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Protein & Peptide Letters

Editor-in-Chief

ISSN (Print): 0929-8665
ISSN (Online): 1875-5305

Research Article

Interaction of Cu+2 with α-Crystallin: A Biophysical and Mass Spectrometric Study

Author(s): Srabani Karmakar* and K.P. Das

Volume 25, Issue 3, 2018

Page: [275 - 284] Pages: 10

DOI: 10.2174/0929866525666171229230611

Price: $65

Abstract

Background: αA- and αB- crystallin are members of small heat shock protein family with chaperone property. Their interactions with Cu2+ ions are reported in neurodegenerative diseases. We have been studying the effect of small ionic molecules on the stability of α-crystallin. Cu2+ is co-ordinated with αB-crystallin involving three histidine residues and one aspartic acid residue as potential binding sites. However, copper binding sites for the oligomeric native protein αA-crystallin protein is not known.

Objective: The objective of this study was to study oligomerization and stability of αA- and αBcrystallin in presence and absence of Cu2+ ions and to find binding sites of Cu2+ on αA-crystallin.

Methods: The recombinant Human αA- and αB-crystallin proteins were purified after overexpression from the E. coli BL21DE3 cell lysate by a combination of ion-exchange and gel filtration chromatography. Mass analysis of αA- and αB-crystallin in absence and presence of Cu2+ were carried out by MALDI TOF MS. Stability of αA-crystallin in presence and absence of Cu2+ was determined by equilibrium urea denaturation experiments. The equilibrium urea unfolding profiles of the αA-crystallin in absence and presence of different Cu2+ concentrations were fitted according to the three state model of protein unfolding. Dynamic Light Scattering (DLS) measurements were carried out to detect the oligomeric size of αA-crystallin in presence and absence of Cu2+ during urea unfolding. Histidine residues were modified by DEPC (Diethyl pyro carbonate). Chemically modified and unmodified αA-crystallin was digested by trypsin prior to MALDI MS analysis. Cu2+ pre-incubation was done before the chemical modification.

Results: Mass spectrometric detection of intact protein allows direct measurement of Cu2+ ions bound to the protein. Thus the average numbers of Cu2+ bound to αA- and αB-crystallin were 4.2 and 3.6 respectively per subunit. It is seen that in presence of Cu2+ ions the free energy (ΔG) of unfolding of αA-crystallin almost doubled. The size analysis by dynamic light scattering data clearly indicated that in presence of Cu2+ ions the oligomeric size remain unchanged with increasing urea solutions. Mass spectrometric detection with chemical modification of histidine residues of αA-crystallin in presence and absence of Cu2+ indicated that amino acid residues H107, H100, H115 of αA-crystallin are involved in Cu2+ binding.

Conclusion: Our results indicated that Cu2+ helped in increasing stability of αA-crystallin and three histidine residues H100, H107 and H115 of αA-crystallin are Cu2+ binding residues.

Keywords: α-crystallin chaperone, stabilization by Cu2+, dynamic light scattering of α-crystallin, urea unfolding of α- crystallin, MALDI TOF mass spectrometry, histidine residues.

Graphical Abstract


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