Metabolism of l- and d-3-hydroxybutyrate by rat liver during development

The metabolism of d- and l-3-hydroxybutyrate by neonatal and suckling rats was investigated. Both isomers of 3-hydroxybutyrate were incorporated into hepatic lipid, amino acids, and protein throughout the developmental period. The enzyme activities of liver 3-oxo-CoA transferase and brain 3-hydroxybutyrate dehydrogenase were compared during the first 3 postnatal weeks. The results suggest that the enzymatic activity of liver 3-oxo-CoA transferase is sufficient to account for a major portion of the d-isomer incorporation. The production of CO₂ by rat liver was greater from d-3-hydroxybutyrate than that measured from the l-isomer. The in vitro oxidation of both the d- and l-isomers by rat liver was stimulated by ATP + CoA or by GTP + CoA which suggests that their utilization may also be mediated by acyl-CoA synthetase enzymes.     

Synthesis of l-3, 4-Dihydroxyphenylalanine from l-Tyrosine by Microorganisms

l-3, 4-Dihydroxyphenylalanine can be synthesized efficiently from l-tyrosine under acidic conditions by Aspergillus oryzae and other fungi.     

Synthesis and anti-viral activity of a series of d- and l-2'-deoxy-2'-fluororibonucleosides in the subgenomic HCV replicon system

Based on the discovery of (2'R)-d-2'-deoxy-2'-fluorocytidine as a potent anti-hepatitis C virus (HCV) agent, a series of d- and l-2'-deoxy-2'-fluororibonucleosides with modifications at 5- and/or 4-positions were synthesized and evaluated for their in vitro activity against HCV and bovine viral diarrhea virus (BVDV). The key step in the synthesis, the introduction of 2'-fluoro group, was achieved by either fluorination of 2,2'-anhydronucleosides with hydrogen fluoride-pyridine or potassium fluoride, or a fluorination of arabinonucleosides with DAST. Among the 27 analogues synthesized, only the 5-fluoro compound, namely (2'R)-d-2'-deoxy-2',5-difluorocytidine (13), demonstrated potent anti-HCV activity and toxicity to ribosomal RNA. The replacement of the 4-amino group with a thiol group resulted in the loss of activity, while the 4-methylthio substituted analogue (25) exhibited inhibition of ribosomal RNA. As N(4)-hydroxycytidine (NHC) had previously shown potent anti-HCV activity, we combined the two functionalities of the N(4)-hydroxyl and the 2'-fluoro into one molecule, resulting (2'R)-d-2'-deoxy-2'-fluoro-N(4)-hydroxycytidine (23). However, this nucleoside showed neither anti-HCV activity nor toxicity. All the l-forms of the analogues were devoid of anti-HCV activity. None of the compounds showed anti-BVDV activity, suggesting that the BVDV system cannot always predict anti-HCV activity.     

Bacterial assimilation of d- and l-2-chloropropionates and occurrence of a new dehalogenase

The occurrence of a new bacterial dehalogenase acting on both the optical isomers of 2-halogenated alkanoic acids was demonstrated. When the haloalkanoic acid-utilizing bacteria were screened in a medium containing dl-2-chloropropionate as a sole carbon source, two types of bacteria were isolated: (1) a few strains utilizing both d- and l-isomers of 2-chloropropionate and (2) strains utilizing only the l-isomer. A dehalogenating enzyme was obtained from the cells of Pseudomonas sp. which is able to utilize both isomers. The crude enzyme catalyzed the dehalogenation of d- and l-2-chloropropionates to yield l- and d-isomers of lactate, respectively. The enzyme showed the same pH optimum and heat inactivation rate for the d- and l-isomers. Apparent K _m values for d- and l-2-chloropropionates were 4.5 and 1.0 mM, respectively. The enzyme acted specifically on 2-haloalkanoic acids. Activity staining of disc-gels electrophoresed witg the crude enzyme preparation showed that the dehalogenation of d- and l-2-chloropropionates, monochloroacetate, dichloroacetate, 2,2-dichloropropionate, and dl-2-chlorobutyrate is due to a single protein.Abbreviations MCA monochloroacetic acid - DCA dichloroacetic acid - TCA trichloroacetic acid - 2 MCPA 2-monochloropropionic acid - 22 DCPA 2,2-dichloropropionic acid - 3 MCPA 3-monochloropropionic acid - 2 MCBA 2-monochlorobutyric acid - 3 MCBA 3-monochlorobutyric acid - 4 MCBA 4-monochlorobutyric acid     

Incorporation of l-[3H]fucose and d-[3H]glucosamine into cell-surface-associated glycoconjugates in epidermis of cultured pig skin slices.

1. Electron microscope autoradiography indicated that L-[3H]fucose and D-[3H]glucosamine were both incorporated into cell-surface-associated glycoconjugates in the epidermis of cultured pig skin slices. 2. Acid hydrolysis and paper chromatography of skin homogenates confirmed that there was little metabolic conversion of the labeled precursors to other sugars. 3. Epidermis was separated from dermis using CaCl2, and was extracted with 8 M-urea/5% (w/v) sodium dodecyl sulphate and was then analysed by gel electrophoresis. The major component labelled with D-[3H]glucosamine had an apparent molecular weight in excess of 200 000. This material was not labelled with L-[3H]fucose. Lower molecular-weight components were labelled to a similar extent with both L-[3H]fucose and D-[3H]glucosamine. 4. The high molecular-weight material labelled with D-[3H]glucosamine was released into the medium when the epidermal cells were dispersed with trypsin, indicating that it was either surface-associated or was extracellular. It was also labelled with D-[14C]glucuronic acid, 35SO4(2-) and to a small extent with 14C-labelled amino acids indicating that it contained glycosaminoglycans derived from epidermal proteoglycans. This was confirmed by the fact that it was degraded by testicular hyaluronoglucosidase. It was not present in isolated membranes but was recovered in the soluble fraction from epidermal homogenates. It is therefore only very loosely bound at the cell surface or is present in the extracellular spaces. 5. Membrane-bound [3H]glycoproteins were identified after differential centrifugation of epidermal homogenates. The radioactivity profiles of membrane glycoproteins were similar whether L-[3H]fucose or D-[3H]glucosamine were used and both consisted of a major heterogeneous peak in the apparent mol.wt. range 70 000--150 000. [3H]Glycoproteins in this molecular-weight range were also major components of a plasma-membrane-enriched fraction. These glycoproteins were probably bound to the membrane by hydrophobic interactions, since they were only solubilized by treatment with detergent or organic solvent. They contained terminal sialic acid residues, since they were degraded by neuraminidase.     

Making 3d-4f hexanuclear clusters from heterotrinuclear cationic building blocks

The syntheses and crystal structures of two new hexanuclear complexes are reported: [{(LCu^II(ONO₂))(LCu^II(H₂O))Nd^III}₂(μ-C₂O₄)](NO₃)₂ · 6H₂O (1) and [{(LNi^II(H₂O))(N(CN)₂)}₂Pr^III}₂(ONO₂)](OH) · 2H₂O · 3CH₃CN (2) (L is the dianion of the Schiff-base resulted from the 2:1 condensation of 3-methoxysalyciladehyde with 1,3-propanediamine). Compounds 1 and 2 were obtained by connecting heterotrinuclear cationic complexes [{LM^II}₂Ln^III]³⁺ with oxalato or nitrato linkers. The structure of the complex cation in 1 shows two almost linear trinuclear [Cu₂Nd] moieties which are linked by a bis-chelating oxalato bridge between the neodymium ions. The hexanuclear cationic moiety in 2 is built up of two heterotrinuclear [Ni₂Pr] units that are linked by a nitrato group bridging two praseodymium(III) ions. The spectroscopic (FTIR, UV-Vis) and magnetic properties of 1 and 2 have been investigated.     

Three-dimensional 3d-4f heterometallic polymers containing both azide and carboxylate as co-ligands

The hydrothermal reaction of Ln(NO₃)₃, Ni(NO₃)₂, NaN₃, and isonicotinic acid (L) yielded two novel 3-D coordination frameworks (1 and 2) of general formula [Ni₂Ln(L)₅(N₃)₂ (H₂O)₃] · 2H₂O (Ln = Pr(III) for 1 and Nd(III) for 2), containing Ni-Pr or Ni-Nd hybrid extended three-dimensional networks containing both azido and carboxylate as co-ligands. Both the compounds are found to be isostructural and crystallize in monoclinic system having P2₁/n space group. Here the lanthanide ions are found to be nonacoordinated. Both bidentate and monodentate modes of binding of the carboxylate with the lanthanides have been observed in the above complexes. Variable temperature magnetic studies of the above two complexes have been investigated in the temperature range 2-300 K which showed dominant antiferromagnetic interaction in both the cases and these experimental results are analyzed with the theoretical models.     

Structure of the major neutral oligosaccharide-alditols released from the egg jelly coats ofAxolotl maculatum. Characterization of the carbohydrate sequence GalNAc({eta}l-4)[Fuc({alpha}l-3)] GlcNAc({eta}l-3 6)

Several O-linked oligosaccharides of the jelly coat surroundingthe eggs of Axolotl maculatum were analysed by ¹H-NMR spectroscopy.The four major oligosaccharide-alditols released by reductive-elimination display either the Lewis^x(Le^x) determinant or thesequence GalNAc(l-4)[Fuc(l-3)]GlcNAc This last structure haspreviously been characterized in allergenically active oligosaccharidesisolated from the sea squirt H-antigen, and hi the N-linkedglycans of Schistosoma mansoni and human urokinase. It representsthe major carbohydrate chain found in A.macu-latum,the oviductof which constitutes an excellent source of l-4-acetylgalactosaminyltransferase activity. Moreover, the carbohydrate chains isolatedfrom A.maculatum are quite different from those found hi sevenother amphibian species, in which the presence of species-specificmaterial has been characterized. The role of carbohydrates appearsmore and more apparent during the fertilization process, andthe diversity of the O-linked oligosaccharides supports sucha biological role. amphibian egg jelly coats Axolotl maculatum/Hnmr/oligosccharide structure     

Self-assembly of 3-D 4d-4f coordination frameworks based on pyridine-3,5-dicarboxylic acid: Syntheses, crystal structures and luminescence

The hydrothermal reactions of H₂PDC, AgNO₃ with Eu₂O₃ or Tb(NO₃)₃·6H₂O gave rise to two novel three-dimensional 4d-4f heterometallic metal-organic coordination polymers, AgEu(PDC)₂ (1) and AgTb(PDC)₂ (2) (H₂PDC = pyridine-3,5-dicarboxylic acid), and characterized by elemental analysis, IR, thermal analysis and single-crystal X-ray diffraction. Complexes 1 and 2 crystallize in the monoclinic system, P2/c space group; the structure determination reveal that both of them are isostructural and feature an unusual three-dimensional heterometallic network structure in which infinite lanthanide-carboxylate chains are linked by [Ag(PDC)₂]³⁻ metalloligands to form a mixed-metal coordination network. Moreover, the luminescent properties of two complexes have also been investigated at room temperature.     

Syntheses and characterization of 3D heterometallic (3d-4f) metal-organic frameworks: Reversible de- and rehydration performance and magnetic properties

By the “metalloligand” strategy, two new 3d-4f heterometallic metal-organic frameworks (MOFs), {[Ln₂Cu₃(IDA)₆] · 1.5H₂O}_n [Ln = Tb (1) and Dy (2); H₂IDA = iminodiacetate acid], had been prepared. X-ray crystal structure analyses show that 1 and 2 possess of 3D frameworks with highly ordered 1D channels along the c axis. The highly stable skeleton and reversible de- and rehydration performance of 1 are demonstrated by thermogravimetric and powder X-ray diffraction analyses, and a low temperature magnetic study of 2 reveals a weak ferromagnetic interaction between the metal ions.     

Separation of d-(+)-Nicotine from a Racemic Mixture by Stereospecific Degradation of the l-(-) Isomer with Pseudomonas putida

Incubation of racemic mixtures of dl-(+/-)-nicotine with Pseudomonas putida resulted in a complete stereoselective degradation of the l-(-) isomer. Unnatural d-(+)-nicotine, which is of pharmacological interest for stereochemical studies of various nicotine-responsive systems, was not affected by the bacterium and was recovered by extraction.