Chemistry: molecular biology and microbiology – Enzyme – proenzyme; compositions thereof; process for... – Hydrolase
Reexamination Certificate
2001-05-17
2002-07-23
Nashed, Nashaat T. (Department: 1652)
Chemistry: molecular biology and microbiology
Enzyme , proenzyme; compositions thereof; process for...
Hydrolase
C435S069100, C435S183000, C435S195000, C435S201000, C435S252300, C435S320100, C536S023200
Reexamination Certificate
active
06423525
ABSTRACT:
TECHNICAL FIELD
The present invention relates to novel glycosidases and their uses.
BACKGROUND OF THE INVENTION
The recognition that carbohydrates play a key role in biological processes of living organisms has made their study of great importance for medicine and basic science. The understanding of carbohydrates has lagged behind that of other types of biological molecules because of the immense complexity and variety of these molecules and the lack of availability of analytic and synthetic tools that enable scientists to differentiate one form from another.
Forms of Carbohydrates in Nature.
In nature, carbohydrates exist as polymers known as polysaccharides, that consist of a series of monosaccharides that are covalently attached by glycosidic bonds to form both branched and linear macromolecules. In addition, polysaccharides or, more commonly, oligosaccharides may be coupled to macromolecules such as proteins or lipids to form glycoproteins or glycolipids. Unlike naturally occurring polysaccharides, the oligosaccharides associated with protein or lipid consist of a relatively small subset of monosaccharide types.
Oligosaccharides associated with glycoproteins have been the focus of much of the carbohydrate research to date largely because the biological properties of these molecules are diverse and their relatively short monosaccharide sequences make the oligosaccharides amenable to study.
Structural Features of Glycoproteins.
Glycoproteins are characterized into two groups according to their linkage to protein. The O-glycosyl linked oligosaccharides including mucin-type oligosaccharides, the proteoglycan type, the collagen-type and the extensin-type are bonded to the hydroxyl oxygen of L-serine or L-threonine. The N-glycosyl linked oligosaccharides are bound to the amido nitrogen of asparagine in a tripeptide generally of the form Asn-Xaa-Ser/Thr (where Xaa represents any amino acid). The N-linked oligosaccharides are further differentiated into 3 subgroups these being the high mannose type, the complex type and the hybrid type. N-linked oligosaccharides are frequently branched where branching commonly occurs either at a mannose residue or at an N-acetylglucosamine residue. These branched structures are called biantennary, if there are two branches, and triantennary if there are three branches.
The oligosaccharide can be characterized by its sequence of monosaccharides. The oligosaccharide is attached at its reducing end to the amino acid sequence of the protein while the non-reducing end is found at the terminal monosaccharide at the other end of the oligosaccharide. Other important characteristics of oligosaccharides are the glycosidic bonds that connect individual monosaccharides. The glycosidic bonds obtain their numerical assignment according to the carbons in the monosaccharide ring where linkage occurs. The carbons are numbered in a clockwise direction from 1 to 6. Any of these carbons can be involved in the glycosidic bond although commonly the carbon-1 on the monosaccharide closer to the non-reducing end forms a glycosidic bond with any other carbon on the monosaccharide toward the reducing end of the oligosaccharide. Because each carbon on a monosaccharide is asymmetric, the glycosidic bond occurs in two anomeric configurations, the alpha and the beta anomer. The type of anomer is determined by the position of the reactive hydroxyl group on the carbon.
FIG. 1
illustrates the possible linkage configurations that may exist between two monosaccharides.
Synthesis and Degradation of Oligosaccharides.
Oligosaccharides are synthesized by a battery of enzymes in the cell known as glycosidases and glycosyltransferases. Typically, an oligosaccharide is assembled on a lipid carrier and transferred to the appropriate amino acid within the protein to be glycosylated. Glycosidase trimming and glycosyltransferase mediated synthesis follows and individual monosaccharides or preassembled oligosaccharide units are removed or added. In addition, microscopic reversibility may occur when the exoglycosidases that are usually hydrolytic enzymes, act as transferases in a synthetic role (Ichikawa et al. 1992
, Anal. Biochem
. 202:215-238). In some cases, removal of a monosaccharide results in a conformational change that facilitates further chain synthesis (Camirand et al. 1992
, J. Biol. Chem
., 266:15120-15127). While not wishing to be bound by theory, one cause of inter-cellular variability in glycosylation patterns for a single protein may arise from different amounts and types of available glycosidases and glycosyltransferases in any single cell.
The availability of individual glycosidases and glycosyltransferases depends on the nutritional environment of the cell (Goochee and Monica 1990
, Bio/Technology
6:67-71) the type of cell (Sheares and Robbins 1986
, PNAS
83:1993) and its homeostatic state (Kobata 1988, Gann Monogr.
Cancer Res
. 34:3-13). Associated with the variation it amounts and type of these intracellular enzymes is the occurrence of multiple glycoforms of a single glycoprotein (Parekh et al. 1987
, EMBO
6:1233-1244). These glycoforms differ in their oligosaccharide sequence and linkage characteristics as well as in the position and number of attachment sites of the oligosaccharide to the protein. Variation in glycosylation of a single glycoprotein made in different cell types is an important aspect of recombinant protein therapeutic production because of the possible impact of structural heterogeneity on biological function (Sasaki et al. 1987
, J. Biol. Chem
. 262:12059-12076; Dube et al. 1988
, J. Biol. Chem
. 263:17516-17521; Lund et al. 1993
, Human Antib. Hybridomas
, 4:20-25; Parekh et al. 1989
, Biochem
. 28:7644-7662; Kagawa et al. 1988
, J. Biol. Chem
. 263:17508-17515; Parekh et al. 1989
, Biochem
. 28:7662-7669; Parekh et al. 1989
, Biochem
. 28:7670-7679).
Not only does the glycosylation pattern of a single protein vary according to which cell it is synthesized within, but individual glycosylation events may be characteristic of certain evolutionarily related animal species only. Galili et al. 1987
, Immunology
84:1369-1373 and Galili et al. 1988
, J. Biol. Chem
. 263:17755-17762 identified the occurrence of Gal&agr;1-3Gal in non-primate mammals and New World monkeys, a glycosylation pattern that was absent in humans and Old World monkeys. The absence of this structure could be demonstrated because the disaccharide elicits an immune response in humans. The immune response to atypical glycosylation patterns presents a yet unsolved antigenicity problem that arises from using glycoproteins derived or manufactured in non-primate sources.
Oligosaccharides are degraded by glycosidases that are often highly specific for the glycosidic linkage and the stereochemistry of the oligosaccharide. An example of the influence of remotely located monosaccharides on the digestion of oligosaccharides is found in human patients suffering from fucosidosis. These patients lack the exoglycosidase required to remove fucose from N-linked oligosaccharides prior to digestion with endoglycosidase. The fucose interferes with the enzymatic activity of the endoglycosidase and causes undigested oligosaccharides to be excreted in their urine. (Kobata 1984
, The Biology of Carbohydrates
, Eds., Ginsberg and Robbins, Wiley, N.Y. vol. 2, pp. 87-162.)
The Biological Impact of Glycosylation of Proteins.
The importance of correct synthesis and degradation of oligosaccharides for the organism has been demonstrated in diseases which result from a single defective glycosidase giving rise to incorrect processing of carbohydrate structures. In the example cited above, disease results from the absence of a Fucosidase resulting in incorrect processing of the glycoprotein. Other examples include human &agr;-Mannosidosis in which the major lysosomal &agr;-Mannosidase activity is severely deficient (Gasperi et al. 1992
, J. Biol. Chem
. 267:9706-9712). Aberrant oligosaccharide structures have also been associated with cancer (Sano et al. 1992
, J. Biol. Chem
. 267:1522-1527).
The oligosaccharide s
Fronda Christian L.
New England Biolabs Inc.
Williams Gregory D.
LandOfFree
Isolation and composition of a novel glycosidase from... does not yet have a rating. At this time, there are no reviews or comments for this patent.
If you have personal experience with Isolation and composition of a novel glycosidase from..., we encourage you to share that experience with our LandOfFree.com community. Your opinion is very important and Isolation and composition of a novel glycosidase from... will most certainly appreciate the feedback.
Profile ID: LFUS-PAI-O-2897694