{"title":"Analysis of Ion and pH Effects on Iron Response Element (IRE) and mRNA-Iron Regulatory Protein (IRP1) Interactions","authors":"Mateen A. Khan","doi":"10.2174/2212796814999200604121937","DOIUrl":null,"url":null,"abstract":"\n\nCellular iron uptake, utilization, and storage are tightly controlled\nthrough the action of iron regulatory proteins (IRPs). IRPs achieve this control by binding to\nIREs-mRNA in the 5'- or 3'-end of mRNAs that encode proteins involved in iron metabolism.\nThe interaction of iron regulatory proteins with mRNAs containing an iron responsive\nelement plays a central role in this regulation. The IRE RNA family of mRNA regulatory\nstructures combines absolutely conserved protein binding sites with phylogenetically conserved\nbase pairs that are specific to each IREs and influence RNA/protein stability. Our\nprevious result revealed the binding and kinetics of IRE RNA with IRP1. The aim of the present\nstudy is to gain further insight into the differences in protein/RNA stability as a function\nof pH and ionic strength.\n\n\n\nTo determine the extent to which the binding affinity and stability of protein/RNA\ncomplex was affected by ionic strength and pH.\n\n\n\nFluorescence spectroscopy was used to characterize IRE RNA-IRP protein interaction.\n\n\n\nScatchard analysis revealed that the IRP1 protein binds to a single IRE RNA molecule.\nThe binding affinity of two IRE RNA/IRP was significantly changed with the change in\npH. The data suggests that the optimum binding of RNA/IRP complex occurred at pH 7.6.\nDissociation constant for two IRE RNA/IRP increased with an increase in ionic strength,\nwith a larger effect for FRT IRE RNA. This suggests that numerous electrostatic interactions\noccur in the ferritin IRE RNA/IRP than ACO2 IRE RNA/IRP complex. Iodide quenching\nshows that the majority of the tryptophan residues in IRP1 are solvent-accessible, assuming\nthat most of the tryptophan residues contribute to protein fluorescence.\n\n\n\nThe results obtained from this study clearly indicate that IRE RNA/IRP complex\nis destabilized by the change in pH and ionic strength. These observations suggest that\nboth pH and ion are important for the assembly and stability of the IRE RNA/IRP complex\nformation.\n","PeriodicalId":10784,"journal":{"name":"Current Chemical Biology","volume":"19 1","pages":"88-99"},"PeriodicalIF":0.0000,"publicationDate":"2020-11-19","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"1","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Current Chemical Biology","FirstCategoryId":"1085","ListUrlMain":"https://doi.org/10.2174/2212796814999200604121937","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"","JCRName":"","Score":null,"Total":0}
引用次数: 1
Abstract
Cellular iron uptake, utilization, and storage are tightly controlled
through the action of iron regulatory proteins (IRPs). IRPs achieve this control by binding to
IREs-mRNA in the 5'- or 3'-end of mRNAs that encode proteins involved in iron metabolism.
The interaction of iron regulatory proteins with mRNAs containing an iron responsive
element plays a central role in this regulation. The IRE RNA family of mRNA regulatory
structures combines absolutely conserved protein binding sites with phylogenetically conserved
base pairs that are specific to each IREs and influence RNA/protein stability. Our
previous result revealed the binding and kinetics of IRE RNA with IRP1. The aim of the present
study is to gain further insight into the differences in protein/RNA stability as a function
of pH and ionic strength.
To determine the extent to which the binding affinity and stability of protein/RNA
complex was affected by ionic strength and pH.
Fluorescence spectroscopy was used to characterize IRE RNA-IRP protein interaction.
Scatchard analysis revealed that the IRP1 protein binds to a single IRE RNA molecule.
The binding affinity of two IRE RNA/IRP was significantly changed with the change in
pH. The data suggests that the optimum binding of RNA/IRP complex occurred at pH 7.6.
Dissociation constant for two IRE RNA/IRP increased with an increase in ionic strength,
with a larger effect for FRT IRE RNA. This suggests that numerous electrostatic interactions
occur in the ferritin IRE RNA/IRP than ACO2 IRE RNA/IRP complex. Iodide quenching
shows that the majority of the tryptophan residues in IRP1 are solvent-accessible, assuming
that most of the tryptophan residues contribute to protein fluorescence.
The results obtained from this study clearly indicate that IRE RNA/IRP complex
is destabilized by the change in pH and ionic strength. These observations suggest that
both pH and ion are important for the assembly and stability of the IRE RNA/IRP complex
formation.
期刊介绍:
Current Chemical Biology aims to publish full-length and mini reviews on exciting new developments at the chemistry-biology interface, covering topics relating to Chemical Synthesis, Science at Chemistry-Biology Interface and Chemical Mechanisms of Biological Systems. Current Chemical Biology covers the following areas: Chemical Synthesis (Syntheses of biologically important macromolecules including proteins, polypeptides, oligonucleotides, oligosaccharides etc.; Asymmetric synthesis; Combinatorial synthesis; Diversity-oriented synthesis; Template-directed synthesis; Biomimetic synthesis; Solid phase biomolecular synthesis; Synthesis of small biomolecules: amino acids, peptides, lipids, carbohydrates and nucleosides; and Natural product synthesis).
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