Summary

Destabilization of the Medial Meniscus and Cartilage Scratch Murine Model of Accelerated Osteoarthritis

Published: July 06, 2022
doi:

Summary

The present protocol describes the controlled microblade scratches on the surface of the articular cartilage after destabilizing the mouse knee by cutting the medial miniscotibial ligament. This animal model presents an accelerated form of osteoarthritis (OA) suitable for studying osteophyte formation, osteosclerosis, and early-stage pain.

Abstract

Osteoarthritis is the most prevalent musculoskeletal disease in people over 45, leading to an increasing economic and societal cost. Animal models are used to mimic many aspects of the disease. The present protocol describes the destabilization and cartilage scratch model (DCS) of post-traumatic osteoarthritis. Based on the widely used destabilization of the medial meniscus (DMM) model, DCS introduces three scratches on the cartilage surface. The current article highlights the steps to destabilize the knee by transecting the medial meniscotibial ligament followed by three intentional superficial scratches on the articular cartilage. The possible analysis methods by dynamic weight-bearing, microcomputed tomography, and histology are also demonstrated. While the DCS model is not recommended for studies that focus on the effect of osteoarthritis on the cartilage, it enables the study of osteoarthritis development in a shorter time window, with special focus on (1) osteophyte formation, (2) osteoarthritic and injury pain, and (3) the effect of cartilage damage in the whole joint.

Introduction

Osteoarthritis (OA) is the most prevalent musculoskeletal disease in people over 45, with over 8.75 million seeking treatment in the UK1. The growing prevalence of the disease has led to an increased economic and societal cost, is a major contributor to disability, and reduces the quality of life for patients1. Without treatments available, there is an urgent need to accelerate research to understand the development and progression of the disease. The disease is complex and also multifactorial in its nature. The main clinical measurements of the disease are pain and joint mobility2, and OA affects all the tissues in the joint, not just the cartilage3. One of the main challenges in understanding OA is that it can take years, sometimes decades, from initial presentation/injury to symptomatic disease progression with pain and immobility.

Modeling osteoarthritis in rodents has enhanced our knowledge of OA pathophysiology by allowing us to understand the initiation and progression in a much shorter time frame and with a detailed examination of the tissues involved. There are numerous murine models of osteoarthritis, from genetically modified animals to surgical intervention models. The most widely used murine model of post-traumatic OA is the destabilization of the medial meniscus (DMM)4,5. A caveat of the model is the variability between different operators. Experienced surgeons can perform the procedure with minimal joint damage, while inexperienced operators expose the joint capsule for longer periods of time and inflict damage on the cartilage. This variability in the process influences the severity of the model, with more initial damage leading to increased cartilage damage scores and osteophyte formation. Intending to reduce the variability between operators and mimic cartilage damage from clinical intervention, a modified version of this model is developed, whereby controlled additional damage onto the cartilage surface in the form of three superficial scratches are inflicted6. This also allows modeling the OA progression resulting from cartilage damage caused by some clinical interventions. Compared to the standard DMM model, the directly induced cartilage damage results in consistently accelerated protruding osteophyte formation, increased cartilage damage and inflammation, and measurable surrogate pain in male mice.

This model is particularly suitable for the study of early-stage post-traumatic OA, focusing on osteophyte formation, pain presentation (in male mice), synovitis, and early changes to bone parameters. The consistency of osteophyte formation in this model makes it pertinent to study bone repair and endochondral ossification since osteophyte formation is a process of repair via endochondral ossification7. The model also mimics damage introduced directly to the cartilage during clinical interventions, such as arthroscopic surgical procedures, and thus it is also suitable for the study of the effect of cartilage damage on the whole joint.

Protocol

All experimental procedures were approved by the Ethical Review Panel of the University of Glasgow and the University of the West of Scotland, and carried out following the Animals (Scientific Procedures) Act 1986 (UK) guidelines. 10-week-old C57Bl6/J male mice, weighing around 25 g, were used for the present study. The mice were obtained from commercial sources (see Table of Materials).

1. Animal preparation

NOTE: Consider mouse gender in regards to the purpose of the study as post-traumatic OA models display important differences depending on gender8,9,10.

  1. Ensure that the anesthetic reagent (2% isoflurane) is ready.
    NOTE: Injectable anesthesia can also be used11. Given the quick duration of the surgery, the use of inhalant anesthesia is recommended.
  2. Use a separate sham-operated age-matched group as surgical control.
    NOTE: The contralateral knee must not be used as a surgical control (sham operation on the contralateral leg). This may have issues in terms of animal welfare, and it will likely affect gait and gait measurements. The contralateral knee normalizes intrinsic bone parameters12 and acts as a paired comparison on evoked pain tests13.
  3. Use skeletally mature mice.
    ​NOTE: Most literature induces OA at 8-12 weeks of age. In the present study, the mice are 10 weeks old.

2. Pre-operative care (carried out by a surgical assistant)

  1. If transported from a different facility, allow at least 1 week prior to surgical intervention for mice to adjust to their new environment.
  2. Carry out surgery in an appropriately designated sterile room, ensuring all surfaces are sterile (e.g., use sterile drapes to cover areas of surgery).
    NOTE: The surgery is aseptic.
  3. Arrange and place sterile instruments on sterile drapes.
  4. Weigh the mouse.
  5. Induce anesthesia by introducing the mouse in an anesthetic cage and then introducing 2% isofluorane for upto 15 min using a standard anesthetic rig (see Table of Materials).
    NOTE: The cage must not have "residual" anesthesia prior to introducing the mouse.
  6. Once anesthetized, take the mouse out of the anesthetic chamber and clip the fur over the knee, front and lateral sides from the mid-shin to the mid-thigh with small hair clippers.
    NOTE: The choice of hindlimb knee is up to the operator's preference on which side they find easier to conduct the surgery. This protocol operated on the left leg.
  7. Ensure the mouse is fully anesthetized (non-responsive to pinching the foot).
  8. Disinfect skin by applying antibacterial skin cleanser (e.g., containing chlorhexidine or iodophor, see Table of Materials) on shaved exposed skin.
  9. For analgesia, administer 0.05 mg/kg of buprenorphine subcutaneously.
  10. Place the mouse on the dorsal side, leaving the knee to be operated on upwards, and place the mouse nose in the nozzle connected to the anesthetic rig.
  11. Cover the mouse with a sterile drape with a small keyhole opening.
  12. Position the leg to be operated on with the knee flexed at less than 90°, with the patellar ligament facing upwards and the foot immobilized with surgical tape.

3. Destabilization of the medial meniscus procedure followed by cartilage scratch

  1. Adjust the microscope to focus on the patellar ligament.
  2. Pinch the skin of the knee on the lateral side with serrated forceps (see Table of Materials), make a small cut parallel to the distal patellar tendon using surgical scissors, introduce the scissors and expand the cut to about 1 cm. Move the skin over to the medial side, exposing the patellar ligament and the proximal tibial plateau (Figure 1).
  3. With a number 11 blade, make an incision along the medial side of the patellar ligament, from the top to the bottom of the ligament (Figure 1A). When reaching the bottom of the patellar ligament, turn the blade 90° and extend the incision away from the patellar ligament toward the medial side to gain access to the joint capsule.
    NOTE: Bleeding may occur in this or the subsequent steps. If bleeding occurs use a sterile cotton bud and apply pressure a few seconds (5 to 30 s).
  4. Pinch the patellar ligament with blunt tip forceps and rotate the wrist to move the patellar ligament to the lateral side, just enough to expose the infrapatellar fat pad (IFP).
    NOTE: To minimize damage to the patellar ligament, do not hold the tweezers too tight, just sufficient to keep the ligament to the side.
  5. While still holding the patellar ligament lightly, pinch the IFP with micro-tweezers (see Table of Materials) to raise it and move it slightly upward. This allows visualizing the medial meniscus ligament.
  6. Identify the medial meniscotibial ligament (MMTL) of the medial meniscus, which anchors the cranial horn of the medial meniscus to the anterior tibial plateau (Figure 1B).
  7. Avoid damage and prolonged cartilage exposure at the tibial plateau or femoral condyle.
  8. Carefully sever the MMTL with small 2 mm blade Vannas spring scissors, leaving the medial meniscus and other ligaments intact. At this point, the surgical procedure for the DMM model is completed (Figure 1C).
  9. With a 3 mm microsurgical knife, mark three evenly spaced indentations on the tibial articular cartilage in a direction from the posterior to the anterior part.
    NOTE: The scores are about 1 mm in length and only damage the surface of the cartilage (Figure 2D).
    1. Do not use excessive force with the blade onto the cartilage (i.e., ensure the scratches are superficial). This additional step inflicts cartilage damage, inducing the DCS model.
  10. Close the skin with two or three small 7 mm wound closure metal clips or absorbable 6-0 subdermal surgical sutures (see Table of Materials).
    NOTE: Subdermal surgical sutures are better as they avoid further intervention, but they extend the surgery duration. External sutures increase the risk of wound opening by the gnawing of the mice.
  11. Identify the medial meniscotibial ligament of the medial meniscus for sham surgery, but do not sever.
  12. For mice only receiving cartilage scratches, make the three superficial scratches without severing the ligament.
    ​NOTE: Between each mouse, change gloves and sterilize instruments via autoclave. Remember to check the instruments have cooled before re-use.

4. Post-operative care

  1. If bleeding has occurred (>50 uL), inject 500 µL of warm sterile saline subcutaneously (on the back of the mouse).
    NOTE: In our experience, although mice have minor bleeds, it never is more than a small drop, and thus fluids do not need to be replenished.
  2. After surgery, place the mouse in a recovery cage on a clean paper tissue and allow recovery from anesthesia (5-10 min).
  3. Transfer the fully conscious mice into a clean cage with fresh bedding after surgery.
  4. In the 72 h after surgical intervention, monitor for any signs of pain or distress. Pay attention to:
    1. Changes in body weight. Although body weight may decrease on the first and second day, this is usually no more than 5% of the pre-surgical body weight.
    2. General lack of grooming or over-grooming around the incision.
    3. Signs of general health deterioration, such as hunched posture, facial grimacing, and/or abnormal respiration.
    4. Wound infection as indicated by any swelling, discharge, or opening of the wound.
      NOTE: Infection may occur if the surgical wound opens. As surgical wound repair (e.g., replacing missing metal clips or re-suturing) is a regulated procedure, ensure relevant approval is obtained prior to performing repairs.
  5. Remove metal clips between 5-7 days post-surgery.
  6. Maintain mice typically 2-52 weeks post-operatively depending on the study design.
  7. Evaluate pain/gait at any point during the study.
    NOTE: The present study uses dynamic weight-bearing as described in step 5.1.
  8. Euthanize the animal by an approved method, according to the national licensing agreements, local guidelines, and experimental approval.
    ​NOTE: In the present study, the animals were euthanized via exsanguination (cardiac puncture) under terminal anesthesia followed by cervical dislocation14.

5. Evaluation of osteoarthritic disease

  1. Measure dynamic weight bearing as a surrogate measurement of pain following the steps below.
    NOTE: As mice are prey animals, they tend to hide pain behaviors. This makes the measurement of pain difficult. There are many ways to measure evoked pain, such as Von Frey15 and gait analysis16. The present study measured the differential load between the operated osteoarthritic leg and the unoperated control leg on a pressure mat while the mouse was in a cage (see Table of Materials, Figure 2A).
    1. Weigh the mouse. Tare and calibrate the pressure mat according to manufacturer's specific instructions (see Dynamic weight-bearing equipment in Table of Materials). Introduce the mouse in the cage.
    2. Record movement and paw pressure of the mouse in the cage for 5 min. Analyze acquired data to validate 1 min, following manufacturer's instructions.
      NOTE: The manufacturer's automated analysis on DWB software (see dynamic weight-bearing equipment in Table of materials) provides measurements on each paw in proportion to the total body weight, the amount of the validated time that each paw remained on the mat, and an estimation of the mat area occupied by each paw. This allows the calculation of the differential load between the two rear paws, the differential load between the front and rear paws, an increase of front paw loading (if the same mouse has been measured over a period of time), the time spent lifting the OA leg in comparison to the contralateral leg and the paw surface.
  2. Quantify calcified tissue through microcomputed tomography (µCT).
    NOTE: Although subchondral bone osteosclerosis and osteophyte formation can be measured in histological sections, µCT offers the opportunity to quantify three-dimensionally. The resolution of image capture in µCT at 5 µm is sufficient, as this allows visualization of smaller structures such as the osteophytes, although the higher the resolution, the better.
    1. Fix knee joints in 4% paraformaldehyde solution for 24 h, then transfer to 70% EtOH.
    2. Scan knee joints in a µCT scanner.
      NOTE: In the present study, the samples were scanned on a µCT scanner (see Table of Materials) with a 0.5 aluminum filter set at 50 kV and 200 µA. Samples were examined at a voxel size of 4.5 µm; 2 µm, 0.2° rotation angle for imaging, and 0.5° rotation angle for quantification.
    3. Reconstruct scans to allow 3D visualization. The scans presented here were reconstructed using compatible software (see Table of Materials).
    4. Analyze subchondral bone sclerosis (Figure 2B) following the steps below.
      1. Select a volume of interest (VOI) of 0.5 mm × 0.9 mm × 0.9 mm in the center of the load of the medial tibial plateau17.
      2. Normalize against the intrinsic bone phenotype of the mouse by analyzing the unoperated leg.
      3. Determine the subchondral bone density and micro-architecture by selecting a region of interest (ROI) delineating the trabecular structure within the tibial epiphysis, the subchondral plate, or the total subchondral bone in the two-dimensional coronal view of the stack using CTan software (see Table of Materials).
        NOTE: As the disease progresses, the separation between the subchondral plate and subchondral trabecular region becomes more difficult to distinguish. It is then recommended to analyze the area of subchondral bone selected from the joint space to the growth plate.
    5. Quantify osteophytes (Figure 2C) following the steps below.
      1. Identify osteophytes in the reconstructed three-dimensional image stacks using CTvol software (see Table of Materials).
        NOTE: Mineralized osteophytes are protrusions similar to woven bone visible on the medial side of the subchondral bone18. An example of these is indicated with yellow arrows in Figure 2C.
      2. Manually count the number of identified osteophytes in the medial side of the knee joint.
      3. Measure osteophyte volume in 2D sequential image analysis (using the CT analyzer) by delineating the edge of osteophytes manually, protruding from the subchondral plate as the region of interest (ROI) for analysis.
      4. Calculate osteophyte bone density as the ratio of bone volume over osteophyte volume using the CT analyzer software (see Table of Materials).
  3. Evaluate cartilage damage and synovitis (Figure 2D) according to the OARSI cartilage damage score19 and synovitis score20 on paraffin-embedded 6 µm sections.
    1. After scanning, decalcify knee joints in 10% EDTA at 4 °C for a minimum of 2 weeks, changing solution twice a week.
    2. Embed samples in paraffin. For treatments and incubation periods, see Supplementary File 1.
    3. Cut 5 µm coronal sections of paraffin-embedded samples on a rotary microtome (see Table of Materials).
    4. Select sections in the area where the tibial and femoral condyles meet (Figure 2D). Select two sections in three equally distanced areas of the joint.
      NOTE: Sections scored in the present study were selected in areas 80-100 µm apart.
    5. Stain sections with Safranin-O and Fast green (see Table of Materials) following the steps below.
      1. Deparaffinize sections by submerging them (in the mentioned sequence) in Xylene for 5 min (2x), 100% ethanol for 2 min, 95% ethanol for 2 min, 80% ethanol for 2 min, and 70% ethanol for 2 min.
      2. Stain with filtered Haematoxylin (see Table of Materials) for 30 s. Then rinse in tap water for 5 min (three times).
      3. Wash with Scott's buffer (2 g of sodium bicarbonate and 10 g of magnesium sulfate in 1 L of distilled water) for 2 min. Rinse in 'tap water' for 5 min (three times).
      4. Stain for 4 min with 0.2% Fast green. Dip in 1% glacial acetic acid, five times (freshly made each session). Rinse quickly in tap water.
      5. Stain for 5 min with 0.5% Safranin-O. Rinse in 95% ethanol. Dehydrate sections in 100% ethanol for 3 min followed by 3 min in Xylene.
    6. Score sections as stated in Glasson et al. for cartilage19 and Jackson et al. for synovitis20.
      NOTE: Other methods of quantification exist, such as the computer-based quantification by Pinamont et al.21.
    7. Validate the scoring system with two different scorers, blinded to the experiment.

Representative Results

The percentage load per total body weight of the rear operated/OA leg was compared to the contralateral/control leg. Although other parameters may also give significant differences, like the increase in front paw load after surgical intervention, a consistent change in rear paw load indicates a preference to use one leg over the other and is a more direct indicator of significant discomfort for the mouse due to OA development. There were no significant changes in rear leg load in the DMM model within 8 weeks post-induction, while DCS mice favor the contralateral/control leg significantly 2 weeks after intervention (Figure 3A).

Subchondral bone was analyzed by focusing on the volume under the medial loaded region of the tibial condyle. Here we assessed the bone density of this area by determining the percentage of mineralized bone within the region of interest and calculated the ratio between the contralateral and the ipsilateral leg. The ratio indicates that both models have increased bone density in the affected limb (ratio above 1) 4 weeks after induction (Figure 3B). The emergence of osteophytes is more prominent in the DCS model, where there is a significant increase in the number and volume compared to the DMM model 2 weeks after intervention (Figure 3C,D). DCS presents elevated cartilage damage in the medial tibial and femoral compartments and synovitis (Figure 3E,F) 4 weeks after induction.

Figure 1
Figure 1: Surgical intervention to induce post-traumatic OA in the mouse. Sequential images represent the different stages of the procedure. (A) Exposure of joint capsule cutting the superficial membrane around the knee by inserting a number 11 scalpel blade on the medial side of the patellar ligament and away from the ligament. This will expose the infrapatellar fat pad. (B) Identification and transection of the medial meniscotibial ligament. To identify the ligament, move the patellar ligament toward the lateral side and then push the fat pad upward. This allows for the visualization of the ligament as a small horizontal white line just above the tibial condyle (indicated here with a black arrow). To cut the ligament, the lower blade of the spring scissors is placed under the ligament, taking care not to damage the cartilage. Move the meniscus towards the medial side to visualize the tibial condyle. (C) Scratching the surface of the exposed cartilage and closure of the wound. To scratch the cartilage, the microblade is inserted toward the posterior side, where it contacts the cartilage and then moves forward toward the anterior part of the joint. Once the scratches are done, pull the skin over the knee and close the wound either by subdermal suturing or with wound clips. Please click here to view a larger version of this figure.

Figure 2
Figure 2: Evaluation of osteoarthritis in the mouse. (A) Dynamic weight-bearing consists of matching the load on a pressure mat to the corresponding paw. The load is then expressed as a percentage of the total weight. (B) Subchondral bone is measured by selecting a volume of interest in the loading region of the medial tibial condyle and selecting the subchondral plate or trabecular bone. These images are at a resolution of 4.5 µm. (C) Osteophytes are identified and quantified in a three-dimensional view of the acquired µCT images. The volume of osteophytes is measured by selecting an ROI delineating the edge of the osteophyte. The bone density is calculated as the bone volume per osteophyte volume. The images presented here were taken at a resolution of 2 µm, but quantification is usually done with a 4.5 µm resolution. (D) Cartilage and synovitis scores are taken from 6 µm sections stained with Safranin-O and Fast green. A coronal section of the mouse knee where all quadrants, marked with a black box, are visible for scoring and a magnification of the medial side is shown. The synovitis surrounding the medial side of the knee joint is also visible, especially above and below the displaced meniscus. Please click here to view a larger version of this figure.

Figure 3
Figure 3: Representative evaluation of OA in the DMM and the DCS models. (A) DWB measured up to 8 weeks post-induction on experiments carried out by the same expert operator. Load is expressed as a ratio between the operated/OA load versus the contralateral/control load. Paired t-tests of both legs are also shown in the Sham (grey), DMM (blue), and DCS (pink) models. µCT analysis 4 weeks after surgical intervention. (B) Subchondral bone was analyzed 4 weeks after surgical intervention and expressed as the ratio of the ipsilateral over the contralateral %BV/TV. (C) Osteophyte number and (D) osteophyte volume was analyzed 2 weeks after induction. Histological evaluation 4 weeks after induction of (E) cartilage damage of the medial tibial and femoral articular cartilage and (F) synovitis were scored with standardized methods19,20. Data are expressed as mean ± standard deviation, n ≥ 5. Data were compared by repeated-measures ANOVA with a Šídák test correction (A), paired t-test (A), or standard Student's t-test (BF). *P < 0.05, **P < 0.01, ***P < 0.001, ns = not significant. Please click here to view a larger version of this figure.

Supplementary File 1: Treatment and incubation condition for paraffin embedding. Please click here to view a larger version of this figure.

Discussion

To perform surgical induction of post-traumatic osteoarthritis (PTOA), support from an assistant is strongly recommended (e.g., to prepare the mice while the operator focuses on the surgery). This facilitates aseptic surgery, thereby reducing the risks of infections and making the intervention more efficient in large experiments. It is easy to lose the plane of focus during the surgery, so a microscope that includes pedals for focusing is a valuable feature in helping to maintain sterility throughout the surgery. The position of the mouse and the knee is crucial. The knee must be facing upward and sufficiently bent to maximize the opening of the knee joint space, facilitating easier access to the ligament for introducing the microblade to scratch the condyle surface. Identifying the MMTL can be challenging, especially when the fat pad is larger than usual or there is a small bleed. To avoid bleeds, push the fat pad upward to prevent tears and subsequent bleeding. If the fat pad is large, this might take a little longer, but patiently continue to push it upwards.

The MMTL is quite close to the tibial condyle, so one must take care not to injure the cartilage when positioning the lower blade of the curved spring scissors under the MMTL. The curved blades should point toward the medial side and slightly upward, parallel to the condyle. For best sectioning of the MMTL, ensure the scissors are sharp. Check that the meniscus can move medially after cutting the ligament, as sometimes a small attachment remains that needs further cutting. When introducing the microblade to scratch the condyle, it must be perpendicular to the condyle. Make the first scratch closer to the middle of the joint but take care not to damage the anterior cruciate ligament. Then move toward the medial side and then behind the meniscus. The scratches might be visible as faint white lines on the cartilage. Because we usually use clips, the initial incision is performed on the lateral side, so the clips are positioned on the side of the leg after closing the wound. This avoids the clips rubbing the knee as the mouse regains movement. When using sutures, the use of subdermal stitches is strongly recommended. If using external stitches, the mice are likely to gnaw at the stitches and open their wound, which will increase the chances of infection. When done right, this surgery must not take more than 5-10 min, from incision to wound closure, thus minimizing the exposure of the cartilage and any additional uncontrolled damage that may occur. After the surgery, the mice recover very quickly and almost immediately can climb into the cage and move around normally. If the mice are not active, the appropriate expert in the unit should be consulted.

For the behavioral evaluation of pain, dynamic weight-bearing was assessed. However, this method may be considered less sensitive than other evoked pain tests, such as von Frey testing15. It is recommended that more than one method is used to monitor and assess pain. The changes observed 2 weeks after intervention in DCS, even though transient, indicate a generally decreased loading of the OA leg compared to the healthy leg. Therefore, 2 weeks after DCS intervention may be used to evaluate early osteoarthritic or injury pain in mouse models. Visualization of mineralized osteophytes by µCT allows for three-dimensional quantification, which can also be matched to the histological sections12, adding another dimension to the study of osteophyte emergence and evolution. In our group, osteophyte presence was variable in the DMM model between and within operators (2.3 ± 1 vs. 1.2 ± 1, n > 7, P = 0.0183), whereas induction of DCS robustly led to osteophyte generation in all cases irrespective of the operator (2.6 ± 0.7 vs. 2.4 ± 0.5, n > 7, P = 0.711). Also, there are significantly more and larger osteophytes in the DCS model compared to DMM. Thus, DCS is an ideal model for the study of osteophyte formation. Quantification of osteosclerosis limited to the loading area of the subchondral bone is also an improvement in detecting small changes. Comparing the medial compartment of the operated leg to the contralateral leg also offers a way to normalize against the intrinsic bone phenotype of that particular mouse12. The addition of the cartilage scratches in the DCS model is a controlled means of inducing focused cartilage damage during surgery that accelerates many of the aspects of the disease. One of the consequences of the experimental procedure involving intentional damage to the cartilage itself is that this artefactual damage needs to be excluded or adjusted for in the cartilage grading system. Because of this limitation, we do not recommend this model if the study's main aim is to understand the effect of osteoarthritis on the cartilage itself. Finally, it is also strongly recommended to have at least two blinded scorers grade the cartilage damage and synovitis scores. This validates and enhances the standardization of the scoring systems.

A limitation of this study is that the extent of variability across all the parameters comparing the DCS and DMM models was not fully evaluated. This will be addressed in the future with more extensive studies, which could also include an assessment of the variability between operators from different institutions.

In conclusion, the accelerated OA pathogenesis in the current DCS model allows representation of post-traumatic OA and provides a powerful and robust research tool to investigate and elucidate underlying OA pathophysiological mechanisms driving this chronic debilitating joint disease. Additionally, it enables OA to be explored in a shorter time window, focusing on osteophytogenesis, OA pain, and the effect of cartilage damage on the whole joint.

Offenlegungen

The authors have nothing to disclose.

Acknowledgements

We would like to acknowledge the work of Gemma Charlesworth and Mandie Prior at the University of Liverpool, who acquired the µCT images used in this publication. Work was funded by Versus Arthritis (grants 20199 and 22483). Lynette Dunning was funded by Versus Arthritis (grant 20199). Kendal McCulloch was funded by a UWS PhD scholarship. Carmen Huesa was funded by Versus Arthritis (grants 20199 and 22483).

Materials

#11 scalpel blade (and scalpel handle). World precision instruments 500240 access the joint capsule
15° Cutting Angle microsurgical stab knife MSP REF7503 scratch the cartilage
6-0 vicryl rapide Any medical supplies provider alternative method to close wound
Anaesthetic rig Generic (many different suppliers)
Antibacterial skin clenser (Hibiscrub) Amazon To sterilise surgical skin area
Applicator for 7 mm clips World precision instruments 500343 close the wound
Balance Generic (many different suppliers) To weigh mouse
Blunt curved forceps Fine science tools 500232 move the patellar ligament to the side
Buprenorphine (Vetergesic) Supplied by unit as it is a prescription drug Analgesia
CT analyser Bruker 3D.SUITE software Software
Ctvol Bruker 3D.SUITE software Software
Data viewer Bruker 3D.SUITE software Software
Dynamic weight bearing equipment Bioseb BIO-DWB-DUAL Measure limb loading and has cage, pressure matt and software for analysis
EDTA Merck E9884 10% solution in PBS (or water) to decalcify bone pH 7.4
Ethanol Generic (many different suppliers) for embedding decalcified bones
Fast Green FCF Merck F7252 For staining sections
Glacial acetic acid Merck 1005706 For stianing sections
Haematoxylin solution Merck GHS132 Nuclear staining in paraffin sections.
Hoskins #21 micro-tweezers. Cameron surgical limited PHF1085 move the fat pad
Isofluorane Supplied by unit as it is a prescription drug
Mice Charles river C57Bl6/J male 8 weeks old (to allow acclimatisation in the unit)
Microcomputed tomography scanner Bruker SKYSCAN 1272 CMOS µCT
Micropore surgical paper tape FisherScientific 12787597 hold leg in position
Paraffin wax Generic (many different suppliers) for embedding decalcified bones
Reflex 7 mm stainless steel wound clips or Fine science tools 12032-07 close the wound
Remover for 7 mm clips World precision instruments 500347 remove wound clips
Rotary Microtome Generic (many different suppliers) To cut section of Paraffin embedded tissue.
Safranin-O Merck S2255 For staining sections
Serrated curved forceps Fine science tools 15915 hold the skin
Sterile Drape Generic (many different suppliers) To ensure sterility of surgical area
Sterile Drape with key hole Generic (many different suppliers) To cover mouse and expose leg
Sterile saline Generic (many different suppliers)
Sterile surgical drape Generic (many different suppliers) maintain sterile environment for surgical tools
Sterile surgical drape with key hole Generic (many different suppliers) cover the mouse and keep leg through key hole
Straight Scissors World precision instruments 14393 open the wound
Surgical microscope. Generic (many different suppliers) Adjustable focus.
Vannas spring scissors with 2 mm blades. Fine science tools 15000-04 cut the MMTL
Xylene Generic (many different suppliers) for embedding decalcified bones

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Dunning, L., McCulloch, K., Lockhart, J. C., Goodyear, C. S., Huesa, C. Destabilization of the Medial Meniscus and Cartilage Scratch Murine Model of Accelerated Osteoarthritis. J. Vis. Exp. (185), e64159, doi:10.3791/64159 (2022).

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