Journal of Lipid Research (Oct 1984)

Mode of action of steroid desmolase and reductases synthesized by Clostridium 'scindens' (formerly Clostridium strain 19).

  • J Winter,
  • G N Morris,
  • S O'Rourke-Locascio,
  • V D Bokkenheuser,
  • E H Mosbach,
  • B I Cohen,
  • P B Hylemon

Journal volume & issue
Vol. 25, no. 10
pp. 1124 – 1131

Abstract

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A recently isolated hitherto unknown Clostridium from human feces, designated Clostridium ''scindens'' (formerly strain 19), synthesizes at least two enzymes active on the side-chain of the steroid molecule and two enzymes active on the hydroxyl groups of the 7-position of bile acids. Steroid desmolase, responsible for side-chain cleavage of corticoids, and 20 alpha-hydroxysteroid dehydrogenase have not been detected in any other bacterial species of the resident colonic flora. Steroid desmolase is Eh-dependent (optimum ca. -130 mV), requires a hydroxy group at C-17, and preferably an alpha-ketol group in the side-chain; an alpha-hydroxy group at C-20 reduces and a beta-hydroxy group at C-20 prevents side-chain cleavage. With suitable substrates, the yield of C-19 steroids is proportional to the bacterial multiplication rate. 20 alpha-Hydroxysteroid dehydrogenase (20 alpha-HSDH) is also Eh-dependent (optimum ca. -300 mV) and reduces the C-20 keto function to an alpha-hydroxy group, regardless of the presence or absence of a hydroxy group at C-17. 7 alpha-Dehydroxylase metabolizes cholic and chenodeoxycholic acid, while 7 beta-hydroxysteroid dehydrogenase acts upon ursodeoxycholic acid. The latter two enzymes are not specific for C. scindens.