NZ534219A - Method for enhancing cellulose and modifying lignin biosynthesis in plants - Google Patents

Method for enhancing cellulose and modifying lignin biosynthesis in plants

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Publication number
NZ534219A
NZ534219A NZ534219A NZ53421900A NZ534219A NZ 534219 A NZ534219 A NZ 534219A NZ 534219 A NZ534219 A NZ 534219A NZ 53421900 A NZ53421900 A NZ 53421900A NZ 534219 A NZ534219 A NZ 534219A
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New Zealand
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plant
cellulose synthase
cellulose
expression
promoter
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NZ534219A
Inventor
Vincent L Chiang
Daniel T Carraway
Luguang Wu
Chandrashekhar P Joshi
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Univ Michigan Tech
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Priority claimed from NZ515459A external-priority patent/NZ515459A/en
Publication of NZ534219A publication Critical patent/NZ534219A/en

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Abstract

An isolated polynucleotide sequence is described to comprise a cellulose synthase promoter of SEQ ID NO:3, a sequence conservative variant thereof, or a functional fragment thereof which binds to a transcription factor in a plant cell. The polynucleotide is described to be a stress-inducible promoter, to comprise at least one MSRE (mechanical stress regulatory element), which can be a tree. A method of increasing expression of a cellulose synthase in a plant involves delivering into the plant a cDNA encoding a protein; and a method for reducing the expression of a cellulose synthase in a plant comprises delivering into the plant a DNA in an antisense orientation. Methods for increasing or reducing cellulose biosynthesis in a plant are also described.

Description

3 4 2 1 9 NEW ZEALAND PATENTS ACT, 1953 No: Divided out of No. 515459 Date: Dated 18 May 2000 COMPLETE SPECIFICATION METHOD FOR ENHANCING CELLULOSE AND MODIFYING LIGNIN BIOSYNTHESIS IN PLANTS We, BOARD OF CONTROL OF MICHIGAN TECHNOLOGICAL UNIVERSITY, of 1400 Townsend Drive, Houghton, Michigan 49931, United States of America, do hereby declare the invention for which we pray that a patent may be granted to us, and the method by which it is to be performed, to be particularly described in and by the following statement: 1 (followed by page 1 a) INTELLECTUAL PROPERTY OFFICE OF N.Z. 21 JUL 2DM RECEIVED -la- METHOD FOR ENHANCING CELLULOSE AND MODIFYING LIGNIN BIOSYNTHESIS IN PLANTS The reader is directed to our related patent specification NZ 515459.
FIELD OF THE INVENTION This invention relates to polynucleotide molecules encoding cellulose synthase and cellulose synthase polypeptides, methods for genetically altering cellulose and lignin biosynthesis, and methods for improving strength properties of juvenile wood and fiber in trees. Described are polynucleotide molecules encoding promoters of cellulose synthase 10 methods for identifying regulatory elements in a cellulose synthase promoter and transcription factors that bind to such regulatory elements, and to methods for augmenting expression of polynucleotides operably linked to a cellulose synthase promoter.
BACKGROUND OF THE INVENTION Lignin and cellulose are the two major building blocks of plant cell walls 15 that provide mechanical strength and rigidity. In plants, and especially in trees, these two organic materials exist in a dynamic equilibrium conferring mechanical strength, water transporting ability and protection from biotic and abiotic environmental stresses. Normally, oven-diy wood contains 30 to 50% cellulose, 20 to 30% lignin and 20 to 30% hemicellulose (Higuchi, 1997).
Proportions of lignin and cellulose are known to change with variation in the natural environment. For example, during the development of compression wood in conifers, the percentage of lignin increases from 30 to 40 %, and cellulose content proportionally decreases from 40 to 30% (Timmell, 1986). Conversely, in angiosperm tension wood the percentage of cellulose increases from 30 to 40%, while lignin content 25 decreases from 30 to 20% (Timmell, 1986).
It was recently discovered that the genetic down-regulation of a key tissue-specific enzyme from the lignin biosynthesis pathway, 4CL, results in reduction of lignin - SKTRUHTTIIAL PROt-Ei;iY OFFICE OF N.Z. 18 JAN content by up to 45% in transgenic aspen trees (Hu et al, 1999). This down-regulation is also associated with a 15% increase in the cellulose content. If the converse were true, i.e., that increasing cellulose content by genetic up-regulation of cellulose biosynthesis results in reduction of lignin content, then the pulp yield could be increased. This would allow 5 tremendous savings in chemical and energy costs during pulping because, for example, lignin must be degraded and removed during the pulping process.
Cellulose is a linear glucan consisting of p-D-l,4-linked glucose residues. It is formed by a cellulose synthase enzyme which catalyzes assembly of UDP-glucose units in plasma membrane complexes known as "particle rosettes" (Delmer and Amor, 10 1995). Cellulose synthase is thought to be anchored to the membrane by eight transmembrane binding domains to form the basis of the cellulose biosynthesis machinery in the plant cell wall (Pear et al, 1996).
In higher plants, the glucan chains in cellulose microfibrils of primary and secondary cell walls are different in their degree of polymerization (Brown et al., 1996). 15 For example, secondary cell walls are known to contain cellulose having a high degree of polymerization, while in primary cell walls the degree of polymerization is lower. In another example, woody cell walls suffering from tension stress produce tension wood on the upper side of a bent angiosperm tree in response to the stress. In these cells, there are elevated quantities of cellulose which have very high crystallinity. The formation of 20 highly crystalline cellulose is important to obtain a higher tensile strength of the wood fiber. Woody cell walls located at the under side of the same stem experience a compression stress, but do not produce highly crystalline cellulose. Such variation in the degree of polymerization in cell walls during development is believed to be due to different types of cellulose synthases for organizing glucose units into different 25 paracrystalline arrays (Haigler and Blanton, 1996). Therefore, it would be advantageous to determine the molecular basis for the synthesis of highly crystalline cellulose so that higher yields of wood pulp having superior strength properties can be obtained from transgenic trees. Production of highly crystalline cellulose in transgenic trees would also markedly improve the mechanical strength properties of juvenile wood formed in normal 30 trees. This would be a great benefit to the industry because juvenile wood is generally undesirable for solid wood applications because it has inferior mechanical properties.
Since the deposition of cellulose and lignin in trees is regulated in a compensatory fashion, genetic augmentation of cellulose biosynthesis might have a repressive effect on lignin deposition. Since the degree of polymerization and crystallinity 35 may depend upon the type of cellulose synthase incorporated in the cellulose biosynthesis machinery, the expression of heterologous cellulose synthase or a UDP-glucose binding region thereof (e.g., sweetgum protein expression in loblolly pine), could increase the quality of cellulose in transgenic plants. Over-expression of a heterologous cellulose synthase may also increase cellulose quantity in transgenic plants. Thus, genetic engineering of cellulose biosynthesis can provide a strategy to augment cellulose quality and quantity, while reducing lignin content in transgenic plants.
A better understanding of the biochemical processes that lead to wood 5 formation would enable the pulp and paper industries to more effectively use genetic engineering as a tool to meet the increasing demands for wood from a decreasing production area. With this objective, many xylem-specific genes, including most lignin biosynthesis genes, have been isolated from developing xylem tissues of various plants including tree species (Ye and Varner, 1993; Fukuda, 1996; Whetten et al, 1998). Genes 10 regulating cellulose biosynthesis in crop plants (Pear et al, 1996 and Arioli et al, 1998), versus in trees, have also been isolated. However, isolation of tree genes which are directly involved in cellulose biosynthesis has remained a great challenge.
For more than 30 years, no gene encoding higher plant cellulose synthase (CelA) was identified. Recently, Pear et al. (1996) isolated the first putative higher plant 15 CelA cDNA, GhCelA (GenBank No. GHU58283), by searching for UDP-glucose binding sequences in a cDNA library prepared from cotton fibers having active secondary wall cellulose synthesis. GhCelA was considered to encode a cellulose synthase catalytic subunit because it is highly expressed in cotton fibers, actively synthesizes secondary wall cellulose, contains eight transmembrane domains, binds UDP-glucose, and contains two 20 other domains unique to plants.
Recently, Arioli et al (1998) cloned a CelA homolog, RSW1 (radial swelling) (GenBank No. AF027172), from Arabidopsis by chromosome walking to a defective locus of a temperature sensitive cellulose-deficient mutant. Complementation of the rswl mutant with a wild type full-length genomic RSW1 clone restored the normal 25 phenotype. This complementation provided the first genetic proof that a plant CelA gene encodes a catalytic subunit of cellulose synthase and functions in the biosynthesis of cellulose microfibrils. The full-length Arabidopsis RSW1 represents the only known, currently available cellulose synthase cDNA available for further elucidating cellulose biosynthesis in transgenic systems (Wu et al, 1998).
The discovery of the RSW1 gene substantiated the belief that the assembly of a cellulose synthase into the plasma membrane is required for functional cellulose biosynthetic machinery and for manufacturing crystalline cellulose microfibrils in plant cell walls. Most significantly, a single CelA gene, e.g. RSW1, is sufficient for the biosynthesis of cellulose microfibrils in plants, e.g. Arabidopsis. Thus, RSW1 is a prime 35 target for engineering augmented cellulose formation in transgenic plants.
Since many of society's fiber, chemical and energy demands are met through the industrial-scale production of cellulose from wood, genetic engineering of the cellulose biosynthesis machinery in trees could produce higher pulp yields. This would allow greater returns on investment by pulp and paper industries. Therefore, it would be advantageous to isolate and characterize genes from trees that are involved in cellulose biosynthesis in order to improve the properties of wood.
SUMMARY OF THE INVENTION Described are polynucleotides comprising a nucleotide sequence that encodes a cellulose synthase, regulatory sequences, including a stress-inducible promoter, of the cellulose synthase, a cellulose synthase protein or a functional domain thereof and methods for augmenting cellulose biosynthesis in plants. 10 In one aspect, the present invention provides a polynucleotide comprising a sequence that encodes a cellulose synthase promoter of SEQ ID NO: 3, a sequence conservative variant thereof, or a functional fragment thereof which binds to a transcription factor in a plant cell.
In another aspect, the present invention provides a method of causing stress-15 induced gene expression in a plant cell comprising delivering into the cell a vector comprising a cellulose synthase promoter operatively linked to a gene, wherein the gene is expressed upon a mechanical stress to the plant.
In another aspect, the present invention provides a method of increasing expression of a cellulose synthase in a plant comprising delivering into the plant a cDNA 20 encoding a protein that binds to a positive MSRE of a cellulose synthase promoter wherein the binding to the positive MSRE results in expression of a cellulose synthase, resulting in increased expression of cellulose in the plant.
In another aspect, the present invention is directed to a method of reducing expression of a cellulose synthase in a plant comprising delivering into the plant a DNA in an 25 antisense orientation, the DNA in a sense orientation encoding protein that binds to a positive MSRE and results in expression of a cellulose synthase.
In yet another aspect, the present invention is directed to a method of increasing cellulose biosynthesis in a plant comprising delivering into the plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter, wherein binding of the 30 protein to the positive MSRE results in expression of a cellulose synthase.
In a further aspect, the present invention is directed to a method of reducing cellulose biosynthesis in a plant comprising delivering into the plant a DNA in an antisense orientation, the DNA in a sense orientation encoding protein that binds to a positive MSRE of a cellulose synthase promoter.
In a still further aspect, the present invention is directed to a method of determining a positive mechanical stress responsive element (MSRE) in a cellulose synthase promoter comprising: (i) introducing into a plant a cellulose synthase promoter that has a portion deleted, the cellulose synthase promoter operatively linked to a polynucleotide INTELLECTUAL PROPERTY OFFlUt OF N.Z. 1 <i NOV 2005 ocrciupn -4a- encoding a reporter, and (ii) detecting a decrease in the amount of reporter in the plant after inducing a stress to the plant.
In a still further aspect, the present invention is directed to a method of determining a negative MSRE in a cellulose synthase promoter comprising: (i) introducing into a plant a cellulose synthase promoter that has a portion deleted, the cellulose synthase promoter operatively linked to a reporter gene, and (ii) detecting an increase in the amount of reporter in the plant after inducing a stress to the plant.
Other aspects of the invention will be appreciated by a consideration of the detailed description of the invention, drawings and appended claims. -4b- Described is a method of increasing expression of a cellulose synthase in a plant comprising delivering into the plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter wherein the binding to the positive MSRE results in expression of a cellulose synthase, resulting in increased expression of cellulose in the plant.
Described is a method of reducing expression of a cellulose synthase in a plant comprising delivering into the plant a cDNA in an antisense orientation, the cDNA in a sense orientation encoding protein that binds to a positive MSRE and results in expression of a cellulose synthase.
Described is a method of increasing cellulose biosynthesis in a plant comprising delivering into the plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter, wherein binding of the protein to the positive MSRE results in expression of a cellulose synthase.
Described is a method of reducing cellulose biosynthesis in a plant comprising delivering into the plant a cDNA in an antisense orientation, the cDNA in a sense orientation encoding protein that binds to a positive MSRE of a cellulose synthase promoter.
In yet another aspect, the present invention provides a method of altering a characteristic of a plant comprising the step of incorporating into the genome of the plant a nucleotide sequence encoding cellulose synthase, a nucleotide sequence encoding a UDP-glucose binding domain thereof, or a non-cellulose synthase encoding nucleotide sequence, wherein the nucleotide sequence is operatively linked to a cellulose synthase promoter comprising a mechanical stress regulatory element (MSRE), such that in response to stress, a transcription factor contacts a MSRE nucleotide sequence of the cellulose synthase promoter, such that when the nucleotide sequence is expressed in the plant, the characteristic of the plant is altered, wherein the characteristic includes a least one of altered growth, altered cellulose content, altered lignin content, and altered strength of juvenile wood and fiber, and combinations thereof compared to a control plant that is not transformed with the nucleotide sequence. -4c- In yet another aspect, the present invention provides a method of regulating cellulose synthase expression in a plant comprising delivering into the plant (a) a cDNA encoding a polypeptide which is a positive MSRE of a cellulose synthase promoter; or (b) a cDNA in an anti sense orientation of the cDNA of (a), in amount and under conditions effective to allow at least a portion of the plant's cells to take up the cDNA.
In still another aspect, the present invention provides a method of altering a characteristic of a plant comprising the step of incorporating into the genome of the plant a nucleotide sequence encoding a UDP-glucose catalytic subunit, such that when the nucleotide sequence is expressed in the plant, the characteristic of the plant is altered, wherein the characteristic includes at least one of accelerated plant growth, increased cellulose content, decreased lignin content, and improved strength of juvenile wood and fiber, and combinations thereof compared to a control plant that is not transformed with the nucleotide sequence.
In still another aspect, the present invention provides a method of altering a characteristic of a plant comprising the step of incorporating into the genome of the plant a cellulose synthase promoter operatively linked to a nucleotide sequence, such that a negative MSRE of the cellulose synthase promoter has been modified, deleted, or blocked, such that when the nucleotide sequence is expressed in the plant, the characteristic of the plant is altered, wherein the characteristic includes at least one of accelerated growth, increased cellulose content, decreased lignin content, and improved strength of juvenile wood and fiber, and combinations thereof compared to a control plant that is not transformed with the nucleotide sequence.
In a further aspect, the present invention provides a method of altering a characteristic of a plant comprising the step of incorporating into the genome of the plant a cellulose synthase promoter operatively linked to a nucleotide sequence, such that a positive MSRE of the cellulose synthase promoter has been modified, deleted, or blocked, such that when the nucleotide sequence is expressed in the plant, the characteristic of the plant is altered, wherein the characteristic includes at least one of decreased cellulose content, and increased lignin content, and combinations thereof compared to a control plant that is not transformed with the nucleotide sequence.
In still a further aspect, the present invention provides a plant or a tree produced by the methods as set forth in the invention. -4d- In still a further aspect, the present invention provides a plant having a characteristic genetically altered through incorporation into the genome of the plant a nucleotide sequence encoding cellulose synthase, such that when the nucleotide sequence is expressed in the plant, the characteristic of the plant is altered, wherein the characteristic includes at least one of altered growth, altered lignin content, altered cellulose content, and altered strength of juvenile wood and fiber, and combinations thereof compared to a control plant that is not transformed with the nutleotide sequence.
Described is a polynucleotide comprising a sequence that encodes a cellulose synthase, or a polynucleotide fragment thereof, the fragment encoding a functional domain of cellulose synthase, such as a UDP-glucose binding domain. Also provided is a cellulose synthase or a functional domain or fragment thereof, including a UDP-glucose binding domain and at least one of eight transmembrane domains. Further provided is a cellulose synthase promoter, or a functional fragment thereof, which fragment contains one or more mechanical stress response elements (MSRE).
Described is a method of improving the quality of wood by altering the quantity of cellulose in plant cells,-and optionally decreasing the content of lignin in the cell. Also described is a method of altering the growth or the cellulose content of a plant by expressing an exogenous polynucleotide encoding a cellulose synthase or a UDP-glucose binding domain thereof in the plant. Further provided is a method for causing a stress-induced gene expression in a plant cell by expressing a polynucleotide of choice using a stresS-inducible cellulose synthase promoter.
Described is a method for determining a mechanical stress responsive element (MSRE) in a cellulose synthase promoters and a method for identifying transcription factors that binds to the MSRE.
Described is a method for altering (increasing or decreasing) i.e., regulating, the expression of a cellulose synthase in a plant by expressing an exogenous polynucleotide encoding a transcription factor having the property of binding a positive MSRE of a cellulose synthase promoter or by expressing an antisense polynucleotide encoding a transcription factor having the property of binding a negative MSRE to block the expression of the transcription factor.
Other aspects of the invention will be appreciated by a consideration of the detailed description of die invention drawings and appended claims.
DESCRIPTION OF THE DRAWINGS Fig. 1 represents a nucleic acid sequence encoding a cellulose synthase from Populus tremuloides [SEQ ID NO: 1] and the protein sequence thereof [SEQ ID NO: 2].
Fig. 2 a-c (collectively referred to as Fig. 2) represent a Southern blot analysis of aspen genomic DNA probed with a fragment of the aspen cDNA represented in Fig. 1 under low (panel a) and high stringency conditions (panel b), and a northern blot analysis of the total aspen RNA from stem intemodes using the same probe (panel c).
Fig. 3 a-d (collectively referred to as Fig. 3) represent in situ localization of 10 the cellulose synthase gene transcripts as shown in the transverse sections from second (panel a), fourth (panel b), sixth (panel c) and fifth (panel d) internode.
Fig. 4 represents a nucleic acid sequence of the 5' region of aspen cellulose synthase gene including the promoter region and the 5' portion of the coding sequence [SEQ ID NO: 3].
Fig. 5 a-f (collectively referred to as Fig. 5) represents a histochemical analysis (panels a-d and f) and fluorescence microscopy (panel e) of transgenic tobacco for GUS gene expression driven by a cellulose synthase promoter of the invention.
Fig. 6 a-d (collectively referred to as Fig. 6) represents a histochemical analysis of GUS gene expression driven by aspen cellulose synthase promoter of the 20 invention; tangential and longitudinal sections were harvested before bending (panel a), and 4 (panel b), 20 (panel c) and 40 (panel d) hours after bending and stained for GUS expression.
Fig. 7 represents a cDNA encoding cellulose synthase isolated from Arabidopsis [SEQ ID NO:4].
Fig. 8 represents an Arabidopsis cellulose synthase [SEQ ID NO:5] encoded by the cDNA represented in Fig. 7.
DF.TATT FD DESCRIPTION OF THE INVENTION All patents, patent applications and references cited in this specification are hereby 30 incorporated herein by reference in their entirety. In case of any inconsistency, the present disclosure governs.
Definitions The terms used in this specification generally have their ordinary meanings 35 in the art, within the context of the invention, and in the specific context where each term is used. Certain terms are discussed below, or elsewhere in the specification, to provide additional guidance to the person of skill in the art in describing the compositions and methods of the invention and how to make and use them. It will be appreciated that the 1 same thing can be said in more than one way. Consequently, alternative language and synonyms may be used for any one or more of the terms discussed herein, nor is any special significance to be placed upon whether or not a term is elaborated or discussed herein. Synonyms for certain terms are provided. A recital of one or more synonyms does 5 not exclude the use of other synonyms. The use of examples anywhere in this specification, including examples of any terms discussed herein, is illustrative only, and in no way limits the scope and meaning of the invention or of any exemplified term. Likewise, the invention is not limited to the preferred embodiments.
The term "plant" includes whole plants and portions of plants, including 10 plant organs (e.g. roots, stems, leaves, etc.).
The term "angiosperm" refers to plants which produce seeds encased in an ovary. A specific example of an angiosperm is Liquidambar styraciflua (L.)[sweetgum].
The term "gymnosperm" refers to plants which produce naked seeds, that is, seeds which are not encased in an ovary. Specific examples of a gymnosperm include 15 Pinus taeda (L.)[loblolly pine].
The term "polynucleotide" or "nucleic acid molecule" is intended to include double or single stranded genomic and cDNA, RNA, any synthetic and genetically manipulated polynucleotide, and both sense and anti-sense strands together or individually (although only sense or anti-sense stand may be represented herein). This includes single-20 and double-stranded molecules, i.e., DNA-DNA, DNA-RNA and RNA-RNA hybrids, as well as "protein nucleic acids" (PNA) formed by conjugating bases to an amino acid backbone. This also includes nucleic acids containing modified bases, for example thio-uracil, thio-guanine and fluoro-uracil.
An "isolated" nucleic acid molecule or polynucleotide refers to a 25 component that is removed from its original environment (for example, its natural environment if it is naturally occurring). An isolated nucleic acid or polypeptide may contains less than about 50%, preferably less than about 75%, and most preferably less than about 90%, of the cellular components with which it was originally associated. A polynucleotide amplified using PCR so that it is sufficiently and easily distinguishable (on 30 a gel, for example) from the rest of the cellular components is considered "isolated". The polynucleotides and polypeptides of the invention may be "substantially pure," i.e., having the highest degree of purity that can be achieved using purification techniques known in the art.
The term "hybridization" refers to a process in which a strand of nucleic 35 acid joins with a complementary strand through base pairing. Polynucleotides are "hybridizable" to each other when at least one strand of one polynucleotide can anneal to a strand of another polynucleotide under defined stringency conditions. Hybridization requires that the two polynucleotides contain substantially complementary sequences; depending on the stringency of hybridization, however, mismatches may be tolerated. Typically, hybridization of two sequences at high stringency (such as, for example, in an aqueous solution of 0.5X SSC at 65 °C) requires that the sequences exhibit some high degree of complementarily over their entire sequence. Conditions of intermediate 5 stringency (such as, for example, an aqueous solution of 2X SSC at 65 °C) and low stringency (such as, for example, an aqueous solution of 2X SSC at 55 °C), require correspondingly less overall complementarily between the hybridizing sequences. (IX SSC is 0.15 M NaCl, 0.015 M Na citrate.) As used herein, the above solutions and temperatures refer to the probe-washing stage of the hybridization procedure. The term "a 10 polynucleotide that hybridizes under stringent (low, intermediate) conditions" is intended to encompass both single and double-stranded polynucleotides although only one strand will hybridize to the complementary strand of another polynucleotide.
A "sequence-conservative variant" is a polynucleotide that contains a change of one or more nucleotides in a given codon position, as compared with another 15 polynucleotide, but the change does not result in any alteration in the amino acid encoded at that position.
A "function-conservative variant" is a polypeptide (or a polynucleotide encoding the polypeptide) having a given amino acid residue that has been changed without altering the overall conformation and function of the polypeptide, including, but 20 not limited to, replacement of an amino acid with one having similar physico-chemical properties (such as, for example, acidic, basic, hydrophobic, and the like). Amino acids with have similar physico-chemical properties are well known in the art. For example, arginine, histidine and lysine are hydrophilic-basic amino acids and may be interchangeable. Similarly, isoleucine, a hydrophobic amino acid, may be replaced with 25 leucine, methionine or valine. Sequence- and function-conservative variants are discussed in greater detail below with respect to degeneracy of the genetic code.
A "functional domain" or a "functional fragment" refers to any region or portion of a protein or polypeptide or polynucleotide which is a region or portion of a larger protein or polynucleotide, the region or portion having the specific activity or 30 specific function attributable to the larger protein or polynucleotide, e.g., a functional domain of cellulose synthase is the UDP-glucose binding domain.
The term "% identity" refers to the percentage of the nucleotides/amino acids of one polynucleotide/polypeptide that are identical to the nucleotides/amino acids of another sequence of polynucleotide/polypeptide as identified by program GAP from 35 Genetics Computer Group Wisconsin (GCG) package (version 9.0) (Madison, WI). GAP uses the algorithm of Needleman and Wunsch (J. Mol. Biol. 48:443-453,1970) to find the alignment of two complete sequences that maximizes the number of matches and minimizes the number of gaps. When parameters required to run the above algorithm are not specified, the default values offered by the program are contemplated. The following parameters are used by the GCG program GAP as default values (for polynucleotides): gap creation penalty:50; gap extension penalty:3; scoring matrix: nwsgapdna.cpm (local data file).
The "% similarity" or "% homology" between two polypeptide sequences is a function of the number of similar positions shared by two sequences on the basis of the scoring matrix used divided by the number of positions compared and then multiplied by 100. This comparison is made when two sequences are aligned (by introducing gaps if needed) to determine maximum homology. PowerBlast program, implemented by the 10 National Center for Biotechnology Information, can be used to compute optimal, gapped alignments. GAP program from Genetics Computer Group Wisconsin package (version 9.0) (Madison, WI) can also be used. GAP uses the algorithm of Needleman and Wunsch (J Mol Biol 48: 443-453, 1970) to find the alignment of two complete sequences that maximizes the number of matches and minimizes the number of gaps. When parameters 15 required to run the above algorithm are not specified, the default values offered by the program are contemplated. The following parameters are used by the GCG program GAP as default values (for polypeptides): gap creation penalty: 12; gap extension penalty:4; scoring matrix:Blosum62.cpm (local data file).
The term "oligonucleotide" refers to a nucleic acid, generally of at least 10, 20 preferably at least 15, and more preferably at least 20 nucleotides, that is hybridizable to a genomic DNA molecule, a cDNA molecule, or an mRNA molecule encoding a gene, mRNA, cDNA, or other nucleic acid of interest. Oligonucleotides can be labeled, e.g., with 32P-nucleotides or nucleotides to which a label, such as biotin, has been covalently conjugated. In one embodiment, a labeled oligonucleotide can be used as a probe to detect 25 the presence of a nucleic acid. In another embodiment, oligonucleotides (one or both of which may be labeled) can be used as PCR primers, either for cloning full length or a fragment of CelA, or to detect the presence of nucleic acids encoding CelA. In a further embodiment, an oligonucleotide of the invention can form a triple helix with a CelA DNA molecule. In still another embodiment, a library of oligonucleotides arranged on a solid 30 support, such as a silicon wafer or chip, can be used to detect various polymorphisms of interest. Generally, oligonucleotides are prepared synthetically, preferably on a nucleic acid synthesizer. Accordingly, oligonucleotides can be prepared with non-naturally occurring phosphoester analog bonds, such as thioester bonds, etc.
The term "coding sequence" refers to that portion of the gene that contains 35 the information for encoding a polypeptide. The boundaries of the coding sequence are determined by a start codon at the 5' (amino) terminus and a translation stop codon at the 3' (carboxyl) terminus. A coding sequence can include, but is not limited to, prokaryotic sequences, cDNA from eukaryotic mRNA, genomic DNA sequences from eukaryotic (e.g., mammalian) DNA, and even synthetic DNA sequences.
A "promoter" is a polynucleotide containing elements (e.g., a TATA box) which are capable of binding RNA polymerase in a cell and initiating transcription of a 5 downstream (3' direction) coding sequence. For purposes of defining the present invention, the promoter sequence is bounded at its 3' terminus by the transcription initiation site and extends upstream (5' direction) to include the minimum number of bases or elements necessary to initiate transcription at levels detectable above background. Within the promoter sequence will be found a transcription initiation site (conveniently 10 defined for example, by mapping with nuclease SI), as well as protein binding domains (consensus sequences) responsible for the binding of RNA polymerase. Examples of promoters that can be used in the present invention include PtCelAP, 4CL-1 and 35S.
The term "constitutive promoter" refers to a promoter which typically, does not require positive regulatory proteins to activate expression of an associated coding 15 sequence, i.e., a constitutive promoter maintains some basal level of expression. A constitutive promoter is commonly used in creation of an expression cassette. An example of a constitutive promoter are 35S CaMV (Cauliflower Mosaic Virus), available from Clonetech, Palo Alto, CA.
The term "inducible promoter" refers to the promoter which requires a 20 positive regulation to activate expression of an associated coding sequence. An example of such a promoter is a stress-inducible cellulose synthase promoter from aspen described herein.
A coding sequence is "under the control" of transcriptional and transnational control sequences in a cell when RNA polymerase transcribes the coding sequence into 25 mRNA, which is then trans-RNA spliced and translated into the protein encoded by the coding sequence.
A "vector" is a recombinant nucleic acid Construct, such as plasmid, phage genome, virus genome, cosmid, or artificial chromosome to which a polynucleotide of the invention may be attached. In a specific embodiment, the vector may bring about the 30 replication of the attached segment, e.g., in the case of a cloning vector.
The term "expression cassette" refers to a polynucleotide which contains both a promoter and a protein coding sequence such that expression of a given protein is achieved upon insertion of the expression cassette into a cell.
A cell has been "transfected" by exogenous or heterologous polynucleotide 35 when such polynucleotide has been introduced inside the cell. A cell has been "transformed" by exogenous or heterologous polynucleotide when the transfected polynucleotide effects a phenotypic change. Preferably, the transforming polynucleotide should be integrated (covalently linked) into chromosomal DNA making up the genome of the cell.
"Exogenous" refers to biological material, such as a polynucleotide or protein, that has been isolated from a cell and is then introduced into the same or a 5 different cell. For example, a polynucleotide encoding a cellulose synthase of the invention can be cloned from xylem cells of a particular species of tree, inserted into a plasmid and reintroduced into xylem cells of the same or different species. The species thus contains an exogenous cellulose synthase polynucleotide.
"Heterologous polynucleotide" refers to an exogenous polynucleotide not 10 naturally occurring in the cell into which it is introduced.
"Homologous polynucleotide" refers to an exogenous polynucleotide that naturally exists in the cells into which it is introduced.
Described is isolation and characterization of polynucleotides encoding cellulose synthases from plants, especially trees, including full 15 length or naturally occurring forms of cellulose synthases, functional domains, promoters and regulatory elements. Therefore, in accordance with the present invention there may be employed conventional molecular biology, microbiology, and recombinant DNA techniques within the skill of the art. Such techniques are explained fully in the literature. See, e.g., Sambrook, Fritsch & Maniatis, Molecular Cloning: A Laboratory Manual, 20 Second Edition (1989) Cold Spring Harbor Laboratory Press, Cold Spring Harbor, New York (herein "Sambrook et al., 1989"); DNA Cloning: A Practical Approach, Volumes I and II (D.N. Glover ed. 1985); Oligonucleotide Synthesis (MJ. Gait ed. 1984); Nucleic Acid Hybridization [B.D. Hames & S.J. Higgins eds. (1985)]; Transcription And Translation [B.D. Hames & S.J. Higgins, eds. (1984)]; Animal Cell Culture [R.I. 25 Freshney, ed. (1986)]; Immobilized Cells And Enzymes [IRL Press, (1986)]; B. Perbal, A Practical Guide To Molecular Cloning (1984); F.M. Ausubel et al. (eds.), Current Protocols in Molecular Biology, John Wiley & Sons, Inc. (1994).
Described is a novel, full-length cellulose synthase gene (CelA), a novel stress inducible promoter of cellulose synthases (CelAP), and cellulose 30 synthase proteins from trees, including UDP-glucose catalytic domains thereof. The invention enables the development of transgenic tree varieties having increased cellulose content, decreased lignin content and, therefore, improved wood fiber characteristics. Production of increased cellulose quantity and quality in multiple varieties of commercially relevant, transgenic forest tree species in operational production scenarios 35 are further contemplated. Described is a new experimental system for study of CelA gene expression and function in trees.
INIELLECTUAt PROPERTY OFFICE OF N.Z. 1 h NOV 2005 -BECElVFn Polvnucleotides encoding cellulose synthase and fragments thereof Described are polynucleotides which comprise the nucleotide sequence that encodes cellulose synthase of the invention or a functional fragment thereof. In a preferred embodiment, the polynucleotide comprises the sequence 5 encoding a tree cellulose synthase and most preferrably, the sequence encoding a cellulose synthase from aspen. In one embodiment, a polynucleotide includes the entire cellulose synthase coding region, e.g., nucleotides 69 to 3,005 of SEQ ID NO: 1. In another aspect of the invention, the polynucleotide encoding an Arabidopsis cellulose synthase is provided (see SEQ ID NO:4 and the translated protein of SEQ ID NO:5). 10 " Described are fragments of the polynucleotides encoding cellulose synthase of the invention, which fragments encode at least one transmembrane domain and/or a UDP-glucose binding domain. For example, a polynucleotide comprising the nucleotides encoding a UDP-glucose binding domain of aspen cellulose synthase (e.g., nucleotides 660 to 2250 of SEQ ID NO:l) or corresponding 15 nucleotides of SEQ ID NO:4 are within the scope of the invention. The nucleotides encoding the UDP-glucose binding domain can be determined by, for example, alignment of protein sequences as described below.
- Described are sequence conservative variants of the coding portion of SEQ ID NOS: 1 and 4.
Polynucleotides that hybridize under conditions of low, medium, and high stringency to SEQ ID NOS: 1 and 4, and their respective coding portions are also described.
Preferably, the polynucleotide that hybridizes to any of SEQ ID NOS: 1 and 4, or their respective coding portions, is about the same length as that sequence, for example, not more than about 10 to about 20 nucleotides longer or shorter. 25 In another embodiment the hybridizable polynucleotide is at least 1500 nucleotides long, preferably at least 2500 nucleotides long and most preferably at least 3000 nucleotides long. In yet another embodiment, the hybridizable polynucleotide comprises the UDP-glucose binding domain as found in SEQ ID NO:l or 4, or at least the conserved region QVLRW. Most preferably, the hybridizable polynucleotide has a UDP-30 glucose binding activity.
The polynucleotides that occur originally in nature may be isolated from the organisms that contain them using methods described herein or well known in the art. The non-naturally occurring polynucleotides may be prepared using various manipulations known in the field of recombinant DNA. For example, the cloned CelA polynucleotide 35 can be modified according to methods described by Sambrook et al., 1989. The sequence can be cleaved at appropriate sites with restriction endonuclease(s), followed by further enzymatic modification if desired, isolated, and ligated in vitro. In the production of the modified polynucleotides, for example, care should be taken to ensure that the modified INTELLECTUAL PROPERTY OFFICE OF N.Z t <1 NOV 2005 \ polynucleotide remains within the appropriate translational reading frame (if to be expressed) or uninterrupted by translational stop signals. As a further example, a CelA-encoding nucleic acid sequence can be mutated in vitro or in vivo, to create and/or destroy translation, initiation, and/or termination sequences, or to create variations in coding 5 regions and/or form new restriction endonuclease sites or destroy preexisting ones, to facilitate further in vitro modification. Preferably, such mutations enhance the functional activity of the mutated CelA polynucleotide. Any technique for mutagenesis known in the art can be used, including but not limited to, in vitro site-directed mutagenesis (Hutchinson, C., et al., 1978, J. Biol. Chem. 253:6551; Zoller and Smith, 1984, DNA 10 3:479-488; Oliphant et al., 1986, Gene 44:177; Hutchinson et al., 1986, Proc. Natl. Acad. Sci. U.S.A. 83:710), use of TAB linkers (Pharmacia), etc. PCR techniques are preferred for site directed mutagenesis (see Higuchi, 1989, "Using PCR to Engineer DNA", in PCR Technology: Principles and Applications for DNA Amplification, H. Erlich, ed., Stockton Press, Chapter 6, pp. 61-70).
The described polynucleotides may be introduced into various vectors adapted for plant or non-plant replication. These are well known in the art, thus, choice, construction and use of such vectors is well within the skill of a person skilled in the art. Possible vectors include, but are not limited to, plasmids or modified viruses of plants, but the vector system must be compatible with the host cell used. An 20 example of a suitable vector is Ti plasmid. The insertion into a cloning vector can, for example, be accomplished by ligating the DNA fragment into a cloning vector which has complementary cohesive termini. However, if the complementary restriction sites used to fragment the DNA are not present in the cloning vector, the ends of the DNA molecules may be enzymatically modified. Alternatively, any site desired may be produced by ^ 25 ligating nucleotide sequences (linkers) onto the DNA termini; these ligated linkers may " comprise specific chemically synthesized oligonucleotides encoding restriction endonuclease recognition sequences. An expression cassette containing cellulose synthase or recombinant molecules thereof can be introduced into host cells via silicon carbide whiskers, transformed protoplasts, transformation, e.g., Agrobacterium vectors (discussed 30 below), electroporation, infection, etc., so that many copies of the gene sequence are generated. Preferably, the cloned gene is contained on a shuttle vector plasmid, which provides for expansion in a cloning cell, e.g., E. coli, and facile purification for subsequent insertion into an appropriate expression cell line, if such is desired. For example, a shuttle vector, which is a vector that can replicate in more than one type of organism, can be 35 prepared for replication in both E. coli and Saccharomyces cerevisiae by linking sequences from an E. coli plasmid with sequences form the yeast 2m plasmid.
Transgenic plants containing the polynucleotides described herein are also / described. Methods for introducing exogenous polynucleotides INTELLECTUAL PROPERTY OFFICE OF N.Z. 1 <1 NOV 2005 into plant cells and regenerating transgenic plants are well known. Some are provided below.
In one embodiment, to introduce a plasmid containing a CelA coding sequence or promoter into a plant, a 1:1 mixture of plasmid DNA containing a selectable marker expression cassette and plasmid DNA containing a cellulose synthase expression cassette is precipitated with gold to form microprojectiles. The microprojectiles are rinsed in absolute ethanol and aliquots are dried onto a suitable macrocarrier such as the macrocarrier available from BioRad in Hercules, CA. Prior to bombardment, embryogenic tissue is preferably desiccated under a sterile laminar-flow 10 hood. The desiccated tissue is transferred to semi-solid proliferation medium. The prepared microprojectiles are accelerated from the macrocarrier into the desiccated target cells using a suitable apparatus such as a BioRad PDS-1000/HE particle gun. In a preferred method, each plate is bombarded once, rotated 180 degrees, and bombarded a second time. Preferred bombardment parameters are 1350 psi rupture disc pressure, 6 mm 15 distance from the rupture disc to macrocarrier (gap distance), 1 cm macrocarrier travel distance, and 10 cm distance from macrocarrier stopping screen to culture plate (microcarrier travel distance). Tissue is then transferred to semi-solid proliferation medium containing a selection agent, such as hygromycin B, for two days after bombardment.
Cellulose synthase protein and fragment thereof A described cellulose synthase is a plant protein that contains a catalytic subunit which has UDP-glucose binding activity for the synthesis of glucan from glucose, and eight transmembrane domains for localizing the cellulose synthase to the cell 25 membrane. The cellulose synthase of the invention has; eight transmembrane binding domains; two at the amino terminal and six at the carboxyl terminal. The UDP-glucose binding domain is located between transmembrane domains two and three. Examples of this protein structure are seen in the aspen cellulose synthase as well as in those of RSW1 and GhCelA. The location of the transmembrane domain may be identified as described 30 below and as exemplified in the Example. Preferably, the described cellulose synthase has an amino acid sequence of a tree cellulose synthase. 1 In one embodiment, the cellulose synthase protein is isolated from aspen. Aspen cellulose synthase contains about 978 amino acids and has a molecular weight of about 110 KDa and a pi of about 6.58. In one embodiment, the aspen 35 cellulose synthase has the amino acid sequence of SEQ ID NO:2 as represented in Fig. 1.
Described is a cellulose synthase of SEQ ED NO: 5.
Described are fragments of plant cellulose synthases, such as fragments containing at least one transmembrane region and/or a UDP-glucose binding INTELLECTUAL PROPERTY OFFICE OF N.Z. 14 NOV 2005 domain. The transmembrane regions may be identified as described in the Example by using the method of Hoffman and Stoffel (1993).
The cellulose synthase fragment containing the UDP-glucose binding domain is functional without the presence of the rest of the protein. This separable activity 5 is as shown in the Example. This result was surprising and unexpected because previously identified UDP-glucose binding domains were not known to be functional when isolated from other portions of the protein. Thus, a fragment of any cellulose synthase (such as PtCelA, RSW1, GhCelA and SEQ ID NO:5) that contains a UDP-glucose binding domain and is independently functional is useful herein. The function of the UDP-glucose binding domain may be determined using the assay described in the Example. The described UDP-glucose binding domain js located between the second and third transmembrane region of the cellulose synthase and has conserved amino acid sequences for UDP-glucose binding, such as the sequence QVLRW and conserved D residues. The UDP-glucose binding domain and the conserved regions therein may be 15 located in a cellulose synthase using the guidance of the present specification and the general knowledge in the art, for example Brown, 1996. In one embodiment, the UDP-glucose binding domain and the conserved regions therein may be identified by comparing the amino acid sequence of cellulose synthase of interest with the amino acid sequence of aspen cellulose synthase using the algorithms described in the specification or generally 20 known in the art. For example, the UDP-glucose binding domain of SEQ ID NO:2 is in the position amino acids 220 to 749. The conserved QVLRW sequence is located at positions 715-719 of SEQ ID NO:2.
Polypeptides having at least 75%, preferably at least 85% and most preferably at least 95% similarity to the amino acid sequence of SEQ ID NO: 2, amino 25 acids 220-749 of SEQ ID NO:2, SEQ ID NO:5 or its UDP-glucose binding domain using Power Blast or GAP algorithm described above. In a preferred embodiment, these polypeptides are of about the same length as the polypeptide of SEQ ID NO: 2 or amino acids 220-749 of SEQ ID NO:2. For example, the polypeptide may be from about 2-3 to about 5-7 and to about 10-15 amino acids longer or shorter. In another embodiment, the 30 polypeptides described in this paragraph are not originally found (i.e., naturally occurring) in Arabidopsis or cotton. These polypeptides may be prepared by, for example, altering the nucleic acid sequence of a cloned polynucleotide encoding the protein of SEQ ID NO:2 or SEQ ID NO:5 using the methods well known in the art.
Function conservative variants of cellulose synthase are also described 35 and can be prepared by altering the sequence of a cloned polynucleotide encoding cellulose synthase or fragments thereof. Conventional methods used in the art can be used to make substitutions, additions or deletions in one or more amino acids, to provide functionally equivalent molecules. For example, a function INTELLECTUAL PROPERTY OFFICE OF N2 1 4 NOV 2005 conservative variant that has substitutions, deletions and/or additions in the amino and/or carboxyl terminus of the protein, outside of the UDP-glucose binding domain is useful.
Preferably, variants are made that have enhanced or increased functional activity relative to native cellulose synthase. Methods of directed evolution can 5 be used for this purpose.
Also described are function conservative variants which include altered sequences in which functionally equivalent amino acid residues are substituted for residues within the sequence resulting in a conservative amino acid substitution. For example* one or more amino acid residues within the sequence can be substituted by 10 another amino acid of a similar polarity, which acts as a functional equivalent, resulting in a silent alteration. Substitutes for an amino acid within the sequence may be selected from other members of the class to which the amino acid belongs. For example, the nonpolar (hydrophobic) amino acids include alanine, leucine, isoleucine, valine, proline, phenylalanine, tryptophan and methionine. Amino acids containing aromatic ring 15 structures are phenylalanine, tryptophan, and tyrosine. The polar neutral amino acids include glycine, serine, threonine, cysteine, tyrosine, asparagine, and glutamine. The positively charged (basic) amino acids include arginine, lysine and histidine. The negatively charged (acidic) amino acids include aspartic acid and glutamic acid. Such alterations will not be expected to affect apparent molecular weight as determined by 20 polyacrylamide gel electrophoresis, or isoelectric point. Particularly preferred substitutions are: (i) Lys for Arg and vice versa such that a positive charge may be maintained; (ii) Glu for Asp and vice versa such that a negative charge may be maintained; (iii) Ser for Thr such that a free -OH can be maintained; and (iv) Gin for Asn such that a free CONH2 can be maintained. Amino acid substitutions may also be introduced to 25 substitute an amino acid with a particularly preferable property. For example, a Cys may be introduced a potential site for disulfide bridges with another Cys. A His may be introduced as a particularly "catalytic" site (i.e., His can act as an acid or base and is the most common amino acid in biochemical catalysis). Pro may be introduced because of its particularly planar structure, which induces b-turns in the protein's structure. 30 The cellulose synthase of the invention can be isolated by expressing a cloned polynucleotide encoding the cellulose synthase as well as using direct protein purification techniques. These methods will be apparent to those of skill in the art. ;Polynucleotides containing cellulose synthase promoter 35 Useful herein is a cellulose synthase promoter. The promoter is a stress-inducible promoter and may be used to synthesize greater quantities of high crystalline cellulose in plant, and preferably in trees. This permits an increase in the ;INTELLECTUAL PROPERTY OFFICE OF N.Z. ;1V NOV 2005 ;Dcr cixicn ;-16- ;1 ;proportion of cellulose in transgenic plants, greater strength of juvenile wood and fiber, and acceleration of overall growth rate. ;- In one embodiment, the promoter is from aspen and is represented in Figure 4. The promoter sequence is located within the region of nucleotides 5 1-840 of SEQ ID NO:3. A person of skill in the art will appreciate that not the entire sequence is required for the promoter function and can easily identify the critical regions by looking for conserves boxes and doing routine deletion analysis. Thus, functional fragments of SEQ ID NO:l are useful. ;Polynucleotides that hybridize under conditions of low, medium, and high 10 stringency to SEQ ID NO:3, and its non-coding portion are also useful. ;The hybridizable polynucleotide may be about the same length as the sequence to which it hybridizes, for example, not more than about 10 to about 20 nucleotides longer or shorter. In another embodiment, the hybridizable polynucleotide is at least about 200 nucleotides long, preferably at least about 400 nucleotides long and most preferably at 15 least 500 nucleotides long. In yet another embodiment, the hybridizable polynucleotide comprises at least one MSRE element identified according to the method described below. ;A cellulose synthase promoter typically provides tissue- ;specific gene regulation in xylem, but also permits up-regulation of gene expression in other tissues as well, e.g., phloem under tension stress. Furthermore, expression of 20 cellulose synthase is localized to an area of the plant under stress. ;This stress-inducible phenomenon is regulated by positive and negative mechanical stress response elements (MSREs). These MSREs upregulate (positive) or downregulate (negative) the expression of a cellulose synthase polynucleotide under stress conditions through binding of transcription factors. MSRE-regulated expression of 25 cellulose synthase permits synthesis of cellulose with high crystallinity. ;The MSREs of cellulose synthase can be modified or employed otherwise in methods to regulate expression of a polynucleotide, including a cellulose synthase, operatively linked to a promoter containing an MSRE in response to mechanical stress (e.g., tension or compression) to a transgenic plant. ;30 Negative MSREs of a cellulose synthase promoter can be modified, ;removed or blocked to improve expression of a cellulose synthase, and thereby increase cellulose production and improve wood quality. Alternatively, positive MSREs can be removed or blocked to decrease expression of a cellulose synthase, which decreases cellulose production and increases lignin deposition. This is useful for increasing the fuel 35 value of wood because lignin has a higher BTU value than cellulose. Moreover, a modified cellulose synthase promoter can be operatively linked to a polynucleotide of interest to control its expression upon mechanical stress to a plant harboring it. ;INTELLECTUAL PROPERTY OFFICE OF N2 ;14 NOV 2005 RECEIVED ;-17- ;The location of MSRE elements in the SEQ ID NO:3 may be identified, for example, using promoter deletion analysis, DNAse Foot Print Analysis, and Southwestern screening of an expression library for an MSRE. In one embodiment, cellulose synthase promoter that has one or more portions deleted, and is operatively linked to a reporter 5 sequence, is introduced into a plant or a plant cell. A positive MSRE is detected by observing no relative change or increase in the amount of reporter in a transgenic plant or tissue, e.g., phloem after inducing a stress to the plant, and a negative MSRE is detected by observing increases in the amount of reporter in the plant in the absence of any stress to the plant. A positive element is detected when by removing it, GUS expression goes down 10 and by adding it kept at the same level or more. The negative element does not support, or suppreses, expression of GUS and by removing it, normal or enhanced GUS expression is observed as compared to when negative element is present. ;Manipulation of a MSRE binding sites and/or providing transcription factors that bind thereto, provides a mechanism to continuously produce high crystalline 15 cellulose in woody plant cell walls of transgenic plants. For example, one having ordinary skill in the art can delete or block negative MSRE elements, or provide cDNA encoding protein(s) that bind the positive MSREs, to enable constitutive expression of a cellulose synthase without the requirement of a mechanical stress. The increased cellulose synthase, and therefore, increased cellulose content, can improve the strength properties of juvenile 20 wood and fiber. It is also contemplated that the positive MSREs can be deleted or blocked, or cDNA in an antisense direction, which in the sense direction encodes a protein that binds a positive MSRE, can be provided, to reduce cellulose synthase activity and decrease cellulose production. ;25 Method of Isolating Polynucleotides Encoding Cellulose Synthase ;Described are methods for identifying and isolating polynucleotides encoding cellulose synthase in plants, e.g., tiees, (in addition to those polynucleotides provided in the Example and represented in Fig. 1 and Fig. 7). These polynucleotides may be used to manipulate expression of cellulose synthase with an objective to improve the 30 cellulose content and properties of wood. ;The method comprises identifying a nucleic acid fragment containing a sequence encoding cellulose synthase or a portion thereof by using a fragment of SEQ ID NOS:l or 4 as a probe or a primer. Once identified, the nucleic acid fragment containing a sequence encoding cellulose synthase or a portion thereof is isolated. 35 Polynucleotides encoding described cellulose synthases, whether genomic DNA, cDNA, or fragments thereof, can be isolated from many sources, particularly from cDNA or genomic libraries from plants, preferably trees (e.g. aspen, sweetgum, loblolly pine, eucalyptus, and other angiosperms and gymnosperms). ;INTELLECTUAL PROPERTY OFFICE OF N.Z. ;1 h NOV 2005 ;-18- ;Molecular biology methods for obtaining polynucleotides encoding a cellulose synthase are well known in the art, as described above (see, e.g., Sambrook et ah, 1989, supra). ;Accordingly, cells from any species of plant can potentially serve as a nucleic acid source for the molecular cloning of a polynucleotide encoding a cellulose 5 synthase* The DNA may be obtained by standard procedures known in the art from cloned DNA (e.g., a DNA "library"), and preferably is obtained from a cDNA library prepared from tissues with high level expression of a cellulose synthase (e.g., xylem tissue, since cells in this tissue evidence very high levels of expression of CelA), by chemical synthesis, by cDNA cloning, or by the cloning of genomic DNA, or fragments 10 thereof, purified from a desired cell (see, for example, Sambrook et al., 1989, supra; Glover, D.M. (ed.), 1985, DNA Cloning: A Practical Approach, MRL Press, Ltd., Oxford, U.K. Vol. I, II). Clones derived from genomic DNA may contain regulatory and intron ^ DNA regions in addition to coding regions; clones derived from cDNA will not contain intron sequences. Whatever the source, a polynucleotide should be molecularly cloned 15 into a suitable vector for its propagation.
In another embodiment for the molecular cloning of a polynucleotide encoding a cellulose synthase from genomic DNA, DNA fragments are generated from a genome of interest, such as from a plant, or more particularly a tree genome, part of which will correspond to a desired polynucleotide. The DNA may be 20 cleaved at specific sites using various restriction enzymes. Alternatively, one may use DNAse in the presence of manganese to fragment the DNA, or the DNA can be physically sheared, as for example, by sonication. The linear DNA fragments can then be separated according to size by standard techniques, including but not limited to, agarose and polyacrylamide gel electrophoresis and column chromatography.
Once the DNA fragments are generated, identification of the specific DNA fragment containing a desired CelA sequence may be accomplished in a number of ways. For example, if an amount of a portion of a CelA sequence or its specific RNA, or a fragment thereof, is available and can be purified and labeled, the generated DNA fragments may be screened by nucleic acid hybridization to a labeled probe (Benton and 30 Davis, 1977, Science 196:180; Grunstein and Hogness, 1975, Proc. Natl. Acad. Sci. U.S.A. 72:3961). For example, a set of oligonucleotides corresponding to the partial amino acid sequence information obtained for a CelA protein from trees can be prepared and used as probes for DNA encoding cellulose synthase, or as primers for cDNA or mRNA (e.g., in combination with a poly-T primer for RT-PCR). Preferably, a fragment is 35 selected that is highly unique to a described cellulose synthase, such as the UDP- glucose binding regions. Those DNA fragments with substantial homology to the probe will hybridize. As noted above, the greater the degree of homology, the more stringent hybridization conditions can be used. In a specific embodiment, stringency hybridization conditions can be used to identify homologous CelA sequences from trees or other plants.
Thus, in one embodiment, a labeled cellulose synthase cDNA from, e.g., Populus tremuloides (PtCelA), can be used to probe a library of genes or DNA fragments 5 from various species of plants, especially angiosperm and gymnosperm, to determine whether any bind to a described CelA. Once genes or fragments are identified, they can be amplified using standard PCR techniques, cloned into a vector, e.g., pBluescript vector (StrataGene of LaJolla, CA), and transformed into a bacteria, e.g., DH5a E. coli strain (Gibco BRL of Gaithersburg, MD). Bacterial colonies are typically tested to 10 determine whether any contains a cellulose synthase-encoding nucleic acid. Once a positive clone is identified through binding, it is sequenced from an end, preferably the 3' end. cDNA libraries can be constructed in various hosts, such as lambda ZAPII, available from Stratagene, LaJolla, CA, using poly(A) +RNA isolated from aspen xylem, 15 according to the methods described by Bugos et al (Biotechniques 19:734-737, 1995 ). The above mentioned probes are used to assay the aspen cDNA library to locate cDNA which codes for enzymes involved in production of cellulose synthases. Once a cellulose synthase sequence is located, it is then cloned and sequenced according to known methods in the art.
Further selection can be carried out on the basis of the properties of the gene, e.g., if the gene encodes a protein product having the isoelectric, electrophoretic, hydropathy plot, amino acid composition, or partial amino acid sequence of a cellulose synthase protein of the invention, as described herein. Thus, the presence of the gene may be detected by assays based on the physical, chemical, or immunological properties of its 25 expressed product. For example, cDNA clones or DNA clones which hybrid-select the proper mRNAs can be used to produce a protein that has similar properties known for 4 cellulose synthases. Such properties may include, for example, similar or identical electrophoretic migration patterns, isoelectric focusing or non-equilibrium pH gel electrophoresis behavior, proteolytic digestion maps, hydropathy plots, or functional 30 properties (such as isolated, functional UDP-glucose binding domains).
A cellulose synthase polynucleotide can also be identified by mRNA selection, i.e., by nucleic acid hybridization followed by in vitro translation. In this procedure, nucleotide fragments are used to isolate complementary mRNAs by hybridization. Such DNA fragments may represent available, purified CelA DNA, or may 35 be synthetic oligonucleotides designed from the partial amino acid sequence information. Functional assays (e.g., UDP-glucose activity) of the in vitro translation products of the products of the isolated mRNAs identifies the mRNA and, therefore, the complementary DNA fragments, that contain the desired sequences. I intellectual property office OF N.Z.
H NOV 2005 RECEIVED A radiolabeled CelA cDNA can be synthesized using a selected mRNA as a template. The radiolabeled mRNA or cDNA may then be used as a probe to identify homologous CelA DNA fragments from amongst other genomic DNA fragments.
It will be appreciated that other polynucleotides, in addition to a CelA 5 can be operatively linked to a CelA promoter to control expression of the polynucleotide upon application of a mechanical stress.
Expression of CelA Polypeptides The nucleotide sequence coding for CelA, or a functional fragment, 10 derivative or analog thereof, including chimeric proteins, can be inserted into an appropriate expression vector, i.e., a vector which contains the necessary elements for the transcription and translation of the inserted protein-coding sequence. Preferably, an expression vector includes an origin of replication. The elements are collectively termed herein a "promoter." Thus, a nucleic acid encoding CelA can be operatively associated with a promoter in an expression vector of the invention. Both cDNA and genomic sequences can be cloned and expressed under control of such regulatory sequences. The necessary transcriptional and translational signals can be provided on a recombinant expression vector, or they may be supplied by the native gene encoding CelA and/or its flanking regions.
In addition to a CelAP, expression of cellulose synthase can be controlled by any promoter/enhancer element known in the art, but these regulatory elements must be functional in the host selected for expression. Promoters which may be used to control CelA polynucleotide expression include, constitutive, development-specific and tissue-specific. Examples of these promoters include 35S Cauliflower Mosaic Virus, terminal 25 flower and 4CL-1. Thus, there are various ways to alter the growth of a plant using different promoters, depending on the needs of the practitioner.
The nucleotide sequence may be inserted in a sense or antisense direction depending on the needs of the practitioner. For example, if augmentation of cellulose biosynthesis is desired then polynucleotides encoding, e.g., cellulose synthase, can be 30 inserted into the expression vector in the sense direction to increase cellulose synthase production and thus cellulose biosynthesis. Alternatively, if it is desired that cellulose biosynthesis is reduced or lignin content is increased, then polynucleotides encoding, e.g., cellulose synthase ,can be inserted in the antisense direction so that upon transcription the antisense mRNA hybridizes to other complementary transcripts in the sense orientation to 35 prevent translation. In other embodiments, the polynucleotide encodes a UDP-glucose binding domain and is used in a similar manner as described.
A recombinant CelA protein of the invention, or functional fragment, derivative, chimeric construct, or analog thereof, may be expressed chromosomally, after INTELLECTUAL PROPERTY OFFICE OF N.Z. 14 NOV 2005 Dcr'cn/cn integration of the coding sequence by recombination. In this regard, any of a number of amplification systems for plants may be used to achieve high levels of stable gene expression, as discussed above. Any of the methods previously described for the insertion of DNA fragments into a cloning vector may be used to construct expression vectors 5 containing a gene consisting of appropriate transcriptional/translational control signals and the protein coding sequences. These methods may include in vitro recombinant DNA and synthetic techniques and in vivo recombination (genetic recombination). i Expression vectors containing a nucleic acid encoding a CelA can be identified by four general approaches: (a) PCR amplification of the 10 desired plasmid DNA or specific mRNA, (b) nucleic acid hybridization, (c) presence or absence of selection marker gene functions, (d) analyses with appropriate restriction endonucleases, and (e) expression of inserted sequences. In the first approach, the nucleic acids can be amplified by PCR to provide for detection of the amplified product. In the second approach, the presence of a foreign gene inserted in an expression vector can be 15 detected by nucleic acid hybridization using probes comprising sequences that are homologous to an inserted marker gene. In the third approach, the recombinant vector/host system can be identified and selected based upon the presence or absence of certain "selection marker" gene functions (e.g., P-glucuronidase activity, resistance to antibiotics, transformation phenotype, etc.) caused by the insertion of foreign genes in the 20 vector. In another example, if the nucleic acid encoding CelA is inserted within the ''selection marker" gene sequence of the vector, recombinants containing the CelA insert can be identified by the absence of the CelA gene function. In the fourth approach, recombinant expression vectors are identified by digestion with appropriate restriction enzymes. In the fifth approach, recombinant expression vectors can be identified by 25 assaying for the activity, biochemical, or immunological characteristics of the gene product expressed by the recombinant, provided that the expressed protein assumes a functionally active conformation.
After a particular recombinant DNA molecule is identified and isolated, several methods known in the art may be used to propagate it. Once a suitable host system 30 and growth conditions are established, recombinant expression vectors can be propagated and prepared in quantity. As previously explained, the expression vectors which can be used include, but are not limited to those vectors or their derivatives described above.
Vectors are introduced into the desired host cells by methods known in the art, e.g., Agrobacterium-mediated transformation (described in greater detail below), 35 transfection, electroporation, microinjection, transduction, cell fusion, DEAE dextran, calcium phosphate precipitation, lipofection (lysosome fusion), use of a gene gun, or a DNA vector transporter (see, e.g., Wu et al., 1992, J. Biol. Chem. 267:963-967; Wu and INTELLECTUAt^PROPERTY OFFICE H NOV 2005 receiver Wu, 1988, J. Biol. Chem. 263:14621-14624; Hartmut et al., Canadian Patent Application No. 2,012,311, filed March 15,1990).
The cell into which the recombinant vector comprising the nucleic acid encoding CelA is cultured in an appropriate cell culture medium under conditions that 5 provide for expression of CelA by the cell. In addition, a host cell strain may be chosen which modulates the expression of the inserted sequences, or modifies and processes the gene product in a specific fashion desired. Different host cells have characteristic and specific mechanisms for the translational and post-translational processing and modification (such as glycosylation, cleavage, e.g., of a signal sequence) of proteins. 10 Appropriate cell lines or host systems can be chosen to ensure the desired modification and processing of the foreign protein expressed.
Aerobacterium-mediated transformation and inducing somatic embryos The culture media used in the invention, and for transforming 15 Agrobacterium, contain an effective amount of each of the medium components (e.g. basal medium, growth regulator, carbon source) described above. As used in describing the present invention, an "effective amount" of a given medium component is the amount necessary to cause a recited effect. For example, an effective amount of a growth hormone in the primary callus growth medium is the amount of the growth hormone that induces 20 callus formation when combined with other medium components. Other compounds known to be useful for tissue culture media, such as vitamins and gelling agents, may also be used as optional components of the culture media of the invention.
Transformation of cells from plants, e.g., trees, and the subsequent production of transgenic plants using Agrobacterium-mediated transformation procedures 25 known in the art, and further described herein, is one example of a method for introducing a foreign gene into trees. Transgenic plants may be produced by various methods, such as by the following steps: (i) culturing Agrobacterium in low-pH induction medium at low temperature and preconditioning, i.e., coculturing bacteria with wounded tobacco leaf extract in order to induce a high level of expression of the Agrobacterium vir genes whose 30 products are involved in the T-DNA transfer, (ii) coculturing a desired plant tissue explants, including zygotic and/or somatic embryo tissues derived from cultured explants, with the incited Agrobacterium; (iii) selecting transformed callus tissue on a medium containing antibiotics; and (v) and converting the embryos into plantlets.
Any non-tumorigenic A. tumefaciens strain harboring a disarmed Ti 35 plasmid may be used in the method of the invention. Any Agrobacterium system may be used. For example, Ti plasmid/binary vector system or a cointegrative vector system with one Ti plasmid may be used. Also, any marker gene or polynucleotide conferring the ability to select transformed cells, callus, embryos or plants and any other gene, such as, for example ,a gene conferring resistance to a disease, or one improving cellulose content, may also be used. Any promoter desired can be used, such as, for example, a PtCelAP of the invention, and those promoters as described above. A person of ordinary skill in the art can determine which markers and genes are used depending on particular needs.
For purposes of the present invention, "transformed" or "transgenic" means that at least one marker gene or polynucleotide conferring selectable marker properties is introduced into the DNA of a plant cell, callus, embryo or plant. Additionally, any gene may also be introduced.
To increase the infectivity of the bacteria, Agrobacterium is cultured in 10 low-pH induction medium, i.e., any bacterium culture media with a pH value adjusted to from 4.5 to 6.0, most preferably about 5.2, and at low temperature such as for example about 19-30°C, preferably about 21-26°C. The conditions of low-pH and low temperature are among the well-defined critical factors for inducing virulence activity in Agrobacterium (e.g., Altmorbe et al, Mol. Plant-Microbe. Interac. 2: 301,1989; Fullner et 15 al., Science 273: 1107,1996; Fullner and Nester, J. Bacteriol. 178:1498, 1996).
The bacteria is preconditioned by coculturing with wounded tobacco leaf extract (prepared according to methods known generally known in the art) to induce a high level of expression of the Agrobacterium vir genes. Prior to inoculation of plant somatic embryos, Agrobacterium cells can be treated with a tobacco extract prepared from 20 wounded leaf tissues of tobacco plants grown in vitro. To achieve optimal stimulation of the expression of Agrobacterium vir genes by wound-induced metabolites and other cellular factors, tobacco leaves can be wounded and pre-cultured overnight. Culturing of bacteria in low pH medium and at low temperature can be used to further enhance the bacteria vir gene expression and infectivity. Preconditioning with tobacco extract and the 25 vir genes involved in the T-DNA transfer process are generally known in the art.
Agrobacterium treated as described above is then cocultured with a plant tissue explant, such as for example zygotic and/or somatic embryo tissue. Non-zygotic (i.e., somatic) or zygotic tissues can be used. Any plant tissue may be used as a source of explants. For example, cotyledons from seeds, young leaf tissue, root tissues, parts of 30 stems including nodal explants, and tissues from primary somatic embryos such as the root axis may be used. Generally, young tissues are a preferred source of explants.
Described are methods of altering the growth of a plant by expressing a described polynucleotide, which as a result alters the growth of the plant. The polynucleotide used in the method may be a homologous polynucleotide or a 35 heterologous polynucleotide and are described in detail above. For example, both full-length and UDP-glucose binding region containing fragments may be expressed. Additionally, depending on the aim of the method, the polynucleotide may be introduced into the plant in the sense or in the antisense orientation. Any suitable promoter may be I INTELLECTUAL PROPERTY OFFICE OF N.Z. 1 V NOV 2005 RECEIVED used to provide expression. The promoter or a functional fragment thereof is operatively linked to the polynucleotide. The promoter may be a constitutive promoter, a tissue-specific promoter or a development-specific plant promoter. Examples of suitable promoters are Cauliflower Mosaic Virus 35S, 4CL, cellulose synthase promoter, PtCelAP 5 and terminal flower promoter.
Described is a method of altering the cellulose content in a plant by expressing a i polynucleotide as described above. The method may be used to increased the ratio of cellulose to lignin in the plant that have an exogenous polynucleotide introduced therein.
Described is a method for altering expression of a cellulose synthase in a plant cell by introducing into the cell a vector comprising a described polynucleotide and expressing the polynucleotide. The polynucleotides and promoters described above may be used.
Described is a method for causing stress-induced gene expression in a plant cell. 15 The method comprises (i) introducing into the plant or a plant cell an expression cassette comprising a cellulose synthase promoter or a functional fragment thereof or providing a plant or a plant cell that comprises the expression cassette (The promoter of the cassette is operatively linked to a coding sequence of choice.); and (ii) applying mechanical stress to the plant to induce expression of the desired coding 20 sequence.
Described is a method for determining a positive mechanical stress responsive element (MSRE) in a cellulose synthase promoter which comprises (i) making serial deletions in the cellulose synthase promoter, such as for example, SEQ ID NO:3; (ii) introducing the deletion linked to a polynucleotide encoding a 25 reporter sequence into a plant cell, and (iii) detecting a decrease in the amount of reporter in the plant after inducing a stress to the plant. Similarly, a method for determining a negative MSRE in a cellulose synthase promoter is provided. It comprises (i) making serial deletions in the cellulose synthase promoter, such as for example, SEQ ID NO:3; (ii) introducing the deletion linked to a polynucleotide encoding a reporter sequence into a 30 plant cell, and (iii) detecting an increase in the amount of reporter in the plant after inducing a stress to the plant.
The following methods are also described and useful herein: a method for expressing cellulose synthase in a tissue-specific manner comprising transforming a plant with a tissue specific promoter operatively linked to a polynucleotide 35 encoding a cellulose synthase; a method for inducing expression of a cellulose synthase in a plant comprising introducing into a plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter, thereby resulting in increased expression of cellulose in the plant, wherein the binding to the positive MSRE results in expression of INTELLECTUAL PROPERTY OFFICE OF N.Z. 1K NOV 2005 a cellulose synthase; a method for reducing expression of a cellulose synthase comprising introducing into a plant a cDNA in an antisense orientation, wherein the cDNA in a sense orientation encodes a protein that binds to a positive MSRE and results in expression of a cellulose synthase; a method for increasing cellulose biosynthesis in a plant comprising 5 introducing into a plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter, whereby binding of the protein to the positive MSRE results in expression of a cellulose synthase, and A method for reducing cellulose biosynthesis in a plant comprising introducing into a plant a cDNA in an antisense orientation, wherein the cDNA in a sense orientation encodes a protein that binds to a positive MSRE of a 10 cellulose synthase promoter.
EXAMPLE Molecular cloning of cellulose synthase This Example describes the first tree cellulose synthase cDNA (PtCelA, 15 GenBank No. AF072131) cloned from developing secondary xylem of aspen trees using RSW1 cDNA.
Prior to the present invention, only partial clones of cellulose synthases from crop species and cotton GhCelA have been discovered, which have significant homology to each other. The present inventors have discovered and cloned a new full-20 length cellulose synthase cDNA, AraxCelA (GenBank No. AF062485) (Fig. 7, [SEQ ID NO: 4]), from an Arabidopsis primary library. AraxCelA is a new member of cellulose synthase and shows 63-85% identity and 72-90% similarity in amino acid sequence with other Arabidopsis CelA members.
Another cellulose synthase was cloned in aspen using a 32P-Iabeled 1651-bp 25 long EcoRI fragment of Arabidopsis CelA cDNA, which encodes a centrally located UDP-glucose binding domain, was used as a probe to screen about 500,000 pfu of a developing xylem cDNA library from aspen (Populus tremuloides) (Ge and Chiang, 1996). Four positive clones were obtained after three rounds of plaque purification. Sequencing the 3' ends of these four cDNAs showed that they were identical clones. The longest cDNA 30 clone was fully sequenced and determined to be a full-length cDNA having a 3232 bp nucleotide sequence (Fig. 1) [SEQ ID NO: 1], which encodes a protein of 978 amino acids [SEQ ID NO: 2].
Characterization of a cellulose synthase from aspen The first AUG codon of PtCelA was in the optimum context for initiation of 35 transcription on the basis of optimal context sequence described by Joshi (1987a) and Joshi et al. (1997). A putative polyadenylation signal (AATACA) was found 16 bp upstream of a polyadenylated tail of 28 bp, which is similar to the proposed plant structure (Joshi, 1987b). The 5' untranslated leader was determined to have 68 bp and the 3' untranslated trailor was 227 bp. Both of these regions have a typical length observed in many plant genes (Joshi, 1987a and Joshi, 1987b). This cDNA clone exhibited 90% amino acid sequence similarity with cellulose synthase from cotton (GhCelA,) and 71% with cellulose synthase from Arabidopsis (RSW1), suggesting that this particular tree 5 homolog also encodes a cellulose synthase.
The full length cDNA was designated PtCelA, and encodes a 110,278 Da polypeptide having an isoelectric point (pi) of 6.58 and 8 charged molecules. The hydropathy curve indicated that this particular cellulose synthase has eight transmembrane binding domains; two at the amino terminal and six at the carboxyl terminal, using the 10 method of Hoffman and Stoffel (1993). This protein structure is analogous to those of RSW1 and GhCelA. All of the conserved domains for UDP-glucose binding, such as QVLRW and conserved D residues, are also present in a cellulose synthase of the invention, e.g., PtCelA (Brown et al, 1996). Thus, based on sequence and molecular analyses, it was concluded that PtCelA encodes a catalytic subunit which, like RSW1 in 15 Arabidopsis, is essential for the cellulose biosynthesis machinery in aspen.
In situ localization of PtCelA mRNA transcripts along the developmental gradient defined by stem primary and secondary growth demonstrated that cellulose synthase expression is confined exclusively to developing xylem cells undergoing secondary wall thickening. This cell-type-specific nature of PtCelA gene expression was 20 also consistent with xylem-specific activity of cellulose synthase promoter (PtCelAP) based on heterologous promoter-B-glucuronidase (GUS) fusion analysis. Overall, the results provide several lines of evidence that cellulose synthase is the gene primarily responsible for cellulose biosynthesis during secondary wall formation in woody xylem of trees, such as aspen. Previous results by the inventors (Hu et al, 1999) showed that 25 cellulose and lignin are deposited in a compensatory fashion in wood. The discovery of a cellulose synthase in trees, such as aspen, permits the up-regulation of the protein to elevate cellulose production. Surprisingly, expression of CelA in trees suppressed lignin biosynthesis to further improve wood properties of trees.
Preparation of transgenic plants 30 The UDP-glucose binding sequence was subcloned into pBI121, which was used to prepare transgenic tobacco plants (Hu et al., 1998). The expression of a heterologous UDP-glucose binding sequence resulted in a remarkable growth-accelerating effect. This was surprising because current knowledge of the function of plant cellulose synthases teaches that a UDP-glucose sequence must remain intact with other functional 35 domains in CelA, e.g., the transmembrane domains, in order for cellulose synthase to initiate cellulose biosynthesis. The remarkable growth and tremendous increase in plant biomass observed in transgenic tobacco was due likely to an augmented deposition of cellulose, indicating that the UDP-glucose domain alone is sufficient for genetic augmentation of cellulose biosynthesis in plants.
Genome organization and expression of a novel cellulose synthase To confirm that the cDNA clone of Fig. 1 [SEQ ID NO: 1] was a cellulose 5 synthase, genomic Southern blot analysis was performed under both high and low stringency conditions using the cDNA. Genomic DNA from aspen was digested with Pstl (lane P), Hindfll (lane H) and EcoRl (lane E), and probed using a lkb 32P-labeled fragment from the 5' end of a cellulose synthase of Fig. 1. The Southern blot suggested the presence of a small family of cellulose synthase genes in aspen genome (Fig. 2, panels 10 a and b). Repeated screening of the aspen xylem cDNA library with various plant CelA gene-related probes always resulted in the isolation of the same cellulose synthase cDNA clone. This suggested that the cellulose synthase cDNA cloned (Fig. 1) [SEQ ID NO: 1], represents the primary and most abundant cellulose synthase-encoding gene in developing xylem of trees, such as aspen, where active cellulose deposition takes place. It also 15 indicates that manipulation of cellulose synthase gene expression can have a profound influence on cellulose biosynthesis in trees.
In situ hybridization Northern blot analysis of total RNA from the internodes of aspen seedling stems (Fig. 2, panel c) using the labeled probe (as described above) revealed the near 20 absence of cellulose synthase transcripts in tissues undergoing primary growth (internodes 1 to 4), and that the presence of cellulose synthase transcripts occurs during the secondary growth of stem tissues (internodes 5 to 11). However, weak northern signals in primary growth may only suggest that cellulose synthase gene expression is specific to xylem, of which there is little in primary growth tissue.
Xylogenesis in higher plants offers a unique model that involves sequential execution of cambium cell division, commitment to xylem cell differentiation, and culmination in xylem cell death (Fukuda, 1996). Although primary and secondary xylem cells originate from different types of cambia, namely procambium and inter/intrafasicular cambium, both exhibit conspicuous secondary wall development with massive cellulose 30 and lignin deposition (Esau, 1965). To further investigate spatial and temporal cellulose synthase gene expression patterns at the cellular level, in situ hybridization was used to localize cellulose synthase mRNA along the developmental gradient defined by stem primary and secondary growth.
Localization of cellulose synthase gene transcripts (RNA) in stem at 35 various growth stages was also observed. Fig. 3 shows transverse sections from 2nd, 4th and 6th internodes hybridized with digoxygenin (DIG)-labeled cellulose synthase antisense or sense (control) RNA probes, as described.
PtCelA transcripts were detected in young aspen stem sections by in situ hybridization with transcripts of highly variable 5' region of PtCelA cDNA (a 771 bp long fragment generated from Pstl and SacI). This region was first subcloned in the plasmid vector, pGEM,-3Zf (+) (Promega) for the production of digoxygenin (DIG)-labeled 5 transcripts using T7 (for antisense transcripts) and SP6 (for sense transcripts) RNA polymerase (DIG system: Boehringer Mannheim). Probes were subjected to mild alkaline hydrolysis by incubation in 100 mM NaHCC>3, pH 10.2 at 60 °C, which produced approximately 200 bp fragments.
Aspen young stems were prepared for sectioning by fixation in 4% (w/v) 10 paraformaldehyde in 100 mM phosphate buffer (pH 7.0) at 4 °C overnight, dehydrated through an ethanol series on ice, and embedded in Paraplast medium (Sigma). Ten jttm sections were mounted on Superfrost/plus (Fisher) slides at 42 °C overnight, dewaxed and then rehydrated through a descending ethanol series. The sections were incubated with proteinase K (10 fig/ml in 100 mM Tris-HCl, 50 mM EDTA, pH 7.5) for 30 min and were 15 post-fixed with FAA. The sections were acetylated with 0.33% (v/v) acetic anhydride in 0.1 M triethanolamine-HCI (pH 8.0) prior to hybridization. The sections were then incubated in a hybridization mixture (approximately 2 /ig/ml DIG-labeled probes, 50% (v/v) formamide, 2 X SSPE, 10% (w/v) dextran sulfate, 125 /ig/ml tRNA, pH 7.5) at 45 °C for 12-16 hrs. Nonhybridized single-stranded RNA probe was removed by treatment with 20 20 /ig/ml RNase A in TE buffer with 500 mM NaCl. The sections were washed at 50 °C. Hybridized DIG-labelled probe was detected on sections using anti-digoxygenin antiserum at a 1:1500 dilution, as described in the manufacturer's instruction (DIG system: Boehringer Mannheim). Sections were examined by Eclipse 400 light microscope (Nikon) and photographed.
During the primary growth stage (Fig. 3, panels a and b), strong expression of cellulose synthase was found localized exclusively to primary xylem (PX) cells. At this stage, young internodes are elongating, resulting in thickening of primary xylem cells through formation of secondary walls (Esau, 1968). The concurrence of shoot elongation with high expression of cellulose synthase strongly suggests the association of cellulose 30 synthase protein with secondary cell wall cellulose synthesis. Later stages of primary growth (Fig. 3, panel b) are characterized by the appearance of an orderly alignment of primary xylem cells. Active cellulose biosynthesis accompanies cell elongation-induced wall thickening, as indicated by the strong expression of cellulose synthase in these primary xylem cells.
At the beginning of secondary growth in older internodes, it was observed that expression of cellulose synthase is also exclusively localized to xylem cells (Fig. 3, panel c). Instead of elongation in internodes distal to the meristematic activity, growth at this stage is mainly radial due to thickening in secondary cell walls of secondary xylem.
At the same time, expression of PtCelA gene becomes localized to the secondary developing xylem cells (SX in Fig. 3, panel c), which is again consistent with the idea that PtCelA encodes a secondary cell wall cellulose synthase. At this stage, secondary xylem cells cover the elongated and differentiated primary xylem cells in which PtCelA gene 5 expression is no longer detectable (Fig. 3, panel c)-. These results demonstrate that expression of PtCelA gene is xylem-specific and the cellulose synthase of Fig. 1 [SEQ ID NO: 1] encodes a cellulose synthase associated with cellulose biosynthesis in secondary walls of xylem cells. To further confirm xylem-specific expression of cellulose synthase, a cellulose synthase gene promoter sequence was cloned and characterized for regulatory 10 activities.
Characterization of expression regulated bv cellulose synthase promoter A 5' 1,200 bp cDNA fragment of a cellulose synthase of Fig. 1 [SEQ ID NO: 1] was used as a probe to screen an aspen genomic library for 5' regulatory sequences of a novel cellulose synthase gene, PtCelA. The library was constructed by cloning aspen 15 genomic DNA fragments, generated from an SauSAl partial-digest and sucrose gradient-selected, into the BamHl site of a Lambda DASH II vector (Stratagene, La Jolla, CA). Five positive clones were obtained from about 150,000 pfu and Lambda DNA was purified. One clone having about a 20 kb DNA insert size was selected for restriction mapping and partial sequencing. This resulted in the identification of a 5' flanking region 20 of PtCelA gene of approximately 1 kb. This genomic fragment, designated PtCelAP (Fig. 4) [SEQ ID NO: 3], contained about 800 bp of promoter sequence, 68 bp of 5' end untranslated region and 160 bp of coding sequence. To investigate regulation of tissue-specific cellulose synthase expression at the cellular level, promoter activity was analyzed in transgenic tobacco plants by histochemical staining of a GUS protein. A PtCelAP-GUS 25 fusion binary vector was constructed in pBI121 with the 35S promoter replaced with PtCelAP [SEQ ID NO: 3) and introduced into tobacco (Nicotiana tabacum) as per Hu et al (1998).
Eleven independent transgenic lines harboring a CelAP-GUS fusion were generated. Fig. 5 shows a histochemical analysis of GUS expression driven by a cellulose 30 synthase promoter of the invention in transgenic tobacco plants. Transverse sections from the 3rd (panel a), 5th (panel b), 7th (panel c), and 8th (panels d and f) internodes were stained from GUS activity, and fluorescence microscopy was used to visualize expression under UV radiation.
GUS staining was detected exclusively in xylem tissue of stems, roots and 35 petioles. In stems, strong GUS activity was found localized to xylem cells undergoing primary (Fig. 5, panel a) and secondary growth (Fig. 5 panels b-d and f). GUS expression was confined to xylem cells in the primary growth stage and became more localized in developing secondary xylem cells during secondary growth. An entire section from the 8th internode stained for GUS activity (Fig. 5, panel f). These results are consistent with the in vivo expression patterns of cellulose synthase in aspen stems. Lignin autofluorescence was visualized after UV radiation. Phloem fibers, which are also active in cellulose and lignin biosynthesis (Fig. 5, panels d and e), did not show GUS activity, 5 suggesting that cellulose synthase gene expression is not associated with cellulose biosynthesis in cell types other than xylem. Examination of GUS activity in roots, stems, leaves, anthers and fruit also showed GUS expression in xylem tissue of all these organs suggesting that the described cellulose synthases are xylem-specific cellulose and expressed in all plant organs.
Characterization of promoter activity and cellular expression of a described cellulose synthase from one particular source (aspen) indicated hat expression produces a protein that encodes a secondary cell wall-specific cellulose synthase and is specifically compartmentalized in developing xylem cells. Characterization of the cellulose synthase gene promoter sequence not only confirms cell type-specific expression 15 of cellulose synthase, but also provides a method for over-expressing cellulose synthase in a tissue-specific manner to augment cellulose production in xylem.
Expression of cellulose synthase under tension stress As described earlier, a cellulose synthase promoter of the invention is involved in a novel gene regulatory phenomenon of cellulose synthase. To further 20 characterize a cellulose synthase of the invention, GUS expression driven by an aspen cellulose synthase promoter (PtCelAP) was observed in transgenic tobacco plants without or under tension stress. The stress was induced by bending and affixing the plants to maintain the bent position (e.g., tying) over a 40 hour period. Tangential and longitudinal sections were taken before bending, and 4 hrs, 20 hrs and 40 hrs after bending (panels a-d, 25 respectively).
The cellulose synthase promoter-Gt/S fusion binary constructs showed exclusive xylem-specific expression of GUS without any tension stress (Fig. 6, panel a). However, under tension stress conditions endured by angiosperms in nature, the transgenic tobacco plants induced xylem and phloem-specific expression on the upper side of the 30 stem within the first four hours of stress (Fig. 6, panel b).
This observation was surprising because during tension wood development fibers produce highly crystalline cellulose in order to provide essential mechanical strength to a bending stem. The present observation was the first showing of transcriptional up-regulation of a cellulose synthase, mediated through a cellulose synthase promoter that is 35 directly responsible for development of highly crystalline cellulose in trees. Furthermore, after 20 hrs of tension stress, both xylem and phloem exhibited GUS expression, but only on the upper side of the stem that was under tensile stress, i.e., GUS expression on the lower side was inhibited (Fig. 6, panel c). With extended stress (up to 40 hrs), GUS INTELLECTUAL PROPERTY OFFICE OF N2. 14 NOV 2005 expression was restricted to only one small region on the upper side of the stem where maximum tension stress was present (Fig. 6, panel d). Based on the observation of GUS signal in woody cells upon tension stress and the absence of GUS under compression or no stress, it was concluded that a cellulose synthase promoter of the invention has mechanical 5 stress responsive elements (MSREs) that turn cellulose synthase genes on and off depending on the presence and type of stress to the stem.
The results indicate that positive MSREs exist in a cellulose synthase promoter of the invention to bind transcription factors in response to tension stress for regulating the expression of cellulose synthase and increasing biosynthesis of higher 10 crystalline cellulose. This is evident based on the expression of GUS in xylem and phloem tissue at the upper side of the stem subjected to tension stress, but not when tissue on the lower side was subjected to compression or no stress. Furthermore, the tissue at the lower side of the stem, which was subjected to compression stress, showed no GUS expression, i.e., expression was turned off. This indicated the presence of negative MSREs, which 15 bind transcription factors to turn off expression of cellulose synthase at the lower side of the stem. Negative MSREs likely suppress development of highly crystalline cellulose in normal wood.
These results provide a mechanism for genetically engineering synthesis of highly crystalline cellulose in juvenile wood for enhancing strength properties, and for 20 synthesizing a higher percentage of cellulose in reaction wood. The positive MSREs and their cognate transcription factors are important in the synthesis of highly crystalline cellulose of high tensile strength, as are the negative MSREs and inhibition of cognate transcription factors thereto. The described method thus provides a starting point for cloning cDNAs for the transcription factors that bind to positive and negative MSREs 25 according to methods known in the art Constitutive expression of cDNAs for positive MSRE transcription factors allows the continuous production of highly crystalline cellulose in transgenic trees, while expression of antisense cDNAs for negative MSRE transcription factors inhibits those transcription factors so that cellulose synthase cannot turn off. This combination will assure continuous production of highly crystalline 30 cellulose in trees. • Genetic engineering of cellulose synthase in transgenic plants As discussed above, the nucleotide sequence of a described cellulose synthase ' e.g., PtCelA cDNA from aspen, shows significant homology with <kher polynucleotides encoding cellulose synthase proteins that have been suggested as authentic 35 cellulose synthase clones. To further characterize the activity of a cellulose synthase, four constructs were prepared in a PBI121 plasmid. 1) A constitutive plant promoter Cauliflower mosaic Virus 35S was operatively linked to PtCelA (35SP-PtCelA-s) and overexpressed in transgenic plants.
INTELLECTUAL PROPERTY OFFICE OF N.Z, 14 NOV 2005 This causes excess production of cellulose, resulting in a reduction in lignin content. Tobacco and aspen have been transformed with this construct. 2) Cauliflower mosaic Virus 35S was operatively linked to antisense RNA from PtCelA (35S-PtCelA-a) and constitutively expressed to reduce production of cellulose and increase lignin content in transgenic plants. This negative control construct may not result in healthy plants since cellulose is essential for plant growth and development. Aspen plants have been transformed with this construct. 3) Aspen 4CL-1 promoter (Hu et al., 1998) was operatively linked to PtCelA (Pt4CLP-PtCelA) (the 35S promoter of PBI121 was removed in this construct) and expressed in a tissue-specific manner in developing secondary xylem of transgenic aspen. This expression augments the native cellulose production and reduces lignin content of angiosperm tissues. Tobacco and aspen have transformed with this construct. 1 4) The cytoplasmic domain of PtCelA which contains three conserved regions thought to be involved in UDP-glucose binding during cellulose biosynthesis, was linked to a 35S promoter to produce binary constructs (35S-PtCelA UDP-glucose). Expression by this promoter permits constitutive expression of a UDP glucose binding domain of PtCelA in transgenic plants. Tobacco and aspen have been transformed with this construct. 35S-GUS constructs (pBI121, ClonTech, CA) were used as controls for 20 each experiment with the constructs. Transgenic tobacco plants were transformed with the constructs. The following table shows the general growth measurements of the TO tobacco plants. Plants carrying a PtCelA construct grew much faster than control plants carrying a pBI121 (control) construct. In comparing developmental 4CL and constitutive 35S promoter control of PtCelA expression, the 35S was more effective, permitting faster 25 growth of transgenic tobacco plants. The fastest growth was seen in transgenic plants carrying a 35S promoter driven UDP-G domain from PtCelA.
It is noted that TO generation plants can have carry over effects from their tissue culture treatments. Therefore, seeds were collected for testing this growth phenomenon in TI generations. The transgenic tobacco plants were analyzed for presence 30 of the transferred genes and all tested positive for the respective gene constructs.
TABLE Transgenic tobacco plant measurements after transfer in soi for about 1.5 months (N = 2) Construct Height Diameter Internode length No. of leaves Longest leaf 3SS-GUS 17 0.5 1 11 17 35S-PtCelA 77 1.0 6 13 37 35S-VDPG 83 1.0 6 13 37 4CLP-PtCelA 41 0.8 29 Note: All values were measured in centimeters, excluding number of leaves.
It will be appreciated by persons of ordinary skill in the art that the examples and preferred embodiments herein are illustrative, and that the invention may be practiced in a variety of embodiments which share the same inventive concept.
BIBLIOGRAPHY Hu et al, 1999, Nature Biotechnology, In Press Whetten etal., 1998, Ann Rev PI Physiol PI Mol Biol, 49: 585-609 5 Arioli et al., 1998, Science, 279: 717-720 Wu etal, 1998, PI Physiol, 117:1125 Hu et al, 1998, PNAS, 95: 5407-5412 Joshi et al, 1997, PMB, 35: 993-1001 Fukuda, 1996, Ann Rev PI Physiol PI Mol Biol, 47: 299-325 10 Pear et al, 1996, PNAS, 93:12637-12642 Haigler and Blanton, 1996, PNAS, 93: 12082-12085 Ge and Chiang, 1996, PI Physiol, 112: 861 Brown et al., 1996, Trends PI Sci., 1: 149-156 Delmer and Amor, 1995, PI Cell, 7: 987-1000 15 Hoffman and Stoffel, 1993, Biol Chem, Hoppe-Seyler 374: 166 Joshi, 1987, NAR, 15:6643-6653 Joshi, 1987, NAR, 15:9627-9640 Timmell, 1986, Compression Wood in Gymnopserms, Springer Verlag Esau, 1967, Plant Anatomy, Wiley and sons, NY 20 Higuchi, 1997, Biochemistry and Molecular Biology of Wood, Springer Verlag

Claims (32)

WHAT WE CLAIM IS:
1. An isolated polynucleotide sequence comprising a cellulose synthase promoter of SEQ ID NO:3, a sequence conservative variant thereof, or a functional fragment thereof which binds to a transcription factor in a plant cell.
2. The polynucleotide as set forth in claim 1 wherein the plant is a tree.
3. The polynucleotide as set forth in claim 1 wherein the polynucleotide is a stress-inducible promoter.
4. The polynucleotide as set forth in claim 1 wherein the polynucleotide comprises at least one MSRE.
5. The polynucleotide as set forth in claim 4 wherein the MSRE is a positive MSRE, a negative MSRE, or a combination thereof.
6. A vector comprising a promoter, a variant, or a fragment thereof as set forth in claim 1.
7. The vector as set forth in claim 6, wherein the promoter, variant, or fragment thereof is operatively linked to a polynucleotide encoding cellulose synthase, a UDP-glucose binding domain, or a polynucleotide encoding a polypeptide other than cellulose synthase.
8. A transgenic plant comprising a promoter, a variant, or a fragment thereof as set forth in claim 1.
9. A transgenic tree comprising a promoter, a variant, or a fragment thereof as set forth in claim 1.
10. A method of causing stress-induced gene expression in a plant cell comprising delivering into the cell a vector comprising a cellulose synthase promoter operatively linked to a gene, wherein the gene is expressed upon a mechanical stress to the plant. INTELLECTUAL PROPERTY OFFICE OF N.Z. 1 h NOV 2005 ^RECEIVED -36-
11. A method of increasing expression of a cellulose synthase in a plant comprising delivering into the plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter wherein the binding to the positive MSRE results in expression of a cellulose synthase, resulting in increased expression of cellulose in the plant.
12. A method as set forth in claim 11 wherein the plant is a tree.
13. A plant produced by the method as set forth in claim 11.
14. A tree produced by the method as set forth in claim 12.
15. A method of reducing expression of a cellulose synthase in a plant comprising delivering into the plant a DNA in an antisense orientation, the DNA in a sense orientation encoding protein that binds to a positive MSRE and results in expression of a cellulose synthase.
16. A plant produced by the method as set forth in claim 15.
17. A method as set forth in claim 15 wherein the plant is a tree.
18. A tree produced by the method as set forth in claim 17.
19. A method of increasing cellulose biosynthesis in a plant comprising delivering into the plant a cDNA encoding a protein that binds to a positive MSRE of a cellulose synthase promoter, wherein binding of the protein to the positive MSRE results in expression of a cellulose synthase.
20. A plant produced by the method as set forth in claim 19.
21. A method as set forth in claim 19 wherein the plant is a tree.
22. A tree produced by the method as set forth in claim 21.
23. A method of reducing cellulose biosynthesis in a plant comprising delivering into the plant a DNA in an antisense orientation, the DNA in a sense orientation encoding protein that binds to a positive MSRE of a cellulose synthase promoter. INTELLECTUAL PROPERTY OFFICE OF N.Z. 14 NOV 2005 RECEIVED -37-
24. A plant produced by the method as set forth in claim 23.
25. A method as set forth in claim 23 wherein the plant is a tree.
26. A tree produced by the method as set forth in claim 25.
27. A method of determining a positive mechanical stress responsive element (MSRE) in a cellulose synthase promoter comprising: (i) introducing into a plant a cellulose synthase promoter that has a portion deleted, the cellulose synthase promoter operatively linked to a polynucleotide encoding a reporter, and (ii) detecting a decrease in the amount of reporter in the plant after inducing a stress to the plant.
28. A method of determining a negative MSRE in a cellulose synthase promoter comprising: (i) introducing into a plant a cellulose synthase promoter that has a portion deleted, the cellulose synthase promoter operatively linked to a reporter gene, and (ii) detecting an increase in the amount of reporter in the plant after inducing a stress to the plant.
29. An isolated polynucleotide as claimed in claim 1 substantially as herein described with reference to any example thereof and with or without reference to the accompanying drawings.
30. A vector as claimed in claim 6 substantially as herein described with reference to any example thereof and with or without reference to the accompanying drawings.
31. A transgenic plant as claimed in any one of claims 8, 13, 16, 20 and 24 substantially as herein described with reference to any example thereof and with or without reference to the accompanying drawings.
32. A transgenic tree as claimed in any one of claims 9, 14, 18, 22 and 26 substantially as herein described with reference to any example thereof and with or without reference to the accompanying drawings. INTELLECTUAL PROPERTY OFFICE OF N2. 14 NOV 2005 RECEIVED -BBSS. A method as claimed in any one of claims 10,11, 15,19,23,27 and 28 substantially as herein described with reference to any example thereof and with or without reference to the accompanying drawings. INTELLECTUAL PROPERTY OFFICE OF N.Z n NOV 2005 RECEIVED
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