said polynucleotide of claim 29 comprises at least about 21 consecutive base pairs of SEQ ID NO. 1. 39) The transgenic plant, or part thereof, according to claim 37, wherein said polynucleotide of claim 29 comprises at least about 21 consecutive base pairs of SEQ IDNO. 6. Z0 40) The transgenic plant according to claim 39, wherein said plant is a monocot plant. 41) The transgenic plant according to claim 39, wherein said plant is a barley, rice, maize, wheat, sorghum, sugar cane or rye. 42) The DNA molecule according to claim 29, wherein said DNA molecule is depicted by SEQ ID NO. 8 or SEQ. ID. NO. 18. 25 43) A method of increasing the starch content in the kernel of a plant comprising the steps of: a) transforming a plant cell with said DNA molecule of claim 1; b) generating a plant from said plant cell; c) inducing expression of said nucleic acid sequence of claim 1 in the vegetative 30 tissue of said plant when said plant is subjected to drought conditions during its reproductive stage; and Page 48 WO 2006/060376 PCT/US2005/043097 d) increasing starch content in the kernel compared to the starch content in the kernel of an isogenic plant not containing said DNA molecule when said transgenic plant and said isogenic plant are grown under substantially the same drought conditions. 44) The method for increasing the starch content in the kernel of a plant according to 5 claim 43, wherein said promoter is endogenous to said plant species. 45) The method for increasing the starch content in the kernel of a plant according to claim 43, wherein said promoter comprises the 5'non-coding regulatory region of a Rabl 17 gene. 46) The method for increasing the starch content in the kernel of a plant according to 10 claim 45, wherein said nucleic acid sequence further comprises the 3'-terminator non coding region of a Rab 17 gene. 47) A transgenic plant prepared by the method of claim 43. 48) Transgenic seeds derived from the plant of claim 47. 49) A double stranded short interfering nucleic acid (siRNA) molecule that down 15 regulates expression of a T6PP gene in the vegetative tissue of a plant, wherein said siRNA molecule comprises at least about 21 base pairs. 50) The siRNA molecule of claim 49, wherein one of the strands of said double stranded siRNA molecule comprises a nucleotide sequence substantially similar to the nucleotide sequence of a T6PP gene or a portion thereof and, wherein the second 20 strand of said double-stranded siRNA molecule comprises a nucleotide sequence that is complementary to a nucleotide sequence of said first strand. 51) The siRNA molecule of claim 49, wherein said siRNA molecule is encoded by at least about 21 consecutive base pairs of SEQ ID NO. 6. 52) The siNA molecule of claim 49, wherein said siNA molecule comprises 25 ribonucleotides. 53) An isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is drought induced in vegetative tissue, wherein said nucleic acid is capable of down-regulating a T6PP gene. Page 49 WO 2006/060376 PCT/US2005/043097 54) The DNA molecule according to claim 53, wherein said polynucleotide is depicted by SEQ ID. NO 6. 55) The DNA molecule according to claim 53, wherein said polynucleotide comprises at least about 21 consecutive base pairs of SEQ ID NO. 6. 5 56) The DNA molecule according to claim 53, wherein said polynucleotide is placed in a sense orientation relative to said promoter. 57) The DNA molecule according to claim 53, wherein said polynucleotide is placed in an antisense orientation relative to said promoter. 58) The DNA molecule according to claim 53, wherein said polynucleotide is a 10 complement to said 21 consecutive base pairs. 59) The DNA molecule according to claim 53, wherein said polynucleotide is placed in a sense orientation relative to said promoter. 60) The DNA molecule according to claim 53, wherein said polynucleotide is placed in an antisense orientation relative to said promoter. 15 61) The DNA molecule according to claim 53, wherein said promoter is derived from the 5' region of a Rabl7 gene and exhibits promoter activity in plants. 62) The DNA molecule according to claim 53, wherein said DNA molecule further comprises a 3' region derived from a Rabl7 gene and exhibits terminator activity in plants. 20 63) The DNA molecule according to claim 53, wherein said promoter comprises about 100-1649 contiguous nucleotides of DNA, wherein said contiguous nucleotides of DNA have from 85% to 100% identity to about 100 to 1649 contiguous nucleotides of DNA having the sequence of SEQ ID NO. 42. 64) The DNA molecule according to claim 53, wherein said nucleic acid is capable of 25 forming into a double stranded RNA. 65) The DNA molecule according to claim 53, wherein said polynucleotide comprises co suppressor RNA. 66) The DNA molecule according to claim 53, wherein said polynucleotide comprises catalytic RNA. 30 67) The DNA molecule according to claim 53, wherein said polynucleotide is capable of forming into a triplex nucleic acid. 68) The DNA molecule according to claim 53 wherein said promoter is also expressed in seed tissue. Page 50 WO 2006/060376 PCT/US2005/043097 69) A plant cell comprising the DNA molecule according to claim 53. 70) A transgenic plant, or a part thereof, comprising the plant cell according to claim 69. 71) The plant cell according to claim 69, wherein said polynucleotide of claim 53 comprises at least about 21 consecutive base pairs of SEQ ID NO. 6. 5 72) The transgenic plant, or part thereof, according to claim 70, wherein said polynucleotide of claim 53 comprises at least about 21 consecutive base pairs of SEQ IDNO. 6. 73) The transgenic plant according to claim 70, wherein said plant is a monocot plant. 74) The transgenic plant according to claim 70, wherein said plant is a barley, rice, maize, 10 wheat, sorghum, sugar cane or rye. 75) The transgenic plant according to' claim 70, wherein said plant is a maize plant. 76) The DNA molecule according to claim 53, wherein said nucleic acid is expressed in seed tissue. 77) The DNA molecule according to claim 53, wherein said DNA molecule is depicted by 15 SEQ ID NO. 8 or SEQ. ID. NO. 18. 78) A method of increasing the starch content in the kernel of a plant comprising the steps of: a) obtaining a plant comprising the DNA molecule of claim 1; b) growing said plant under drought conditions; 20 c) inducing expression of said nucleic acid sequence of claim 1 in the vegetative tissue of said plant when said plant is subjected to drought conditions during its reproductive stage; and d) increasing starch content in the kernel of said plant compared to the starch content in the kernel of an isogenic plant not containing said DNA molecule when said plant 25 and said isogenic plant are grown under substantially the same drought conditions. 79) An isolated DNA molecule comprising a polynucleotide encoding a nucleic acid, said polynucleotide is operatively linked to a promoter that is stress inducible in vegetative tissue of a plant and developmentally expressed in kernels of said plant, wherein said nucleic acid is capable of down-regulating a T6PP gene. 30 Page 51