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"Structure, Assembly And Dynamics Of Macromolecular Complexes By Single Particle Cryo-electron Microscopy." and the language of the book is English.


“Structure, Assembly And Dynamics Of Macromolecular Complexes By Single Particle Cryo-electron Microscopy.” Metadata:

  • Title: ➤  Structure, Assembly And Dynamics Of Macromolecular Complexes By Single Particle Cryo-electron Microscopy.
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  • Language: English

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  • Internet Archive ID: pubmed-PMC4028798

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This article is from <a href="//archive.org/search.php?query=journaltitle%3A%28Journal%20of%20Nanobiotechnology%29" rel="nofollow">Journal of Nanobiotechnology</a>, <a href="//archive.org/search.php?query=journaltitle%3A%28Journal%20of%20Nanobiotechnology%29%20AND%20volume%3A%2811%29" rel="nofollow">volume 11</a>.<h2>Abstract</h2>Background: Proteins in their majority act rarely as single entities. Multisubunit macromolecular complexes are the actors in most of the cellular processes. These nanomachines are hold together by weak protein-protein interactions and undergo functionally important conformational changes. TFIID is such a multiprotein complex acting in eukaryotic transcription initiation. This complex is first to be recruited to the promoter of the genes and triggers the formation of the transcription preinitiation complex involving RNA polymerase II which leads to gene transcription. The exact role of TFIID in this process is not yet understood. Methods: Last generation electron microscopes, improved data collection and new image analysis tools made it possible to obtain structural information of biological molecules at atomic resolution. Cryo-electron microscopy of vitrified samples visualizes proteins in a fully hydrated, close to native state. Molecular images are recorded at liquid nitrogen temperature in low electron dose conditions to reduce radiation damage. Digital image analysis of these noisy images aims at improving the signal-to-noise ratio, at separating distinct molecular views and at reconstructing a three-dimensional model of the biological particle. Results: Using these methods we showed the early events of an activated transcription initiation process. We explored the interaction of the TFIID coactivator with the yeast Rap1 activator, the transcription factor TFIIA and the promoter DNA. We demonstrated that TFIID serves as an assembly platform for transient protein-protein interactions, which are essential for transcription initiation. Conclusions: Recent developments in electron microscopy have provided new insights into the structural organization and the dynamic reorganization of large macromolecular complexes. Examples of near-atomic resolutions exist but the molecular flexibility of macromolecular complexes remains the limiting factor in most case. Electron microscopy has the potential to provide both structural and dynamic information of biological assemblies in order to understand the molecular mechanisms of their functions.

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