Finding Needles in a Haystack with Light: Resolving the Microcircuitry of the Brain with Fluorescence Microscopy

To understand the microcircuitry of the brain, the anatomical and functional connectivity among neurons must be resolved. One of the technical hurdles to achieving this goal is that the anatomical connections, or synapses, are often smaller than the diffraction limit of light and thus are difficult to resolve by conventional microscopy, while the microcircuitry of the brain is on the scale of 1 mm or larger. To date, the gold standard method for microcircuit reconstruction has been electron microscopy (EM). However, despite its rapid development, EM has clear shortcomings as a method for microcircuit reconstruction. The greatest weakness of this method is arguably its incompatibility with functional and molecular analysis. Fluorescence microscopy, on the other hand, is readily compatible with numerous physiological and molecular analyses. We believe that recent advances in various fluorescence microscopy techniques offer a new possibility for reliable synapse detection in large volumes of neural circuits. In this minireview, we summarize recent advances in fluorescence-based microcircuit reconstruction. In the same vein as these studies, we introduce our recent efforts to analyze the long-range connectivity among brain areas and the subcellular distribution of synapses of interest in relatively large volumes of cortical tissue with array tomography and superresolution microscopy.     

Analysis of the Late Steps of Exocytosis: Biochemical and Total Internal Reflection Fluorescence Microscopy (TIRFM) Studies

1. Time with Julie in his laboratory at the NIH in the early 1970s is remembered. The experience led to a life-long interest in the regulation of catecholamine secretion. Here are summarized aspects of this work.2. The relationship between ATP-dependent priming of exocytosis and the polyphosphoinositides is reviewed. In addition, studies are summarized in which total internal reflection fluorescent microscopy (TIRFM) was used to visualize secretory granule behavior before exocytosis and individual exocytotic events.3. Quantitative optical analysis indicates that chromaffin granule motion is highly restricted but regulated. Granules can undergo significant motion in the 100 ms prior to fusion and interactions with the plasma membrane leading to fusion can occur within this time. The small motions may permit granules adjacent to the plasma membrane to repetitively sample microdomains of the plasma membrane, thereby increasing the probability of fruitful interactions that lead to fusion.     

Fluorescence Microscopy of Single Viral Capsids

To build a foundation for the single-molecule fluorescence microscopy of protein complexes, the present study achieved fluorescence microscopy of single, nucleic acid-free protein capsids of bacteriophage T7. The capsids were stained with Alexa 488 (green emission). Manipulation of the capsids' thermal motion was achieved in three dimensions. The procedure for manipulation included embedding the capsids in an agarose gel. The data indicate that the thermal motion of capsids is reduced by the sieving of the gel. The thermal motion can be reduced to any desired level. A semilogarithmic plot of an effective diffusion constant as a function of gel concentration is linear. Single, diffusing T7 capsids were also visualized in the presence of single DNA molecules that had been both stretched and immobilized by gel-embedding. The DNA molecules were stained with ethidium (orange emission). This study shows that single-molecule (protein and DNA) analysis is possible for both packaging of DNA in a bacteriophage capsid and other events of DNA metabolism. The major problem is the maintenance of biochemical activity.     

Improved-Throughput Traction Microscopy Based on Fluorescence Micropattern for Manual Microscopy

Traction force microscopy (TFM) is a quantitative technique for measuring cellular traction force, which is important in understanding cellular mechanotransduction processes. Traditional TFM has a significant limitation in that it has a low measurement throughput, commonly one per TFM dish, due to a lack of cell position information. To obtain enough cellular traction force data, an onerous workload is required including numerous TFM dish preparations and heavy cell-seeding activities, creating further difficulty in achieving identical experimental conditions among batches. In this paper, we present an improved-throughput TFM method using the well-developed microcontact printing technique and chemical modifications of linking microbeads to the gel surface to address these limitations. Chemically linking the microbeads to the gel surface has no significant influence on cell proliferation, morphology, cytoskeleton, and adhesion. Multiple pairs of force loaded and null force fluorescence images can be easily acquired by means of manual microscope with the aid of a fluorescence micropattern made by microcontact printing. Furthermore, keeping the micropattern separate from cells by using gels effectively eliminates the potential negative effect of the micropattern on the cells. This novel design greatly improves the analysis throughput of traditional TFM from one to at least twenty cells per petri dish without losing unique advantages, including a high spatial resolution of traction measurements. This newly developed method will boost the investigation of cell-matrix mechanical interactions.     

Recent Developments in Correlative Super-Resolution Fluorescence Microscopy and Electron Microscopy

The recently developed correlative super-resolution fluorescence microscopy (SRM) and electron microscopy (EM) is a hybrid technique that simultaneously obtains the spatial locations of specific molecules with SRM and the context of the cellular ultrastructure by EM. Although the combination of SRM and EM remains challenging owing to the incompatibility of samples prepared for these techniques, the increasing research attention on these methods has led to drastic improvements in their performances and resulted in wide applications. Here, we review the development of correlative SRM and EM (sCLEM) with a focus on the correlation of EM with different SRM techniques. We discuss the limitations of the integration of these two microscopy techniques and how these challenges can be addressed to improve the quality of correlative images. Finally, we address possible future improvements and advances in the continued development and wide application of sCLEM approaches.     

Cell Electrofusion Visualized with Fluorescence Microscopy

Cell electrofusion is a safe, non-viral and non-chemical method that can be used for preparing hybrid cells for human therapy. Electrofusion involves application of short high-voltage electric pulses to cells that are in close contact. Application of short, high-voltage electric pulses causes destabilization of cell plasma membranes. Destabilized membranes are more permeable for different molecules and also prone to fusion with any neighboring destabilized membranes. Electrofusion is thus a convenient method to achieve a non-specific fusion of very different cells in vitro. In order to obtain fusion, cell membranes, destabilized by electric field, must be in a close contact to allow merging of their lipid bilayers and consequently their cytoplasm. In this video, we demonstrate efficient electrofusion of cells in vitro by means of modified adherence method. In this method, cells are allowed to attach only slightly to the surface of the well, so that medium can be exchanged and cells still preserve their spherical shape. Fusion visualization is assessed by pre-labeling of the cytoplasm of cells with different fluorescent cell tracker dyes; half of the cells are labeled with orange CMRA and the other half with green CMFDA. Fusion yield is determined as the number of dually fluorescent cells divided with the number of all cells multiplied by two.     

Measuring Phagosome pH by Ratiometric Fluorescence Microscopy

Phagocytosis is a fundamental process through which innate immune cells engulf bacteria, apoptotic cells or other foreign particles in order to kill or neutralize the ingested material, or to present it as antigens and initiate adaptive immune responses. The pH of phagosomes is a critical parameter regulating fission or fusion with endomembranes and activation of proteolytic enzymes, events that allow the phagocytic vacuole to mature into a degradative organelle. In addition, translocation of H⁺ is required for the production of high levels of reactive oxygen species (ROS), which are essential for efficient killing and signaling to other host tissues. Many intracellular pathogens subvert phagocytic killing by limiting phagosomal acidification, highlighting the importance of pH in phagosome biology. Here we describe a ratiometric method for measuring phagosomal pH in neutrophils using fluorescein isothiocyanate (FITC)-labeled zymosan as phagocytic targets, and live-cell imaging. The assay is based on the fluorescence properties of FITC, which is quenched by acidic pH when excited at 490 nm but not when excited at 440 nm, allowing quantification of a pH-dependent ratio, rather than absolute fluorescence, of a single dye. A detailed protocol for performing in situ dye calibration and conversion of ratio to real pH values is also provided. Single-dye ratiometric methods are generally considered superior to single wavelength or dual-dye pseudo-ratiometric protocols, as they are less sensitive to perturbations such as bleaching, focus changes, laser variations, and uneven labeling, which distort the measured signal. This method can be easily modified to measure pH in other phagocytic cell types, and zymosan can be replaced by any other amine-containing particle, from inert beads to living microorganisms. Finally, this method can be adapted to make use of other fluorescent probes sensitive to different pH ranges or other phagosomal activities, making it a generalized protocol for the functional imaging of phagosomes.     

Light Sheet Fluorescence Microscopy: A Review

Light sheet fluorescence microscopy (LSFM) functions as a non-destructive microtome and microscope that uses a plane of light to optically section and view tissues with subcellular resolution. This method is well suited for imaging deep within transparent tissues or within whole organisms, and because tissues are exposed to only a thin plane of light, specimen photobleaching and phototoxicity are minimized compared to wide-field fluorescence, confocal, or multiphoton microscopy. LSFMs produce well-registered serial sections that are suitable for three-dimensional reconstruction of tissue structures. Because of a lack of a commercial LSFM microscope, numerous versions of light sheet microscopes have been constructed by different investigators. This review describes development of the technology, reviews existing devices, provides details of one LSFM device, and shows examples of images and three-dimensional reconstructions of tissues that were produced by LSFM.     

Enhancing Biochemical Resolution by Hyperdimensional Imaging Microscopy

Two decades of fast-paced innovation have improved the spatial resolution of fluorescence microscopy to enable molecular resolution with low invasiveness and high specificity. Fluorescence microscopy also enables scientists and clinicians to map and quantitate the physicochemical properties (e.g., analyte concentration, enzymatic activities, and protein-protein interactions) of biological samples. But the biochemical resolving power of fluorescence microscopy is not as well optimized as its spatial resolution. Current techniques typically observe only the individual properties of fluorescence, thus limiting the opportunities for sensing and multiplexing. Here, we demonstrate a new, to our knowledge, imaging paradigm, hyperdimensional imaging microscopy, which quantifies simultaneously and efficiently all the properties of fluorescence emission (excited-state lifetime, polarization, and spectra) in biological samples, transcending existing limitations. Such simultaneous detection of fluorescence features maximizes the biochemical resolving power of fluorescence microscopy, thereby providing the means to enhance sensing capabilities and enable heavily multiplexed assays. Just as multidimensional separation in mass-spectroscopy and multidimensional spectra in NMR have empowered proteomics and structural biology, we envisage that hyperdimensional imaging microscopy spectra of unprecedented dimensionality will catalyze advances in systems biology and medical diagnostics.     

Evanescent Excitation and Emission in Fluorescence Microscopy

Evanescent light—light that does not propagate but instead decays in intensity over a subwavelength distance—appears in both excitation (as in total internal reflection) and emission (as in near-field imaging) forms in fluorescence microscopy. This review describes the physical connection between these two forms as a consequence of geometrical squeezing of wavefronts, and describes newly established or speculative applications and combinations of the two. In particular, each can be used in analogous ways to produce surface-selective images, to examine the thickness and refractive index of films (such as lipid multilayers or protein layers) on solid supports, and to measure the absolute distance of a fluorophore to a surface. In combination, the two forms can further increase selectivity and reduce background scattering in surface images. The polarization properties of each lead to more sensitive and accurate measures of fluorophore orientation and membrane micromorphology. The phase properties of the evanescent excitation lead to a method of creating a submicroscopic area of total internal reflection illumination or enhanced-resolution structured illumination. Analogously, the phase properties of evanescent emission lead to a method of producing a smaller point spread function, in a technique called virtual supercritical angle fluorescence.     

Supercritical Angle Fluorescence Microscopy and Spectroscopy

Fluorescence detection, either involving propagating or near-field emission, is widely being used in spectroscopy, sensing, and microscopy. Total internal reflection fluorescence (TIRF) confines fluorescence excitation by an evanescent (near) field, and it is a popular contrast generator for surface-selective fluorescence assays. Its emission equivalent, supercritical angle fluorescence (SAF), is comparably less established, although it achieves a similar optical sectioning as TIRF does. SAF emerges when a fluorescing molecule is located very close to an interface and its near-field emission couples to the higher refractive index medium (n₂ > n₁) and becomes propagative. Then, most fluorescence is detectable on the side of the higher-index substrate, and a large fraction of this fluorescence is emitted into angles forbidden by Snell’s law. SAF, as well as the undercritical angle fluorescence (UAF; far-field emission) components, can be collected with microscope objectives having a high-enough detection aperture (numerical aperture > n₂) and be separated in the back focal plane by Fourier filtering. The back focal plane image encodes information about the fluorophore radiation pattern, and it can be analyzed to yield precise information about the refractive index in which the emitters are embedded, their nanometric distance from the interface, and their orientation. A SAF microscope can retrieve this near-field information through wide-field optics in a spatially resolved manner, and this functionality can be added to an existing inverted microscope. Here, we describe the potential underpinning of SAF microscopy and spectroscopy, particularly in comparison with TIRF. We review the challenges and opportunities that SAF presents from a biophysical perspective, and we discuss areas in which we see potential.     

Visualizing Single-molecule DNA Replication with Fluorescence Microscopy

We describe a simple fluorescence microscopy-based real-time method for observing DNA replication at the single-molecule level. A circular, forked DNA template is attached to a functionalized glass coverslip and replicated extensively after introduction of replication proteins and nucleotides (Figure 1). The growing product double-strand DNA (dsDNA) is extended with laminar flow and visualized by using an intercalating dye. Measuring the position of the growing DNA end in real time allows precise determination of replication rate (Figure 2). Furthermore, the length of completed DNA products reports on the processivity of replication. This experiment can be performed very easily and rapidly and requires only a fluorescence microscope with a reasonably sensitive camera.     

X-Ray Fluorescence Microscopy Reveals the Role of Selenium in Spermatogenesis

Selenium (Se) is a trace element with important roles in human health. Several selenoproteins have essential functions in development. However, the cellular and tissue distribution of Se remains largely unknown because of the lack of analytical techniques that image this element with sufficient sensitivity and resolution. Herein, we report that X-ray fluorescence microscopy (XFM) can be used to visualize and quantify the tissue, cellular, and subcellular topography of Se. We applied this technique to characterize the role of Se in spermatogenesis and identified a dramatic Se enrichment specifically in late spermatids, a pattern that was not seen in any other elemental maps. This enrichment was due to elevated levels of the mitochondrial form of glutathione peroxidase 4 and was fully dependent on the supplies of Se by selenoprotein P. High-resolution scans revealed that Se concentrated near the lumen side of elongating spermatids, where structural components of sperm are formed. During spermatogenesis, maximal Se associated with decreased phosphorus, whereas Zn did not change. In sperm, Se was primarily in the midpiece and colocalized with Cu and Fe. XFM allowed quantification of Se in the midpiece (0.8 fg) and head (0.2 fg) of individual sperm cells, revealing the ability of sperm cells to handle the amounts of this element well above its toxic levels. Overall, the use of XFM allowed visualization of tissue and cellular Se and provided important insights in the role of this and other trace elements in spermatogenesis.     

Quantitative Analysis of Three-Dimensional Fluorescence Localization Microscopy Data

Identifying the three-dimensional molecular organization of subcellular organelles in intact cells has been challenging to date. Here we present an analysis approach for three-dimensional localization microscopy that can not only identify subcellular objects below the diffraction limit but also quantify their shape and volume. This approach is particularly useful to map the topography of the plasma membrane and measure protein distribution within an undulating membrane.Single molecule localization microscopy (SMLM) (1–3) is a superresolution fluorescence microscopy technique that produces coordinate data for single molecule localizations with a precision of tens of nanometers in live and fixed cells. These methods have mainly been performed with total internal reflectance fluorescence microscopy and therefore have generated two-dimensional molecular coordinates. Such two-dimensional data sets have revealed nanosized clusters of membrane proteins at the cell surface (4–7). This was achieved with analysis routines based on pair-correlation analysis (8), Ripley’s K function (9), and related techniques. While three-dimensional localization microscopy techniques such as biplane imaging (10), astigmatic spot analysis (11), and depth-encoding point-spread functions (12) have now been developed, quantitative analysis approaches of three-dimensional coordinate patterns have not.Here, we describe an approach based on Getis and Franklin''s local point pattern analysis to quantitatively analyze three-dimensional subcellular structures and map plasma membrane topography. The latter can also be used to account for topography-induced clustering of membrane proteins in an undulating membrane. To illustrate the approach, we generated three-dimensional SMLM data of the membrane dye DiI and the protein Linker for Activation of T cells (LAT) fused to the photoswitchable fluorescent protein mEos2 in T cells. It has been previously shown that LAT resides within the plasma membrane as well as membrane-proximal vesicles (5,13). The data were acquired using the biplane SMLM technique and highly inclined and laminated optical sheet illumination (14). Three-dimensional molecular coordinates were calculated by fitting a three-dimensional theoretical point-spread-function to the acquired data.As previously described for two-dimensional SMLM data analysis (5), Ripley’s K-function is calculated according to Eq. 1 where V is the analyzed volume, n is the total number of points, and r is the radius of a sphere (a circle for the two-dimensional case) centered on each point. The value K(r) is thus a measure of how many points are encircled within a sphere of radius r:K(r)=V∑i=1n∑j=1n(δij/n2);δij=1ifd(pointi,pointj)<r,0else.(1)For completely spatially random (CSR) data, K(r) scales with the volume of the sphere. We therefore linearize the K-function such that it scales with radius (the L-function) using:L(r)=(3K(r)4π)1/3.(2)The value of L(r)−r is then zero for the CSR case. Values of L(r)−r above zero indicate clustering at the length scale, r.Next we used the related Getis and Franklin''s local point pattern analysis to generate a clustering value (L(r) at r = 50 nm; L(50)) for each point, j, based on the local three-dimensional molecular density. This was calculated using:Lj(50)=((3V4π)∑i=1n(δijn))1/3;δij=1ifd(pointi,pointj)<50,0else.(3)These values can then be interpolated such that every voxel in a volume is assigned a cluster value based on the number of encircled points, relative to the expected CSR case. This allows construction of isosurfaces where all points on the surface have an identical L(50) value. A high threshold imparts a strict criterion for cluster detection compared to a lower one, and this allows users to, for example, determine the efficiency of sequestration into clusters by quantifying the cluster number and size as a function of the threshold.To illustrate the identification of subcellular structures, Lat-mEos2 was imaged by three-dimensional SMLM in activated T cells at the immunological synapse (Fig. 1 A). Three-dimensional projections of isosurfaces (for L(50) = 200) clearly identified intracellular LAT vesicles at varying depths within the synapse (Fig. 1, B and C). Cluster statistics were extracted from this data set to quantify the distribution of clusters in the z direction as well as the volume and sphericity of the LAT objects themselves (Fig. 1, D–F).Open in a separate windowFigure 1Identification of subcellular objects in three dimensions by isosurface rendering of molecular distribution. (A) Schematic of a T cell synapse formed against an activating coverslip where subsynaptic LAT vesicles (red dots) can be imaged with three-dimensional SMLM. (B and C) Isosurfaces, shown in x,z view (B) and as projection (C), identify T cell vesicles as LAT objects with L(50) > 200 (Eq. 3). (D–F) Distribution of LAT objects in z direction (D), volume (E), and sphericity (F) of LAT objects in T cells.Membrane undulations can cause clustering artifacts when the distribution of membrane proteins is recorded as a two-dimensional projection (15) (Fig. 2 A), as is the case in two-dimensional SMLM under total internal reflectance fluorescence illumination. To illustrate a solution to this problem, we obtained three-dimensional SMLM data sets of the membrane dye DiI (16) in resting T cells adhered onto nonactivating coverslips. With appropriately short labeling times to prevent dye internalization, it can be assumed that all DiI molecules reside in the plasma membrane. In this case, as is the case for plasma membrane proteins, neither two-dimensional nor three-dimensional analysis is appropriate, as it is a priori known the points must be derived from a two-dimensional membrane folded in three-dimensional space. To correct for membrane undulations, the plasma membrane topography must first be mapped so that molecular coordinates of membrane molecules can be appropriately corrected in two-dimensional projections. The position of the plasma membrane in three dimensions, i.e., the membrane topography, was determined by averaging the z position of all DiI molecules within a 100-nm radius in x-y at each point. The averaged z-position of DiI molecules was then displayed as a map, which exhibits a smooth, undulating profile (Fig. 2 B). The selection of this radius determines the accuracy of the assigned z position but also causes smoothing of the membrane profile.Open in a separate windowFigure 2Mapping of membrane topography and correction of molecular distributions in undulating membranes. (A) Two-dimensional projections can cause cluster artifacts, for example in membrane ruffles. Molecules (red rectangles) in the upper image are equally spaced along the membrane but appear as clusters in two-dimensional projections in areas with high gradient. (B) Three-dimensional membrane topography of a 2 × 2 μm plasma membrane area of a resting T cell obtained from averaged z positions of DiI molecules. Note that membrane undulation is ∼100 nm. (C) Map of membrane gradient, corresponding to the topography map shown in panel B, with an area of high gradient highlighted (dashed red box). (D) Correction of the circle radii in the Getis and Franklin cluster map calculations to account for projection artifacts. (E and F) Cluster map of data shown in panel C before (E) and after (F) correction for membrane gradient. Boxes in panels C, E, and F highlight the regions with high membrane gradient.Next, the gradient at the position of each DiI molecule was determined and interpolated into a gradient map (Fig. 2 C). Here, blue represents horizontal, i.e., flat membrane areas, whereas red regions indicate areas of high gradient. The information from the gradient map was then used to ensure that the two-dimensional circles in the Getis and Franklin cluster map calculations each correspond to an identical area of membrane, hence accounting for two-dimensional projection artifacts. To do this, the size of the circle (r) used to calculate the L value for each molecule was modified using Eq. 4, where c is calculated for the surface, S, using Eq. 5:r(corr)=r(uncorr)(1+c2)1/4,(4)c=((∂S∂x)2+(∂S∂y)2)1/2.(5)This operation is shown schematically in Fig. 2. The comparison of Getis and Franklin cluster maps before (Fig. 2 E) and after (Fig. 2 F) correction for the gradient shows that cluster values for DiI molecules were substantially reduced by up to 5–10% at sites where the plasma membrane had a high gradient (area highlighted in red box), and where the two-dimensional projection of three-dimensional structures caused an overestimation of clustering.In conclusion, we demonstrated that three-dimensional superresolution localization microscopy data can be used to identify and quantify subcellular structures. The approach has the distinct advantage that subcellular structures are solely identified by the distribution of the fluorescent marker so that no a priori knowledge of the structure is necessary. How precisely the subcellular structures are identified only depends on how efficiently the fluorescent maker is recruited to the structure, and hence does not depend on the resolution limits of optical microscopy. We applied the methods to two very different structures in T cells: small intracellular vesicles and the undulating plasma membrane. Importantly, the topography of plasma membrane can also be used to correct clustering artifacts in two-dimensional projections, which may be useful for distribution analysis within membranes.     

Rapid Analysis and Exploration of Fluorescence Microscopy Images

Despite rapid advances in high-throughput microscopy, quantitative image-based assays still pose significant challenges. While a variety of specialized image analysis tools are available, most traditional image-analysis-based workflows have steep learning curves (for fine tuning of analysis parameters) and result in long turnaround times between imaging and analysis. In particular, cell segmentation, the process of identifying individual cells in an image, is a major bottleneck in this regard.Here we present an alternate, cell-segmentation-free workflow based on PhenoRipper, an open-source software platform designed for the rapid analysis and exploration of microscopy images. The pipeline presented here is optimized for immunofluorescence microscopy images of cell cultures and requires minimal user intervention. Within half an hour, PhenoRipper can analyze data from a typical 96-well experiment and generate image profiles. Users can then visually explore their data, perform quality control on their experiment, ensure response to perturbations and check reproducibility of replicates. This facilitates a rapid feedback cycle between analysis and experiment, which is crucial during assay optimization. This protocol is useful not just as a first pass analysis for quality control, but also may be used as an end-to-end solution, especially for screening. The workflow described here scales to large data sets such as those generated by high-throughput screens, and has been shown to group experimental conditions by phenotype accurately over a wide range of biological systems. The PhenoBrowser interface provides an intuitive framework to explore the phenotypic space and relate image properties to biological annotations. Taken together, the protocol described here will lower the barriers to adopting quantitative analysis of image based screens.     

Tentative Identification of Methanogenic Bacteria by Fluorescence Microscopy

Methanogenic bacteria, which are presently identified on the basis of cell morphology and substrate conversion to CH₄, can be differentiated from nonmethanogens and identified in pure or mixed culture on the basis of their autofluorescence under ultraviolet illumination.