8 research outputs found
Investigating the kinetochore complex in Schizosaccharomyces pombe using advanced fluorescence microscopy techniques
Major insights into various biological processes and structures could be achieved using fluorescence
microscopy, which is a non-invasive, live- and fixed cell compatible, high contrast imaging technique.
Here, the molecule of interest can be specifically labeled with a fluorescent marker using a multitude of
different labeling techniques, best suited for the individual biological research question. The location
of the molecule of interest can be deduced from the emitted fluorescent signal of the marker due to
their immediate proximity.
However, structures smaller than the diffraction limit of light of about 200 nm can not be resolved
by conventional fluorescence microscopy. Other techniques, such as e.g. electron microscopy
(EM) or X-ray crystallography allow for higher resolutions, but lack the target specific read-out
or are not compatible with in vivo studies. Nevertheless, by utilizing advanced optical components
and illumination patterns and designing fluorophores with tightly controllable photophysics,
the diffraction limit of light could be circumvented leading to improved resolutions. From these
super-resolution techniques, only single-molecule localization microscopy (SMLM) allows for a
quantitative analysis of the target molecule due to the spatiotemporal detection of the fluorescent marker.
The segregation of sister-chromatids to the corresponding daughter cells is a vital and irreversible
process, which needs to be tightly regulated. Here, a multi-protein complex called the kinetochore
(KT), which serves as a force-sensing linker between the centromere in chromosomes and kinetochore
microtubules (kMTs) originating from the spindle pole body (SPB), plays a pivotal role as errors
in this process lead to aneuploidy or cell death. Thus, understanding the architecture and regulation
of this complex is essential. However, even though certain subcomplexes of the KT could be
resolved by EM or X-ray crystallography in vitro, the full KT nanostructure was not resolved in vivo yet.
Hence in chapter 2, the in vivo nanoscale structure of the fission yeast KT complex was investigated
using SMLM. The fission yeast Schizosaccharomyces pombe was used as the model organism of
choice, due to its small regional centromeres. It acts as an intermediate between the point centromere
in the budding yeast Saccharomyces cerevisiae, on which only one KT assembles, and the larger
regional centromeres in humans. To investigate the KT in fission yeast, a structure smaller than the
diffraction limit of light, different SMLM imaging and labeling strategies in microbes were developed
or applied fitting this research question. However, for the creation of the KT map at least two different
super-resolved targets are required: one reference protein at the centromere and one protein of interest
(POI) a time in the KT complex. As no combination of commonly used photoswitchable organic dyes
for SMLM proved to be applicable in fission yeast, the focus was shifted towards photoactivatable
and - convertable fluorescent proteins (FPs) as alternative fluorescent markers. Knowing this, the KT
structure was investigated using a multi-color SMLM approach based on FPs utilizing an orthogonal
sequential illumination pattern and a KT protein database was generated. Developing novel image
analysis tools and controls allowed for the extraction of intra- KT distances and POI copy numbers.
Based on these parameters, first conclusions on the structure, preferred KT assembly pathways and
stoichiometries were drawn and a model of the fission yeast KT was proposed.
Finally, to investigate the KT structure in even greater detail, a new imaging technique combining
expansion microscopy (ExM) and SMLM, termed single-molecule expansion microscopy in fission
yeast (SExY) was developed in chapter 3, which increases the imaging resolution of SMLM by the
corresponding expansion factor (EF) of the sample. For this, the fixed sample was first embedded
in a hydrogel and then expanded upon incubation in aqueous media. To achieve an even expansion,
the proteins were covalently linked to the gel mesh and obstacles like protein connections, cell
walls or membranes were dissolved in homogenization steps prior to expansion. Then, the sample
was imaged using the SMLM based imaging technique photoactivated localization microscopy
(PALM), which lead to single-digit nanometer resolutions. Since KT proteins are low abundant,
we optimized for an increase in protein retention yield, which we could improve by half compared
to the initial protocol. We also optimized for an isotropic expansion of the sample, which we
controlled by determining the EFs of different cell organelles and the distribution of cytosolic FPs
compared to non-expanded cells. With the final SExY protocol at hand we were than able to visualize
KT proteins as well as other nuclear targets in vivo at a single digit nanometer range for the first time
Visualizing the inner life of microbes: practices of multi-color single-molecule localization microscopy in microbiology
SI figure 4 from Combining single-molecule and expansion microscopy in fission yeast to visualize protein structures at the nanostructural level
In this work, we have developed an expansion microscopy (ExM) protocol that combines ExM with photoactivated localization microscopy (ExPALM) for yeast cell imaging, and report a robust protocol for single-molecule and expansion microscopy of fission yeast, short SExY. Our optimized SExY protocol retains about 50% of the fluorescent protein signal, doubling the amount obtained compared to the original protein retention ExM (proExM) protocol. It allows for a fivefold, highly isotropic expansion of fission yeast cells, which we carefully controlled while optimizing protein yield. We demonstrate the SExY method on several exemplary molecular targets and explicitly introduce low-abundant protein targets, e.g. nuclear proteins such as cbp1 and mis16 and the centromere-specific histone protein cnp1. The SExY protocol optimizations increasing protein yield could be beneficial for many studies, i.e. when targeting low abundance proteins or studies that rely on genetic labelling for various reasons, e.g. for proteins that cannot be easily targeted by extrinsic staining or in case artefacts introduced by unspecific staining interfere with data quality
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Unraveling the kinetochore nanostructure in Schizosaccharomyces pombe using multi-color SMLM imaging.
Funder: Boehringer Ingelheim FondsFunder: Bonn UniversityFunder: Max Planck SocietyFunder: Carnegie Mellon UniversityThe key to ensuring proper chromosome segregation during mitosis is the kinetochore (KT), a tightly regulated multiprotein complex that links the centromeric chromatin to the spindle microtubules and as such leads the segregation process. Understanding its architecture, function, and regulation is therefore essential. However, due to its complexity and dynamics, only its individual subcomplexes could be studied in structural detail so far. In this study, we construct a nanometer-precise in situ map of the human-like regional KT of Schizosaccharomyces pombe using multi-color single-molecule localization microscopy. We measure each protein of interest (POI) in conjunction with two references, cnp1CENP-A at the centromere and sad1 at the spindle pole. This allows us to determine cell cycle and mitotic plane, and to visualize individual centromere regions separately. We determine protein distances within the complex using Bayesian inference, establish the stoichiometry of each POI and, consequently, build an in situ KT model with unprecedented precision, providing new insights into the architecture
SI figure 3 from Combining single-molecule and expansion microscopy in fission yeast to visualize protein structures at the nanostructural level
In this work, we have developed an expansion microscopy (ExM) protocol that combines ExM with photoactivated localization microscopy (ExPALM) for yeast cell imaging, and report a robust protocol for single-molecule and expansion microscopy of fission yeast, short SExY. Our optimized SExY protocol retains about 50% of the fluorescent protein signal, doubling the amount obtained compared to the original protein retention ExM (proExM) protocol. It allows for a fivefold, highly isotropic expansion of fission yeast cells, which we carefully controlled while optimizing protein yield. We demonstrate the SExY method on several exemplary molecular targets and explicitly introduce low-abundant protein targets, e.g. nuclear proteins such as cbp1 and mis16 and the centromere-specific histone protein cnp1. The SExY protocol optimizations increasing protein yield could be beneficial for many studies, i.e. when targeting low abundance proteins or studies that rely on genetic labelling for various reasons, e.g. for proteins that cannot be easily targeted by extrinsic staining or in case artefacts introduced by unspecific staining interfere with data quality
Supplementary Code from Combining single-molecule and expansion microscopy in fission yeast to visualize protein structures at the nanostructural level
In this work, we have developed an expansion microscopy (ExM) protocol that combines ExM with photoactivated localization microscopy (ExPALM) for yeast cell imaging, and report a robust protocol for single-molecule and expansion microscopy of fission yeast, short SExY. Our optimized SExY protocol retains about 50% of the fluorescent protein signal, doubling the amount obtained compared to the original protein retention ExM (proExM) protocol. It allows for a fivefold, highly isotropic expansion of fission yeast cells, which we carefully controlled while optimizing protein yield. We demonstrate the SExY method on several exemplary molecular targets and explicitly introduce low-abundant protein targets, e.g. nuclear proteins such as cbp1 and mis16 and the centromere-specific histone protein cnp1. The SExY protocol optimizations increasing protein yield could be beneficial for many studies, i.e. when targeting low abundance proteins or studies that rely on genetic labelling for various reasons, e.g. for proteins that cannot be easily targeted by extrinsic staining or in case artefacts introduced by unspecific staining interfere with data quality
SI figure 1 from Combining single-molecule and expansion microscopy in fission yeast to visualize protein structures at the nanostructural level
In this work, we have developed an expansion microscopy (ExM) protocol that combines ExM with photoactivated localization microscopy (ExPALM) for yeast cell imaging, and report a robust protocol for single-molecule and expansion microscopy of fission yeast, short SExY. Our optimized SExY protocol retains about 50% of the fluorescent protein signal, doubling the amount obtained compared to the original protein retention ExM (proExM) protocol. It allows for a fivefold, highly isotropic expansion of fission yeast cells, which we carefully controlled while optimizing protein yield. We demonstrate the SExY method on several exemplary molecular targets and explicitly introduce low-abundant protein targets, e.g. nuclear proteins such as cbp1 and mis16 and the centromere-specific histone protein cnp1. The SExY protocol optimizations increasing protein yield could be beneficial for many studies, i.e. when targeting low abundance proteins or studies that rely on genetic labelling for various reasons, e.g. for proteins that cannot be easily targeted by extrinsic staining or in case artefacts introduced by unspecific staining interfere with data quality
SI figure 2 from Combining single-molecule and expansion microscopy in fission yeast to visualize protein structures at the nanostructural level
In this work, we have developed an expansion microscopy (ExM) protocol that combines ExM with photoactivated localization microscopy (ExPALM) for yeast cell imaging, and report a robust protocol for single-molecule and expansion microscopy of fission yeast, short SExY. Our optimized SExY protocol retains about 50% of the fluorescent protein signal, doubling the amount obtained compared to the original protein retention ExM (proExM) protocol. It allows for a fivefold, highly isotropic expansion of fission yeast cells, which we carefully controlled while optimizing protein yield. We demonstrate the SExY method on several exemplary molecular targets and explicitly introduce low-abundant protein targets, e.g. nuclear proteins such as cbp1 and mis16 and the centromere-specific histone protein cnp1. The SExY protocol optimizations increasing protein yield could be beneficial for many studies, i.e. when targeting low abundance proteins or studies that rely on genetic labelling for various reasons, e.g. for proteins that cannot be easily targeted by extrinsic staining or in case artefacts introduced by unspecific staining interfere with data quality