AI Article Synopsis

  • * It was found that CB-F3GA binds to two different sites on HSA, with one site (PBS-II) showing a much stronger affinity compared to the other (PBS-I), which suggests varied strength in the binding interactions.
  • * Binding at the high-affinity site promotes the formation of dimeric clusters, while binding at the low-affinity site leads to larger tetramers, indicating that drug binding could impact how HSA aggregates, which is important for understanding drug delivery

Article Abstract

Binding interactions between Cibacron Blue-F3GA (CB-F3GA) and human serum albumin (HSA, at physiologically ten-fold lower concentration) was studied by isothermal titration calorimetry (ITC) and in-silico docking computations. ITC experiments revealed two separate binding sites on HSA with different binding affinities for CB-F3GA. The high-affinity binding site (PBS-II) on HSA binds CB-F3GA at nanomolar scale (K  = 118 ± 107 nM) with favorable binding enthalpy (ΔH  = - 6.47 ± 0.44 kcal/mol) and entropy (-TΔS  = -2.98 kcal/mol) energies. CB-F3GA binds to the low-affinity binding site (PBS-I) at μM scale (K  = 31.20 ± 18.40 μM) with favorable binding enthalpy (ΔH  = - 5.03 ± 3.86 × 10 kcal/mol) and entropy (-TΔS  = -1.12 kcal/mol) energies. ITC binding data strongly suggest that CB-F3GA binding to PBS-II site increases the formation of dimeric-HSA clusters (N  = 2.43 ± 0.50), while binding to PBS-I leads to tetrameric-HSA clusters (N  = 4.61 ± 0.90). These results suggest that a higher degree of HSA aggregation upon drug binding may be expected under physiological conditions, a notion that should be further investigated for the delivery and toxicity of drug-HSA interactions.

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Source
http://dx.doi.org/10.1002/jmr.3040DOI Listing

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