TY - JOUR
T1 - Hydrophobic vitamin B12. Part 15 1. Carbon-skeleton rearrangement reactions mediated by hydrophobic vitamin B12 covalently bound to an anionic lipid species in aqueous media
AU - Hisaeda, Yoshio
AU - Ogawa, Akihiro
AU - Ohno, Teruhisa
AU - Murakami, Yukito
N1 - Funding Information:
The present work was supported in part by a Grant-in-Aid for Scientific Research from the Ministry of Education, Science, Sports and Culture of Japan, the Ministry of Agriculture, Forestry and Fisheries of Japan in the framework of the Pioneering Research Project in Biotechnology, and a grant from the Nagase Science and Technology Foundation.
PY - 1998/5/15
Y1 - 1998/5/15
N2 - A novel artificial vitamin B12 holoenzyme was prepared in aqueous media by combination of a hydrophobic vitamin Bi2 covalently bound to an anionic lipid species and a bilayer matrix of sodium N,N-dihexadecyl-Nα-(6-sulfohexanoyl)-L-alaninamide. Microenvironmental properties around a hydrophobic vitamin B12 placed in the bilayer membrane were examined by electronic spectroscopy and fluorescence polarization measurements. The hydrophobic vitamin B12 was well separated from a bulk aqueous phase, and its molecular motion was markedly suppressed. A reaction mimicking catalytic functions of methylmalonyl-CoA mutase was carried out by using hydrophobic vitamin B12 derivatives having a diethyl 2,2-bis(ethoxycarbonyl)propyl group at an axial site of the nuclear cobalt. A carbon-skeleton rearrangement of the alkyl ligand bound to a hydrophobic vitamin B12 was markedly promoted in the bilayer matrix, relative to the reaction in methanol and benzene, via formation of a radical intermediate. A reaction simulating catalysis by α-methyleneglutarate mutase was also carried out. The cyanide ion enhanced a carbon-skeleton rearrangement of the 2,3-bis(ethoxycarbonyl)-l-butene moiety bound to hydrophobic vitamin B12 derivatives in the bilayer membrane under photolysis conditions via formation of an anionic intermediate. As an extension of such mimicking reactions, a carbon-skeleton rearrangement reaction of diethyl 2-acetylamino-2-methylpropanedioate coordinated to a hydrophobic vitamin B12 covalently bound to a lipid species, which afforded diethyl 2-acetylaminobutanedioate, was also examined in the bilayer membrane under photolysis conditions. The motional repression and desolvation effects operated on the substrate-bound hydrophobic vitamin B12 were found to be responsible for enhancement of the rearrangement reactions of the substrate radicals formed under photolysis conditions.
AB - A novel artificial vitamin B12 holoenzyme was prepared in aqueous media by combination of a hydrophobic vitamin Bi2 covalently bound to an anionic lipid species and a bilayer matrix of sodium N,N-dihexadecyl-Nα-(6-sulfohexanoyl)-L-alaninamide. Microenvironmental properties around a hydrophobic vitamin B12 placed in the bilayer membrane were examined by electronic spectroscopy and fluorescence polarization measurements. The hydrophobic vitamin B12 was well separated from a bulk aqueous phase, and its molecular motion was markedly suppressed. A reaction mimicking catalytic functions of methylmalonyl-CoA mutase was carried out by using hydrophobic vitamin B12 derivatives having a diethyl 2,2-bis(ethoxycarbonyl)propyl group at an axial site of the nuclear cobalt. A carbon-skeleton rearrangement of the alkyl ligand bound to a hydrophobic vitamin B12 was markedly promoted in the bilayer matrix, relative to the reaction in methanol and benzene, via formation of a radical intermediate. A reaction simulating catalysis by α-methyleneglutarate mutase was also carried out. The cyanide ion enhanced a carbon-skeleton rearrangement of the 2,3-bis(ethoxycarbonyl)-l-butene moiety bound to hydrophobic vitamin B12 derivatives in the bilayer membrane under photolysis conditions via formation of an anionic intermediate. As an extension of such mimicking reactions, a carbon-skeleton rearrangement reaction of diethyl 2-acetylamino-2-methylpropanedioate coordinated to a hydrophobic vitamin B12 covalently bound to a lipid species, which afforded diethyl 2-acetylaminobutanedioate, was also examined in the bilayer membrane under photolysis conditions. The motional repression and desolvation effects operated on the substrate-bound hydrophobic vitamin B12 were found to be responsible for enhancement of the rearrangement reactions of the substrate radicals formed under photolysis conditions.
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U2 - 10.1016/s0020-1693(97)06036-2
DO - 10.1016/s0020-1693(97)06036-2
M3 - Article
AN - SCOPUS:0000460878
VL - 273
SP - 299
EP - 309
JO - Inorganica Chimica Acta
JF - Inorganica Chimica Acta
SN - 0020-1693
IS - 1-2
ER -