How does intraarticular dexmedetomidine injection effect articular cartilage and synovium? An animal study

No patients were involved.

After obtaining approval from the Animal Experimentations Local Ethics Board of Hacettepe University (approval number: 52338575–47), this study was conducted in accordance with certain binding guidelines (European Union Strategy for the Protection and Welfare of Animals).

We enrolled twenty male Sprague-Dawley rats with a mean age of 12 months and weighing 300–350 g. Rats were obtained commercially from a private source (Kobay A.Ş, Ankara/TURKEY-www.​kobay.​com.​tr). Rats were housed in appropriate pathogen-free conditions at a temperature of 20 °C–24 °C (in separate cages, enough for normal activity). The light cycle was fixed at 12 h (12 h light and 12 h dark). All rats received standard food and water ad libitum.

All rats were anesthetized with an intraperitoneal ketamine (75 mg/kg) injection. Under aseptic conditions, 0.25 ml dexmedetomidine (100 mcg/ml) (group D) was injected into the right knee joint, and 0.25 ml normal saline (the control group, group C) was injected into the left knee joint of the rats. In our previous study, we tested the injection technique and determined the intraarticular injection and the volume of the injection by injecting the same amount (0.25 ml) of methylene blue into both knees of an anesthetized rat [14]. After the injections, postoperative care was provided, and then all the rats were placed in their cages. Four rats from each group were sacrificed under ketamine anesthesia (120 mg/kg intraperitoneally) by cervical dislocation as described in “AVMA Guidelines for the Euthanasia at Animals [15]” on days 1, 2, 7, 14, and 21, and knee joint samples were obtained.

The samples were fixed with 10% buffered formalin for 2 weeks and decalcified in “De Castro” solution for 6 weeks at room temperature as in a previous trial [14]. Routine light microscopy was used to assess the decalcified samples. The decalcified samples were processed for routine light microscopy. Briefly, the samples were dehydrated and embedded in paraffin. Five-micrometer-thick serial sections were cut and stained with hematoxylin–eosin and Masson’s trichrome stains according to standard procedures. The sections were examined under a light microscope (Leica DM 6000B) and photographed with a DFC490 digital camera (Leica, Wentzler, Germany).

The histological evaluation of all the articular/periarticular regions and the synovium was performed by two separate histologists in a blinded manner. A four-point scale was used to grade the inflammatory changes in four fields per section and four sections per knee. The histological sections of the periarticular regions and synovium were examined for edema, neutrophil infiltration and congestion. Inflammatory changes were evaluated according to a four-point scale (0/1/2/3 = normal/mild/moderate/severe). Synovial hyperplasia was scored according to the ranking of synovitis (0: single layer of synovium, 1: two layers of synovium, 2: three layers of synovium, 3: four layers of synovium). The percentage of fibrotic tissue was evaluated in Masson’s trichrome-stained sections of loose joint tissue. Fibrotic tissue < 10% was scored as 0, 10–30% fibrotic tissue as 1, 30–50% fibrotic tissue as 2, and > 50% fibrotic tissue as 3.

Changes in the structure of the joint cartilage were evaluated using a modified Mankin score [16] with four parameters as in a previous trial [16] (Table 1) and were graded according to a five-point scale in a blinded manner [14].

Four knee samples in each group were required to show a difference of 65% in inflammation scores in the first 2 days (power 80%, α = 0.05), as determined from our previous studies [16‐18]. To sacrifice the minimal available number of rats, we decided to use the right knee of each rat as the study group and the left knee as the control group. Using this technique, we also maintained overall homogeneity among the rat groups. As a result, we ended with a total sample size of twenty rats.

Sprague-Dawley rats are widely used in toxicology studies as standard models; however, articular changes in rats may not be directly comparable to those in humans and thus may not reflect the response in humans ¹⁰. On the other hand, the results of our study, which examined the histopathological changes in the cartilage and synovium in healthy rat knees, may not reflect any impact of dexmedetomidine on damaged knee structures or any effect of repetitive administration. In the study by Cheng et al., dexmedetomidine was investigated for its effect on osteoarthritis induced by papain in rat knees, and it was reported that dexmedetomidine improved the damage in cartilage tissue in osteoarthritis [31]. In our study, our primary outcome was not to determine the treatment effect of dexmedetomidine on cartilage tissue but to investigate the safety of this drug in healthy chondrocytes in advance. The lack of a group of rats that had chondroarthritis may be considered a limitation to our study. In the in vitro study conducted by Mancini et al., it was concluded that dexmedetomidine may cause signs of late apoptosis and necrosis at high doses, and the researchers recommended using these high doses with care for intra-articular injection [30]. In our study, we did not use such high doses, and apoptosis and necrosis were not the parameters that we evaluated for the effects of dexmedetomidine on healthy chondrocytes. These parameters may have led to more detailed information about the potential effects of dexmedetomidine on chondrocytes, which may be considered a limitation to our study.

Another major limitation of our study is the small sample size. Although the type II error was acceptable (power 80%) and we used Bonferroni correction to control type I error, a larger sample size would probably be needed to detect a smaller percentage of difference in inflammation between dexmedetomidine and saline. However, this is the first study to examine the histopathological effects of dexmedetomidine on knee joint structures, which is widely used in humans although still not approved for the intraarticular route.

Furthermore, we observed significant sedation in all groups although dexmedetomidine was injected intraarticularly, so a central analgesic effect resulting from systemic absorption cannot be excluded [3]; however, the plasma concentration of the analgesics used was not measured.