Name: 视频: 伤口测定评估共培养中小鼠成肌细胞的迁移能力 - 概念
Uploaded: 2023-04-30T15:05:17.000+00:00
Duration: 1 min 52 s
Description: 198 次观看. 来源:Toubat， O. et al.， 体外旁分泌非经典 Wnt 信号传导建模。J. Vis. Exp. （2021）。 该视频介绍了一种非接触式共培养伤口愈合试验，用于评估小鼠成肌细胞的迁移能力。这有助于了解体外旁分泌非经典 Wnt 信号相互作用的信号发送和信号接收成分。

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1. Wound assay:
(Figure 1 outlines the schematic model of the assay)
<ol>
	<li>Allow the O9-1 cell inserts and C2C12 cell chamber wells to adhere and proliferate in the incubator until both cells are at ~70-80% confluency before proceeding with this portion of the protocol. If cells grow &#62;90% confluent, do not proceed with the scratch assay, as cells will merely detach from the well.</li>
	<li>Warm 1x PBS and C2C12 medium by placing them in a 37 &#176;C water bath.</li>
	<li>Remove supernatant medium from the C2C12 chamber well and wash the cells once with 1x PBS. Remove the 1x PBS and immediately scratch the cells with a sterile P10 pipette tip.
	<ol>
		<li>Pass the sterile P10 pipette tip firmly in a single direction to span the entire length or width of the cell monolayer (e.g., right to left, top to bottom). Be sure to scratch each well containing cells only once. 
		NOTE: To optimize scratching results, scratch wells of different experimental conditions at a similar level of confluency. To do this, ensure that each 4-chambered well has cells for each required experimental condition (e.g., well #1 negative control, well #2 positive control). In addition, use a new sterile P10 pipette for each scratch and apply a similar amount of force to the pipette each time. Do not attempt to create more than one scratch in each well.</li>
		<li>After scratching, quickly add 1 mL of 1x PBS back into the well using a P1000 pipette tip. Repeat this process for each well that will be scratched. 
		NOTE: Given the variability associated with each scratch, it is recommended that multiple wells (n = 3) are used for wound creation in each experimental condition. Work expeditiously as it is critical to minimize the duration for which the cells are without 1x PBS during these steps. After removing 1x PBS from each well, one should not take more than 5 s to generate a wound in each well.</li>
	</ol>
	</li>
	<li>After generating a wound and adding 1x PBS back into each well, image the scratch using a brightfield inverted microscope and use this image as the baseline wound size (time 0). To take images, perform the following steps:
	<ol>
		<li>Turn on the computer and the microscope (see the Table of Materials) by pressing the power button. Place the chamber slide on the stage and rotate the objective dial to 5x magnification.</li>
		<li>Open the imaging software (see the Table of Materials) by double-clicking the software icon on the computer desktop. Click the Camera tab on the software home screen. Click the Live button to visualize the cells on the AxioCam IC tab.</li>
		<li>Ensure that the light filter is pulled all the way out to allow light to pass to the camera and computer screen. Manually move and/or rotate the chamber slide to position the wound area in the center of the live image on the AxioCam IC tab.</li>
		<li>To take images, click snap to open a new tab next to the AxioCam IC tab that contains the image.</li>
		<li>To save this still image, click file on the top left of the software home page | save as | enter the file name in the file name box. Save the figure in Carl Zeiss image (*.czi) format (the default setting), and select desktop on the bar on the left to save the file to the desktop as a .czi file, which can only be opened in the Zen lite 2012 software program.</li>
		<li>To save the picture as a .tiff, click file | save as | enter file name in the file name box. Save the figure as tagged image file (*.tiff) by clicking the save as type button and selecting *.tiff from the dropdown menu. 
		NOTE: The .tiff format can be opened in any image processing software.</li>
		<li>Manually reposition the chamber slide to take 2-3 more images at other points of the wound in the same well. 
		NOTE: In total, this will result in 3-4 non-overlapping, high-magnification images of the wound in each well.</li>
	</ol>
	</li>
	<li>Remove the 1x PBS from each well and add 1 mL of C2C12 medium. 
	NOTE: Be cautious not to pipette too aggressively when removing or adding solutions to the chamber well following wound generation, as this may cause cells to detach from the chamber well. In addition, tilt the chamber well so that aspiration and reintroduction of solutions can be done at the corners of each well to minimize cell monolayer disruption.</li>
	<li>Assemble the well insert coculture system by manually placing the inserts containing the O9-1 cells in each well of the chamber well. Gently push the inserts down into the well such that the bottom of the insert sits just above the underlying C2C12 cells. Return the well insert constructs to the incubator. 
	NOTE: Do not allow the bottom of the insert to physically touch and mechanically disrupt the underlying C2C12 cells.</li>
	<li>Allow the cells to migrate for a total of 9-12 h. To determine the optimal migration time, check the cells at 6 h following wound creation, then every 2-3 h thereafter. End the experiment when the cells in control or positive control conditions begin to completely cover the wound. 
	NOTE: Given the non-contact nature of the construct, the overlying insert does not need to be removed from the wells when checking interval migration progression. Migratory variability will be observed depending on factors such as the cell types used in this assay, cellular density at the time of wound generation, the width of the wound created, and experimental conditions of manipulated cells (e.g., gene knockdown, recombinant protein addition). Concentrations of these reagents should be determined experimentally with guidance from manufacturer recommendations.</li>
</ol>

<table><tbody><tr><td>C2C12 murine myoblast cell line&amp;nbsp;</td><td>ATCC</td><td>CRL-1772</td><td></td></tr><tr><td>Chamber Slide System, 4-well</td><td>ThermoFisher Scientific</td><td>154526</td><td></td></tr><tr><td>Dulbecco&amp;rsquo;s Modified Eagle&amp;rsquo;s Medium (DMEM), high glucose (4.5 g/L), Lglutamine (2 mM)&amp;nbsp;</td><td>Corning</td><td>10-017-CV</td><td>Stored at 4 &amp;deg;C</td></tr><tr><td>Graduated and sterile pipette tips, 10 &amp;micro;L</td><td>USA Scientific</td><td>1111-3810</td><td></td></tr><tr><td>O9-1 neural crest cell line&amp;nbsp;</td><td>Millipore Sigma</td><td>SCC049</td><td></td></tr><tr><td>Phosphate-buffer saline (PBS), 1x, without calcium and magnesium, pH 7.4</td><td>Corning</td><td>21-040-CV</td><td>Stored at 4 &amp;deg;C</td></tr><tr><td>Falcon permeable support for 24-well plate with 0.4 &amp;micro;M transparent PET membrane</td><td>Corning</td><td>353095</td><td></td></tr><tr><td>Fetal bovine serum</td><td>Fisher Scientific&amp;nbsp;</td><td>W3381E</td><td>Stored in 50 mL aliquots at -20 &amp;deg;C</td></tr><tr><td>Zeiss inverted Axio Vert.A1 light microscope</td><td>Carl Zeiss AG</td><td></td><td></td></tr><tr><td>Zen lite 2012 microscopy software</td><td>Carl Zeiss AG</td><td></td><td>Imaging software</td></tr></tbody></table>

wound assay to evaluate the migratory capacity of murine myoblasts in co-culture

Source: Toubat, O. et al., <a href="https://app-jove-com.remotexs.ntu.edu.sg/v/63247">Modeling Paracrine Noncanonical Wnt Signaling In Vitro.</a> J. Vis. Exp. (2021).
This video describes a non-contact co-culture wound healing assay to evaluate the migratory capacity of murine myoblasts. This helps to understand signal-sending and signal-receiving components of the paracrine non-canonical Wnt signaling interactions in vitro.

<img alt="Figure 1" src="/files/ftp_upload/21287/21287_Figure1.jpg" /> 
Figure 1: Schematic model of the assay.&#160;Step 1 includes the&#160;in vitro&#160;expansion of C2C12 myoblasts and NCCs using STO feeder cells. Step 2 involves the plating of NCCs and C2C12 cells in the coculture system. Step 3 includes the wound assay performed in underlying C2C12 cells to evaluate cellular migratory capacity. Step 4 involves immunostaining for phalloidin to evaluate cytological architecture and morphology of migrated cells. Abbreviations: NCCs = neural crest cells; Ab = antibody.

Wound Assay to Evaluate the Migratory Capacity of Murine Myoblasts in Co-Culture

Source: Toubat, O. et al., Modeling Paracrine Noncanonical Wnt Signaling In Vitro. J. Vis. Exp. (2021).
This video describes a non-contact co-culture ...

In response to a wound, secretory cells produce paracrine signaling molecules to activate myoblasts &#8212; undifferentiated muscle cells. Activated myoblasts migrate toward the wound site, where they proliferate, causing the wound to heal.
To evaluate the migratory capacity of myoblasts in vitro, take a multiwell plate containing a confluent monolayer of murine myoblasts. Using a pipette tip, scratch the monolayer to create a linear, cell-free patch inside the well, which simulates the wound site.
Carefully supplement the well with the growth medium without disturbing the wound patch.
Take a membranous insert containing an adherent culture of neural crest cells, or NCCs &#8212; secretory cells &#8212; in a suitable medium. Place the insert inside the well, so that the NCCs at the base are near the wound patch. Incubate the co-culture for the desired duration.
During incubation, the NCCs release signaling molecules that bind to the specific receptors on the myoblasts, initiating a signaling cascade. This signaling facilitates actin reorganization in the myoblasts, and as a result, these cells develop cytoplasmic projections such as lamellipodia and filopodia, at their edges. These projections help the myoblasts migrate toward the wounded area and gradually repopulate, leading to wound healing.
Place the plate under a microscope, and observe the wound healing, the extent of which correlates with the migratory capacity of myoblasts in co-culture.

wound-assay-to-evaluate-migratory-capacity-murine-myoblasts-co

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198 次观看. 来源:Toubat， O. et al.， 体外旁分泌非经典 Wnt 信号传导建模。J. Vis. Exp. （2021）。 该视频介绍了一种非接触式共培养伤口愈合试验，用于评估小鼠成肌细胞的迁移能力。这有助于了解体外旁分泌非经典 Wnt 信号相互作用的信号发送和信号接收成分。 

视频: 伤口测定评估共培养中小鼠成肌细胞的迁移能力 - 概念

In Vitro Scratch Assay to Demonstrate Effects of Arsenic on Skin Cell Migration

Understanding the physiologic mechanisms of wound healing has been the focus of ongoing research for many years. This research directly translates into changes in clinical standards used for treating wounds and decreasing morbidity and mortality for patients. Wound healing is a complex process that requires strategic cell and tissue interaction and function. One of the many critically important functions of wound healing is individual and collective cellular migration. Upon injury, various cells from the blood, surrounding connective, and epithelial tissues rapidly migrate to the wound site by way of chemical and/or physical stimuli. This migration response can largely dictate the outcomes and success of a healing wound. Understanding this specific cellular function is important for translational medicine that can lead to improved wound healing outcomes. Here, we describe a protocol used to better understand cellular migration as it pertains to wound healing, and how changes to the cellular environment can significantly alter this process. In this example study, dermal fibroblasts were grown in media supplemented with fetal bovine serum (FBS) as monolayer cultures in tissue culture flasks. Cells were aseptically transferred into tissue culture treated 12-well plates and grown to 100% confluence. Upon reaching confluence, the cells in the monolayer were vertically scratched using a p200 pipet tip. Arsenic diluted in culture media supplemented with FBS was added to individual wells at environmentally relevant doses ranging 0.1-10 &#956;M. Images were captured every 4 hours (h) over a 24 h period using an inverted light microscope to observe cellular migration (wound closure). Images were individually analyzed using image analysis software, and percent wound closure was calculated. Results demonstrate that arsenic slows down wound healing. This technique provides a rapid and inexpensive first screen for evaluation of the effects of contaminants on wound healing.

In Vitro Scratch Assay to Demonstrate Effects of Arsenic on Skin Cell Migration

This study focuses on an in vitro model of wound healing (scratch assay) as a mechanism for determining how environmental contaminants such as arsenic influence cellular migration. The results demonstrate that this in vitro assay provides rapid and early indications of changes to cellular migration prior to in vivo experimentation.

在体外显示砷对皮肤细胞迁移影响的划痕测定

Understanding the physiologic mechanisms of wound healing has been the focus of ongoing research for many years. This research directly translates into ...

科研

JoVE Journal

环境科学

Microscopy Based Methods for the Assessment of Epithelial Cell Migration During In Vitro Wound Healing

Cell migration is a mandatory aspect for wound healing. Creating artificial wounds on research animal models often results in costly and complicated experimental procedures, while potentially lacking in precision. In vitro culture of epithelial cell lines provides a suitable platform for researching the cell migratory behavior in wound healing and the impact of treatments on these cells. The physiology of epithelial cells is often studied in non-confluent conditions; however, this approach may not resemble natural wound healing conditions. Disrupting the epithelium integrity by mechanical means generates a realistic model, but may impede the application of molecular techniques. Consequently, microscopy based techniques are optimal for studying epithelial cell migration in vitro. Here we detail two specific methods, the artificial wound scratch assay and the artificial migration front assay, that can obtain quantitative and qualitative data, respectively, on the migratory performance of epithelial cells.

Microscopy Based Methods for the Assessment of Epithelial Cell Migration During  In Vitro Wound Healing

This manuscript describes how incision-like lesions made on cultured epithelial cell monolayers conveniently model wound healing in vitro, allowing for imaging by confocal or laser scanning microscopy, and which can provide high-quality quantitative and qualitative data for studying both cell behavior and the mechanisms involved in migration.

以显微镜为基础的方法评估上皮细胞迁移过程中的体外创面愈合

Cell migration is a mandatory aspect for wound healing. Creating artificial wounds on research animal models often results in costly and complicated ...

医学

Scratch Migration Assay and Dorsal Skinfold Chamber for In Vitro and In Vivo Analysis of Wound Healing

Impaired cutaneous wound healing is a major concern for patients suffering from diabetes and for elderly people, and there is a need for an effective treatment. Appropriate in vitro and in vivo approaches are essential for the identification of new target molecules for drug treatments to improve the skin wound healing process. We identified the &#946;3 subunit of voltage-gated calcium channels (Cav&#946;3) as a potential target molecule to influence the wound healing in two independent assays, i.e., the in vitro scratch migration assay and the in vivo dorsal skinfold chamber model. Primary mouse embryonic fibroblasts (MEFs) acutely isolated from wild-type (WT) and Cav&#946;3-deficient mice (Cav&#946;3 KO) or fibroblasts acutely isolated from WT mice treated with siRNA to down-regulate the expression of the Cacnb3 gene, encoding Cav&#946;3, were used. A scratch was applied on a confluent cell monolayer and the gap closure was followed by taking microscopic images at defined time points until complete repopulation of the gap by the migrating cells. These images were analyzed, and the cell migration rate was determined for each condition. In an in vivo assay, we implanted a dorsal skinfold chamber on WT and Cav&#946;3 KO mice, applied a defined circular wound of 2 mm diameter, covered the wound with a glass coverslip to protect it from infections and desiccation, and monitored the macroscopic wound closure over time. Wound closure was significantly faster in Cacnb3-gene-deficient mice. Because the results of the in vivo and the in vitro assays correlate well, the in vitro assay may be useful for the high-throughput screening before validating the in vitro hits by the in vivo wound healing model. What we have shown here for wild-type and Cav&#946;3-deficient mice or cells might also be applicable for specific molecules other than Cav&#946;3.

Here, we present a protocol for an in vitro scratch assay using primary fibroblasts and for an in vivo skin wound healing assay in mice. Both assays are straightforward methods to assess in vitro and in vivo wound healing.

划痕迁移分析和背皮折叠室的体外和在Vivo分析伤口愈合

Impaired cutaneous wound healing is a major concern for patients suffering from diabetes and for elderly people, and there is a need for an effective ...

Wound Assay to Evaluate the Migratory Capacity of Murine Myoblasts in Co-Culture

成績單

Wound Assay to Evaluate the Migratory Capacity of Murine Myoblasts in Co-Culture