Literature DB >> 28990867

Characterization of colchicine binding with normal and glycated albumin: In vitro and molecular docking analysis.

Nayyar Rabbani1, Shams Tabrez2, Badar Ul Islam3, Md Tabish Rehman4, Abdulrahman M Alsenaidy1, Mohamed F AlAjmi4, Rais Ahmad Khan5, Mohammad A Alsenaidy6, Mohd Shahnawaz Khan1.   

Abstract

The transport of more than 90% of the drugs viz. anticoagulants, analgesics, and general anesthetics in the blood takes place by albumin. Hence, albumin is the prime protein needs to be investigated to find out the nature of drug binding. Serum albumin molecules are prone to glycation at elevated blood glucose levels as observed in diabetics. In this piece of work, glycation of bovine serum albumin (BSA) was carried out with glyceraldehyde and characterized by molecular docking and fluorometry techniques. Glycation of BSA showed 25% loss of free amino groups and decreased protein fluorescence (60%) with blue shift of 6 nm. The present study was also designed to evaluate the binding of colchicine (an anti-inflammatory drug) to native and glycated BSA and its ability to displace 8-analino-1-nephthalene sulfonic acid (ANS), from the BSA-ANS complex. Binding of ANS to BSA showed strong binding (Ka = 4.4 μM) with native conformation in comparison to glycated state (Ka = 8.4 μM). On the other hand, colchicine was able to quench the fluorescence of native BSA better than glycated BSA and also showed weaker affinity (Ka = 23 μM) for glycated albumin compared with native state (Ka = 16 μM). Molecular docking study showed that both glyceraldehyde and colchicine bind to common residues located near Sudlow's site I that explain the lower binding of colchicine in the glycated BSA. Based on our results, we believe that reduced drugs-binding affinity to glycated albumin may lead to drugs accumulation and precipitation in diabetic patients.

Entities:  

Keywords:  bovine serum albumin; colchicine; drug-binding capability; glycation; glyceraldehyde

Mesh:

Substances:

Year:  2017        PMID: 28990867     DOI: 10.1080/07391102.2017.1389661

Source DB:  PubMed          Journal:  J Biomol Struct Dyn        ISSN: 0739-1102


  9 in total

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  9 in total

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