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Plant Physiology 132:1153-1161 (2003) © 2003 American Society of Plant Biologists Possibility of Bacterial Recruitment of Plant Genes Associated with the Biosynthesis of Secondary Metabolites1German Research Centre Biotechnology-Gesellschaft für Biotechnologische Forschung, Mascheroder Weg 1, 38124 Braunschweig, Germany (H.B.B., R.M.); and Institut für Pharmazeutische Biologie, Technical University Braunschweig, Mendelssohnstrasse 1, 38106 Braunschweig, Germany (R.M.)
Microorganisms and plants synthesize an immense variety of metabolites,
which are generally classified into two major groups based on their function.
Primary metabolites are essential for growth and universally used, whereas
secondary metabolism is highly diverse and variable and plays a role for the
survival of the producing organism within its natural habitat
(Demain, 1989
The ability to form thousands of structurally diverse natural products due
to secondary metabolism is considered a typical feature of plants and
microbes. These compounds are usually classified into major groups depending
on the basic building blocks of the final structure, e.g. the terpenes that
are formed from isoprenoid moieties, or the polyketides, which are assembled
from short chain carboxylic acids. These products not only play an important
role for their producers in the natural habitat, but also for human health (as
opposed to their name indicating "of secondary interest"), because
almost 50% of the most important medications are derived from these so-called
natural products (Demain,
1999 Although approximately 170,000 secondary metabolites are known according to the Chapman & Hall dictionary of natural products (see http://www.chemnetbase.com/scripts/dnpweb.exe), there is a clear trend as to which group of organisms produces what type of compounds. For example, alkaloids (e.g. morphine) and phenylpropanoids are considered typical plant metabolites, whereas nonribosomally biosynthesized peptides (e.g. cyclosporin) are regarded as microorganism specific. Thus, a variety of structures, biosynthetic pathways, proteins, and genes are believed to be only found in plants, raising a question of the origin of biosynthetic pathways. Did plants "invent" all of these pathways without using and adapting genetic information from prokaryotes?
In contrast to this generally accepted hypothesis, this update will show
that a variety of metabolic pathways that were regarded to be present only in
plants have in the recent years also been found in prokaryotes. Microorganisms
with a complex life cycle and large genomes (e.g. myxobacteria
[Shimkets, 1993
PAL is a ubiquitous enzyme in higher plants; it catalyzes the deamination of L-Phe to trans-cinnamic acid (Fig. 1). Without PAL, our world would be less colorful due to the lack of flavonoids and anthocyanins. Moreover, plants would most likely not exist in their current form due to the lack of lignin. PAL is the first enzyme in the conversion of L-Phe to benzoic acid (Fig. 1), an important structural element in a variety of natural products from plants (e.g. cocaine [Leete, 1990  ],
paclitaxel [Walker and Croteau,
2000], and fungi, e.g. zaragozic acid
[Bergstrom et al., 1995]).
In prokaryotes, only very few cinnamic and benzoic acid derived metabolites
have been described, presumably due to the rarity of PAL in these organisms.
However, there is evidence for two PAL independent pathways to benzoate: the
anaerobic degradation of L-Phe
(Schneider et al., 1997
PAL is highly homologous to His ammonia lyase (HAL), the enzyme catalyzing
an analogous deamination of His to trans-urocanate in pro- and eukaryotes and,
therefore, initiates His degradation in almost all organisms
(Michal, 1999
The presence of a PAL activity in prokaryotes was first described in 1970
for Streptomyces verticillatus, which produces cinnamide
(Emes and Vining, 1970
The only case in which prokaryotic PAL activity has been clearly correlated
to a biosynthetic protein is EncP from S. maritimus, which is needed
for enterocin biosynthesis (Xiang and
Moore, 2002
The absence of steroids in prokaryotes has been close to a dogma for many years. Until recently, only two bacterial species were known to have the triterpenes typical for eukaryotes: 4,4-dimethyl, 4-methyl, and 4-desmethylcholesterols in the methylotrophic bacterium Methylococcus capsulatus (Bird et al., 1971 ) and 8(9)-cholesten-3 -ol in the myxobacterium
Nannocystis excedens (Kohl et
al., 1983). Instead of steroids, bacteria often employ
squalene-derived pentacyclic terpenes of the hopanoid type to build their
membranes (Kannenberg and Poralla,
1999). Very recently, a detailed analysis of many myxobacterial
strains from different genera revealed the presence of several steroids, which
were previously only known from eukaryotes
(Bode et al., 2003;
Fig. 3).
Strains of the myxobacterium N. excedens are potent prokaryotic
steroid producers that contain more than 2% steroids in their cellular dry
weight and 10 distinct steroids. Almost all intermediates and side products of
the biosynthesis of the major steroid in mammals, 5-cholesten-3
Studies with different types of steroid biosynthesis inhibitors underline
the differences between the prokaryotic and the eukaryotic enzymes. No
inhibition was observed in vivo in myxobacteria by terbinafin, tolnaftat, or
AMO1618, well-known inhibitors of the eukaryotic squalene epoxidase. No
inhibition of hydroxymethyl glutaryl-CoA reductase with fluvastatin was
observed (Bode et al., 2003
Although Nannocystis strains produce quantities of steroids equal
to that in eukaryotes, their function in myxobacteria remains a mystery. No
difference in reproduction time, ethanol tolerance, fatty acid composition, or
swarming could be observed upon comparing a wild-type strain of S.
aurantiaca with a cycloartenol knockout
(Bode et al., 2003
The CHS and stilbene synthase (STS) superfamily of PKSs appears to be ubiquitous in higher plants. STSs, e.g. resveratrol synthase, produce the stilbene backbone as a key reaction in the biosynthesis of stilbene type phytoalexins (Fig. 1). CHS is a key enzyme in the biosynthesis of flavonoids, which exhibit a wide range of biochemical, physiological, and ecological activities. Resveratrol and CHSs condense 4-coumaroyl-CoA with three molecules of malonyl-CoA, which results in products differing in the newly formed ring systems (resveratrol and naringenin chalcone; see Figs. 1 and 4). The same type of condensing reaction is utilized by the 2-ketoacyl-ACP synthases of fatty acid biosynthesis. However, the available data show that these enzymes share little overall homology with either resveratrol synthase or CHS (Schröder, 1999 ). Over
the last couple of years, a series of new additions to the CHS/STS superfamily
has been reported from plants, which differ from the enzymes described above
by utilizing non-phenylpropanoid starter units, varying numbers of
condensation reactions, and different cyclization patterns (e.g. acridone
synthase [Junghanns et al.,
1995] and 2-pyrone synthases
[Eckermann et al., 1998;
compare with Fig. 5]).
Unexpectedly, in 1999, "a new type of polyketide biosynthetic
pathway" was reported in bacteria. This pathway is used for the assembly
of flaviolin (Fig. 5), a small
aromatic metabolite in streptomycetes
(Funa et al., 1999
Thus far, none of the few characterized bacterial type III PKSs employs the
typical plant starter molecule, 4-coumaroyl-CoA (see Figs.
4 and
5), suggesting a distinction
between bacterial and plant type III PKS enzymes. This suggestion might in
fact be wrong because several bacterial gene products might employ
4-coumaroyl-CoA as a starter molecule. For example, the purple photosynthetic
bacterium Rhodospirillum centenum has a photoactive yellow protein
(PYP) domain containing the chrompohore 4-coumarate that is part of a
bacterial photoreceptor with similarity to plant phytochromes
(Jiang et al., 1999
Dopa-decarboxylase, an enzyme that was considered to be plant and animal specific, can also be found in myxobacteria. It is closely related to plant enzymes and does not group phylogenetically with bacterial amino acid decarboxylases (AADs). AADs belong to the large group of pyridoxalphosphate-dependent enzymes, which contain a conserved domain (protein families database 00282 of the Sanger Centre). They are necessary for the formation of biogenic amines with important physiological properties in animals (Voet and Voet, 1995 ).
In plants, the AADs catalyzing Tyr, L-dopa, and Trp decarboxylation
represent branching points from primary into secondary metabolism. Tyramine
and dopamine serve as precursors for the formation of a variety of alkaloids
such as isoquinoline alkaloids (see Fig.
1, e.g. morphine and codeine;
Kutchan and Zenk, 1993;
Facchini et al., 2000).
Phylogenetic analysis of nine different types of
pyridoxalphosphate-dependent AADs
(Sandmeier et al., 1994
Group II contains prokaryotic and eukaryotic AADs of different function
(but only L-Glu decarboxylase and L-His decarboxylase
had been reported from prokaryotes before the Sandmeier study was published),
which led the investigators to assume that the divergence between these
enzymes occurred before the development of their catalytic specificities.
Thus, one would expect a DDC of prokaryotic origin to show the highest
similarities to group II AADs of prokaryotic origin, despite possible
differences in substrate specificity
(Müller et al.,
2000
A DDC encoded in the chromosome of the myxobacterium S. cellulosum
So ce90 was found and initially characterized after functional expression in
Escherichia coli. Although the function of the corresponding protein
in the bacterium is still unclear, it could be shown that the DDC shares more
biochemical properties with the subgroup of plant DDCs than with those of
animal origin (Müller et al.,
2000
We show the presence of what was formerly regarded as plant-specific biosyntheses and pathways in prokaryotes, mostly in actinomycetes and myxobacteria. The question as to which class of organisms invented these genes, enzymes, and pathways cannot yet be answered because we are only beginning to reveal these features common to prokaryotes and eukaryotes. However, there is certainly a possibility that at least some of the genes that were regarded as typical for plants might originate from prokaryotes. What is the function of these pathways in prokaryotes, and why were they discovered only recently? The answer to the second part of the question is the wealth of information only now becoming available from various sequencing projects of prokaryotic organisms. The first part of the question is more difficult to answer. First, the accumulation of typical plant biosynthetic pathways in myxobacteria and actinomycetes might be due to their saprophytic life style and close proximity to plants in their soil environment as mentioned in the introduction. However, several other soil-inhabiting bacteria have been sequenced (e.g. B. subtilis) that do not show the observed accumulation of plant-like genes. Secondly, myxobacteria and actinomycetes have the largest genomes of all bacteria known so far with 12.2 Mb for S. cellulosum (Pradella et al., 2002 ) and 8.6 Mb for S. coelicolor
(Bentley et al., 2002). These
larger sized genomes might have resulted from "gene picking" from
various sources during their evolution. However, integrating and maintaining
additional genes should result in some benefit for the organism because a
large genome requires more energy to maintain. Why are there not more
soil-inhabiting genera of prokaryotes with large genomes? Perhaps the reason
is that we only know a small fraction of the microorganisms present in the
soil environment. This is due to our inability to isolate and grow most of
them (Zengler et al., 2002).
The lifestyle of myxobacteria and streptomycetes might be an additional reason
because they can be regarded as two of the most complex prokaryotes.
Myxobacteria build tree-like fruiting bodies
(Reichenbach, 1993;
Fig. 6) and streptomycetes form
aerial mycelium (Hopwood,
1999) under starvation conditions, and their development
culminates in the formation of spores for survival under stressful
conditions.
These are exciting times to study metabolism in plants and microbes because we are currently gaining a deeper insight into the processes underlying development and evolution. In the future, we will be able to base our research on genome and proteome data, which will hopefully reveal further details of the molecular basis of complex developmental processes and the function of "plant-like" genes in microorganisms.
We would like to thank Eric Nudleman and Lars Jelsbak for critical reading of the manuscript and Thomas Hartmann and Dale Kaiser for helpful comments. Received December 26, 2002; returned for revision March 8, 2003; accepted April 17, 2003.
http://www.plantphysiol.org/cgi/doi/10.1104/pp.102.019760.
1 This work was supported by the Deutsche Forschungsgemeinschaft (research
grant nos. Mu 1254/3, Mu 1254/4, and Bo 1834/1).
2 Present address: Biochemistry Department, Bademan Center B400, Stanford
University, CA 94305-5307. * Corresponding author; e-mail ROM{at}GBF.DE; fax 49–531–6181284.
Bangera MG, Thomashow LS (1999) Identification and characterization of a gene cluster for synthesis of the polyketide antibiotic 2,4-diacetylphloroglucinol from Pseudomonas fluorescens Q2–87. J Bacteriol 181: 3155–3163 Bentley SD, Chater KF, Cerdeno-Tarraga AM, Challis GL, Thomson NR, James KD, Harris DE, Quail MA, Kieser H, Harper D et al. (2002) Complete genome sequence of the model actinomycete Streptomyces coelicolor A3(2). Nature 417: 141–147[CrossRef][Medline] Bergstrom JD, Dufresne C, Bills GF, Nallin-Omstead M, Byrne K (1995) Discovery, biosynthesis, and mechanism of action of the zaragozic acids: potent inhibitors of squalene synthase. Annu Rev Microbiol 49: 607–639[CrossRef][Medline] Bird C, Lynch J, Pirt F, Reid W, Brooks C (1971) Steroids and squalene in Methylococcus capsulatus grown on methane. Nature 230 Bode HB, Zeggel B, Silakowski B, Wenzel SC, Reichenbach H, Müller R (2003) Steroid biosynthesis in prokaryotes: identification of myxobacterial steroids and cloning of the first bacterial 2,3(S)-oxidosqualene cyclase from the myxobacterium Stigmatella aurantiaca. Mol Microbiol 47: 471–481[CrossRef][Web of Science][Medline] Breese K, Boll M, Alt-Morbe J, Schagger H, Fuchs G (1998) Genes coding for the benzoyl-CoA pathway of anaerobic aromatic metabolism in the bacterium Thauera aromatica. Eur J Biochem 256: 148–154[Medline]
Christenson J, Dairman W, Udenfired S (1972) On
the identity of DOPA decarboxylase and 5-hydroxytryptophan decarboxylase.
Proc Natl Acad Sci USA 69:
343–347 Croteau R, Kutchan T, Lewis N (2000) Natural products (secondary metabolites). In B Buchanan, W Gruissem, R Joneas, eds, Biochemistry and Molecular Biology of Plants. American Society of Plant Biologists, Rockville, MD, pp 1250–1268 Demain A (1989) Functions of secondary metabolites. In C Hirshberger, S Queener, G Hegemann, eds, Genetics and Molecular Biology of Industrial Microorganisms. American Society for Microbiology, Washington, DC, pp 1–11 Demain A (1999) Pharmaceutically active secondary metabolites of microorganisms. Appl Microbiol Biotechnol 52: 455–463[CrossRef][Web of Science][Medline] Eckermann S, Schröder G, Schmidt J, Strack D, Edrada RA, Helariutta Y, Elomaa P, Kotilainen M, Kilpeläinen I, Proksch P et al. (1998) New pathway to polyketides in plants. Nature 396: 387–390[CrossRef] Emes AV, Vining LC (1970) Partial purification and properties of L-phenylalanine ammonia-lyase from Streptomyces verticillatus. Can J Biochem 48: 613–622[Medline] Facchini PJ, Huber-Allanach KL, Tari LW (2000) Plant aromatic-amino acid decarboxylases: evolution, biochemistry, regulation, and metabolic engineering applications. Phytochemistry 54: 121–138[CrossRef][Web of Science][Medline] Funa N, Ohnishi Y, Fujii I, Shibuya M, Ebizuka Y, Horinouchi S (1999) A new pathway for polyketide synthesis in microorganisms. Nature 400: 897–899[CrossRef][Medline] Gerth K, Jansen R, Reifenstahl G, Höfle G, Irschik H, Kunze B, Reichenbach H, Thierbach G (1983) The myxalamids, new antibiotics from Myxococcus xanthus (Myxobacterales): I. Production, physico-chemical and biological properties, and mechanism of action. J Antibiotics 36: 1150–1156[Medline] Grabley S, Thiericke R (1999) The impact of natural products on drug discovery. In S Grabley, R Thiericke, eds, Drug Discovery from Nature. Springer, Berlin, pp 3–37 Grond S, Langer HJ, Henne P, Sattler I, Thiericke R, Grabley S, Zähner H, Zeeck A (2000) Secondary metabolites by chemical screening: 39. Acyl alpha-L-rhamnopyranosides, a novel family of secondary metabolites from Streptomyces sp.: isolation and biosynthesis. Eur J Org Chem 6: 929–937 Harborne J (1993) Introduction to Ecological Biochemistry, Ed 4. Academic Press, London Hartmann T (1996) Diversity and variability of plant secondary metabolism: a mechanistic view. Entomol Exp Applic 80: 177–188 Hellingwerf KJ (2002) The molecular basis of sensing and responding to light in microorganisms. Int J Gen Mol Microbiol 81: 51–59 Hertweck C, Moore BS (2000) A plant-like biosynthesis of benzoyl-CoA in the marine bacterium "Streptomyces maritimus." Tetrahedron 56: 9115–9120[CrossRef] Hill AM, Harris JP, Siskos AP (1998) Investigation of glycerol incorporation into soraphen A. Chem Commun: 2361–2362
Hopwood DA (1999) Forty years of genetics with
Streptomyces: from in vivo through in vitro to in silico.
Microbiology 145:
2183–2202 Jansen R, Washausen P, Kunze B, Reichenbach H, Höfle G (1999) Antibiotics from gliding bacteria: LXXXIII. The crocacins, novel antifungal and cytotoxic antibiotics from Chondromyces crocatus and Chondromyces pediculatus (Myxobacteria): isolation and structure elucidation. Eur J Org Chem 5: 1085–1089
Jiang Z, Swem LR, Rushing BG, Devanathan S, Tollin G, Bauer
CE (1999) Bacterial photoreceptor with similarity to
photoactive yellow protein and plant phytochromes. Science
285:
406–409 Junghanns KT, Kneusel RE, Baumert A, Maier W, Gröger D, Matern U (1995) Molecular cloning and heterologous expression of acridone synthase from elicited Ruta graveolens L. cell suspension cultures. Plant Mol Biol 27: 681–692[CrossRef][Web of Science][Medline] Kannenberg EL, Poralla K (1999) Hopanoid biosynthesis and function in bacteria. Naturwissenschaften 86: 168–176[CrossRef][Web of Science]
Kawalleck P, Keller H, Hahlbrock K, Scheel D, Somssich I
(1993) A pathogen-responsive gene of parsley encodes tyrosine
decarboxylase. J. Biol. Chem.
268:
2189–2194 Kohl W, Gloe A, Reichenbach H (1983) Steroids from the myxobacterium Nannocystis exedens. J Gen Microbiol 129: 1629–1635 Kutchan T, Zenk M (1993) Enzymology and molecular biology of benzophenanthridine alkaloid biosynthesis. J Plant Res 3: 165–173
Kutchan TM (2001) Ecological arsenal and
developmental dispatcher. The paradigm of secondary metabolism. Plant
Physiology 125:
58–60 Kyndt JA, Meyer TE, Cusanovich MA, Van Beeumen JJ (2002) Characterization of a bacterial tyrosine ammonia lyase, a biosynthetic enzyme for the photoactive yellow protein. FEBS Lett 512: 240–244[CrossRef][Medline] Leete E (1990) Recent developments in the biosynthesis of the tropane alkaloids. Planta Med 56: 339–352[Medline] Li T, Choroba O, Hong H, Williams D, Spencer J (2001) Biosynthesis of the vancomycin group of antibiotics: characterisation of a type III polyketide synthase in the pathway to (S)-3,5-dihydroxyphenylglycine. Chem Commun 20: 2156–2157[CrossRef] Mahmud T, Bode HB, Silakowski B, Kroppenstedt RM, Xu M, Nordhoff S, Höfle G, Müller R (2002) A novel biosynthetic pathway providing precursors for fatty acid biosynthesis and secondary metabolite formation in myxobacteria. J Biol Chem 277: 23768–32774 Michal G (1999) Biochemical Pathways, Vol 1: Spektrum Akad. Verlag, Heidelberg Moore BS, Höpke JN (2001) Discovery of a new bacterial polyketide biosynthetic pathway. ChemBioChem 2: 35–38[CrossRef][Web of Science][Medline] Müller R, Gerth K, Brandt P, Blöcker H, Beyer S (2000) Identification of an L-dopa decarboxylase gene from Sorangium cellulosum So ce90. Arch Microbiol 173: 303–306[CrossRef][Medline] Ourisson G, Nakatani Y (1994) The terpenoid theory of the origin of cellular life: the evolution of terpenoids to cholesterol. Chem Biol 1: 11–23[CrossRef][Medline]
Pfeifer V, Nicholson GJ, Ries J, Recktenwald J, Schefer AB,
Shawky RM, Schroder J, Wohlleben W, Pelzer S (2001) A
polyketide synthase in glycopeptide biosynthesis: the biosynthesis of the
non-proteinogenic amino acid (S)-3,5-dihydroxyphenylglycine. J Biol
Chem 276:
38370–38377 Poralla K, Muth G, Hartner T (2000) Hopanoids are formed during transition from substrate to aerial hyphae in Streptomyces coelicolor A3(2). FEMS Microbiol Lett 189: 93–95[CrossRef][Web of Science][Medline]
Porter JA, Young KE, Beachy PA (1996)
Cholesterol modification of hedgehog signaling proteins in animal development.
Science 274:
255–259 Pradella S, Hans A, Sproer C, Reichenbach H, Gerth K, Beyer S (2002) Characterisation, genome size and genetic manipulation of the myxobacterium Sorangium cellulosum So ce56. Arch Microbiol 178: 484–492[CrossRef][Medline] Reichenbach H (1993) Biology of the myxobacteria: ecology and taxonomy. In M Dworkin, D Kaiser, eds, Myxobacteria II. American Society for Microbiology, Washington, DC, pp 13–62 Reichenbach H, Dworkin M (1992) The Myxobacteria. In A Balows, HG Trüper, M Dworkin, W Harder, K-H Schleifer, eds, The Procaryotes, Ed 2. Springer-Verlag, New York, pp 3416–3487 Reichenbach H, Höfle G (1994) Discovery of a new antifungal mechanism of action, soraphen: an almost-success story. In JH Walsdorff, ed, Scientific Annual Report. Gesellschaft für Biotechnologische Forschung mbH, Braunschweig, Germany, pp 5–22 Reichenbach H, Höfle G (1999) Myxobacteria as producers of secondary metabolites. In S Grabley, R Thieriecke, eds, Drug Discovery from Nature. Springer Verlag, Berlin, pp 149–179 Rother R, Poppe L, Viergutz S, Langer B, Retey J (2001) Characterization of the active site of histidine ammonia-lyase from Pseudomonas putida. Eur J Biochem 268: 6011–6019[Web of Science][Medline] Sandmeier E, Hale T, Christen P (1994) Multiple evolutionary origin of pyridoxal-5'-phosphate-dependent amino acid decarboxylases. Eur J Biochem 221: 997–1002[Web of Science][Medline] Schneider S, Mohamed ME, Fuchs G (1997) Anaerobic metabolism of L-phenylalanine via benzoyl-CoA in the denitrifying bacterium Thauera aromatica. Arch Microbiol 168: 310–320[CrossRef][Medline] Schröder J (1999) The chalcone/stilbene synthase-type family of condensing enzymes. In D Barton, K Nakanishi, O Meth-Cohn, eds, Comprehensive Natural Products Chemistry, Vol 1. Elsevier, Amsterdam, pp 749–771
Schuster B, Retey J (1995) The mechanism of
action of phenylalanine ammonia-lyase: the role of prosthetic dehydroalanine.
Proc Natl Acad Sci U S A 92:
8433–8437 Schwede TF, Retey J, Schulz GE (1999) Crystal structure of histidine ammonia-lyase revealing a novel polypeptide modification as the catalytic electrophile. Biochemistry 38: 5355–5361[CrossRef][Medline] Shimkets L (1993) The myxobacterial Genome. In M Dworkin, D Kaiser, eds, Myxobacteria II. American Society for Microbiology, Washington, DC, pp 85–108 Silakowski B, Nordsiek G, Kunze B, Blöcker H, Müller R (2001) Novel features in a combined polyketide synthase/non-ribosomal peptide synthetase: the myxalamid biosynthetic gene cluster of the myxobacterium Stigmatella aurantiaca Sg a15. Chem Biol 8: 59–69[CrossRef][Web of Science][Medline] Staunton J, Weissman KJ (2001) Polyketide biosynthesis: a millennium review. Nat Prod Rep 18: 380–416[CrossRef][Web of Science][Medline] Strohl W (1997) Biotechnology of Antibiotics, Ed 2, Vol 82. Marcel Dekker, New York Stryer L (1995) Biochemistry, Ed 4. W. H. Freeman and Company, New York Trowitzsch-Kienast W, Forche E, Wray V, Reichenbach H, Jurkiewicz E, Hunsmann G, Höfle G (1992) Phenalamide, neue HIV-Inhibitoren aus Myxococcus stipitatus Mx s40. Liebigs Ann Chem 16: 659–664 Voet D, Voet J (1995) Biochemistry, Ed 2. Wiley, New York
Walker K, Croteau R (2000) Taxol biosynthesis:
molecular cloning of a benzoyl-CoA:taxane 2alpha-O-benzoyltransferase
cDNA from taxus and functional expression in Escherichia coli.
Proc Natl Acad Sci USA 97:
13591–13596
Ware J, Dworkin M (1973) Fatty acids of
Myxococcus xanthus. J Bacteriol
115:
253–261
Xiang LK, Moore BS (2002) Inactivation,
complementation, and heterologous expression of encP, a novel bacterial
phenylalanine ammonia-lyase gene. J Biol Chem
277:
32505–32509
Zengler K, Toledo G, Rappe M, Elkins J, Mathur EJ, Short JM,
Keller M (2002) Cultivating the uncultured. Proc Natl
Acad Sci USA 99:
15681–15686 This article has been cited by other articles:
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PHE AMMONIUM LYASE (PAL),...
TRUE STEROIDS FROM PROKARYOTES
