The interaction of human and bovine serum proteins with CYP3A in human liver microsomes: inhibition of testosterone 6β-hydroxylation by albumin, α-globulins, α 1-acid glycoprotein and γ-globulins

The effects of human and bovine serum proteins on CYP3A activity, using testosterone as the probe substrate, were investigated in human liver microsomes. Serum albumin, α-globulins, and α 1-acid glycoprotein (α 1-AGP) of both species significantly inhibited testosterone 6β-hydroxylation. When the in...

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Published inToxicology letters Vol. 136; no. 1; pp. 33 - 41
Main Authors Matsumoto, Satoshi, Ding, Li R, Ishii, Mikio, Fischer, Nancy E, Inaba, Tadanobu
Format Journal Article
LanguageEnglish
Published Elsevier Ireland Ltd 15.11.2002
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Abstract The effects of human and bovine serum proteins on CYP3A activity, using testosterone as the probe substrate, were investigated in human liver microsomes. Serum albumin, α-globulins, and α 1-acid glycoprotein (α 1-AGP) of both species significantly inhibited testosterone 6β-hydroxylation. When the inhibitory effects of serum proteins were compared with serum protein binding data, human α-globulins, with a ratio (relative metabolic activity/unbound fraction) of 0.3, showed higher, and bovine α 1-AGP, with the ratio of 1.4, showed lower inhibitory effects than those expected from protein binding of testosterone. The effects of the other serum proteins were close to those expected from protein binding, according to the free drug hypothesis. The K i values obtained from the Dixon plots were 0.32% (w/v, 48 μM) for human serum albumin (HSA), 0.48% for human α-globulins, and 0.23% (52 μM) for human α 1-AGP. K i values of bovine serum albumin, bovine α-globulins and bovine α 1-AGP were 3–5 times higher than those of the respective human proteins. The results suggest a direct interaction of some of these serum proteins with the active site of the CYP3A isoform. Since the bovine serum proteins showed weaker inhibitory effects than human serum proteins, the wide use of BSA, which is viewed as interchangeable with HSA, needs to be cautioned.
AbstractList The effects of human and bovine serum proteins on CYP3A activity, using testosterone as the probe substrate, were investigated in human liver microsomes. Serum albumin, α-globulins, and α 1-acid glycoprotein (α 1-AGP) of both species significantly inhibited testosterone 6β-hydroxylation. When the inhibitory effects of serum proteins were compared with serum protein binding data, human α-globulins, with a ratio (relative metabolic activity/unbound fraction) of 0.3, showed higher, and bovine α 1-AGP, with the ratio of 1.4, showed lower inhibitory effects than those expected from protein binding of testosterone. The effects of the other serum proteins were close to those expected from protein binding, according to the free drug hypothesis. The K i values obtained from the Dixon plots were 0.32% (w/v, 48 μM) for human serum albumin (HSA), 0.48% for human α-globulins, and 0.23% (52 μM) for human α 1-AGP. K i values of bovine serum albumin, bovine α-globulins and bovine α 1-AGP were 3–5 times higher than those of the respective human proteins. The results suggest a direct interaction of some of these serum proteins with the active site of the CYP3A isoform. Since the bovine serum proteins showed weaker inhibitory effects than human serum proteins, the wide use of BSA, which is viewed as interchangeable with HSA, needs to be cautioned.
Author Matsumoto, Satoshi
Ishii, Mikio
Fischer, Nancy E
Ding, Li R
Inaba, Tadanobu
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Keywords Albumin
CYP3A
Testosterone
Globulins
α 1-AGP
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Snippet The effects of human and bovine serum proteins on CYP3A activity, using testosterone as the probe substrate, were investigated in human liver microsomes. Serum...
SourceID elsevier
SourceType Publisher
StartPage 33
SubjectTerms Albumin
CYP3A
Globulins
Testosterone
α 1-AGP
Title The interaction of human and bovine serum proteins with CYP3A in human liver microsomes: inhibition of testosterone 6β-hydroxylation by albumin, α-globulins, α 1-acid glycoprotein and γ-globulins
URI https://dx.doi.org/10.1016/S0378-4274(02)00285-0
Volume 136
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