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- W1490299216 abstract "Degradation of heat-treated cells of Proteus vulgaris P 18 with a protease preparation from a soil Bacillus subtilis allowed the isolation of a cell envelope structural entity, 60–70 Å thick, consisting of two electron-dense layers separated by a light one and composed, at least in part, of lipopolysaccharide O-antigen and of peptidoglycan. An enriched preparation, of which 55% of the dry weight consisted of an intact peptidoglycan, was obtained through the sequential action upon lyophilized cells of hot aqueous sodium dodecyl sulfate and B. subtilis protease. Both Chalaropsis B endo-N-acetylmuramidase and Streptomyces DD carboxypeptidase solubilized the enriched peptidoglycan preparation. The Chalaropsis enzyme completely degraded the glycan moiety into peptide-substituted disaccharide units. The DD carboxypeptidase hydrolyzed the d-alanyl-(d)-meso-diaminopimelic acid linkages involved in peptide cross-linking. In the intact peptidoglycan, about 35% of the l-alanyl-γ-d-glutamyl-(l)-meso-diaminopimelic acid-(l)-d-alanine residues occurred as uncross-linked monomers, 40% of them as peptide dimers and 16% as peptide trimers. It is likely that not all the peptides retained the d-alanine residue at their C-termini. About half of the N-acetylmuramic acid residues in the glycan moiety are O-acetylated, a property which is compatible with high lysozyme resistance exhibited by the P. vulgaris peptidoglycan." @default.
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- W1490299216 date "1971-06-01" @default.
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- W1490299216 title "The cell envelope in Proteus vulgaris P 18" @default.
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- W1490299216 doi "https://doi.org/10.1016/0005-2736(71)90149-0" @default.
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