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      Unusual sequence organization in CenB, an inverting endoglucanase from Cellulomonas fimi.

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      Journal of Bacteriology
      American Society for Microbiology

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          Abstract

          The nucleotide sequence of the cenB gene was determined and used to deduce the amino acid sequence of endoglucanase B (CenB) of Cellulomonas fimi. CenB comprises 1,012 amino acids and has a molecular weight of 105,905. The polypeptide is divided by so-called linker sequences rich in proline and hydroxyamino acids into five domains: a catalytic domain of 607 amino acids at the N terminus, followed by three repeats of 98 amino acids each which are greater than 60% identical, and a C-terminal domain of 101 amino acids which is 50% identical to the cellulose-binding domains of C. fimi cellulases Cex and CenA. A deletion mutant of the cenB gene encodes a polypeptide lacking the C-terminal 333 amino acids of CenB. The truncated polypeptide is catalytically active and, like intact CenB, binds to cellulose, suggesting that CenB has a second cellulose-binding site. The sequence of amino acids 1 to 461 of CenB is 35% identical, with a further 15% similarity, to that of a cellulase from avocado, which places CenB in cellulase family E. CenB releases mostly cellobiose and cellotetraose from cellohexaose. Like CenA, CenB hydrolyzes the beta-1,4-glucosidic bond with inversion of the anomeric configuration. The pH optimum for CenB is 8.5, and that for CenA is 7.5.

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          Author and article information

          Journal
          Journal of Bacteriology
          J. Bacteriol.
          American Society for Microbiology
          0021-9193
          1098-5530
          January 01 1991
          January 1991
          January 01 1991
          : 173
          : 1
          : 308-314
          Article
          10.1128/jb.173.1.308-314.1991
          207188
          1987122
          0d964845-d4b5-40ff-930c-7afbb812d8fc
          © 1991
          History

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