lattice light sheet microscopy to visualize receptor-ligand interactions in live cells

Lattice Light Sheet Microscopy to Visualize Receptor-Ligand Interactions in Live Cells

Add 10 milliliters of water and 30 microliters of fluorescein to the LLSM bath. First, press Image (Home) to move the object to image position, and look at a single vessel laser beam pattern.
Align the laser beam using the guide and preset region of interest to make the beam a thin pattern that is balanced in all directions. The beam should also appear focused in the finder camera. Use the two mirror tilt adjusters, the top focus micrometer, and the objective color to adjust the beam.
Next, wash the bath and the objectives with at least 200 milliliters of water to completely remove any fluorescein.
To image standard fluorescent beads, turn on Dither by setting to 3 in the &#39;X Galvo Range&#39; box, and press Live to view current field. Manually adjust the tilt mirror, objective color, and focus micrometer for highest gray values. Then, adjust as necessary to obtain proper patterns for objective scan, Z galvo, Z plus objective, and sample scan capture modes. After this, press Execute in Sample Scan Mode to collect the sample point spread function for de-skewing and de-convolution. Change the lasers to three-color mode, and press Execute again.
To begin, add 100,000 antigen-presenting cells to the prepared 5-millimeter diameter circular coverslip, and allow them to settle for 10 minutes. Grease the sample holder and add the coverslip to it Cell-side-up.
Next, add a drop of imaging media to the back of the coverslip. Screw the sample holder onto the piezo, and press Image (Home). Find an antigen-presenting cell to image and ensure that the LLSM and imaging software are functioning properly.
Press Live to view the current image. Move along Z to find the coverslip and cells. Find the center of an antigen-presenting cell by moving in the Z direction, then, press Stop to pause the laser. Check 3D and input the desired settings. Press Enter and then press Execute to collect the data.
Lower the stage to the Load position, and add 50 microliters of T cells in imaging media drop-wise, directly over the coverslip. It is best to let a drop form on the end of the pipette tip and then, touch the tip to the bath liquid. Raise the stage back by clicking Image (Return).
Begin imaging. Be sure to set the desired Z-stack and timelapse length. For example, image 60 Z-stacks at a 0.4-micrometer step size and input 500th-time frames. Stop recording before 500 frames are reached to avoid photobleaching. Use Live mode to search for cell pairs, and when ready and desired settings have been entered, press Execute to collect data.

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1. Conducting LLSM Daily Alignment
NOTE: (Important) This alignment protocol is based on the LLSM instrument used (see the Table of Materials). Each LLSM may be different and require different alignment strategies, especially those that are home-built. Carry out the appropriate routine alignment and continue to section 2.
<ol>
	<li>Add 10 mL of water plus 30 &#181;L fluorescein (1 mg/mL stock) to the LLSM bath (~10 mL volume), press Image (Home) to move the objective to the image position, and look at a single Bessel laser beam pattern. Align the laser beam using the guides and pre-set region of interest (ROI) to make the beam a thin pattern balanced in all directions.
	<ol>
		<li>The beam should also appear focused in the finder camera. Use two mirror tilt adjustors, a top micrometer, focus, and an emission objective collar to adjust. See Figure 1 A, and B for the correctly aligned beam.</li>
	</ol>
	</li>
	<li>Wash the bath and objectives with at least 200 mL of water to completely remove fluorescein.</li>
	<li>Image standard fluorescent beads in the imaging media (prepared by adhering beads to a 5 mm coverslip with poly-L-lysine, see the Table of Materials; this can be pre-prepared and re-used) for physical point spread function (PSF) in imaging media. 
	NOTE: There can only be one bead in view for later processing, so try to find a bead that is by itself in the viewer or can easily be cropped to obtain a single bead.
	<ol>
		<li>Turn on dither by setting it to 3 in the &#39;X Galvo range&#39; box. Press Live to view the current field. Move along the Z direction to find the coverslip and beads. Find the center of a bead by moving along Z, press Stop to pause the laser. Check 3D, press Center and then press Execute. This will collect the data.</li>
		<li>Manually adjust the tilt mirror, objective collar, and focus micrometer for the highest gray values, then adjust as necessary to obtain proper patterns for objective scan, z galvo, z+objective (totPSF), and sample scan (samplePSF) capture modes. See Figure 1 C-F for properly adjusted maximum intensity projections (MIPs). 
		NOTE: The various capture modes (objective scan, z galvo, z+objective, and sample scan) change how the light sheet moves through the sample. All scan modes should be used for alignment.</li>
		<li>The sample scan shows how data will be collected during the experiment. Collect the sample PSF by pressing Execute in sample scan mode for deskewing and deconvolution. Change lasers to three color modes (488, 560, 647) and press Execute again. 
		NOTE: Since the LLSM images are at an angle (57.2&#176;), images captured in the &#34;sample scan&#34; mode are collected at this angle, and are therefore &#34;skewed&#34;. De-skewing is the process of correcting for this angle and &#34;re-aligning&#34; the image to a true z-stack. These data must be collected in imaging media and in all channels that will be imaged during the experiment. If this is not collected properly, the data will not be properly de-skewed. Similarly, make sure the media has been warmed to 37 &#176;C (or desired experimental temperature).</li>
	</ol>
	</li>
</ol>
2. Setting Up Cells with LLSM
<ol>
	<li>Add 100,000 antigen-presenting cells (APCs) (50 &#181;L) to a 5 mm-diameter circular coverslip and allow them to settle for 10 min.</li>
	<li>Grease the sample holder then add the coverslip cell-side-up to it. Add a drop of imaging media to the back of the coverslip to avoid bubbles before placing it in the bath. Screw the sample holder onto the piezo, and press Image (Home).</li>
	<li>Find an APC to image to ensure that the LLSM and imaging software (see Table of Materials) are functioning properly. 
	NOTE: We image at 0.4 &#181;m step size with 60 z-steps and 10 ms exposure for two colors with a dither set to 3, which results in 1.54 s per frame of the 3D image with ~200 nm XY and 400 nm Z resolution. These settings may need to be adjusted based on cell size, desired z-resolution, and strength of the signal from the fluorescent labeling technique used. Laser power usage will also vary based on the fluorescent labeling technique used.
	<ol>
		<li>Press Live to view the current image. Move along Z to find the coverslip and cells.</li>
		<li>Find the center of an APC by moving in the Z direction, then press Stop to pause the laser. Check 3D and input the desired settings, press Center and then press Execute. This will collect the data.</li>
	</ol>
	</li>
	<li>Lower the stage to load position and add 50 &#181;L of T cells in imaging media (100,000 cells) dropwise directly over the coverslip. It is best to let a drop form on the end of the pipette tip and then touch the tip to the bath liquid. Raise the stage back by clicking &#34;Image (Return)&#34;.</li>
	<li>Begin imaging. Be sure to set the desired stack size and time-lapse length. For example, image 60 z-stacks at a 0.4 &#181;m step size and input 500-time frames. (Typically) stop recording before 500 frames are reached to avoid photobleaching. Use Live mode to search for cell pairs, and when ready and desired settings have been entered, press Execute to collect data. See Figure 2 for an example.</li>
</ol>

<table><tbody><tr><td>5 mm round coverslips</td><td>World Precision Instruments</td><td>502040</td><td>For Imaging</td></tr><tr><td>Alexa Fluor 488 anti-mouse TCR &amp;beta; chain Antibody</td><td>BioLegend</td><td>109215</td><td>For Imaging</td></tr><tr><td>Fluorescein sodium salt</td><td>Sigma-Aldrich</td><td>F6377</td><td>For microscope alignment</td></tr><tr><td>FluoSpheres Carboxylate-Modified Microspheres</td><td>Thermo Fisher Scientific</td><td>F8810</td><td>For microscope alignment</td></tr><tr><td>Imaris</td><td>Bitplane</td><td>N/A</td><td>Tracking Software; Other options for tracking software include Amira or Trackmate (Fiji).</td></tr><tr><td>Lattice Light-Sheet Microscope</td><td>3i</td><td>N/A</td><td>Microscope Used</td></tr><tr><td>Leibovitz&#039;s L-15 Medium, no phenol red</td><td>Thermo Fisher Scientific</td><td>21083027</td><td>For Imaging</td></tr><tr><td>Slidebook</td><td>3i</td><td>N/A</td><td>LLSM imaging software</td></tr><tr><td>Poly-L-Lysine&amp;nbsp;</td><td>Phenix Research Products&amp;nbsp;</td><td>P8920-100ML&amp;nbsp;</td><td>For Imaging</td></tr></tbody></table>

Source: Rosenberg, J., et al. <a href="https://app.jove.com/v/59914">Visualizing Surface T-Cell Receptor Dynamics Four-Dimensionally Using Lattice Light-Sheet Microscopy.</a> J. Vis. Exp. (2020).
In this video, we describe the lattice light-sheet microscopy technique to visualize interactions between live T-cells and antigen-presenting cells. The method involves focusing an ultrathin lattice light sheet on an interacting cell pair to obtain a series of two-dimensional images, which are combined to obtain high-resolution four-dimensional images that reveal the spatiotemporal dynamics of the cell-cell interaction.

<img alt="Figure 1" src="/files/ftp_upload/21457/21457_Figure1.jpg" /> 
Figure 1: LLSM alignment. (A) Desired beam pattern for LLSM imaging experiment. (B) Screenshot of the beam alignment process; on the left is the focus window showing the narrowed, focused beam; at the top right is a graph showing that the beam is centered within the window; at the bottom right is the finder camera, which should also be a thin, focused beam. (C) ...

Source: Rosenberg, J., et al. Visualizing Surface T-Cell Receptor Dynamics Four-Dimensionally Using Lattice Light-Sheet Microscopy. J. Vis. Exp. (2020).
...

Lattice light-sheet microscopy, LLSM, enables the visualization of cell-surface receptor-ligand interactions in live cells with high spatiotemporal resolution.
Take a coverslip containing transduced ligand-expressing cells emitting red fluorescence. Attach the coverslip cell-side-up onto a greased sample holder. Fix the holder on the piezo of a microscope stage to allow precise sample positioning and scanning during imaging. Adjust the software settings to focus on a single ligand-expressing cell.
Pipette the receptor-expressing cell suspension onto the coverslip. The receptors are tagged with green fluorophore-labeled antibodies. Image the interacting cell pairs.
The microscope&#39;s excitation laser emits a circular, linearly-polarized laser beam that passes through cylindrical lenses to create a light sheet. The light sheet is projected onto a modulator that removes excess diffraction and transforms it into an ultrathin lattice pattern.
The lattice light sheet illuminates an ultrathin section of the interacting cell pair, and the fluorescence emitted by the interacting cells is captured perpendicular to the incident beam. Image the interacting cell pair in multiple Z-planes, and capture two-dimensional images in each focal plane with a high-speed camera.
Using suitable software, combine these images to form a z-stack &#8212; a high-resolution four-dimensional image demonstrating the spatiotemporal dynamics of the cell-surface receptor-ligand interaction.

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Lattice Light Sheet Microscopy to Visualize Receptor-Ligand Interactions in Live Cells

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Lattice Light Sheet Microscopy to Visualize Receptor-Ligand Interactions in Live Cells