Organic compounds -- part of the class 532-570 series – Organic compounds – Carbohydrates or derivatives
Reexamination Certificate
1999-02-09
2002-07-23
Geist, Gary (Department: 1623)
Organic compounds -- part of the class 532-570 series
Organic compounds
Carbohydrates or derivatives
C536S001110, C536S115000, C536S124000
Reexamination Certificate
active
06423834
ABSTRACT:
DESCRIPTION
Technical Field
The invention relates to KDO aldolase (EC 4.1.2.23) having a broad substrate specificity with respect to its reverse reaction and to condensation reactions employing such KDO aldolase for synthesizing a broad range of 6-9 carbon 2-keto-3-deoxy-onic acids, viz. 2-keto-3-deoxy-hexulosonate, 2-keto-3-deoxy-heptulosonate, 2-keto-3-deoxy-octulosonate, and 2-keto-3-deoxy-nonulosonate. More particularly, the invention relates to
Aureobacterium barkerei
strain KDO-37-2 (ATCC 49977), to KDO aldolase produced by and isolated from such bacteria, to the employment of such KDO aldose with respect to the synthesis of 2-keto-3-deoxy-onic acids such as 3-deoxy-D-manno-2-octulosonic acid (D-KDO) and to the use of protected forms of such 2-keto-3-deoxy-onic acids for the production of 7 and 8 carbon aldoses by means of radical mediated decarboxylation.
BACKGROUND OF THE INVENTION
2-Keto-3-deoxy-octulosonic acid (KDO) appears as a ketosidic component of all Gram-negative bacteria for which a KDO determination has been made. More particularly, 3-deoxy-D-manno-2-octulosonic acid (D-KDO) is widely found in Gram-negative bacteria. KDO is incorporated into lipopolysaccharides and is localized, as such, within the outer membrane compartment of Gram-negative bacteria. KDO appears to be a vital component of Gram-negative bacteria. KDO can also occur as an acidic exopolysaccharide. In such instances, the KDO can serve as part of a K-antigen.
As illustrated in
FIG. 7
, the biosynthetic incorporation of KDO into lipopolysaccharides consists of two steps, i.e.:
1. Activation of KDO to form CMP-KDO by means of CMP-KDO synthetase (EC 2.7.7.38); and then
2. Coupling of the activated CMP-KDO to lipid A precursor to form lipid A-KDO by means of KDO transferase.
The rate-limiting step with respect to the biosynthesis of KDO containing lipopolysaccharides is the activation of the KDO moiety, i.e., the formation of CMP-KDO. Accordingly, inhibitors of CMP-KDO synthetase are potentially useful as antibacterial agents.
Several chemical and enzymatic synthetic routes have been developed for the synthesis of KDO and its analogs. One route for the chemical synthesis of KDO employs Cornforth's method. (Ghalambor, M. et al.
J. Biol. Chem.
1966, 241, 3207 and Hershberger, C. et al.
J. Biol. Chem.
1968, 243, 1585.) The chemical synthesis of KDO produces multiple enantiomers. In order to obtain enantiomerically pure D-KDO, a separation step must be incorporated into the chemical synthetic route.
Synthetic routes employing enzymes are more stereospecific than chemical synthetic routes. An enzymatic synthetic route employing KDO-8 phosphate synthase and KDO-8-P phosphatase as catalysts and arabinose-5-P and PEP as substrates is illustrated in FIG.
7
. (Bednarski, M. et al.
Tetrahedron Letters
1988, 29, 427.) An alternative enzymatic synthetic route employs sialic acid aldolase. (Augé, C. et al.
Tetrahedron
1990, 46, 201.)
An enzymatic synthetic route employing the reverse reaction of KDO aldolase for a micromolar scale synthesis of KDO is disclosed by Ghalambor. (Ghalambor, M. et al.,
J. Biol. Chem.
1966, 241, 3222.) The synthetic route described by Ghalambor employs KDO aldolase isolated from
Aerobacter cloacae
. The reverse reaction of KDO aldolase is driven by employing high substrate levels, i.e. high concentrations of D-arabinose and D-pyruvate. Ghalambor discloses that there is a 41% yield with this enzyme and narrow substrate specificity.
KDO aldolase (EC 4.1.2.23) is known to be inductively produced by several bacteria, viz.
Escherichia coli
, strains 0111, B, and K-12,
Salmonella typhimurium, Salmonella aldelaide
, and
Aerobacter cloacae
. Ghalambor discloses that all of these known KDO aldolases have comparable activities. For example, all of these KDO aldolases hydrolyze 3-deoxy-D-manno-2-octulosonic acid to form D-arabinose and pyruvate in a forward reaction. As indicated above, Ghalambor also discloses that known KDO aldolase may be employed in a reverse reaction to condense D-arabinose and pyruvate to form 3-deoxy-D-manno-2-octulosonic acid. The substrate specificity of known KDO aldolases with respect to this reverse reaction is confined to D-arabinose and has been specifically shown to lack a measurable specificity for D-ribose in connection with this reverse reaction.
What was needed was an enzymic synthetic route for the production of a wide range of 2-keto-3-deoxy-onic acids and analogs thereof potentially having activity as inhibitors of CMP-KDO synthetase.
What was also needed was a method of converting 2-keto-3-deoxy-onic acids to high-carbon 2-deoxy aldoses.
SUMMARY OF THE INVENTION
Aureobacterium barkerei
strain KDO-37-2 (ATCC 49977) and KDO aldolase (EC 4.1.2.23) isolated therefrom are disclosed therein. KDO aldolase catalyzed condensation employing this enzyme has been demonstrated to be effective for the synthesis of KDO and analogs. The reactions are stereospecific with formation of a new R-stereocenter at C-3 from D-arabinose and related substrates. Decarboxylation of the aldolase products provides a new route to heptose and octose derivatives.
Unlike known KDO aldolases which have a narrow substrate specificity, the KDO aldolase isolated from this source is disclosed to have a very wide substrate specificity with respect to catalyzing its reverse reaction, i.e. the condensation of aldoses with pyruvate. In particular, 3-deoxy-D-manno-2-octulosonic acid (D-KDO) can be synthesized from D-arabinose and pyruvate in 67% yield. Furthermore, studies with respect to the substrate specificity of the enzyme using more than 20 natural and unnatural sugars indicate that this enzyme widely accepts trioses, tetroses, pentoses and hexoses as substrates, especially the ones with R configuration at 3 position. The substituent on 2 position has little effect on the aldol reaction. Nine of these substrates are submitted to the aldol reaction to prepare various 2-keto-3-deoxy-onic acids, including D-KDO, 3-deoxy-D-arabino-2-heptulosonic acid (D-DAH), 2-keto-3-deoxy-L-gluconic acid (L-KDG), and 3-deoxy-L-glycero-L-galacto-nonulosonic acid (L-KDN). The attack of pyruvate appears to take place on the re face of the carbonyl group of acceptor substrates, a facial selection complementary to sialic acid aldolase (si face attack) reactions. The aldolase products can be converted to aldoses via radical-mediated decarboxylation. For example, decarboxylation of pentaacetyl KDO and hexaacetyl neuraminic acid gives penta-O-acetyl-2-deoxy-&bgr;,3-D-manno-heptose and penta-O-acetyl-4-acetamido-2,4-dideoxy-&bgr;-D-glycero-D-gala cto-octose, respectively.
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Madson, et al., “The Oxidation of 3-Deoxy-D-erythro-hexos-2-ulose (“3-Deoxyglucosone”) to 3-Deoxy-D-erythro-2-hexulosonic acid (“2-Keto-3-deoxy-D-gluconate”) by D-Glucose Oxidase”,Carbohyd. Res. 115: 288-291 (1983).
Sengupta, et al., “Structural Analogs of 2-Keto-3-deoxy-D-mannooctulosonic Acid”,Ind. J. Chem. Sect. B 25B: 85-87 (1986).
Augé, et al., “Sialyl Aldolase in Organic Synthesis: From the Trout Egg Acid, 3-Deoxy-D-Glycero-D-Galacto-2-Nonulosonic Acid (KDN), to Branched-Chain Higher Ketoses as Possible New Chirons.”,Tetrahedron 46: 201-214 (1990).
Knappmann, et al., “Localization of the enzyme 3-Deoxy-D-Manno-2-Octulosonic Acid Aldolase”,Appl. Microbiol. Biotechnol. 33: 324-329 (1990).
Auzanneau, et al., “Formation of methyl (2,7-anhydro-3-deoxy-&agr;-D-manno-2-octulofuranos)onate upon methanolysis of 2,4,7,8-tetra-O-acetyl-3-deoxy-&agr;-D-manno-2-octulopyranosono-1,5-lactone”,Carbohyd. Res. 201: 337-241 (1990).
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Ramage, et al., “Dioxalanones as
Shen Gwo-Jenn
Sugai Takeshi
Wong Chi-Huey
Fitting Thomas
Geist Gary
Lewis Donald G.
Owens, Jr. Howard V.
The Scripps Research Institute
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