Reconstruction of large segmental bone defects in rabbit using the Masquelet technique with α-calcium sulfate hemihydrate

The treatment of large segmental bone defects caused by acute high-energy trauma, tumor destruction or resection after infection remains challenging for most orthopedic and trauma surgeons [1]. The approaches currently used to treat large segmental bone defects including autologous bone graft, vascularized free bone transfer, and the Ilizarov intercalary bone method [2]. Autologous bone graft remains the gold standard treatment for bone defects less than 5 cm because of their osteogenicity, osteoinductivity, and osteoconductivity [3‐5]. Vascularized free bone transfer [6‐8] and the Ilizarov intercalary bone method [9, 10] are used most commonly to treat large segmental bone defects more than 5 cm. However, vascularized free bone transfer is microsurgically demanding. In addition, there are associated with donor site morbidity and a high failure rate [11]. The Ilizarov intercalary bone method is technically demanding, time-consuming, and associates with a high complication rate [12].

The Masquelet technique, an emerging alternative approach first described by Alain Masquelet [13, 14], consists of a two-stage procedure that allows reconstruction of large segmental bone defects of up to 25 cm [15, 16]. In the first stage, the defect is temporarily filled with a polymethyl methacrylate (PMMA) spacer. The spacer serves both a mechanical and a biological role. It gives structural support, hinders fibrous invasion, and importantly, induces a vascularized membrane [17]. The induced membrane has been shown to produce growth factors and osteogenic factors, supporting the differentiation and proliferation of bone mesenchymal stem cells (BMSCs) [18, 19]. Moreover, the induced membrane inhibits soft tissue invasion of the defect, thereby potentially preventing autologous cancellous bone (ACB) resorption [4]. In the second stage, the foreign-body PMMA spacer is removed after 6–8 weeks and the membranous tube is filled with ACB [16, 20]. However, ACB is severely restricted by the scarce supply of donors. In addition, regardless of technique, ACB harvesting can also be associated with complications such as bleeding, hematoma, and infection [21‐23]. For these disadvantageous reasons, the use of bone substitute would be of great interest, such as α-calcium sulfate hemihydrate.

In recent years, α-calcium sulfate hemihydrate (α-CSH), an important class of highly cementitious bone substitute, has been clinically used to treat large bone defect. Excellent biocompatibility, biodegradability, and osteoconductivity of α-CSH biomaterial make it an outstanding bone substitute with properties that are more similar to the autologous bone [24]. Interestingly, it has been found to be potentially osteoinductive like differentiation of BMSCs into osteoblasts [25]. Furthermore, the pH environment and the ion release behavior of α-CSH provide an appropriate microenvironment for bone regeneration [26, 27]. However, the resorption rate of α-CSH is too fast to match the rate of new bone formation.

Based on these studies, we found that the Masquelet technique can produce growth factors and osteogenic factors and protect ACB against degradation. On the other hand, α-CSH is a sufficient bone substitute and has excellent biocompatibility, biodegradability, osteoconductivity, and osteoinductivity. In this study, we hypothesized that by replacing or reducing ACB demanding, the combination of the Masquelet technique and isolated α-CSH or an α-CSH/ACB mix can heal large segmental bone defect, which may represent a promising bone substitute to reduce ACB demands to treat large segmental bone defect.

All surgeries went well, and the rabbits recovered successfully from the operation and remained in good health. The implanted PMMA spacer and α-CSH did not cause any symptoms of infection or inflammation.

Reconstruction of large segmental bone defects remains a difficult challenge for orthopedic and trauma surgeons. Current solutions to manage large segmental bone defects include vascularized bone transfer and the Ilizarov intercalary bone method. However, these approaches have limitations because they are microsurgically and technically demanding. The Masquelet technique with ACB graft is a novel approach allowing reconstruction of large segmental bone defects [15, 29, 30]. Several research have highlighted the advantages of using the Masquelet technique: (1) maintain of ACB volume over time through protection of the ACB against resorption [4]; (2) restraint of the ACB in place [31]; (3) inhibit soft tissue invasion into the defect [18]; (4) produce growth factors and osteogenic factors, supporting the proliferation and differentiation of BMSCs [19, 32]. However, the Masquelet technique has limitations because of the supply of ACB and the complications of donor site [21‐23]. Therefore, the use of bone substitute would be of great interest.

To the best of our knowledge, which is the most appropriate bone substitute remains controversial. Bone substitute must be selected for their properties to optimize bone repair, promote cell survival, proliferation, and differentiation, while exhibiting appropriate degradation rate, mechanical strength, excellent osteoconductivity, and osteoinductivity [33]. α-CSH is an outstanding bone substitute due to its easy availability, good biocompatibility, biodegradability, osteoconductivity, and a long history of use in bone reconstruction [34‐36]. Moreover, it has been found to be potentially osteoinductive-like differentiation of BMSCs into osteoblasts [25]. A probable mechanism by which α-CSH can promote bone regeneration is by maintaining a high concentration of extracellular calcium ions, which is well known to have the effects of promoting osteoblast activity and inhibiting osteoclast activity [37‐39]. However, the resorption rate of α-CSH is too fast to match the rate of new bone formation.

In this study, the combination of the Masquelet technique and isolated α-CSH or an α-CSH/ACB mix was investigated in a rabbit critical-sized defect model as they possessed the combined effects—sufficient supply of α-CSH and low resorption of the Masquelet technique. A practical definition of a critical-sized bone defect was suggested as a segmental bone defect of a length exceeding 2 to 2.5 times the diameter of the affected bone and will not heal spontaneously during the lifetime [17, 40]. To evaluate the optimal alternative solutions, we designed four groups: sham, isolated α-CSH, α-CSH/ACB mix (1:1, w/w), and isolated ACB group. The sham group is the negative control group to confirm that the critical-sized defect cannot heal spontaneously. The isolated ACB group is the positive control group to confirm that the critical-sized defect can heal using isolated ACB grafts. Our results showed that the sham group did not heal spontaneously. The Masquelet technique in conjunction with isolated α-CSH can partially heal critical-sized bone defect, while α-CSH/ACB mix (1:1, w/w) can approximately complete heal critical-sized bone defect. These results demonstrated that the Masquelet technique in conjunction with isolated α-CSH does not have enough capacity to repair a critical-sized defect. The bone repair capacity of α-CSH/ACB mix (1:1, w/w) is similar to isolated ACB (P > 0.05). This suggests that α-CSH can replace at least half of ACB, thus reducing the supply of ACB and the complication of donor site. In a further study, more ratio of α-CSH/ACB mixture should be investigated. In addition, α-CSH or α-CSH/ACB mix can be doped with osteogenic factors like bone morphogenetic protein (BMP) and vascular endothelial growth factor (VEGF) to further improve its ability to promote bone repair.

To further investigate the capacity of new bone formation of α-CSH at a molecular level, we examined the expression levels of ALP and OCN. Osteoblasts play a key role in bone formation [41]. ALP and OCN, known as the most abundant bone matrix enzyme and protein, are preferentially expressed by osteoblasts [42]. Therefore, ALP and OCN are often used as a typical biomarker for bone formation and maturation [43]. Our results showed that the ALP and OCN expression of the α-CSH/ACB mix group were higher than the isolated α-CSH group (P < 0.05) and were similar to the isolated ACB group (P s> 0.05). These results suggest that α-CSH and α-CSH/ACB mix can stimulate ALP and OCN expressions and then improve bone formation. In a further study, the definitive mechanism for stimulating ALP and OCN expression should be investigated.

In the first stage of the Masquelet technique, a PMMA spacer is inserted into the bone defect during surgery. In clinical practices, the spacer is molded in vivo. In this study, the spacer is molded in vitro. There is a shortcoming that the spacer does not completely match the diameter and length of the bone defect, which may affect the stabilization of the spacer and the formation of the induced membrane. In addition, another limitation of this study was the lack of an external fixation or a plate, as rabbit radius is too small to match the size of human external fixation and plate. Instead, a small splint fixation was used to enhance the stabilization of the PMMA spacer at the bone defect.

In the second stage of the Masquelet technique, we used α-CSH granules to fill the membranous tubes. In clinical practice, the shape and size of patients’ defects are highly variable. Standardized granules could fill defects of any size and shape and thus abolish the complex computer-assisted customization [44]. In a further study, which is the optimal size and shape of α-CSH or other bone substitute should be investigated.

In conclusion, this study demonstrates that the Masquelet technique in conjunction with α-CSH/ACB mix (1:1, w/w) can complete repair rabbit critical-sized bone defect. When the amount of ACB is not sufficient in clinical practice, α-CSH might be a promising bone substitute to replace at least half of ACB to repair large segmental bone defect.