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Purification and Characterization of Conjugated Bile Salt Hydrolase from Bifidobacterium longum BB536
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Bifidobacterium species deconjugate taurocholic, taurodeoxycholic, taurochenodeoxycholic, glycocholic, glycodeoxycholic, and glycochenodeoxycholic acids. The enzyme level increases in the growth phase. No increase in activity is observed for the cytoplasmic enzyme after addition of conjugated bile acids to a stationary-phase culture. Conjugated bile salt hydrolase (BSH) was purified from Bifidobacterium longum BB536. Its apparent molecular mass in denaturing polyacrylamide gel electrophoresis was ca. 40,000 Da. The intact enzyme had a relative molecular weight of ca. 250,000 as determined by gel filtration chromatography, suggesting that the native BSH of B. longum is probably a hexamer. The purified enzyme is active towards both glycine and taurine conjugates of cholate, deoxycholate, and chenodeoxycholate. The pH optimum is in the range of 5.5 to 6.5. A loss of BSH activity is observed after incubation at temperatures higher than 42(deg)C; at 60(deg)C, 50% of the BSH activity is lost. The importance of free sulfhydryl groups at the enzyme active center is suggested. For B. longum BB536, no significant difference in the initial rate of deconjugation and enzymatic efficiency appears between bile salts. The enzymatic efficiency is higher for B. longum BB536 than for other genera. In this paper, a new method which permits a display of BSH activity directly on polyacrylamide gels is described; this method confirms the molecular weight obtained for B. longum BB536 BSH.
American Society for Microbiology
Title: Purification and Characterization of Conjugated Bile Salt Hydrolase from Bifidobacterium longum BB536
Description:
Bifidobacterium species deconjugate taurocholic, taurodeoxycholic, taurochenodeoxycholic, glycocholic, glycodeoxycholic, and glycochenodeoxycholic acids.
The enzyme level increases in the growth phase.
No increase in activity is observed for the cytoplasmic enzyme after addition of conjugated bile acids to a stationary-phase culture.
Conjugated bile salt hydrolase (BSH) was purified from Bifidobacterium longum BB536.
Its apparent molecular mass in denaturing polyacrylamide gel electrophoresis was ca.
40,000 Da.
The intact enzyme had a relative molecular weight of ca.
250,000 as determined by gel filtration chromatography, suggesting that the native BSH of B.
longum is probably a hexamer.
The purified enzyme is active towards both glycine and taurine conjugates of cholate, deoxycholate, and chenodeoxycholate.
The pH optimum is in the range of 5.
5 to 6.
5.
A loss of BSH activity is observed after incubation at temperatures higher than 42(deg)C; at 60(deg)C, 50% of the BSH activity is lost.
The importance of free sulfhydryl groups at the enzyme active center is suggested.
For B.
longum BB536, no significant difference in the initial rate of deconjugation and enzymatic efficiency appears between bile salts.
The enzymatic efficiency is higher for B.
longum BB536 than for other genera.
In this paper, a new method which permits a display of BSH activity directly on polyacrylamide gels is described; this method confirms the molecular weight obtained for B.
longum BB536 BSH.
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