4.4 Article

Characterization of an acid-dependent arginine decarboxylase enzyme from Chlamydophila pneumoniae

Journal

JOURNAL OF BACTERIOLOGY
Volume 189, Issue 20, Pages 7376-7383

Publisher

AMER SOC MICROBIOLOGY
DOI: 10.1128/JB.00772-07

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Funding

  1. NIAID NIH HHS [AI064444, R21 AI064444, R21 AI064444-01A2] Funding Source: Medline
  2. NIEHS NIH HHS [ES07784, P30 ES007784] Funding Source: Medline

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Genome sequences from members of the Chlamydiales encode diverged homologs of a pyruvoyl-dependent arginine decarboxylase enzyme that nonpathogenic euryarchaea use in polyamine biosynthesis. The Chlamydiales lack subsequent genes required for polyamine biosynthesis and probably obtain pollyamines from their host cells. To identify the function of this protein, the CPn1032 homolog from the respiratory pathogen Chlamydophila pneumoniae was heterologously expressed and purified. This protein self-cleaved to form a reactive pyruvoyl group, and the subunits assembled into a thermostable (4)3 complex. The mature enzyme specifically catalyzed the decarboxylation of L-arginine, with an unusually low pH optimum of 3.4. The CPn1032 gene complemented a mutation in the Escherichia coli adiA gene, which encodes a pyridoxal 5'phosphate-dependent arginine decarboxylase, restoring arginine-dependent acid resistance. Acting together with a putative arginine-agmatine antiporter, the CPn1032 homologs may have evolved convergently to form an arginine-dependent acid resistance system. These genes are the first evidence that obligately intracellular chlamydiae may encounter acidic conditions. Alternatively, this system could reduce the host cell arginine concentration and produce inhibitors of nitric oxide synthase.

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