Name: ビデオ: Safranin-O染色:軟骨の構造的完全性と細胞性を可視化する方法 - 概念
Uploaded: 2023-04-30T14:58:00.000+00:00
Duration: 1 min 45 s
Description: 1.7K ビュー. 出典:Zhao, Y., et al. Establishment of a Surgically-induced Model in Mice to Investigate the Protective Role of Progranulin in Osteoarthritis. J. Vis. Exp. (2014). このビデオでは、サフラニンオレンジを使用した軟骨の染色手順を実演します。この方法は、軟骨を視覚化し、損傷を検出するのに役立ちます。

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1. Safranin O staining
<ol>
	<li>Begin with the glass slides containing serial sagittal sections spanning a region from the center of the lateral condyle to the center of the medial condyle of a euthanized mouse model with the destabilized medial meniscus.</li>
	<li>Next, deparaffinize the slides in oxylene, and hydrate them in an ethanol gradient to distilled water. Thereafter, the slides are stained through Weigert&#39;s Iron Hematoxylin Solution, 0.05% Fast Green (FCF) Solution, 1% Acetic Acid Solution, and 0.1% Safranin O Solution. Mount the slides using resinous medium.</li>
	<li>Score the Safranin O-stained slides based on loss of proteoglycan (red color) in cartilage and percentage of destruction in cartilage structure, do statistical analysis for the histological score.</li>
</ol>

safranin-o staining: a method to visualize the structural integrity and cellularity of cartilage

Source: Zhao, Y., et al. <a href="https://www.jove.com/v/50924">Establishment of a Surgically-induced Model in Mice to Investigate the Protective Role of Progranulin in Osteoarthritis.</a> J. Vis. Exp. (2014).
In this video, we demonstrate a staining procedure for cartilage using safranin-orange. This method helps visualize the cartilage and detect any damage.

Safranin-O Staining: A Method to Visualize the Structural Integrity and Cellularity of Cartilage

Source: Zhao, Y., et al. Establishment of a Surgically-induced Model in Mice to Investigate the Protective Role of Progranulin in Osteoarthritis. J. Vis. ...

For cartilage staining, begin with a formalin-fixed, paraffin-embedded cartilage section from a euthanized mouse.
First, immerse the sample in the xylene substitute - a non-hazardous clearing agent that removes the paraffin wax and exposes the dehydrated tissue. Next, treat the sample with decreasing ethanol concentrations to rehydrate the tissue for subsequent staining.
Now, stain the sample with Weigert&#8217;s iron hematoxylin - an organic stain containing ferrous ions - and incubate briefly. The hematoxylin molecules form complexes with ferrous ions and penetrate the cell. The ferrous ions act as a mordant and facilitate binding of the hematoxylin to the nucleic acids, imparting them a blue color.
Then, treat the sample with the fast green dye - a counterstain that binds to the connective tissue and imparts a green color. Thereafter, treat the sample with an acetic acid solution to stabilize the dye molecules. Lastly, stain the sample with safranin-orange - a cationic dye - and incubate.
The positively charged safranin molecules migrate toward the negatively charged proteoglycans in the cartilage and bind to them, imparting a red color. Subsequently, mount the slide in a resin medium and visualize it under a microscope.
Healthy cartilage appears intensely red due to the proteoglycan-rich extracellular matrix, while unhealthy cartilage appears less red with signs of tissue damage.

safranin-o-staining-method-to-visualize-structural-integrity

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Biological Techniques

Staining Techniques

Tissue staining

1.7K ビュー. 出典:Zhao, Y., et al. Establishment of a Surgically-induced Model in Mice to Investigate the Protective Role of Progranulin in Osteoarthritis. J. Vis. Exp. (2014). このビデオでは、サフラニンオレンジを使用した軟骨の染色手順を実演します。この方法は、軟骨を視覚化し、損傷を検出するのに役立ちます。 

ビデオ: Safranin-O染色:軟骨の構造的完全性と細胞性を可視化する方法 - 概念

Standardized Histomorphometric Evaluation of Osteoarthritis in a Surgical Mouse Model

One of the most prevalent joint disorders in the United States, osteoarthritis (OA) is characterized by progressive degeneration of articular cartilage, primarily in the hip and knee joints, which results in significant impacts on patient mobility and quality of life. To date, there are no existing curative therapies for OA able to slow down or inhibit cartilage degeneration. Presently, there is an extensive body of ongoing research to understand OA pathology and discover novel therapeutic approaches or agents that can efficiently slow down, stop, or even reverse OA. Thus, it is crucial to have a quantitative and reproducible approach to accurately evaluate OA-associated pathological changes in the joint cartilage, synovium, and subchondral bone. Currently, OA severity and progression are primarily assessed using the Osteoarthritis Research Society International (OARSI) or Mankin scoring systems. In spite of the importance of these scoring systems, they are semiquantitative and can be influenced by user subjectivity. More importantly, they fail to accurately evaluate subtle, yet important, changes in the cartilage during the early disease states or early treatment phases. The protocol we describe here uses a computerized and semiautomated histomorphometric software system to establish a standardized, rigorous, and reproducible quantitative methodology for the evaluation of joint changes in OA. This protocol presents a powerful addition to the existing systems and allows for more efficient detection of pathological changes in the joint.

The current protocol establishes a rigorous and reproducible method for quantification of morphological joint changes that accompany osteoarthritis. Application of this protocol can be valuable in monitoring disease progression and evaluating therapeutic interventions in osteoarthritis.

外科用マウスモデルにおける変形性関節症の標準化組織形態評価

One of the most prevalent joint disorders in the United States, osteoarthritis (OA) is characterized by progressive degeneration of articular cartilage, ...

JoVE Journal

医学

An Ex Vivo Tissue Culture Model of Cartilage Remodeling in Bovine Knee Explants

Ex vivo culture systems cover a broad range of experiments dedicated to studying tissue and cellular function in a native setting. Cartilage is a unique tissue important for proper function of the synovial joint and is constituted by a dense extracellular matrix (ECM), rich in proteoglycan and type II collagen. Chondrocytes are the only cell type present within cartilage and are widespread and relatively low in number. Altered external stimuli and cellular signalling can lead to changes in ECM composition and deterioration, which are important pathological hallmarks in diseases such as osteoarthritis (OA) and rheumatoid arthritis.
Ex vivo cartilage models allow 1) profiling of chondrocyte mediated alterations of cartilage tissue turnover, 2) visualizing the cartilage ECM composition, and 3) chondrocyte rearrangement directly in the tissue. Profiling these alterations in response to stimuli or treatments are of high importance in various aspects of cartilage biology, and complement in vitro experiments in isolated chondrocytes, or more complex models in live animals where experimental conditions are more difficult to control.
Cartilage explants present a translational and easily accessible method for assessing tissue remodeling in the cartilage ECM in controllable settings. Here, we describe a protocol for isolating and culturing live bovine cartilage explants. The method uses tissue from the bovine knee, which is easily accessible from the local butchery. Both explants and conditioned culture medium can be analyzed to investigate tissue turnover, ECM composition, and chondrocyte function, thus profiling ECM modulation.

Here, we present a protocol describing isolation and culturing of cartilage explants from bovine knees. This method provides an easy and accessible tool to describe tissue changes in response to biological stimuli or novel therapeutics targeting the joint.

牛膝剥離植物における軟骨改造のEx Vivo組織培養モデル

Ex vivo culture systems cover a broad range of experiments dedicated to studying tissue and cellular function in a native setting. Cartilage is a unique ...

生物学

Detecting Migration and Infiltration of Neutrophils in Mice

Neutrophils are a major member of the innate immune system and play pivotal roles in host defense against pathogens and pathologic inflammatory reactions. Neutrophils can be recruited to inflammation sites via the guidance of cytokines and chemokines. Overwhelming infiltration of neutrophils can lead to indiscriminate tissue damage, such as in rheumatoid arthritis (RA). Neutrophils isolated from peritoneal exudate respond to a defined chemoattractant, N-formyl-Met-Leu-Phe (fMLP), in vitro in Transwell or Zigmond chamber assays. The air pouch experiment can be used to evaluate the chemotaxis of neutrophils towards lipopolysaccharide (LPS) in vivo. The adjuvant-induced arthritis (AA) mouse model is frequently used in RA research, and immunohistochemical staining of joint sections with anti-myeloperoxidase (MPO) or anti-neutrophil elastase (NE) antibodies is a well-established method to measure neutrophil infiltration. These methods can be used to discover promising therapies targeting neutrophil migration.

Here, we present three methods to assess neutrophil migration and infiltration both in vivo and in vitro. These methods can be used to discover promising therapeutics targeting neutrophil migration.

マウスの好中球の遊走と浸潤の検出

Neutrophils are a major member of the innate immune system and play pivotal roles in host defense against pathogens and pathologic inflammatory reactions. ...

Safranin-O Staining: A Method to Visualize the Structural Integrity and Cellularity of Cartilage

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Safranin-O Staining: A Method to Visualize the Structural Integrity and Cellularity of Cartilage

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