Genetic engineering of syringyl-enriched lignin in plants

Details Genetic engineering of syringyl-enriched lignin in plants Genetic engineering of syringyl-enriched lignin in plants

2001-09-05

2004-11-02

Fox, David T. (Department: 1638)

Multicellular living organisms and unmodified parts thereof and

Method of introducing a polynucleotide molecule into or...

C800S287000, C800S298000, C800S319000, C536S023600, C536S024100, C435S069100, C435S468000, C435S419000

Reexamination Certificate

active

06812377

ABSTRACT:

BACKGROUND OF THE INVENTION
The invention relates to a novel DNA sequence, which encodes a previously unidentified lignin biosynthetic pathway enzyme, sinapyl alcohol dehydrogenase (SAD), that regulates the biosynthesis of syringyl lignin in plants. Methods for incorporating this novel SAD gene sequence or sequences similar to this SAD gene into plant genome for genetic engineering of syringyl-enriched lignin in plants are also provided.
Lignin, a complex phenolic polymer, is a major part of the supportive structure of most woody plants including angiosperm and gymnosperm trees which, in turn, are the principal sources of fiber for making paper and cellulosic products. Lignin generally constitutes about 25% of the dry weight of the wood, making it the second most abundant organic compound on earth after cellulose. Lignin provides rigidity to wood for which it is well suited due, in part, to its resistance to biochemical degradation.
Despite its importance to plant growth and structure, lignin is nonetheless problematic to post-harvest, cellulose-based wood/crop processing for fiber, chemical, and energy production because it must be removed or degraded from cellulose at great expense. Certain structural constituents of lignin, such as the guaiacyl moiety, promote monomer cross-linkages that increase lignin resistance to degradation (Sarkanen, 1971; Chang and Sarkanen, 1973; Chiang and Funaoka, 1990). In angiosperms, lignin is composed of a mixture of guaiacyl and syringyl monolignols, and can be degraded at considerably less energy and chemical cost than gymnosperm lignin, which consists almost entirely of guaiacyl moieties (Freudenberg, 1965). It has been estimated that, if syringyl lignin through genetic engineering, could be incorporated into gymnosperm guaiacyl lignin or into angiosperms to increase the syringyl lignin content, the annual saving in processing of such genetically engineered plants as opposed to their wild types would be in the range of $6 to $10 billion in the U.S. alone. Consequently, there has been long-standing incentive to understand the biosynthesis of syringyl monolignol to genetically engineer plants to contain more syringyl lignin, thus, facilitating wood/crop processing (Trotter, 1990; Bugos et al., 1991; Boudet et al., 1995; Hu et al., 1999).
Although it has been known that syringyl lignin is derived from guaiacyl lignin, only a partial syringyl monolignol pathway and its genes encoding the enzymes that catalyze the steps of the pathway have been uncovered. This partial syringyl monolignol pathway, which diverges from guaiacyl pathway at coniferaldehyde, is mediated by genes encoding the enzymes coniferyl aldehyde 5-hydroxylase (CAld5H) (Osakabe et al., 1999) and S-adenosyl-L-methionine (SAM)-dependent 5-hydroxyconiferaldehyde O-methyltransferase (AldOMT) (Li et al., 2000), respectively, for the formation of sinapaldehyde (see, FIG.
1
). However, sinapaldehyde must be enzymatically converted into sinapyl alcohol, the syringyl monolignol, for the biosynthesis of syringyl lignin in plants (see, FIG.
1
). The gene encoding such an enzyme, i.e., a sinapyl alcohol dehydrogenase (SAD), has never been identified nor cloned and represents a missing gene that is indispensable for genetic engineering of syringyl lignin in plants. Thus, there is a need for the identification and isolation of this key gene (SAD) for genetic augmentation of syringyl monolignol biosynthesis in plants and for the methods for such genetic manipulation comprising the use of this key gene.
BRIEF SUMMARY OF THE INVENTION
The present invention provides an isolated complete DNA sequence encoding a novel enzyme, sinapyl alcohol dehydrogenase, SAD, that is obligatory to and plays a dominant role in the biosynthesis of syringyl lignin in plants. SAD catalyzes the conversion of sinapaldehyde to sinapyl alcohol, the syringyl monolignol. The production of SAD, and hence, the production of syringyl monolignol may be increased by supplying extra copies of the SAD gene, or decreased by insertion of the SAD gene or a portion thereof into the genome of a plant, in antisense orientation so that the amount of SAD for catalyzing the sinapyl alcohol is reduced, if so desired.
In one aspect, the invention provides whole gymnosperm plants containing genes which increase production of syringyl lignin and repress production of guaiacyl lignin. Thus the invention addresses the problem of providing gymnosperm species which are easier to delignify in pulping processes.
In another aspect, the invention provides a method for making an expression cassette insertable into a gymnosperm cell for the purpose of inducing formation of syringyl lignin in a gymnosperm plant derived from the cell.
In an additional aspect, the present invention provides a method for modifying genes involved in lignin biosynthesis in gymnosperm species so that production of syringyl lignin is increased while production of guaiacyl lignin is suppressed.
The invention advantageously identifies, isolates, and/or clones those genes in angiosperms responsible for production of syringyl lignin. The invention also advantageously provides for identification and isolation of a polynucleotide encoding a sinapyl alcohol dehydrogenase (SAD) from an angiosperm species and for the use of such polynucleotide to alter the lignin biosynthesis in a gymnosperm.


REFERENCES:
patent: 5451514 (1995-09-01), Boudet et al.
patent: 5633439 (1997-05-01), Walter
patent: 6066780 (2000-05-01), Boudet et al.
patent: 2002/0062496 (2002-05-01), Chapple et al.
patent: 2002/0078474 (2002-06-01), Chiang et al.
patent: 2002/0078477 (2002-06-01), Chiang et al.
patent: 01/27241 (2001-04-01), None
Medina-Escobar et al. (Jan. 29, 1999. NCBI Accession No. U63534).*
Fourgoux-Nicol et al. (1999, Plant Molecular Biology 40: 857-872).*
Bowie et al (1990, Science 247:1306-10).*
McConnell et al (2001, Nature 411) (6838):709-713).*
Lazar et al. (1988, Molecular and Cellular Biology 8:1247-1252).*
Hill et al (1998, Biochem. Biophys. Res. Comm. 244:573-577).*
Hu et al (1999, Nature Biotechnology 17:808-812).*
Kajita et al (1997), Plant Science 128:109-118).*
Piquemal et al (1998, Plant Journal 13(1):71-83).*
Franke et al (2000, Plant Journal 22(3):223-234).*
Bland, D.E., 1966,Holzforschung20:12.
Chandler et al., 1989,The Plant Cell,1:1175.
Chiang, V.L., and Funaoka, M., 1990,Holzforschung44:309.
Corner, E.J.H., 1968,The Life of Plants(New York: New American Library) [Book].
Ebert, et al., 1987,PNAS USA,84:5745.
Fergus, B.J., and Goring, D.A.I., 1970a,Holzforschung24:113.
Fergus, B.J., and Goring, D.A.I., 1970b,Holzforschung24:118.
Frey-Wyssling, A. and Bossard, H.H., 1959 Cytology of ray cells in sapwood and heartwood,Holzforschung13:129-137.
Grand, et al., 1982, Natural variations and controlled in lignification process,Holzforschung36:217-223.
Hahlbrock, K., and Scheel, D., 1989,Plant Mol. Biol.40:347.
Kawamura. I. and Higuchi, T., 1963, Studies on the lignin of young tissues of wood, I. On lignin ofPseudoacacia, J. Jpn. Wood Res. Soc.8:148-153.
Li et al, 2001, The Last Step of Syringyl Monolignol Biosynthesis in Angiosperms is Regulated by a Novel Gene Encoding Sinapyl Alcohol Dehydogenase,The Plant Cell,vol. 13, pp. 1567-1585, Jul. 2001.
MacKay, et al., 1995, Genetic analysis of cinnamyl alcohol dehydrogenase in loblolly pine: Single gene inheritance, molecular characterization and evolution,Mol. Gen. Genet.247:537-545.
Musha, Y. and Goring, D.A.I., 1975, Distribution of syringle and guaiacyl moieties in hardwoods as indicated by ultraviolet microscopy,Wood Sci. Technol.9:45-58.
Napoli et al., 1990,The Plant Cell2:279-289.
Osakabe et al., 1999,Proc. Nat. Acad. Sci. USA96:8955.
Saka, S., and Goring, D.A.I., 1988,Holzforschung42:149.
Sambrook et al., 1982, Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Laboratory, New York.
Sullivan et al., 1989,Mol. Gen. Genet.,215:431.
Terashima et al., 1986,Holzforschung42:101.
van der Krol, A.R., et al., 1988, An anti-sense chalcone cynthase gene in transgenic plants inhibits flower pigmentation,Nature,vol. 333, 866-869.

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