Sequential Interchange of Four Amino Acids from Blood Group B to Blood Group A Glycosyltransferase Boosts Catalytic Activity and Progressively Modifies Substrate Recognition in Human Recombinant Enzymes*

(Received for publication, February 4, 1997, and in revised form, March 19, 1997)

Nina O. L. Seto Dagger §, Monica M. Palcic , Catherine A. Compston , Hong Li , David R. Bundle and Saran A. Narang Dagger

From the Dagger  Institute for Biological Sciences, National Research Council of Canada, Ottawa, Ontario, Canada K1A 0R6 and the  Department of Chemistry, University of Alberta, Edmonton, Alberta, Canada T6G 2G2

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES


ABSTRACT

The human blood group A and B glycosyltransferase enzymes are highly homologous and the alteration of four critical amino acid residues (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser, Leu-266 right-arrow Met, and Gly-268 right-arrow Ala) is sufficient to change the enzyme specificity from a blood group A to a blood group B glycosyltransferase. To carry out a systematic study, a synthetic gene strategy was employed to obtain their genes and to allow facile mutagenesis. Soluble forms of a recombinant glycosyltransferase A and a set of hybrid glycosyltransferase A and B mutants were expressed in Escherichia coli in high yields, which allowed them to be kinetically characterized extensively for the first time. A functional hybrid A/B mutant enzyme was able to catalyze both A and B reactions, with the kcat being 5-fold higher for the A donor. Surprisingly, even a single amino acid replacement in glycosyltransferase A with the corresponding residue from glycosyltransferase B (Arg-176 right-arrow Gly) produced enzymes with glycosyltransferase A activity only, but with very large (11-fold) increases in the kcat and increased specificity. The increases observed in kcat are among the largest obtained for a single amino acid change and are advantageous for the preparative scale synthesis of blood group antigens.


INTRODUCTION

Complex carbohydrates are becoming increasingly important for the key roles they play in cell signaling, molecular recognition, and many other biological processes (1). Specific glycosyltransferase enzymes are responsible for the synthesis of different disaccharide linkages in complex oligosaccharides by transferring a single monosaccharide unit from a nucleotide donor to the hydroxyl group of an acceptor saccharide. Cloned glycosyltransferase enzymes are powerful new tools in small to large scale synthesis of therapeutically significant oligosaccharides (2, 3). Glycosyltransferases are highly specific for the donor and acceptor substrates and have been grouped into families according to the type of sugar they transfer (4, 5). With a few exceptions, a different glycosyltransferase is required to synthesize each different glycosidic linkage, and it is estimated that there are over 100 different glycosyltransferases to account for all the documented oligosaccharides (6). Mammalian oligosaccharide chains are largely composed of nine monosaccharide units, which are transferred by glycosyltransferases to different acceptor structures, but there have been no extensive sequence similarities found among different glycosyltransferases. However, there are common structural features among mammalian transferases as they are all classified as type II integral membrane proteins, with a short amino-terminal cytoplasmic tail, a membrane-anchoring domain, a short proteolytically sensitive stem region, and a large catalytic domain that includes the carboxyl terminus (6).

The most homologous glycosyltransferase sequences are the A and B glycosyltransferases of the human ABO blood group system (7). The histo-blood group ABO(H) antigens are defined carbohydrate determinants found on the surface of red blood cells and are largely responsible for failure of mismatched blood transfusions. These ABO carbohydrate antigens occur on other cell types and are important in cell development, cell differentiation, and oncogenesis (8-10). Blood group A individuals express alpha (1-3)N-acetylgalactosaminyltransferase (GTA),1 which catalyzes the transfer of GalNAc from the donor UDP-GalNAc to the (O)H-precursor structure Fucalpha (1-2)Galbeta -OR to give the A determinant GalNAcalpha (1-3)[Fucalpha (1-2)]Galbeta -OR. Blood group B individuals express alpha (1-3)galactosyltransferase (GTB), which uses the same (O)H-structure but catalyzes the transfer of Gal from UDP-Gal to make the B determinant Galalpha (1-3)[Fucalpha (1-2)]Galbeta -OR (7, 11) (Fig. 1). Blood group O individuals do not express either enzyme, and AB individuals express both (7).


Fig. 1. Biosynthesis of the blood group A and B antigens from the O(H) precursor. The human GTA enzyme catalyzes the transfer of GalNAc from the donor UDP-GalNAc (b) to the (O)H-precursor structure Fucalpha (1-2)Galbeta -OR (a) to give the A antigen Fucalpha (1-2)[GalNAcalpha (1-3)]Galbeta -OR (c). The human GTB enzyme catalyzes the transfer of Gal from UDP-Gal (d) to the same (O)H-precursor (a) to make the B antigen Fucalpha (1-2)[Galalpha (1-3)]Galbeta -OR (e). R = carbohydrate residue attached to a glycoprotein or glycolipid.
[View Larger Version of this Image (22K GIF file)]

The cDNA sequences of the GTA and GTB genes show that they are highly homologous and that alteration of only four critical amino acid residues (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser, Leu-266 right-arrow Met, and Gly-268 right-arrow Ala) is sufficient to change the enzyme specificity from a blood group A to a blood group B enzyme (7, 12, 13). GTA and GTB transfer to the same (O)H acceptor structure Fucalpha (1-2)Galbeta -OR, but use different UDP-sugar donors. Therefore, it is assumed that these four amino acids form the basis for the differential affinity of the A and B glycosyltransferases for their nucleotide donors UDP-GalNAc and UDP-Gal, respectively (13). In previous studies, transient gene expression in human HeLa cells of combinatorial A-B transferase chimera constructions which differed at the four critical amino acids suggested that substitutions at positions 266 and 268 were crucial for the nucleotide donor specificity of the enzyme (13). However, the authors note that transient expression in HeLa cells may not be the true representation of in vivo conditions and, moreover, does not provide any mechanistic information about the enzymes. Therefore, detailed kinetic analyses of purified enzymes are necessary to determine the exact effects of the residue changes on substrate recognition and catalytic activity (14).

There is a need for economical production of oligosaccharides, especially for the purpose of studying their biochemical function and assessing their potential in therapeutics or as diagnostic tools. Enzymatic oligosaccharide synthesis using glycosyltransferases proceeds regio- and stereoselectively and is less laborious and less costly compared with chemical synthesis. The limitation to the use of glycosyltransferases as synthetic tools is their scarcity from natural sources. The expression of recombinant glycosyltransferases in bacterial systems makes milligram scale synthesis by the enzymatic approach more practical (15).

Previously, we described the expression in Escherichia coli of a soluble recombinant GTB and the kinetic characterization of its acceptor specificity using synthetic analogs of the H disaccharide acceptor (16). In this paper, we report the chemical synthesis and expression of DNA encoding GTA and a series of mutants. The sequence of the synthetic DNA was designed to contain codons preferred for optimal expression in E. coli and unique restriction sites to permit systematic study of the specific effect of amino acid changes to important residues. We also describe the extensive kinetic characterization of wild-type GTA and a set of mutants where one, two, and then three critical amino acid positions of GTA were substituted with the corresponding amino acids found in GTB (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser, and Leu-266 right-arrow Met). Wild-type GTA and the mutant proteins were purified, kinetically characterized, and utilized in the preparative scale synthesis of blood group A and B trisaccharides.


EXPERIMENTAL PROCEDURES

Materials and General Techniques

Oligodeoxyribonucleotides were synthesized using model 380A and 394 DNA/RNA synthesizers (Applied Biosystems). Restriction enzymes and DNA-modifying enzymes were purchased from New England Biolabs and Life Technologies, Inc. All general molecular biology procedures were performed according to standard procedures (17). Gene design, extinction coefficients at 280 nm, and molecular weights of proteins were determined using the Wisconsin Sequence Analysis Software (Genetics Computer Group, Inc.). Pefabloc protease inhibitor (Boehringer Mannheim); UDP, UDP-GalNAc, and UDP-Gal (Sigma); UDP-[6-3H]GalNAc (10 Ci/mmol) and UDP-[6-3H]Gal (15 Ci/mmol) (American Radiolabeled Chemicals); Sep-Pak C18 reverse phase cartridges (Waters); Ecolite (+) liquid scintillation mixture (ICN); and Centriplus-10 protein concentrators (Amicon) were purchased commercially.

Construction of the Synthetic Glycosyltransferase Wild-type A Gene and Mutants

The ompA-GTA gene (1034 base pairs) was designed and synthesized as described previously for GTB (16). The mutant proteins were named based on their amino acid status at the four locations where GTA and GTB differ. The synthetic wild-type GTA (designated AAAA) and GTB (BBBB) genes were designed with unique restriction sites throughout the gene to facilitate mutagenesis. Glycosyltransferase mutants BAAA, BBAA, and BBBA were synthesized by digesting the GTB gene with KpnI/SphI and ligating in oligonucleotides to form the desired gene sequence. The DNA sequences of all four genes were confirmed on both strands.

Expression in E. coli

Plasmids harboring the wild-type ompA-GTA, and the mutant BAAA, BBAA, and BBBA genes were used to transform E. coli TG-1 cells. To produce the recombinant glycosyltransferase proteins, E. coli strains containing the 5 different plasmids were grown at 30 °C in M-9 minimal medium supplemented with 0.4% casamino acids and 100 µg/ml ampicillin. After 18-24 h the cultures were induced with 1 mM isopropyl-1-thio-beta -D-galactopyranoside and made up to 1 × TB (12 g of tryptone, 24 g of yeast extract, and 4 ml of glycerol/liter of culture), a rich growth medium that maximizes cell density. The cultures were harvested 48-64 h later, and periplasmic extracts were prepared by a one-step osmotic shock. Cells from 2 liters of culture were resuspended thoroughly in 60 ml of ice-cold shock buffer (20 mM Tris-HCl, 1 mM EDTA (pH 7.2), 1.0 mM Pefabloc) and incubated on ice for 30-60 min. Proteins were analyzed as described previously (16).

Purification of Wild-type GTA and Mutants

Soluble proteins were purified from 60 ml of periplasmic extracts by precipitating with ammonium sulfate. The 20-60% ammonium sulfate fraction was resuspended in 1.5-3.0 ml of column buffer (20 mM Tris (pH 7.2), 1 mM dithiothreitol, 0.5 M NaCl) and dialyzed extensively against the same buffer. The extracts were made up to 2 mM MnCl2, spun in a microcentrifuge for 5 min to remove any insoluble material and loaded onto a 10-ml UDP-hexanolamine-Sepharose column at 0.4 ml/h with column buffer containing 2 mM MnCl2 and washed extensively until the A280 nm was at background levels. GTA was eluted with column buffer containing 20 mM MnCl2 and 2 mM UDP (18). Since 2 mM UDP has a strong absorbance at 280 nm, the purified protein peak in the column fractions was determined by taking 20 µl of each fraction and measuring the protein concentration using the Bio-Rad Micro Protein Assay. Pooled column fractions (3-4 ml) containing pure GTA enzyme were concentrated to 600-1000-µl volumes using Centriplus-10 units, dialyzed extensively against 20 mM sodium cacodylate (pH 6.8) containing 1 mM dithiothreitol before activity assays or use in enzymatic synthesis. The protein concentration of all the enzymes was determined using the Bradford method with bovine gamma  globulin as a standard (Bio-Rad).

Kinetic Properties of Transferase A and Transferase AB Mutants

For the kinetic analysis of GTA and GTB activity, Sep-Pak radiochemical C18 assays were used with the hydrophobic acceptor Fucalpha (1-2)Galbeta -O-(CH2)7CH3 essentially as described previously (19-21). Reactions to measure glycosyltransferase A activity were incubated at 37 °C for 20-60 min and carried out in a 33-µl total volume with 50 mM sodium cacodylate buffer (pH 7.0), 20 mM MnCl2, 0.2 µCi of UDP-[6-3H]GalNAc, and 0.0005-0.2 µl of purified GTA or mutant enzymes. Initial rate conditions were linear under these conditions, where no more than 10-15% of substrate was consumed. Six different concentrations of donor and acceptor were employed generally covering the range from about 0.3 up to 8 Km for the substrate. Data were analyzed for a general two-substrate system using Equation 1.
v=<FR><NU>v[<UP>A</UP>][<UP>B</UP>]</NU><DE>K<SUB>ia</SUB>K<SUB>B</SUB>+K<SUB>B</SUB>[<UP>A</UP>]+K<SUB>A</SUB>[<UP>B</UP>]+[<UP>A</UP>][<UP>B</UP>]</DE></FR> (Eq. 1)
The kinetic parameters vmax, Km, and Km/vmax were derived from the best fit of the Michaelis-Menten equation using unweighted nonlinear regression with the SigmaPlot 4.1 program. Replots of the values of 1/vmax and Km/vmax versus 1/[acceptor] of the six primary plots were all linear and gave KA (the apparent Michaelis constant for the acceptor), vmax and Kia (the apparent Michaelis constant that is independent of the concentration of donor and reflects the effect that the binding of one substrate has on the binding of the other substrate). Replots of the values from the six primary plots of 1/vmax and Km/vmax versus 1/[donor] were all linear and gave KB (the apparent Michaelis-Menten constant for donor) and vmax. It is noted that the extent to which donor affects the Km for the acceptor is the same as the effect of acceptor on donor Km, that is KA Kib = KB Kia (where Kib is the apparent Michaelis constant for donor that is independent of the concentration of acceptor).

The reactions to measure glycosyltransferase B activity were incubated at 37 °C for 30-120 min and carried out in 33 µl total volume with 50 mM sodium cacodylate buffer (pH 7.0), 20 mM MnCl2, 0.2 µCi of UDP-[6-3H]Gal, and 0.05-4.0 µl of purified GTA or mutant enzymes. Six different concentrations of donor and acceptor were employed and analysis carried out as described for the glycosyltransferase A activity.

One milliunit of activity is defined as the amount that catalyzes the conversion of 1 nmol of sugar transferred/min. The catalytic constant or turnover number, kcat, is the maximum number of substrate molecules converted to product per active site per unit time, obtained from vmax/[E].

The Preparative Scale Enzymatic Synthesis of the Blood Group A and B Trisaccharides

The preparative scale enzymatic synthesis of 6.0 mg of blood group A trisaccharide was carried out in a reaction mixture, which contained 6.0 mg (13.7 µmol) of precursor H oligosaccharide Fucalpha (1-2)Galbeta -O-(CH2)7CH3, 15 mg (22.4 µmol) of UDP-GalNAc, 100 mM sodium cacodylate (pH 7.0), 5 mM MnCl2, 1 mg/ml bovine serum albumin, and 50 milliunits of recombinant GTA or BAAA enzyme in a total volume of 0.8-1.0 ml. The reaction was incubated overnight at 37 °C with GTA enzyme and UDP-GalNAc being added in two aliquots. The progress of the reaction was monitored by thin layer chromatography with the product purified upon completion using two Sep-Pak C18 reverse phase cartridges as described previously (15). Similarly, BBBA was used in reactions with either UDP-GalNAc or UDP-Gal, for the preparative scale synthesis of both A and B trisaccharide products. The products were characterized by 1H NMR spectroscopy on a Varian Unity 500 spectrophotometer at 500 Mhz.


RESULTS

Gene Design and Synthesis of GTA and Mutants

The amino acid sequence of membrane-bound human GTA deduced from cDNA (7, 12) was used to redesign a 1034-base pair synthetic GTA gene to contain E. coli preferred codons to maximize gene expression and unique restriction sites to facilitate mutagenesis (Fig. 2). The putative transmembrane domain (amino acids 1-53) was replaced with the bacterial ompA secretory signal to target GTA into the periplasm as a soluble protein. A DNA segment encoding the c-myc epitope and an affinity purification tail consisting of five histidine residues was added to the carboxyl terminus of the GTA gene in front of two termination codons (Fig. 2). GTA (AAAA) and GTB (BBBB) differ by only four essential amino acids (residues 176, 235, 266, and 268), and the mutant proteins were named based on their amino acid status at the four locations. Only the unique restriction enzymes sites in GTA are shown in Fig. 2, but other restriction sites that differ between the GTA and GTB sequences are also present.


Fig. 2. Amino acid and nucleotide sequence of synthetic DNA used to encode the human glycosyltransferase A. The residue numbers appear on top of the amino acid sequence and are numbered according to the membrane-anchored form. The amino acid sequence begins with the ompA secretion leader (bold italics) fused to the catalytic domain of GTA, which starts at residue 54. A c-myc peptide (italic) and a His affinity tail are added to the carboxyl end. The four essential amino acids (residues 176, 235, 266, and 268) that differ between the blood group A and B glycosyltransferases are boxed. The nucleotide numbers are on the right-hand side of the figure. Only unique restriction enzyme sites are shown.
[View Larger Version of this Image (66K GIF file)]

Expression and Purification

The soluble form of GTA and its mutants were purified from the periplasm to apparent homogeneity and characterized as described previously for GTB (16). The mutations in BAAA (Arg-176 right-arrow Gly) and BBAA (Arg-176 right-arrow Gly and Gly-235 right-arrow Ser) enhanced total expression levels of the enzymes compared with that of GTA and BBBA (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser, and Leu-266 right-arrow Met), with a corresponding increased secretion of soluble recombinant protein into the periplasm (data not shown). In terms of enzymatic activity, the average yield of pure BAAA was 19 times higher than for GTA, due to being more highly expressed in E. coli and having increased catalytic activity.

Kinetic Characterization

Using a suitable range of six acceptor concentrations and six donor concentrations and then measuring the rate with all possible combinations of these substrate concentrations (i.e. 6 × 6 grid), the kinetic constants KA, KB, kcat, and kcat/Km were determined. In comparing wild-type glycosyltransferase A and B enzymes with each using their preferred donors, the kcat (maximum rate possible when both acceptor and donor is saturated) is similar. However, glycosyltransferase A has a Kia for its preferred donor UDP-GalNAc that is 5.5 times lower than the Kia of the B enzyme for its preferred donor UDP-Gal, which results in a higher specificity constant (kcat/Km) for the A enzyme (Table I).

Table I. Kinetic parameters of wild-type and mutant glycosyltransferase A and B enzymes

KA is the Michaelis-Menten constant for the acceptor. KB is the Michaelis-Menten constant for the donor, and Kia is the apparent Michaelis constant for acceptor independent of donor. These were obtained by analysis of secondary plots of the slopes and intercepts of primary plots for six concentrations of both donor and acceptor. KA is the Michaelis-Menten constant for the acceptor. KB is the Michaelis-Menten constant for the donor, and Kia is the apparent Michaelis constant for acceptor independent of donor. These were obtained by analysis of secondary plots of the slopes and intercepts of primary plots for six concentrations of both donor and acceptor.

Enzyme UDP-GalNAc
UDP-Gal
KA KB Kia kcat kcat/KA kcat/KB KA KB Kia kcat kcat/KA kcat/KB

µM µM µM s-1 mM-1s-1 mM-1s-1 µM µM µM s-1 mM-1s-1 mM-1s-1
AAAA 15 13 4.9 4.9 330 380 23 6.3 23 0.020 0.87 3.2
BAAA 43 126 12 55 1300 440 68 43 76 0.037 0.54 0.86
BBAA 206 51 121 24 120 470 708 36 644 0.030 0.042 0.83
BBBA 348 253 139 10 29 40 420 56 105 2.1 5.0 38
BBBB 281 285 122 0.3 1.1 1.1 54 34 27 6.5 120 190

Wild-type GTA and mutant BAAA and BBAA enzymes showed predominantly glycosyltransferase A activity (UDP-GalNAc) only. It was possible to kinetically characterize the small amounts of glycosyltransferase B activity (UDP-Gal) that was detectable in these glycosyltransferase A enzymes by using comparatively high concentrations of the recombinant enzymes in the assays for B activity. Kinetic analysis of the GTA enzyme using the B donor UDP-Gal shows that the wild-type A enzyme does not transfer the B donor (UDP-Gal) efficiently, largely because of a much lower kcat. Similarly, the decreased kcat also accounts for the lack of A activity (transferring of UDP-GalNAc) displayed by the B enzyme (Table I). KA and KB for GTA was similar for both UDP-GalNAc and UDP-Gal. Thus, the difference in the donor specificity of the glycosyltransferase A and B enzymes is largely due to a difference in kcat rather than Km values.

The single mutant BAAA (Arg-176 right-arrow Gly) showed a very large 11-fold increase in kcat and a 4-fold increase in the specificity constant kcat/KA compared to wild-type A enzyme (Table I). Although the single amino acid change in BAAA was due to the substitution of residue Gly-176 from the B enzyme for Arg in the A enzyme, this enzyme did not show any additional ability to catalyze the B reaction, but instead showed an increased ability to catalyze the A reaction.

A further additional amino acid change in the double mutant BBAA (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser) results in an enzyme with a 5-fold increase in kcat compared with the wild-type A enzyme. In contrast to BAAA, the specificity constant kcat/KB is only increased slightly. Despite two amino acid substitutions with the corresponding residues in the B enzyme, BBAA is not able to catalyze either the A or B reaction with the same specificity as either the wild-type A or B enzyme.

BBBA (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser, and Leu-266 right-arrow Met) has the ability to catalyze both the A and B reactions and is a functional hybrid A/B enzyme. With UDP-GalNAc, BBBA has a 2-fold increase in kcat, but also a larger KA and KB, which results in lower specificity constants compared with wild-type (Table I).

Enzymatic Synthesis of Blood Group A and B Trisaccharides

GTA and BAAA were used in preparative scale synthesis of the blood group A trisaccharide. Recombinant GTA (50 milliunits) was used in the preparative scale synthesis of 6 mg of the blood group A trisaccharide from the H disaccharide acceptor Fucalpha (1-2)Galbeta -O-(CH2)7CH3. The reaction was judged to be 50% complete after 6 h at 37 °C. The reaction was left for another 16-20 h, which resulted in 100% conversion to the A trisaccharide product. Aliquots of the reaction mixture were removed at different times, and the enzyme activity was found to be relatively stable at 37 °C for 2 days. Under the preparative scale synthesis conditions, the mutant BAAA has the advantage of having a higher specific activity, kcat, and kcat/Km compared to wild-type GTA. The use of the glycosyltransferase AB mutant BBBA with either UDP-GalNAc or UDP-Gal donors in enzymatic synthesis also resulted in 100% conversion to the blood group A or B trisaccharide determinants.

The structures of the synthetic A (Fucalpha (1-2)[GalNAcalpha (1-3)]Galbeta -O-(CH2)7CH3) and B trisaccharide products (Fucalpha (1-2)[Galalpha (1-3)]Galbeta -O-(CH2)7CH3) were confirmed by 1H NMR. In the A trisaccharide product, the terminal GalNAc is linked to Gal in an alpha 1right-arrow3 linkage. The resonance of the alpha -anomeric H of GalNAc was at delta  5.32 ppm (J1,2 3.8 Hz) and that of the alpha -anomeric H of Fuc was at delta  5.17 ppm (J1,2 3.8 Hz). For the B trisaccharide product, the alpha -anomeric H of the terminal Gal linked to the inner Gal in an alpha 1right-arrow3 linkage results in the H-1 resonance at delta  5.30 ppm (J1,2 3.8 Hz) and the alpha -anomeric H of Fuc at delta  5.24 ppm (J1,2 2.8 Hz) (22) (data not shown).


DISCUSSION

In this paper, we describe the chemical synthesis and expression of functional human GTA genes and its mutants using the synthetic gene strategy. Purified recombinant GTA and its mutant BAAA from 1 liter of E. coli had enzymatic activity equivalent to that recoverable from 0.2 and 32 million liters of human blood group A sera (19-21, 23-25), without the need for laborious multistep chromatographic purification (23, 26). It is interesting to note that the improved yield of active blood group A enzyme was accomplished without significantly altering the Km for the acceptor, and, surprisingly, mutant BAAA showed 11-fold higher A activity resulting from a single amino acid change of Arg-176 right-arrow Gly. The availability of large quantities of the recombinant enzymes has made possible the first systematic kinetic characterization of the human blood group A and B enzymes. This allowed for an exact comparison of steady-state kinetic parameters of wild-type A enzyme, the mutants, and the B enzyme for both UDP-GalNAc and UDP-Gal donors.

Although GTA and GTB differ by only four amino acids and use the same acceptor, the alteration of these amino acids affects the binding of both the UDP-sugar donor and the acceptor. Kinetic characterization revealed that alteration of even one of the four amino acids that differ between these two enzymes may affect the Km of both the acceptor and the donor substrates. The Km for the acceptor also differed depending on whether UDP-GalNAc or UDP-Gal was used as the donor (Table I). GTB has a KB for the donor UDP-Gal higher than the KB that GTA has for the donor UDP-GalNAc, which suggests that the binding of GTB to UDP-Gal is weaker than the binding of GTA to UDP-GalNAc, with the corresponding kcat values being similar.

The major difference in the utilization of the alternate donors by the glycosyltransferase A and B enzymes is largely due to a difference in kcat rather than Km. For GTA the kcat for UDP-Gal is only 0.4% that of UDP-GalNAc. GTA had an apparent Km for UDP-Gal similar to the Km for UDP-GalNAc, indicating that the enzyme was able to bind both donors, but the significantly decreased kcat for UDP-Gal showed that it was not able to readily catalyze the transfer. Similarly, the lack of GTB activity observed for BAAA (Arg-176 right-arrow Gly) and BBAA (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser) was not necessarily due to an increased Km, but also largely due to a decreased kcat.

The mutant BAAA was similar to GTA in that it possessed essentially only GTA activity. Alteration of GTA by the single mutation (Arg-176 right-arrow Gly) did not alter the donor substrate specificity but did alter the kinetic properties of the enzyme by increasing kcat 11-fold, as well as increasing the specificity constant, with respect to both the acceptor (kcat/KA) and the donor UDP-GalNAc (kcat/KB) (Table I). It is surprising that substitution of the corresponding residues from GTB into GTA in these two mutant enzymes did not result in any additional glycosyltransferase B activity but instead produced enzymes with glycosyltransferase A activity higher than that found in wild-type GTA. Indeed these are among the largest increases in kcat observed for a single amino acid change.

It is interesting to note that transient expression studies in HeLa cells suggest BAAA is half as active as wild-type A enzyme (13). In contrast, detailed kinetic analysis of the purified enzymes illustrates that it is essential to determine the exact effects of residue changes on substrate recognition and catalytic activity. The transient expression studies provide no mechanistic information (14).

The triple mutant BBBA (Arg-176 right-arrow Gly, Gly-235 right-arrow Ser, and Leu-266 right-arrow Met) was a functional hybrid A/B enzyme, which was used to synthesize both the blood group A and B trisaccharides, since it had significant A and B activity. The structural difference between alpha Gal and alpha GalNAc is spatially significant as the 2-deoxy-2-acetamido group in alpha GalNAc is larger than the 2-hydroxyl group in alpha Gal. Glycosyltransferase AB enzymes exist in nature and may provide an explanation for the rare cis-AB phenotype observed (27).

The maximum rate possible when both substrates are saturated (kcat) is often affected by rate-limiting substrate binding or product release steps. The specificity constant (kcat/Km), which combines the effects of both rate and binding, was greatly increased in BAAA for both the acceptor and the donor. Generally, irrespective of the mechanism, the major factor governing specificity is the stability of the enzyme-bound transition state, which exists during the conversion of the enzyme-bound substrate to product. It is possible that the removal of the Arg side chain at position 176 in mutant BAAA stabilizes the transition state with the donor alpha GalNAc more effectively, resulting in the higher specificity observed.

Our results suggest that alteration of the four critical amino acids that differ between GTA and GTB affected the kinetic constants of both the acceptor and the donor, possibly due to topologically close binding of the donor and acceptor. Mutations at residue 176 in BAAA appear to have little effect on the binding of the acceptor, but do affect the enzyme turnover, as this mutant showed a very large increase in kcat. Mutations at residues 176 and 235 in BBAA showed a 5-fold increase in kcat and weaker acceptor binding, and the binding of the donor was not greatly affected. These results suggest a role in enzyme turnover for residue 176. Residue 235 could affect the binding of the acceptor, and segments around residues 266 and 268 could be most critical for binding of the nucleotide sugar donor.

Recombinant GTA and BAAA enzymes were used in the preparative scale synthesis of the blood group A trisaccharide, with BAAA having the advantage of having a 11-fold higher kcat compared with wild-type GTA. A further systematic mutagenesis of GTA and GTB may lead to glycosyltransferase enzymes with even more significant increases in catalytic activity.

Very little is known about structure/function relationships in glycosyltransferases. With a few exceptions, there is very little nucleotide or amino acid sequence similarity among glycosyltransferases even if they use the same acceptor or nucleotide donors. There are no x-ray crystal structures of mammalian glycosyltransferases known, and the large scale fermentation of E. coli to produce unglycosylated glycosyltransferases may produce enough protein for crystallization and subsequent three-dimensional structure determination. The availability of recombinant GTA, GTB, and their mutants can form the framework for further genetic engineering of new glycosyltransferases, allowing investigation into structure and function relationships to produce new glycosyltransferase enzymes as synthetic tools and diagnostic reagents.


FOOTNOTES

*   This work was supported in part by a collaborative grant from the Natural Sciences and Engineering Research Council of Canada (to M. M. P. and D. R. B.). This is NRCC Publication 39548.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) Y11891[GenBank].


§   To whom correspondence should be addressed. Tel.: 613-990-7206; Fax: 613-941-1327; E-mail: nina.seto{at}nrc.ca.
1   The abbreviations used are: GTA, glycosyltransferase A encoded by the blood group A gene (EC 2.4.1.40); GTB, glycosyltransferase B encoded by the blood group B gene (EC 2.4.1.37).

ACKNOWLEDGEMENTS

We thank Dr. Ole Hindsgaul for providing the acceptor substrates, helpful discussions throughout this work, and reading of the manuscript. We also thank Dr. A. Otter for the NMR spectra, D. Bilous for the synthesis of the oligonucleotides, J. Michniewicz for assistance with DNA sequence analysis, D. Pope for general assistance, and Dr. N. M. Young for reading of the manuscript.


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