One-Step Synthesis of Cellulose from Cellobiose via Protic Acid-Assisted Enzymatic Dehydration in Aprotic Organic Media

Direct and efficient enzymatic synthesis of long-chain cellulose from cellobiose in its original form was successfully achieved via the combination of a surfactant-enveloped enzyme (SEE) and a protic acid in an aprotic organic solvent, lithium chloride/N,N-dimethylacetamide system. The SEE biocatalyst was prepared by protecting the surface of cellulase with the nonionic surfactant dioleyl-N-d-glucona-l-glutamate for keeping its enzymatic activity in nonaqueous media. Fourier transform infrared and nuclear magnetic resonance analyses elucidated the successful synthesis of cellulose, β-1,4-linked d-glucopyranose polymer, through the reverse hydrolysis of cellobiose. By using protic acid cocatalysts, a degree of polymerization of as-synthesized cellulose reached more than 120, in a ca. 26% conversion, which was 5 times higher than that obtained in an acid-free SEE system. A novel-concept biocatalysis, i.e., a protic acid-assisted SEE-mediated reaction, enables a facile, one-step chain elongation of carbohydrates without any activation via multistep organic chemistry, and can provide potential applications in the functional design of glycomaterials.     

Isotopic Determination and Optimum Reaction Conditions of Pantothenic Acid Synthetase

When yeast protoplasts that were producing repressible acid phosphatase (r-APase) were treated with tunicamycin (TM), three specific proteins of 59k, 57k, and 55k daltons were accumulated in the membrane fraction in addition to the usual membrane proteins and these proteins were not detected in the secreted fraction. These proteins were immunoprecipitated with anti r-APase antiserum. Their molecular sizes were almost the same as those endo-H treated r-APase. Therefore these proteins were considered to be nonglycosylated forms of r-APase proteins. These results proved that nonglycosylated forms of r-APase produced by TM-treatment were not secreted by yeast protoplasts.     

Engineered Sialylation of Pathogenic Antibodies In Vivo Attenuates Autoimmune Disease

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Characterization of Three ��-Galactoside Phosphorylases from Clostridium phytofermentans: DISCOVERY OF d-GALACTOSYL-��1��4-l-RHAMNOSE PHOSPHORYLASE*

We characterized three d-galactosyl-β1→3-N-acetyl-d-hexosamine phosphorylase (EC 2.4.1.211) homologs from Clostridium phytofermentans (Cphy0577, Cphy1920, and Cphy3030 proteins). Cphy0577 and Cphy3030 proteins exhibited similar activity on galacto-N-biose (GNB; d-Gal-β1→3-d-GalNAc) and lacto-N-biose I (LNB; d-Gal-β1→3-d-GlcNAc), thus indicating that they are d-galactosyl-β1→3-N-acetyl-d-hexosamine phosphorylases, subclassified as GNB/LNB phosphorylase. In contrast, Cphy1920 protein phosphorolyzed neither GNB nor LNB. It showed the highest activity with l-rhamnose as the acceptor in the reverse reaction using α-d-galactose 1-phosphate as the donor. The reaction product was d-galactosyl-β1→4-l-rhamnose. The enzyme also showed activity on l-mannose, l-lyxose, d-glucose, 2-deoxy-d-glucose, and d-galactose in this order. When d-glucose derivatives were used as acceptors, reaction products were β-1,3-galactosides. Kinetic parameters of phosphorolytic activity on d-galactosyl-β1→4-l-rhamnose were k_cat = 45 s⁻¹ and K_m = 7.9 mm, thus indicating that these values are common among other phosphorylases. We propose d-galactosyl-β1→4-l-rhamnose phosphorylase as the name for Cphy1920 protein.Phosphorylases are a group of enzymes involved in formation and cleavage of glycoside linkage together with glycoside hydrolases and glycosyl-nucleotide glycosyltransferases (synthases). Phosphorylases, which reversibly phosphorolyze oligosaccharides to produce monosaccharide 1-phosphate, are generally intracellular enzymes showing strict substrate specificity. Physiologically, such strict substrate specificity is considered to be closely related to the environment containing bacteria possessing them. For example, d-galactosyl-β1→3-N-acetyl-d-hexosamine phosphorylase (GalHexNAcP²; EC 2.4.1.211) from Bifidobacterium longum, an intestinal bacterium, forms part of the pathway metabolizing galacto-N-biose (GNB; d-Gal-β1→3-d-GalNAc) from mucin and lacto-N-biose I (LNB; d-Gal-β1→3-d-GlcNAc) from human milk oligosaccharides, both of which are present in the intestinal environment, with GNB- and LNB-releasing enzymes and GNB/LNB transporter (1–8). Another example is cellobiose phosphorylase from Cellvibrio gilvus, which is a cellulolytic bacterium. Cellobiose phosphorylase forms an important cellulose metabolic pathway with an extracellular cellulase system producing cellobiose (9, 10).The reversible catalytic reaction of phosphorylases is one of the most remarkable features that make them suitable catalysts for practical syntheses of oligosaccharides. An oligosaccharide can be produced from inexpensive material by combining reactions of two phosphorylases, one for phosphorolyzing the material and the other for synthesizing the oligosaccharide, in one pot. Based on this idea, LNB is synthesized on a large (kg) scale using sucrose phosphorylase and GalHexNAcP (11). Practical synthesis methods of trehalose and cellobiose have also been developed (12, 13). However, only 14 kinds of substrate specificities have been reported among phosphorylases (13), thus restricting their use. Therefore, it would be useful to find a phosphorylase with novel activity.GalHexNAcP phosphorolyzes GNB and LNB to produce α-d-galactose 1-phosphate (Gal 1-P) and the corresponding N-acetyl-d-hexosamine. To date, GalHexNAcP is the only phosphorylase known to act on β-galactoside. This enzyme was first found in the cell-free extract of Bifidobacterium bifidum (14) and then in B. longum (1, 15), Clostridium perfringens (16), Propionibacterium acnes (17), and Vibrio vulnificus (18). These studies revealed that GalHexNAcPs were classified into three subgroups based on substrate preference between GNB and LNB. These subgroups are as follows: 1) galacto-N-biose/lacto-N-biose I phosphorylase (GLNBP), showing similar activity on both GNB and LNB (B. longum and B. bifidum); 2) galacto-N-biose phosphorylase (GNBP), preferring GNB to LNB (C. perfringens and P. acnes); and 3) lacto-N-biose I phosphorylase (LNBP), preferring LNB to GNB (V. vulnificus) (18). The ternary structure of GLNBP from B. longum (GLNBP_Bl) has been revealed recently (19). Based on the similarity in ternary structures between GLNBP_Bl and β-galactosidase from Thermus thermophilus, which belongs to glycoside hydrolase family 42 (19, 20), GalHexNAcP homologs are classified as GH112 (glycoside hydrolase family 112), although phosphorylases are glycosyltransferases (21, 22).Clostridium phytofermentans is an anaerobic cellulolytic bacterium. It is found in soil and grows optimally at 37 °C (23). Its whole genome sequence has been revealed (GenBank^TM accession number {"type":"entrez-nucleotide","attrs":{"text":"CP000885","term_id":"160426828","term_text":"CP000885"}}CP000885). The bacterium possesses three GalHexNAcP homologous genes (cphy0577, cphy1920, and cphy3030 genes; GenBank^TM accession numbers are {"type":"entrez-protein","attrs":{"text":"ABX40964.1","term_id":"160427401","term_text":"ABX40964.1"}}ABX40964.1, {"type":"entrez-protein","attrs":{"text":"ABX42289.1","term_id":"160428726","term_text":"ABX42289.1"}}ABX42289.1, and {"type":"entrez-protein","attrs":{"text":"ABX43387.1","term_id":"160429824","term_text":"ABX43387.1"}}ABX43387.1, respectively). C. phytofermentans has the ability to utilize a wide range of plant polysaccharides (23), and substrate specificities of these three gene products (Cphy0577, Cphy1920, and Cphy3030 proteins) are considered to be responsible for this ability. Furthermore, the three proteins have not been clearly categorized as GLNBP, GNBP, or LNBP, based on the phylogenetic tree shown in Fig. 1.Open in a separate windowFIGURE 1.Phylogenetic tree of GalHexNAcP homologs in GH112. Multiple alignment was performed using ClustalW2 (available on the World Wide Web). A phylogenetic tree was constructed using Treeview version 1.6.6. The proteins characterized in this study are represented with boldface letters in boxes with a heavy outline. The other proteins are numbered serially in boxes. Characterized GLNBP, GNBP, and LNBP are represented with boldface black letters on a gray background, boldface white letters on a gray background, and boldface white letters on a black background, respectively. Organisms and GenBank^TM accession numbers of numbered proteins are as follows: 1, CPF0553 (C. perfringens ATCC13124, {"type":"entrez-protein","attrs":{"text":"ABG83511.1","term_id":"110674524","term_text":"ABG83511.1"}}ABG83511.1) (16); 2, CPE0573 (C. perfringens str.13, {"type":"entrez-protein","attrs":{"text":"BAB80279.1","term_id":"18144232","term_text":"BAB80279.1"}}BAB80279.1); 3, CPR0537 (C. perfringens SM101, {"type":"entrez-protein","attrs":{"text":"ABG86710.1","term_id":"110683340","term_text":"ABG86710.1"}}ABG86710.1); 4, LnpA2 (B. bifidum JCM1254, {"type":"entrez-protein","attrs":{"text":"BAE95374.1","term_id":"107597820","term_text":"BAE95374.1"}}BAE95374.1) (14, 15); 5, LnpA1 (B. bifidum JCM1254, {"type":"entrez-protein","attrs":{"text":"BAD80752.1","term_id":"56676017","term_text":"BAD80752.1"}}BAD80752.1) (14, 15); 6, GLNBP_Bl (B. longum subsp. longum JCM 1217, {"type":"entrez-protein","attrs":{"text":"BAD80751.1","term_id":"56676015","term_text":"BAD80751.1"}}BAD80751.1) (1, 16); 7, Blon_2174 (B. longum subsp. infantis ATCC 15697, {"type":"entrez-protein","attrs":{"text":"ACJ53235.1","term_id":"213524488","term_text":"ACJ53235.1"}}ACJ53235.1); 8, BL1641 (B. longum NCC2705, {"type":"entrez-protein","attrs":{"text":"AAN25428.1","term_id":"23326930","term_text":"AAN25428.1"}}AAN25428.1); 9, BLD_1765 (B. longum DJO10A, {"type":"entrez-protein","attrs":{"text":"ACD99210.1","term_id":"189429062","term_text":"ACD99210.1"}}ACD99210.1); 10, GnpA (P. acnes JCM6473, {"type":"entrez-nucleotide","attrs":{"text":"AB468065","term_id":"219807264","term_text":"AB468065"}}AB468065) (17); 11, GnpA (P. acnes JCM6425, {"type":"entrez-nucleotide","attrs":{"text":"AB468066","term_id":"219807262","term_text":"AB468066"}}AB468066) (17); 12, PPA0083 (P. acnes KPA171202, {"type":"entrez-protein","attrs":{"text":"AAT81843.1","term_id":"50839176","term_text":"AAT81843.1"}}AAT81843.1); 13, VV2_1091 (V. vulnificus CMCP6, {"type":"entrez-protein","attrs":{"text":"AAO07997.1","term_id":"27359049","term_text":"AAO07997.1"}}AAO07997.1) (18); 14, VVA1614 (V. vulnificus YJ016, {"type":"entrez-protein","attrs":{"text":"BAC97640.1","term_id":"37201820","term_text":"BAC97640.1"}}BAC97640.1); 15, Oter_1377 (Opitutus terrae PB90-1, {"type":"entrez-protein","attrs":{"text":"ACB74662.1","term_id":"177840410","term_text":"ACB74662.1"}}ACB74662.1); 16, BCQ_1989 (B. cereus Q1, {"type":"entrez-protein","attrs":{"text":"ACM12417.1","term_id":"221239707","term_text":"ACM12417.1"}}ACM12417.1); 17, BCAH187_A2105 (Bacillus cereus AH187, {"type":"entrez-protein","attrs":{"text":"ACJ78918.1","term_id":"217064668","term_text":"ACJ78918.1"}}ACJ78918.1).In this study, we characterized the three proteins. We reported that two of them were GalHexNAcPs and that the other was a β-galactoside phosphorylase showing unique substrate specificity.     

Stereoscopic Analysis of Optic Nerve Head Parameters in Primary Open Angle Glaucoma: The Glaucoma Stereo Analysis Study

PurposeThe Glaucoma Stereo Analysis Study (GSAS), a cross sectional multicenter collaborative study, used a stereo fundus camera to assess various morphological parameters of the optic nerve head (ONH) in glaucoma patients and investigated the relationships between these parameters and patient characteristics.ResultsPatient characteristics included refractive error of −3.38±3.75 diopters, intraocular pressure (IOP) of 13.6±2.6 mmHg, and visual field mean deviation (MD) of −4.71±3.26 dB. Representative ONH parameters included a horizontal disc width of 1.66±0.28 mm, vertical disc width of 1.86±0.23 mm, disc area of 2.42±0.63 mm², cup area of 1.45±0.57 mm², and cup volume of 0.31±0.22 mm³. Correlation analysis revealed significant negative associations between vertical cup-to-disc ratio (0.82±0.08) and MD (r = −0.40, P<0.01) and between disc tilt angle (10.5±12.5 degrees) and refractive error (r = −0.36, P<0.01). Seventy-five percent of the eyes had a positive value for rim decentering (0.30±0.42), indicating that rim thinning manifested more often as an inferior lesion than a superior lesion.ConclusionWe used stereoscopic analysis to establish a database of ONH parameters, which may facilitate future studies of glaucomatous changes in ONH morphology.