dc.contributor
Universitat de Barcelona. Facultat de Farmàcia i Ciències de l'Alimentació
dc.contributor.author
Cuppari, Anna
dc.date.accessioned
2017-02-13T13:27:38Z
dc.date.available
2017-12-21T06:45:09Z
dc.date.issued
2016-12-21
dc.identifier.uri
http://hdl.handle.net/10803/400213
dc.description.abstract
The mitochondrial transcription factor A, TFAM, has a dual function in the organelle: it activates mitochondrial DNA transcription by binding to the HSP and LSP promoters, while in higher concentrations compacts the mtDNA. In this thesis the mechanism of complex formation between the mitochondrial transcription factor A (TFAM) and its cognate DNA binding sequences is analysed. TFAM is a DNA binding protein that belongs to the HMG- box family. Previous crystallographic works have shown that, by its two HMG-boxes and the intervening linker, TFAM binds to the DNA minor groove of mitochondrial DNA promoters imposing severe DNA distortions. These include two sharp 90-degree kinks that bend the cognate DNA into a U-turn. We here present the crystallographic structure of TFAM in complex with site Y, which together with site X are protein binding sites alternative to the promoter binding regions at the control region of mitochondrial DNA (mtDNA). The structure of the TFAM/site Y complex shows the two HMG-box domains (HMG-box1 and 2) organized in an “L”-shape fold that bends the contacted DNA by 90 degrees. Each HMG-box domain inserts a leucine, Leu 58 from HMG-box1 and Leu182 from HMG-box2, into a base-pair step from respective DNA contacted regions. The two DNA steps are separated by a DNA helix turn. Each insertion disrupts the DNA stacking and, together with additional interactions, facilitates the 90º DNA bending, the two bends resulting in the U-turn conformation. A structural comparison between available TFAM/DNA complexes shows that the linker between HMG-domains is instrumental for the protein to adapt to a conformation variability induced by the different DNA sequences. In addition, while all other crystal structures are unambiguous in the assigned DNA sequence, TFAM/site Y electron density maps indicated a surprising DNA disorder that suggested to trace the DNA in an alternative, not predicted, orientation.
Thus in order to better characterize the binding mechanism of TFAM to the DNA and the role of the DNA properties in this process, we further studied the TFAM/site Y, TFAM/site X and TFAM/LSP complexes by molecular dynamics (MD) simulations, isothermal titration calorimetry (ITC) and electrophoretic mobility shift assays (EMSA). All these techniques showed a recurrent result, which is that TFAM has a clear preference in binding and bending site Y over site X and LSP. The three DNAs present intrinsic distortions that
facilitate binding, which occurs by a mechanism in all cases endothermic and spontaneous and TFAM presents similar affinities to all of them. However, site Y is intrinsically more rigid but easier to distort into the shape found in the crystal, it competes better for TFAM binding, and the enthalpy and entropy of binding are much higher than for the other two sequences. These results suggest a specific binding and bending mechanism significantly dependent on the DNA sequence.
Finally, by multi-angle laser light scattering (MALLS) and analytical ultracentrifugation the multimerization ability of TFAM detected by EMSA and size exclusion chromatography was analysed. The results indicate multimerization of the protein either alone or on the DNA in a cooperative manner at increased complex concentrations, which is consistent with the alternative function of TFAM as an mtDNA packaging protein. Altogether, our results suggest that the DNA sequence properties mediate TFAM binding, involving either specific interactions at the mtDNA control region, or non-specific contacts during mtDNA compaction. For this latter, the regulation of TFAM binding exerted by the DNA sequence might be combined with regulation of protein multimerization processes, all together determining mtDNA compaction, which is essential for cell life.
en_US
dc.description.abstract
Este trabajo de tesis doctoral está centrado en el análisis del mecanismo de unión del factor A de transcripción mitocondrial (TFAM) con sus secuencias de reconocimiento en la región control del ADN mitocondrial (mtADN). En la mitocondria TFAM está implicado en dos procesos fundamentales: la regulación de la trascripción del mtADN, cuando está unido a las secuencias promotoras del filamento ligero y pesado (HSP y LSP), y la compactación del mismo ADN cuando está presente en alta concentración. TFAM pertenece a la familia de los HMG-box y está constituida por dos dominios HMG conectados por un “linker” de 20 residuos. En este trabajo se presenta la estructura cristalográfica de TFAM en complejo con su sitio de reconocimiento alternativo a los promotores, site Y. Desde el análisis de la estructura se ha evidenciado que TFAM presenta el mismo plegamiento observado también cuando está en complejo con LSP, HSP, ADN no específico (nsADN) y su otro sitio de unión site X. Además en todos estos complejos el ADN resulta doblado 180° por medio de dos inserciones mediadas por LEU58 y 182, cada una responsable de un “kink” de 90°. La diferencia principal entre todas las estructuras se observa a nivel del linker que presenta una desviación en respuesta a las diferentes propiedades de los ADNs que contacta.
Para caracterizar mejor el mecanismo de unión de TFAM con sus secuencias de reconocimiento en la región control del mtADN (LSP, site Y and site X), se realizaron diferentes análisis de tipo biofísico y bioquímico. La flexibilidad de estas secuencias se estudió primero por dinámica molecular. Estudios de “isothermal titration calorimetry” y “electrophoresis mobility shift assays” permitieron evidenciar que también si TFAM tiene el mismo mecanismo de unión y la misma afinidad por las tres secuencias, la cinética de formación de los complejos parece ser diferente. Para el análisis de la estequiometria de la unión de TFAM a los diferentes ADN fueron empleadas las técnicas de “multi angle laser light scattering” y “analytical ultracentrifugation”. Estos estudios evidenciaron la tendencia de TFAM de multimerizar, en presencia y ausencia de ADN, en respuesta a aumento de su concentración.
en_US
dc.format.extent
135 p.
en_US
dc.format.mimetype
application/pdf
dc.language.iso
eng
en_US
dc.publisher
Universitat de Barcelona
dc.rights.license
L'accés als continguts d'aquesta tesi queda condicionat a l'acceptació de les condicions d'ús establertes per la següent llicència Creative Commons: http://creativecommons.org/licenses/by-nc-nd/4.0/
dc.rights.uri
http://creativecommons.org/licenses/by-nc-nd/4.0/
*
dc.source
TDX (Tesis Doctorals en Xarxa)
dc.subject
ADN mitocondrial
en_US
dc.subject
Mitochondrial DNA
en_US
dc.subject
Àcids nucleics
en_US
dc.subject
Ácidos nucleicos
en_US
dc.subject
Nucleic acids
en_US
dc.subject
Cromatografia
en_US
dc.subject
Cromatografía
en_US
dc.subject
Chromatography
en_US
dc.subject.other
Ciències de la Salut
en_US
dc.title
Structure and biophysical studies of mitochondrial Transcription Factor A in complex with DNA
en_US
dc.type
info:eu-repo/semantics/doctoralThesis
dc.type
info:eu-repo/semantics/publishedVersion
dc.contributor.director
Solà Vilarrubias, Maria
dc.contributor.tutor
Badia Palacín, Josefa
dc.embargo.terms
12 mesos
en_US
dc.rights.accessLevel
info:eu-repo/semantics/openAccess