| dc.contributor.advisor | Atreya, H S | |
| dc.contributor.advisor | D'Silva, Patrick | |
| dc.contributor.author | Thakur, Anushikha | |
| dc.date.accessioned | 2026-03-26T05:59:30Z | |
| dc.date.available | 2026-03-26T05:59:30Z | |
| dc.date.submitted | 2012 | |
| dc.identifier.uri | https://etd.iisc.ac.in/handle/2005/9868 | |
| dc.description.abstract | Research Focus
This research explores the application of NMR spectroscopy in protein biochemistry, specifically in:
Structure determination of human J-protein co-chaperone Dph4 and yeast Tim23.
Functional analysis of human Dph4 using biophysical and biochemical techniques.
Characterization of hydrogen exchange in proteins using ^13C-detected 2D CON experiments.
Chapter 1 - Introduction
Scope of NMR spectroscopy in protein structure determination.
Advantages of NMR over X-ray crystallography for natively unfolded and multi-domain proteins.
Residue-specific insights into dynamics, conformational exchange, and allostery.
Overview of human Dph4 (a type III J-protein) and yeast Tim23 (a mitochondrial translocon component).
Development of new NMR methods for solvent-exchangeable proton analysis.
Chapter 2 - Functional Analysis of Human Dph4
J-proteins are obligate partners of Hsp70s, stimulating ATPase activity.
Dph4, a type III J-protein, shows unique iron-binding ability with 16-fold higher affinity than zinc.
Fe-Dph4 undergoes oligomerization, potentially functioning as a transient iron-storage protein.
Exhibits redox and electron carrier activity critical for diphthamide biosynthesis.
Fe-binding stabilizes Dph4 and enhances its Hsp70-dependent functions.
Conserved Fe-binding property observed in yeast ortholog Jjj3.
Chapter 3 - Structural Analysis of Human Dph4
NMR structure of Zn-Dph4 solved.
Protein consists of an N-terminal helical domain and a C-terminal -sheet domain connected by a helical linker.
Domains fold independently but show inter-domain mobility.
Linker undergoes conformational changes leading to open/closed states; closed conformation stabilizes Hsp70:Dph4 interaction.
Chemical shift differences highlight the importance of Fe-binding in functional regulation.
Chapter 4 - Structural Analysis of Yeast Tim23 (IMS Domain)
Tim23 is essential for mitochondrial protein import.
NMR analysis of IMS domain revealed large intrinsically disordered regions with a single helical region.
Provides first structural insights into the molecular details of mitochondrial translocation machinery.
Chapter 5 - NMR-Based Hydrogen Exchange Studies
Developed a rapid method using modified ^13C-detected 2D CON experiments.
Enables simultaneous measurement of exchange rates and fractionation factors.
Illustrated on three proteins: Tim23 IMS-domain, ubiquitin, and a Dph4 truncation mutant.
Method provides efficient characterization of hydrogen exchange kinetics and thermodynamics. | |
| dc.language.iso | en_US | |
| dc.relation.ispartofseries | T07660 | |
| dc.rights | I grant Indian Institute of Science the right to archive and to make available my thesis or dissertation in whole or in part in all forms of media, now hereafter known. I retain all proprietary rights, such as patent rights. I also retain the right to use in future works (such as articles or books) all or part of this thesis or dissertation | |
| dc.subject | NMR Spectroscopy in Protein Structure | |
| dc.subject | Human J-Protein Dph4 Structure and Function | |
| dc.subject | Yeast Tim23 IMS Domain | |
| dc.title | Structure, function and dynamics of proteins by NMR spectroscopy : Application to human J-Protein co-chaperone Dph4 and yeast Tim23-IMS | |
| dc.type | Thesis | |
| dc.degree.name | PhD | |
| dc.degree.level | Doctoral | |
| dc.degree.grantor | Indian Institute of Science | |
| dc.degree.discipline | Science | |
