Multicellular living organisms and unmodified parts thereof and – Plant – seedling – plant seed – or plant part – per se – Higher plant – seedling – plant seed – or plant part
Reexamination Certificate
1992-12-07
2002-02-19
Nelson, Amy J. (Department: 1638)
Multicellular living organisms and unmodified parts thereof and
Plant, seedling, plant seed, or plant part, per se
Higher plant, seedling, plant seed, or plant part
C435S320100, C435S419000, C536S023200, C536S023600
Reexamination Certificate
active
06348642
ABSTRACT:
FIELD OF INVENTION
The present invention is directed to synthase enzymes relevant to fatty acid synthesis in plants, protein preparations, amino acid and nucleic acid sequences related thereto, and methods of use for such compositions.
INTRODUCTION
BACKGROUND
Plant oils are used in a variety of industrial and edible uses. Novel vegetable oils compositions and/or improved means to obtain oils compositions, from biosynthetic or natural plant sources, are needed. Depending upon the intended oil use, various different fatty acid compositions are desired.
For example, in some instances having an oilseed with a higher ratio of oil to seed meal would be useful to obtain a desired oil at lower cost. This would be typical of a high value oil product. In some instances, having an oilseed with a lower ratio of oil to seed meal would be useful to lower caloric content. In other uses, edible plant oils with a higher percentage of unsaturated fatty acids are desired for cardiovascular health reasons. And alternatively, temperate substitutes for high saturate tropical oils such as palm and coconut, would also find uses in a variety of industrial and food applications.
One means postulated to obtain such oils and/or modified fatty acid compositions is through the genetic engineering of plants. However, in order to genetically engineer plants one must have in place the means to transfer genetic material to the plant in a stable and heritable manner. Additionally, one must have nucleic acid sequences capable of producing the desired phenotypic result, regulatory regions capable of directing the correct application of such sequences, and the like. Moreover, it should be appreciated that in order to produce a desired phenotype requires that the Fatty Acid Synthetase (FAS) pathway of the plant is modified to the extent that the ratios of reactants are modulated or changed.
Higher plants appear to synthesize fatty acids via a common metabolic pathway. In developing seeds, where fatty acids attached to triglycerides are stored as a source of energy for further germination, the FAS pathway is located in the proplastids. The first step is the formation of acetyl-ACP (acyl carrier protein) from acety-CoA and ACP catalyzed by the enzyme, acetyl-CoA:ACP transacylase (ATA). Elongation of acetyl-ACP to 16- and 18- carbon fatty acids involves the cyclical action of the following sequence of reactions: condensation with a two-carbon unit from malonyl-ACP to form a &bgr;-ketoacyl-ACP (&bgr;-ketoayl-ACP synthase), reduction of the keto-function to an alcohol (&bgr;-keyoayl-ACP reductase), dehydration to form an enoyl-ACP (&bgr;-hydroxyacyl-ACP dehydrase), and finally reduction of the enoyl-ACP to form the elongated saturated acyl-ACP (enoyl-ACP reductase). &bgr;-ketoacyl-ACP synthase I, catalyzes elongation up to palmitoyl-ACP (C16:0), whereas &bgr;-ketoacyl-ACP synthase II catalyzes the final elongation to stearoyl-ACP (C18:0). Common plant unsaturated fatty acids, such as oleic, linoleic and &agr;-linolenic acids found in storage triglycerides, originate from the desaturation of stearoyl-ACP to form oleoyl-ACP (C18:1) in a reaction catalyzed by a soluble plastid &Dgr;-9 desaturase (also often referred to as “stearoyl-ACP desaturase”). Molecular oxygen is required for desaturation in which reduced ferredoxin serves as an electron co-donor. Additional desaturation is effected sequentially by the actions of membrane bound &Dgr;-12 desaturase and &Dgr;-15 desaturase. These “desaturases” thus create mono- or polyunsaturated fatty acids respectively.
A third &bgr;-keyoayl-ACP synthase has been reported in
S. oleracea
leaves having activity specific toward very short acyl-ACPs. This acetoacyl-ACP synthase or “&bgr;-ketoacyl-ACP” synthase III has a preference to acetyl-CoA over acetyl-ACP, Jaworski, J. G., et al.,
Plant Phys.
(1989) 90:41-44. It has been postulated that this enzyme may be an alternate pathway to begin FAS, instead of ATA.
Obtaining nucleic acid sequences capable of producing a phenotypic result in FAS, desaturation and/or incorporation of fatty acids into a glycerol backbone to produce an oil is subject to various obstacles including but not limited to the identification of metabolic factors of interest, choice and characterization of a protein source with useful kinetic properties, purification of the protein of interest to a level which will allow for its amino acid sequencing, utilizing amino acid sequence data to obtain a nucleic acid sequence capable of use as a probe to retrieve the desired DNA sequence, and the preparation of constructs, transformation and analysis of the resulting plants.
Thus, the identification of enzyme targets and useful plant sources for nucleic acid sequences of such enzyme targets capable of modifying fatty acid compositions are needed. Ideally an enzyme target will be amenable to one or more applications alone or in combination with other nucleic acid sequences, relating to increased/decreased oil production, the ratio of saturated to unsaturated fatty acids in the fatty acid pool, and/or to novel oils compositions as a result of the modifications to the fatty acid pool. Once enzyme target(s) are identified and qualified, quantities of protein and purification protocols are needed for sequencing. Ultimately, useful nucleic acid constructs having the necessary elements to provide a phenotypic modification and plants containing such constructs are needed.
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Bibb et al., “Analysis of the Nucleotide Sequence of theStreptomyces glaucescenstcmI Genes Provides Key Information About the Enzymology of Polyketide Antibiotic Biosynthesis,”EMBO J.(1989) 8:2727-2736.
MacKintosh et al., “A New Assay Procedure to Study the Induction of &bgr;-Ketoacyl-ACP Synthase I and II, and the Complete Purification of &bgr;-Ketoacyl-ACP Synthase I from Developing Seeds of Oilseed Rape (Brassica napus),”Biochem. Biophys. Acta(1989) 1002:114-124.
Siggard-Andersen, “Purification and Characterization of a &bgr;-Ketoacyl-ACP Synthase from Barley Chloroplasts,”The Ninth International Symposium on Plant Lipids(1990) Plant Lipid Biochemistry —Structure, Utilisation and Function, Abstract 53.
Kauppinen, “Molecular Cloning of the Gene(s) Coding for Barley &bgr;-Ketoacyl-ACP Synthase,”The Ninth International Symposium on Plant Lipids(1990) Plant Lipid Biochemistry —Structure, Utilisat
Knauf Vic C.
Thompson Gregory A.
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