Advanced imaging

  • Teaching

    Details

    Faculty Faculty of Science and Medicine
    Domain Biology
    Code UE-SBL.00419
    Languages English
    Type of lesson Lecture
    Level Master
    Semester SP-2023

    Schedules and rooms

    Summary schedule Thursday , Cours bloc (Spring semester)
    Contact's hours 8

    Teaching

    Responsibles
    • Egger Boris August
    Teachers
    • Acuna Guillermo Pedro
    • Stefani Fernando Daniel
    Description

    Fluorescence microscopy has become the preferred imaging tool for biological systems due to its capability to visualize specifically the target biomolecules under conditions compatible with life, like room temperature, liquid environment and irradiation with visible light. Fluorescence microscopy also provides very high sensitivity down to the detection of single molecules. As drawback, as it happens with any a far-field optical technique, the spatial resolution is limited by the wavelength of light to a few hundreds of nanometres (the so-called diffraction limit). Remarkably, in the mid 2000s, a series of imaging methods using fluorescence readout were developed that deliver images with resolution beyond the diffraction limit. These methods, called super-resolution fluorescence microscopy or far-field fluorescence nanoscopy and whose pioneers were awarded with the Nobel Prize in Chemistry in 2014(13), have revolutionized biological imaging and continued to be developed until the present day.

     

    In these lectures, we will revise the working principles of super-resolution microscopy and its development from the first generation of methods up to the newest methods capable of achieving 1 nm resolution under ambient conditions(47). We will discuss the performance and technical aspects of the necessary hardware and sample preparation for each one of the different modalities of super-resolution microscopy existing today. Also, we will perform experiments hands-on to obtain super-resolved fluorescence images, including the acquisition and analysis of data.

    Training objectives

    After this course, the student will know:

    • The fundamental principles of superresolution fluorescence microscopy in its different modalities: coordinate stochastic single-molecule localization microscopy (e.g., STORM, PALM, DNA-PAINT), coordinate targeted super-resolution microscopy (e.g., STED, RESOLFT), and single-molecule localization through sequential structured illumination (e.g., MINFLUX, RASTMIN).
    • How to choose the best suited superresolution method for specific applications: visualizing fixed or living specimens, compromise between resolution and throughput (image acquisition speed), visualizing structures or trajectories.
    • How acquire singlemolecule localization data and analyse it to obtain a super-resolved fluorescence image
    Comments

    Jupyter Python course for image processing and analysis. 

     

    Teachers: Ferndando Stefani (Buenos Aires) and Guillermo Acuna (Fribourg)

    Softskills No
    Off field No
    BeNeFri Yes
    Mobility Yes
    UniPop No
  • Dates and rooms
    Date Hour Type of lesson Place
    20.04.2023 13:15 - 17:00 Cours PER 17, Room 001
    21.04.2023 13:15 - 16:00 Cours PER 17, Room 001
  • Assessments methods

    Written exam

    Assessments methods By rating
    Descriptions of Exams

    Written exam (60 min.) during the semester. One mark.

    Written exam MC. 

  • Assignment
    Valid for the following curricula:
    Additional Courses in Sciences
    Version: ens_compl_sciences
    Paquet indépendant des branches > Specialized courses in Biology (Master level)

    Additional programme requirements for PhD studies [PRE-DOC]
    Version: 2020_1/v_01
    Additional programme requirements for PhD studies (Faculty of Science and Medicine) > Specialized courses in Biology (Master level)

    Biology [3e cycle]
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    Biology [POST-DOC]
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