Molecular characterization and protein analysis of the cap region, which is essential for encapsulation in Bacillus anthracis.

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J Bacteriol. 1989 February; 171(2): 722-730

research-article

Molecular characterization and protein analysis of the cap region, which is essential for encapsulation in Bacillus anthracis.

S Makino, I Uchida, N Terakado, C Sasakawa and M Yoshikawa

Department of Bacteriology, University of Tokyo, Japan.

ABSTRACT

By using genetic complementation tests with various in vitro-constructedmutants with mutations in the cap region (which is essentialfor encapsulation in Bacillus anthracis), we identified threecistrons, capB, capC, and capA, in this order of arrangement.Minicell analysis revealed that these cistrons produce proteinsof 44, 16, and 46 kilodaltons, respectively. The complete nucleotidesequence of 3,244 base pairs covering the whole cap region wasdetermined and revealed the existence of the three open readingframes of capB (397 amino acid residues; molecular weight, 44,872),capC (149 amino acid residues; molecular weight, 16,522), andcapA (411 amino acid residues; molecular weight, 46,420) arrangedin the order predicted by complementation tests. These threecistrons were all transcribed in the same direction from promotersunique to each cistron. Judging from the predicted amino acidsequence of the three proteins and from their localization andtheir sensitivity to various physicochemical treatments, theyappeared to be membrane-associated enzymes mediating the polymerizationof D-glutamic acid via the membrane. Capsular peptides immunologicallyidentical to that of B. anthracis were found in B. subtilis,B. megaterium, and B. licheniformis, but no sequence homologousto the cap region was found in any of these bacilli other thanB. anthracis. Using strains of B. anthracis with or withoutinsertional inactivation of the cap region, we found that thecapsule of B. anthracis conferred strong resistance to phagocytosisupon the bacterial host.

J Bacteriol. 1989 February; 171(2): 722-730

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