vibratome sectioning of whole murine kidney: a technique to generate thin sections of murine kidney

Vibratome Sectioning of Whole Murine Kidney: A Technique to Generate Thin Sections of Murine Kidney

Use blunt-ended forceps to gently grasp and remove the prepared kidney from ice-cold KRB solution. Immediately place the kidney on absorbent paper for approximately 2 to 4 seconds to remove excess external moisture. Gently roll the kidney across the absorbent paper to ensure that all sides of the parenchyma have dried so that there is optimal adhesion of the kidney to the vibratome stage.
Immediately apply a thin layer of cyanoacrylate glue to the base of the vibratome specimen plate and use blunt-ended forceps to place the kidney, ureter side down, on the area covered in glue. Gently apply downward pressure to the top of the kidney with the flat edge of the forceps for approximately 10 to 20 seconds to dry the glue.
Firmly secure the specimen plate to the bottom of the buffer tray and adjust the level of KRB solution so that the top of the kidney is fully immersed. For automatic vibratome sectioning, select the start and end positions of the vibratome blade cutting cycle, 0.5 to 1 centimeter clear of the kidney, to ensure that the entire kidney plane is getting sectioned.
Start the automatic cutting process, making sure that the blade makes contact with the kidney. Using forceps, collect sections that are liberated from the kidney and immediately transfer them to individual wells.

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All procedures involving animal models have been reviewed by the local institutional animal care committee and the JoVE veterinary review board.
1. Prepare Solutions
<ol>
	<li>Prepare 1 L of Krebs-Ringer Bicarbonate (KRB) solution containing 120.35 mM NaCl, 5.9 mM KCl, 15.5 mM NaHCO3, 1.2 mM Na2HPO4,1.2 mM MgCl2, 11.5 mM glucose, and 2.5 mM CaCl2. On the day of use, maintain the KRB solution on ice. 
	NOTE: KRB can be stored at 4 &#176;C for up to one week and should be pre-bubbled with a mix of 97% O2&#160;and 3% CO2&#160;for at least 10 min prior to use.</li>
</ol>
2. Vibratome Sectioning of the Kidney
<ol>
	<li>Use blunt-ended forceps to gently grasp and remove the prepared kidney from the ice-cold KRB solution. Immediately place the kidney on absorbent paper for ~2&#8211;4 s to remove excess external moisture. Gently roll the kidney across the absorbent paper to ensure that all sides of the parenchyma have dried so that there is optimal adhesion of the kidney to the vibratome stage. 
	NOTE: As the renal pelvis is located inside the kidney and therefore protected by the outer parenchyma, this short drying period would not be detrimental to tissue integrity.</li>
	<li>Immediately apply a thin layer of cyanoacrylate glue (~1 cm2) to the base of the vibratome specimen plate and use blunt-ended forceps to place the kidney, ureter side down, on the area covered in glue. Gently apply downward pressure to the top of the kidney with the flat edge of the forceps for approximately 10&#8211;20 s to dry the glue. 
	NOTE: To stabilize the kidney during this procedure, use an additional pair of forceps to keep the kidney upright as the glue dries. It is critical that the kidney adheres to the specimen plate in an upright position so that sections are cut straight. To ensure that the kidney has successfully adhered to the specimen plate, gently push the side of the kidney. If the kidney has successfully adhered to the plate, the base of the kidney should stay secured to the plate.</li>
	<li>Firmly secure the specimen plate to the bottom of the buffer tray. Adjust the level of KRB solution so that the top of the kidney is fully immersed. During sectioning steps, as the vibratome blade moves deeper into the buffer tray, remove KRB solution so that the blade holder does not become immersed in solution. 
	NOTE: If the glue has not completely dried before proceeding with this step, the glue will often move up from the base and onto the kidney parenchyma. This excess glue will make sectioning more variable. If this does happen, remove the kidney from the plate and proceed with a fresh kidney preparation.</li>
	<li>For automatic vibratome sectioning, select the start and end positions of the vibratome blade-cutting cycle. Verify these positions are ~0.5&#8211;1 cm clear of the kidney to ensure that with each blade advancement, the entire kidney plane is sectioned.</li>
	<li>Prepare a multi-well plate (24- or 48-well) by filling wells with KRB solution, and place the plate on ice. 
	NOTE: When generated, individual sections should be placed into separate wells to keep track of section depth.</li>
	<li>Start the automatic cutting process. During the initial pass of the blade, ensure that the blade makes contact with the very top of the kidney. If contact is not made, adjust the starting Z-position of the blade.</li>
	<li>Using forceps, collect sections that are liberated from the kidney. Immediately transfer the sections to individual wells and note the Z-depth of the sections to gauge the approximate PKJ location within kidney sections. 
	NOTE: Depending on the cut parameters, some sections may not be cut free from the kidney block. If this occurs, carefully use fine spring scissors to cut sections from the kidney block. Users are also encouraged to actively visualize sections under a light microscope whilst free-floating in individual wells to ensure optimal cut settings and tissue location. Sections containing the PKJ will typically be derived ~ 1000&#8211;1500 &#181;m from the top of the kidney.</li>
	<li>Continue the sectioning protocol until the PKJ regions become more apparent. Refer to the representative results section for a description of the PKJ regions as sectioning proceeds.</li>
	<li>At this point, optimize the sectioning parameters to ensure that the sections are liberated from the kidney block uniformly and are intact. Additionally, make sure that the PKJ regions are continuous and unbroken because broken PKJ walls will not allow adequate imaging of cells within the wall due to collapse. If walls become broken, decrease the sectioning speed and increase the section thickness and continue to observe sections under a light microscope to fine-tune the cutting parameters.</li>
	<li>Store sections at 4&#176;C in KRB solution until experimentation begins.</li>
</ol>

<table><tbody><tr><td>24-well culture plate</td><td>ThermoFisher Scientific</td><td>142485</td><td>To store kidney slices in</td></tr><tr><td>48-well culture plate</td><td>ThermoFisher Scientific</td><td>152640</td><td>To store kidney slices in</td></tr><tr><td>Absorbent paper</td><td>Fisher Scientific</td><td>06-666A</td><td>To dry the kidney before applying glue</td></tr><tr><td>Cyanoacrylate glue</td><td>Amazon</td><td>B001PILFVY</td><td>For adhering the kidney to the specimen plate</td></tr><tr><td>B6;129S-Gt(ROSA)26Sor/J</td><td>The Jackson Laboratory</td><td>13148</td><td>GCaMP3 Mice</td></tr><tr><td>B6;129S-Gt(ROSA)26Sor/J</td><td>The Jackson Laboratory</td><td>24105</td><td>GCaMP6f Mice</td></tr><tr><td>B6.FVB-Tg(Myh11-cre/ERT2)1Soff/J</td><td>The Jackson Laboratory</td><td>19079</td><td>smMHC-CRE Mice</td></tr><tr><td>C57BL/6-Tg(Pdgfra-cre)1Clc/J</td><td>The Jackson Laboratory</td><td>13148</td><td>PDGFRa-CRE Mice</td></tr><tr><td>Fine-tip forceps</td><td>Fine Science Tools</td><td>11254-20</td><td>Used for fine dissection of kidney</td></tr><tr><td>Gillette Silver Blue double-edge blades</td><td>Amazon</td><td>B009XHQGYO</td><td>For insertion into blade holder of vibratome</td></tr><tr><td>Student Adson Forceps</td><td>Fine Science Tools</td><td>91106-12</td><td>For gently holding and moving the kidney</td></tr><tr><td>Student Dumont Forceps</td><td>Fine Science Tools</td><td>91150-20</td><td>Used for internal dissecting forceps</td></tr><tr><td>Vibrocheck</td><td>Leica</td><td>14048142075</td><td>Optional component for calibrating blade movement during cutting</td></tr><tr><td>VT1200 S Vibrating Blade Microtome</td><td>Leica</td><td>14912000001</td><td>Configuration 1 is used in our protocol</td></tr></tbody></table>

Source: Grainger, N. et al. <a href="https://www.jove.com/video/62040" target="_blank">Isolating and Imaging Live, Intact Pacemaker Regions of Mouse Renal Pelvis by Vibratome Sectioning.</a> J. Vis. Exp. (2021)
In this video, we demonstrate the vibratome sectioning of a whole mouse kidney to obtain thin slices. These sliced tissue sections can be stored at low temperatures until further downstream analysis.

Source: Grainger, N. et al. Isolating and Imaging Live, Intact Pacemaker Regions of Mouse Renal Pelvis by Vibratome Sectioning. J. Vis. Exp. (2021)
In ...

To prepare thin sections of a mouse kidney, first, obtain a freshly harvested mouse kidney. Transfer the kidney onto a filter paper and dry it to ensure optimal adhesion to the vibratome specimen holder.
Next, mount the kidney, ureter side down, using a thin layer of cyanoacrylate glue applied to the base of the vibratome specimen holder, securing the kidney in an upright position. Transfer the specimen holder onto a buffer tray.
Fill the tray with a suitable buffer to fully immerse the top surface of the kidney. An ice bath surrounds the tray to prevent tissue damage from heat buildup during slicing. Set the vibratome blade to an appropriate angle, speed, and amplitude. Adjust the thickness parameter to obtain tissue sections of desired thickness.
During operation, the blade vibrates laterally and advances, penetrating through the tissue specimen. The vibrating blade allows the sectioning with less pressure and minimizes the tissue deformation, generating uniform kidney tissue sections of interest while maintaining the tissue morphology.
Meanwhile, assemble a multi-well plate containing a suitable chilled buffer solution to mimic the physiological conditions of the tissue. Now, transfer the sliced tissue sections into the buffer. Finally, store the tissue sections at low temperature until further downstream analysis.

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Vibratome Sectioning of Whole Murine Kidney: A Technique to Generate Thin Sections of Murine Kidney

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Vibratome Sectioning of Whole Murine Kidney: A Technique to Generate Thin Sections of Murine Kidney