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Summary

This protocol presents an economical and efficient method for quantitative evaluation of bone microarchitecture in a mouse model of osteoporosis by combining Hematoxylin-Eosin (HE) staining and micro-computed tomography (Micro-CT) techniques.

Abstract

Bone microstructure refers to the arrangement and quality of bone tissue at the microscopic level. Understanding the bone microstructure of the skeleton is crucial for gaining insight into the pathophysiology of osteoporosis and improving its treatment. However, handling bone samples can be complex due to their hard and dense properties. Secondly, specialized software makes image processing and analysis difficult. In this protocol, we present a cost-effective and easy-to-use solution for trabecular bone microstructure analysis. Detailed steps and precautions are provided. Micro-CT is a non-destructive three-dimensional (3D) imaging technique that provides high-resolution images of trabecular bone structure. It allows for the objective and quantitative evaluation of bone quality, which is why it is widely regarded as the gold standard method for bone quality assessment. However, histomorphometry remains indispensable as it offers crucial cellular-level parameters, bridging the gap between two-dimensional (2D) and 3D assessments of bone specimens. As for the histologic techniques, we chose to decalcify the bone tissue and then perform traditional paraffin embedding. In summary, combining these two methods can provide more comprehensive and accurate information on bone microstructure.

Introduction

Osteoporosis is a prevalent metabolic bone disease, especially among the elderly, and is associated with an increased risk of fragility fractures. As osteoporosis becomes more common in China1, there will be a growing demand for studying the bone structures of small animals2,3. The previous methods of measuring bone loss rely on the outcomes of two-dimensional dual-energy x-ray absorptiometry. However, this does not capture the changes in the architectural microstructure of the trabecular bone, which is a key factor for skeletal strength4. The microstructure of bone affects its strength, stiffness, and fracture resistance. By comparing bone microarchitecture in normal and pathological states, changes in bone tissue morphology, structure, and function caused by osteoporosis can be identified. This information contributes to the understanding of the development of osteoporosis and its association with other diseases.

Micro-computed tomography (Micro-CT) imaging has recently become a popular technique for bone morphology assessment, where it can provide accurate and comprehensive data on bone structure and density parameters such as bone volume fraction, thickness, and separation5,6. At the same time, the Micro-CT results can be affected by the analysis software7. Different methods of image acquisition, evaluation, and reporting are used by various commercial Micro-CT systems. This inconsistency makes it hard to compare and interpret the results reported by different studies5. Also, it cannot currently replace bone histomorphometry in providing researchers with information on cellular-level parameters in the skeletal system8. Meanwhile, histologic techniques allow direct observation and measurement of the microscopic morphology of bone. Hematoxylin and eosin (HE) staining is a common staining technique used in histology to visualize the general structure of cells and tissues. It is used to identify the presence of bone tissue and its microarchitecture.

This article uses Micro-CT combined with tissue slicing technique (Hematoxylin-Eosin [HE] staining) to collect bone tissue images and perform quantitative analysis of trabecular bone to evaluate the changes of bone microstructure in an osteoporosis mouse model.

Protocol

The animal protocol has been approved by the Animal Ethical Committee of Chengdu University of Traditional Chinese Medicine (Record number: 2020-34). Female C57BL/6J mice (12-week old, n = 14) were divided into two groups randomly, a sham-operated group (Sham group, n = 7) and a model group (OVX group, n = 7). Animals were purchased from a commercial supplier (see Table of Materials). All mice were kept in individual cages at 22-26 °C with 45%-55% humidity, allowed to adapt to their new environment for 1 week, and provided free access to water and diet. All animal experimental studies were conducted at Chengdu University of Traditional Chinese Medicine, and all efforts were made to minimize animal suffering.

1. Animal model preparation

  1. Anesthetize the 12-week-old mouse by intraperitoneal injection with 1.25% Avertin (Tribromoethanol in tert-amyl alcohol, see Table of Materials) at a dosage of 0.02 mL/g. Position the mouse prone on a sterile surgical operating table, and immobilize its limbs by taping them securely.
  2. Use scissors (see Table of Materials) to trim any hair that may affect the surgical operation.
    NOTE: It is recommended to avoid skin damage while preparing the surgical site.
  3. Wash hands thoroughly and put on surgical gloves. Disinfect the mouse's back three times with povidone-iodine (see Table of Materials), and use medical gauze (see Table of Materials) to dry it off.
    NOTE: Be cautious; getting the hair too wet during disinfection may lead to postoperative hypothermia in mice.
  4. Make an incision approximately 0.5-1.0 cm long, located 1 cm away from one-third of the midline of the mouse's back, using a scalpel (see Table of Materials). Gently separate the fascia and cut through the muscle with tissue scissors (see Table of Materials) until the ovary is visible. Ligate the surrounding blood vessels with non-absorbable sutures (see Table of Materials) and remove the ovary.
  5. Rinse the cavity using 0.9% saline solution, then suture the skin, muscle, and fascia separately (see Table of Materials).
  6. Repeat the same sequence of steps on the other side.
  7. Remove peri-ovarian fat of the same size as the ovary, and perform the same surgery procedure mentioned above for the remaining steps to establish the sham-operated model.
  8. Allow a recovery period of 1 week after the surgery. After 8 weeks, osteoporotic mouse models will be successfully established9,10.

2. Micro-CT scanning

  1. Euthanize the mouse by excess CO2 inhalation. Remove as much soft tissue as possible from the mouse femur after euthanasia and obtain a fresh sample for scanning.
    NOTE: While there is no perfect solution for sample preservation, certain steps can be taken to maximize the quality of Micro-CT scan results. Before fixation, take care to remove as much surrounding tissue as possible. Formalin or buffered formalin is the most preferred method of fixation with storage in PBS11,12.
  2. Double-click the micro-CT imaging system software icon on the desktop to start the system (see Table of Materials). Select a sample bed compatible with the sample field of view (FOV) of 18 mm x 18 mm. Load the appropriate sample bed into the machine and close the hatch.
  3. Click the Warm-up button in the Control Panel.
    NOTE: A short warm-up time was required. Do not attempt to open the hatch when X-rays are being generated. Check the X-Ray On light on the front panel and computer monitor to confirm if X-rays are being generated.
  4. Click the Menu button to set a new database, then create a new sample and study.
  5. Select Manual from the Menu drop-down list and enter custom voltage and current values in the Control Panel. Set Voltage (kV) to 90, Current (µA) to 80, Scan Mode to High resolution, 14 min, and FOV (mm) to 18 mm x 18 mm.
    NOTE: Refer to the manual for different micro CT systems to set the appropriate parameters.
  6. Position the bone securely with plastic film in the sample bed. Close the hatch. Ensure that the subject is centered precisely in the X-capture window by pressing the adjustment buttons on the machine.
    NOTE: Adjusting the sample must be slow and gentle to avoid it falling into the machine by accident.
  7. Click the Start button to start the CT scan.

3. CT data analysis

  1. Enter the software (see Table of Materials), and select the data to be analyzed. Click Sub and set Pixel Size to 10 µm. Move and resize the region of interest (ROI) to include the distal femur above the growth plate. Click on Start (see Figure 1).
    NOTE: The subvolume reconstruction pixel size was selected at 10 µm since the thickness of the imaging trabeculae was estimated to be about 20-30 µm based on histological data from previous studies13. If the signal-to-noise ratio is insufficient for data processing, a high-resolution 1 h scan must be performed.
  2. Click the Analysis 3D button to get the resulting 3D reconstruction.
  3. Export the data from the micro-CT system to the computer for analysis.
  4. Import the reconstructed CT data. Click Process > Image Calculator, then click Region Pad > Interactive. Adjust the yellow checkbox to the appropriate ROI.
    NOTE: The region of interest (ROI) begins approximately 540 µm proximal to the growth plate and extends 1600 µm proximally to assess the actual bone metabolism and remodeling.
  5. Select the Bone Microarchitecture Analysis (BMA) add-on (see Table of Materials). Click Segment Cortex and then Segment Trabeculae.
    NOTE: Both trabecular and cortical boneare automatically selected. Normally no manual adjustment is required.
  6. Click on Save Final Object Map and then click Measure Bone to calculate bone morphometric indices.
    ​NOTE: Only relative bone mineral density (BMD) was calculated here since no control was added.

4. Decalcification of bone tissue

  1. Fix the bone specimens in 4% paraformaldehyde (see Table of Materials) for 24 h. Wash the specimens thrice with PBS (see Table of Materials) for 20 min each time.
  2. Rinse the tissue thrice with distilled water for 20 min each time. Transfer the tissue to a decalcification solution containing EDTA (see Table of Materials) and decalcify for 30 days with a weekly solution change until endpoint.
    NOTE: Needle pricking, hand pinching, and clamping are used to terminate decalcification when the bone tissue becomes soft, or there is no sense of resistance when needling. The physical method of detection can cause some damage to the tissue structure, so try to avoid excessive force or repeated testing.
  3. Take the tissue out of the fixative and use a scalpel to trim the tissue in a fume hood. Put the trimmed tissue and the corresponding label in a dehydration box.
  4. Put the dehydration box in a basket and dehydrate it in a tissue processor (see Table of Materials) with gradient alcohol (75% ethanol for 4 h, 85% ethanol for 2 h, 90% ethanol for 2 h, 95% ethanol for 1 h, anhydrous ethanol for 30 min, anhydrous ethanol II for 30 min, xylene I for 5-10 min, xylene II for 5-10 min, wax I for 1 h, wax II for 1 h, wax III for 1 h).
  5. Use an embedding machine (see Table of Materials) to embed the wax-soaked tissue. Pour the melted wax into an embedding box and place the tissue from the dehydration box before the wax hardens.
  6. Orient the tissue according to the embedding surface and attach the corresponding label. Cool on a -20 °C freezing table (see Table of Materials). Remove the wax block from the embedding box after solidifying and trim the wax block as needed (see Table of Materials).
  7. Cut the trimmed wax block into 3 µm thick slides on a microtome (see Table of Materials). Float the slides on 40 °C warm water on a tissue spreading machine (see Table of Materials) to flatten the tissue and scoop them up with a slide.
  8. Bake in a 60 °C oven (see Table of Materials) until the water evaporates and the wax melts. Take out and store at room temperature (RT) for later use.

5. HE staining

  1. Put the slides in xylene I for 20 min, then in xylene II for 20 min. Further, put the slides in anhydrous ethanol I and anhydrous ethanol II for 5 min each, 75% alcohol for 5 min, and then wash the slides with tap water (see Table of Materials).
  2. Incubate in hematoxylin (see Table of Materials) for 3-5 min. Differentiate the specimens with a hydrochloric acid solution (see Table of Materials). Treat the slides with an ammonia solution (see Table of Materials) for bluing, and then wash the slides with water.
  3. Put the slides in 85%, 95% gradient alcohol for dehydration, and stain with eosin solution (see Table of Materials) for 5 min.
  4. Put the slides in anhydrous ethanol I for 5 min, anhydrous ethanol II for 5 min, and anhydrous ethanol III for 5 min. Treat the slides with xylene I for 5 min, xylene II for 5 min, and mount with neutral balsam (see Table of Materials).
  5. Examine each slide under the microscope. Then, choose the representative slices for panoramic scanning (see Table of Materials).
    ​NOTE: At least three consecutive slices are required for each sample. Before panoramic scanning, the slices must be examined under a microscope to ensure that they are complete and clear. Ensure that the bone marrow cavity, cortical bone, and cancellous bone are fully displayed and that different types of bone cells can be seen.

6. HE image analysis

  1. Open HE images with CaseViewer software (see Table of Materials). Select the region of interest (ROI) on the slide, and save it as a color image.
    NOTE: The selection of ROI is consistent with the above-mentioned software.
  2. Open the image in ImageJ (see Table of Materials). Select the Wand tool from the toolbar. Click on the trabecular bone.
  3. Adjust the tolerance and contiguous settings as needed. Go to Image > Adjustments > Black & White and click OK. Repeat the steps for other areas of the bone.
  4. Invert the selection and fill it with white color. Save the image as a mask for analysis (see Figure 2).
    NOTE: For the detailed methodology, refer to the previously published work14.
  5. Open the mask in the analysis software15,16 (see Table of Materials). Run Process > Binary > Make Binary to convert the color image to a binary image.
  6. Use plugin17 (see Table of Materials) in the software to analyze structural parameters: Run Area/Volume Fraction to calculate bone volume to total volume of bone (BV/TV [%])18,19.
    NOTE: This method is applicable for bone trabeculae and bone marrow, filling the entire ROI in the HE images.

Results

Micro-CT analysis
We measured the trabecular microarchitectural parameters in mice from both groups and reported their mean values and SDs in Table 1. The distribution of some parameters (i.e., the ratio of bone volume to total tissue volume, trabecular thickness, trabecular separation) within each group are illustrated in Figure 3.

These results indicate significant differen...

Discussion

Osteoporosis can lead to frequent fractures, which are costly, can cause pain, disability, or even death, and seriously affect the quality of life of patients20. Over the years, the ovariectomy model has been recognized as one of the standard methods for studying osteoporosis21. The most common preclinical animal model for osteoporosis is the ovariectomized (OVX) rat. Despite this, the majority of research into the mechanisms of bone disorders, including osteoporosis, has b...

Disclosures

The authors have nothing to disclose.

Acknowledgements

This work was supported by the Sichuan Provincial Administration of Traditional Chinese Medicine (2021YJ0175) and the Graduate Research Innovation Project of the School of Clinical Medicine (LCYJSKT2023-11), Chengdu University of Traditional Chinese Medicine.

Materials

NameCompanyCatalog NumberComments
4% ParaformaldehydeBiosharpBL539A
Adobe PhotoshopAdobe Inc.
Ammonia SolutionChengdu Kolon Chemical Co., Ltd2021070101
Analyze 12.0AnalyzeDirect, Inc
Anatomical ForcepsJinzhong surgical instrument Co., LtdJ3C030
Anhydrous EthanolChengdu Kolon Chemical Co., Ltd2022070501
Automatic Dyeing MachineThermo scientificVaristain™ Gemini ES
Bone Microarchitecture Analysis Add-onAnalyzeDirect, Inc
C57BL/6J miceSPF (Beijing) Biotechnology Co., Ltd.
Carrier SlidesNantong Mei Wei De Experimental Equipment Co., Ltd220518001
CoverslipsNantong Mei Wei De Experimental Equipment Co.220518001
Decalcification SolutionWuhan Xavier Biotechnology Co., LtdCR2203047
Delicate ScissorsJinzhong surgical instrument Co., LtdZJA010
Embedding box marking machineThermo scientific PrintMate AS
Embedding MachineWuhan Junjie Electronics Co., LtdJB-P5
Fiji: ImageJNational Institutes of Health, USA
Film SealerThermo scientificAutostainer 360
Freezing TableWuhan Junjie Electronics Co., LtdJB-L5
H&E Staining KitLeageneDH0020
Hydrochloric Acid SolutionSichuan Xilong Science Co., Ltd210608
ImageJ2 PluginBoneJ 7.0.16
Medical GauzeShandong Ang Yang Medical Technology Co.
Mersilk 3-0 Silk Braided Non-Absorbable SuturesEthicon, Inc.SA84G
Needle HolderJinzhong surgical instrument Co., LtdJ32010
Neutral BalsamSinopharm Group Chemical Reagent Co., Ltd10004160
OvenShanghai Yiheng Scientific Instruments Co., LtdDHG-9240A
PANNORAMIC Digital Slide Scanners3DHISTECH Ltd. PANNORAMIC DESK/MIDI/250/1000
PBS bufferBiosharpG4202
Povidone-iodine solution 5%Chengdu Yongan Pharmaceutical Co., Ltd
Quantum GX2 microCT Imaging SystemPerkinElmer, Inc.
Rotary MicrotomeThermo scientificHM325
ScalpelQuanzhou Excellence Medical Co., Ltd20170022
Scan & Browse Software3DHISTECH Ltd. CaseViewer2.4
Single-Use Sterile Rubber Surgical GlovesGuangdong Huitong Latex Products Group Co., Ltd22B141EO
Sodium Chloride Solution 0.9%Sichuan Kelun Pharmaceutical Co., Ltd
Sterile Hypodermic Syringes for Single UseShandong Weigao Group Medical Polymer Products  Co., Ltd
Sterile Medical Suture NeedlesShanghai Pudong Jinhuan Medical Products Co., Ltd. PW8068
Tissue ProcessorThermo scientificSTP420 ES
Tissue Spreading and Baking MachineWuhan Junjie Electronics Co., LtdJK-6
TribromoethanolNanjing Aibei Biotechnology Co., LtdM2920
Wax TrimmerWuhan Junjie Electronics Co., LtdJXL-818
XyleneChengdu Kolon Chemical Co., Ltd2022051901

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Trabecular BoneMicroarchitectureOsteoporosisMouse ModelMicro computed TomographyTCMTraditional Chinese MedicineBone MorphologyBone StructureBone DensityBone VolumeFracture ThicknessBone MicrostructureHistomorphometryBone Quality Assessment3D Imaging2D Assessment

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