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Probing the Influence of Single-Site Mutations in the Central Cross-β Region of Amyloid β (1–40) PeptidesFritzsch, Jacob, Korn, Alexander, Surendran, Dayana, Krueger, Martin, Scheidt, Holger A., Mote, Kaustubh R., Madhu, Perunthiruthy K., Maiti, Sudipta, Huster, Daniel 02 May 2023 (has links)
Amyloid β (Aβ) is a peptide known to form amyloid fibrils in the brain of patients suffering from Alzheimer’s disease. A complete mechanistic understanding how Aβ peptides form neurotoxic assemblies and how they kill neurons has not yet been achieved. Previous analysis of various Aβ40 mutants could reveal the significant importance of the hydrophobic contact between the residues Phe19 and Leu34 for cell toxicity. For some mutations at Phe19, toxicity was completely abolished. In the current study, we assessed if perturbations introduced by mutations in the direct proximity of the Phe19/Leu34 contact would have similar relevance for the fibrillation kinetics, structure, dynamics and toxicity of the Aβ assemblies. To this end, we rationally modified positions Phe20 or Gly33. A small library of Aβ40 peptides with Phe20 mutated to Lys, Tyr or the non-proteinogenic cyclohexylalanine (Cha) or Gly33 mutated to Ala was synthesized. We used electron microscopy, circular dichroism, X-ray diffraction, solid-state NMR spectroscopy, ThT fluorescence and MTT cell toxicity assays to comprehensively investigate the physicochemical properties of the Aβ fibrils formed by the modified peptides as well as toxicity to a neuronal cell line. Single mutations of either Phe20 or Gly33 led to relatively drastic alterations in the Aβ fibrillation kinetics but left the global, as well as the local structure, of the fibrils largely unchanged. Furthermore, the introduced perturbations caused a severe decrease or loss of cell toxicity compared to wildtype Aβ40. We suggest that perturbations at position Phe20 and Gly33 affect the fibrillation pathway of Aβ40 and, thereby, influence the especially toxic oligomeric species manifesting so that the region around the Phe19/Leu34 hydrophobic contact provides a promising site for the design of small molecules interfering with the Aβ fibrillation pathway.
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Quantitative molecular orientation imaging of biological structures by polarized super-resolution fluorescence microscopy / Imagerie quantitative d'orientation moléculaire dans les structures biologiques par microscopiesuper-résolution polariséeAhmed, Haitham Ahmed Shaban 02 April 2015 (has links)
Dans cette thèse, nous avons construit et optimisé des méthodes de microscopie de fluorescence super-résolue stochastique, polarisée et quantitative qui nous permettent d'imager l'orientation moléculaire dans des environnements dynamiques et statiques a l’échelle de la molécule unique et avec une résolution nanoscopique. En utilisant un montage de microscopie super-résolue à lecture stochastique en combinaison avec une détection polarisée, nous avons pu reconstruire des images d'anisotropie de fluorescence avec une résolution spatiale de 40 nm. En particulier, nous avons pu imager l'ordre orientationnel d'assemblages biomoléculaires et cellulaires. Pour l'imagerie cellulaire, nous avons pu étudier la capacité d'étiquettes de marquer fluorophoresde reporter quantifier l'orientation moléculaire dans l'actine et les microtubules dans des cellules fixées. Nous avons également mis à profit la meilleure résolution et la détection polarisée pour étudier l'ordre moléculaire d’agrégats d’amyloïdes a l’échelle nanoscopique. Enfin, nous avons étudié l'interaction de la protéine de réparation RAD51 avec l'ADN par microscopie de fluorescence polarisée super-résolue pour quantifier l'ordre orientationnel de l'ADN et de la protéine RAD51 afin de comprendre la recombinaison homologue du mécanisme de réparation de l'ADN. / .In this thesis we built and optimized quantitative polarized stochastic super-resolution fluorescence microscopy techniques that enabled us to image molecular orientation behaviors in static and dynamic environments at single molecule level and with nano-scale resolution. Using a scheme of stochastic read-out super resolution microscopy in combination with polarized detection, we can reconstruct fluorescence anisotropy images at a spatial resolution of 40 nm. In particular, we have been able to use the techniques to quantify the molecular orientationalorder in cellular and bio-molecular assemblies. For cellular imaging, we could quantify the ability of fluorophore labels to report molecular orientation of actin and microtubules in fixed cells. Furthermore, we used the improvements of resolution and polarization detection to study molecular order of amyloid aggregates at a nanoscopic scale. Also, we studied repair protein RAD51` s interaction with DNA by using dual color polarized fluorescence microscopy, to quantify the orientational order of DNA and RAD51 to understand the homologous recombination of DNA repair mechanism.
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Structure and Dynamics of the Y145Stop Variant of the Human Prion Protein Studied by Magic-Angle Spinning Solid State NMRHelmus, Jonathan Jaye 06 September 2011 (has links)
No description available.
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