Introduction
There have been numerous reports on the use of cultured cells to treat cartilage injuries of the knee. One of the most prominent reports, by Brittberg et al. [
1], is on autologous chondrocyte implantation (ACI). In that work, the authors used monolayer culture to increase the number of chondrocytes from cartilage harvested from healthy non-weight-bearing sites, and then transplanted these cells to repair articular cartilage defects after covering the defects with a periosteal flap with stitches. Although a number of concerns relating to this conventional ACI have been highlighted in subsequent reports, or adverse events after implantation were reported [
2‐
5], it appears that this new surgical technique has now become an established procedure, and excellent results have been reported [
6‐
9]. Recently, the autologous periosteum was replaced by a collagen membrane used as a covering material to avoid some adverse events and the invasion of healthy tissue [
10]. Moreover, options for ACI are already commercially available, and this treatment approach is now considered to have become routine.
Through an assessment of normal chondrocytes cultured three-dimensionally in agarose gel, Benya and Shaffer [
11] found that these cells maintained a cartilage-organizing potential similar to that in living organisms without dedifferentiation, in contrast to the results obtained in a monolayer culture. In addition to showing that cultured chondrocytes in atelocollagen gel maintained their cartilage-organizing potential, we have demonstrated the usefulness of this cultured cartilage in animal experiments [
12,
13]. Based on these studies, we modified the conventional ACI approach using isolated cultured chondrocytes to devise a method for implanting tissue-engineered cartilage using three-dimensional culture in atelocollagen gel [
14]. In short, we performed transplant procedures in 28 knees and conducted follow-ups for at least 25 months, reporting excellent results in 26 knees. Using this technique, we sought to address the potential disadvantages of conventional ACI, such as dedifferentiation in monolayer culture and leakage of chondrocytes. Recently, many types of biodegradable materials have been used as scaffolding to make three-dimensional cultured cartilage [
15‐
17].
Approaches to the clinical evaluation of therapies for knee injury such as ACI include subjective evaluations by patients using various clinical scores. Two of these, the knee injury and osteoarthritis outcome score (KOOS) [
18] and the Lysholm knee score (LKS) [
19], are important indicators for elucidating clinical usefulness. Meanwhile, objective evaluation methods include arthroscopically-guided diagnostic imaging and magnetic resonance imaging (MRI) evaluation. The greatest advantage of MRI evaluation is that it permits noninvasive imaging and evaluation, and a comparison of MRI changes over time is useful. However, since it requires specialized equipment and is burdensome for certain patients, and moreover, since routine evaluation indicators are not especially well established, few reports have been published on MRI changes in the long-term follow-up of patients who have undergone ACI.
With the aim of further establishing the usefulness of tissue-engineered cartilage using atelocollagen, a multicenter study was conducted in 2009 by a group that included the authors, in which cartilage defects of the knee in 27 patients were treated [
20]. This was conducted as a sponsor-initiated clinical study on behalf of a company which focuses solely on regenerative medicine. In short, the study was conducted at six orthopaedic centers that specialize in the treatment of knees. Evaluations of variables such as clinical symptoms and arthroscopic findings revealed improvement according to our original knee-function score, and arthroscopic examination yielded evaluations of normal or nearly normal results in 92 % of knees, demonstrating the usefulness of cultured cartilage grown in three-dimensional culture using atelocollagen.
In contrast to the number of reports on the long-term follow-up of patients with conventional ACI [
6,
7,
21], there are few reports on the long-term follow-up of the fate of three-dimensionally cultured chondrocytes. Furthermore, for the reasons presented above, the literature is silent on longitudinal studies of MRI evaluations. Therefore, for patients who were part of the multicenter study and were then followed up at our centers, we describe in this report a comprehensive investigation of changes over the follow-up duration in these patients’ clinical symptoms and MRI findings for a mean duration of at least 6.2 years after implantation.
Materials and methods
Subjects
The subjects of this investigation were drawn from the 31 patients described in the report published by Tohyama et al
. [
20]. From the 30 patients who were included in the efficacy evaluation set, we recruited those who were available for a 5-year follow-up at two medical institutions in Japan.
The inclusion criteria in the clinical study conducted by Tohyama et al. were as follows: adults aged 20 years or older; patients with full-thickness defects of cartilage in knees caused by trauma, or osteochondritis dissecans (OCD) or osteoarthritis (OA); and patients who had either failed to respond to conventional methods or for whom it was judged that a benefit could not be anticipated. Similarly, the study was conducted with appropriately-selected exclusion criteria such as a history of rheumatoid arthritis and other systemic diseases, or of malignant tumor. Patients were also subjected to intradermal testing to establish that they were not allergic to atelocollagen gel.
From the 30 patients evaluated for efficacy in the above multicenter study in six medical institutions, the present follow-up research was conducted for 18 patients at two centers. We evaluated a total of 14 patients, excluding those who were unable to visit the centers for personal reasons. The mean age of these evaluated patients was 33.1 years (21–52), six being male and eight female. The causes of the osteochondral defects were trauma (11 knees) and osteoarthritis (3 knees), and the mean (±SD) lesion size was 3.4 (±2.7) cm (Table
1). Two patients underwent simultaneous surgical procedures, with concomitant reconstruction of the medial patellofemoral ligament (case nos. 3, 10). Details of the patients are summarized in Table
1.
Table 1
Details of the 14 knee with cartilage defects treated with cultured cartilage transplantation
1 | F | 36 | 152 | 45.0 | Trauma | L | MFC | 1.3 | III | 0 | 11 | 6.7 |
2 | M | 26 | 173 | 74.0 | Trauma | L | LFC | 2.4 | III | 1 | 24 | 6.6 |
3a
| F | 21 | 152 | 42.8 | Trauma | L | Patella | 2.0 | IV | 0 | 60 | 6.4 |
4 | M | 45 | 169 | 87.0 | Trauma | L | MFC | 2.9 | IV | 1 | 12 | 6.3 |
5 | M | 30 | 169 | 52.2 | Trauma | L | MFC | 2.0 | IV | 0 | 3 | 6.1 |
6 | M | 42 | 167 | 74.6 | OA | L | MFC | 2.4 | III | 0 | 24 | 6.1 |
7 | M | 23 | 177 | 75.0 | Trauma | R | MFC | 1.6 | IV | 1 | 3 | 6 |
8 | F | 22 | 168 | 62.0 | Trauma | R | MFC | 3.8 | IV | 0 | 3 | 6.6 |
9 | F | 47 | 160 | 65.0 | OA | R | Patellar fossa | 2.8 | IV | 1 | 9 | 6.3 |
Patella | 1.3 |
MFC | 0.6 |
10a
| F | 21 | 151 | 45.0 | Trauma | L | LFC | 2.0 | IV | 0 | 3 | 6.3 |
11 | M | 40 | 171 | 91.0 | Trauma | R | LFC | 4.9 | IV | 1 | 36 | 6 |
12 | F | 37 | 160 | 59.0 | Trauma | L | Patella | 4.1 | IV | 0 | 3 | 5.9 |
Patellar fossa | 2.9 |
13 | F | 52 | 162 | 82.0 | OA | L | MFC | 11.3 | IV | 0 | 24 | 5.7 |
14 | F | 22 | 171 | 44.0 | Trauma | L | Patella | 4.2 | IV | 1 | 60 | 5.7 |
Preparation of tissue-engineered cartilage
Tissue-engineered cartilage was prepared according to the method described by Ochi et al. In short, approximately 300 mg of normal cartilage was harvested from an unloaded site under arthroscopic guidance from each individual patient and delivered to a facility belonging to Japan Tissue Engineering Co., Ltd. (Gamagori, Japan). All tissue-engineered cartilage used in this multicenter study was prepared at this facility. After arrival at the facility, the patient’s cartilage tissue was processed with collagenase (type XI; Sigma-Aldrich, St. Louis, MO, USA) to produce a suspension of isolated chondrocytes. The medium used for seeding was Dulbecco’s Modified Eagle Medium (DMEM; GIBCO Invitrogen, Carlsbad, CA, USA) supplemented with 10 % fetal bovine serum (FBS) (JRH Biosciences, St. Lenexa, KS, USA) and 20 mg of HEPES buffer (GIBCO Invitrogen).
To perform the three-dimensional culture in atelocollagen, the suspension of isolated chondrocytes in the above medium and atelocollagen (3 % type I collagen; Koken, Tokyo, Japan) were mixed in a 1:4 ratio and then stirred thoroughly to produce a uniform mixture. The mixture of thoroughly-dispersed cells and atelocollagen was added to culture dishes using a special-purpose seeding ring, and the dishes were heated at 37 °C for 1 h to harden the gel.
The medium used for cell culture was DMEM supplemented with 10 % fetal bovine serum (FBS), 50 μg/ml l-ascorbic acid phosphate magnesium salt (Nikko Chemicals, Tokyo, Japan), 50 μg/ml gentamicin sulfate (Schering-Plough, Munich, Germany), 0.25 μg/ml amphotericin B (Bristol-Myers Squibb, New York, NY, USA), and HEPES buffer. FBS was selected in accordance with the requirements of the Standards for Biological Ingredients (notification no. 210 of the Japanese Ministry of Health, Labor and Welfare).
The tissue-engineered cartilage was incubated in an atmosphere of 5 % carbon dioxide and 95 % air at 37 °C. The culture medium, which was well qualified by means such as a sterility test, was changed every 3–4 days. As the cell culture progressed, the collagen became opaque and acquired a certain level of hardness. Furthermore, cell outgrowths were observed from the locations where the gel was attached to the dish, and cells also became visible on the dish surface.
Implantation of cultured cartilage
Chondrocytes were three-dimensionally cultured in atelocollagen gel for 28 days. The atelocollagen gel containing these chondrocytes was used as the tissue-engineered cartilage for grafting. Before being shipped as tissue-engineered cartilage from the culture facility, a suite of quality tests was performed. Briefly, the results of these pre-shipment quality tests consisted of a negative bacterial cultivation test of the medium, a negative membrane filter sterility test, a negative Mycoplasma screening test using polymerase chain reaction (PCR), a negative endotoxin test, the number of viable cells (by microscopic examination to determine cell number) and the viability (with a hemocytometer and Trypan blue staining), cellular outgrowth from the tissue-engineered cartilage, glycosaminoglycan content, and bovine serum albumin content.
A medial or lateral parapatellar arthrotomy was carried out under tourniquet control. The chondral lesion was debrided as far as the normal surrounding cartilage and until subchondral bone was visible. The defect was covered with a sutured periosteal flap taken from the proximal medial tibia. The flap was shaped and sutured to the surrounding rim of normal cartilage with interrupted 5-0 nylon. After suturing half of the border of the flap, the tissue-engineered cartilage was placed in the defect, and the remaining border of the flap was sutured. The joint capsule, retinaculum, and skin were sutured in separate layers. The knee was supported by a lightweight brace. Two weeks after transplantation, continuous passive movement of the joint was begun. Partial weight-bearing was introduced 3 weeks after surgery, and was gradually increased to full weight-bearing with muscle training during the first 8 weeks after surgery.
Multicenter study procedures
As described above, 14 patients treated at two medical institutions were selected as the subjects of this study. Before the study commenced, the ethics committees of each university reviewed and approved the ethical validity of the study. Written informed consent was obtained from all patients, and the rights of the patients were protected. All patients agreed that any results of this study would be published. Patients selected as subjects were asked to visit the appropriate hospital, and MRI scans were obtained after interviews about their clinical findings at that time. Further details of the procedures are provided below.
Evaluation by clinical outcome
To produce a score for clinical symptoms, the interview included questions about symptoms such as motion pain, rest pain, and knee motion, and the Lysholm–Gillquist scores [
19] were determined from the responses. These scores were also converted to a numerical value using our original knee-function score [
20], which is optimized for evaluating the implantation of tissue-engineered cartilage (Table
2).
Table 2
Descriptions of the Lysholm knee score and the original knee function score
Limp | Knee motion pain |
None | 5 | No motion pain | 50 |
Slight or periodic | 3 | Mild motion pain (rare, relieved) | 35 |
Severe and constant | 0 | Moderate motion pain (frequent, limiting) | 20 |
Support | Severe motion pain (constant, not relieved) | 0 |
None | 5 | Rest knee pain |
Stick or crutch needed | 2 | No rest pain | 25 |
Weight-bearing impossible | 0 | Mild rest pain (rare, relieved) | 15 |
Locking | Moderate or severe rest pain (frequent or constant) | 0 |
None | 15 | Range of knee motion |
None, but catching sensation present | 10 | No loss of motion | 25 |
Occasional | 6 | Mild loss of motion (total are ≥90°) | 16 |
Frequent | 2 | Moderate loss of motion (total are <90°) | 8 |
At examination | 0 | Ankylosis | 0 |
Stairs | Total | 100 |
No problem | 10 | |
Slight problem | 6 |
One step at a time | 2 |
Impossible | 0 |
Instability |
Never | 25 |
Rarely during athletic activities | 20 |
Frequently during athletic activities | 15 |
Occasionally during daily activities | 10 |
Often during daily activities | 5 |
Every step | 0 |
Pain |
None | 25 |
Inconstant and slight during strenuous activities | 20 |
Marked during or after walking more than 2 km | 10 |
Marked during or after walking less than 2 km | 5 |
Constant | 0 |
Swelling |
None | 10 |
After strenuous activities | 5 |
After ordinary activities | 2 |
Constant | 0 |
Squatting |
No problem | 5 |
Slight problem | 4 |
Not beyond 90° of knee flexion | 2 |
Impossible | 0 |
Total | 100 |
An evaluation of the clinical course was made by comparing the scores obtained pre-implantation (pre-operation period; PP) and at 1 year post-implantation (evaluation period I; EP I). At each final hospital visit, patients were asked about their clinical symptoms at the time of evaluation [evaluation period II; EP II, 6.2 (5.7~6.7) years post-implantation].
We selected our original knee function score because, in contrast to the Lysholm knee score (LKS), which includes items relevant to evaluating therapeutic efficacy after ligament reconstruction, such as limping and knee stability, our score minimizes the effects of such factors and considers only the effects of cartilage.
We not only inquired into the level of knee loading in daily activities, but also ascertained whether patients had undergone additional surgical interventions since implantation.
Evaluation by MRI
Magnetic resonance imaging was done on a 3.0 T magnet system (Signa EXCITE HD 3T, Signa HDx 3T; GE Healthcare, Little Chalfont, UK). During imaging, the knee was flexed slightly and scans were acquired under proton density-weighted conditions. Coronal and sagittal scans were acquired for the femoral condyle, and axial and sagittal scans for the patellofemoral joint surface.
After imaging, a modified version of the magnetic resonance observation of cartilage repair tissue (MOCART) system [
22,
23] was used to score the extent of cartilage formation at the transplanted site (Table
3). Evaluations were done by an orthopaedic surgeon who was involved in clinical and basic research into cultured cartilage, but was not involved in treating the patients of this study. Multiple defects were evaluated individually, and the worst score was adopted as the patient MOCART score. The modifications were as follows: under the original MOCART method, images were obtained using fast spin echo and 3D-gradient echo-FSE sequences, while we employed a single imaging sequence and scored a maximum of 30 points for items relevant to the signal intensity of the image (in the original method, a total of 30 points, comprising 15 points per item, was used). For the reconstructed region of cartilage visualized on the MRI scans, the height of the formed cartilage, the integration to the border zone, the surface of the repaired tissue, and other variables were evaluated on a score with a maximum score of 100. For these items, we compared scores obtained at three times: pre-implantation (PP), at 1 year post-implantation (EP I), and at the final evaluation time (EP II).
Table 3
Description of the modified MOCART score
Degree of defect repair and defect filling | Complete (on a level with adjacent cartilage) | 20 |
Hypertrophy (over the level of the adjacent cartilage) | 15 |
Incomplete (under the level of the adjacent cartilage: underfilling) | |
>50 % of the adjacent cartilage | 10 |
<50 % of the adjacent cartilage | 5 |
Subchondral bone exposed (complete delamination or dislocation and/or loose body) | 0 |
Integration to border zone | Complete (complete integration with adjacent cartilage) | 15 |
Incomplete (incomplete integration with adjacent cartilage), demarcating border visible (split-like) | 10 |
Defect visible |
<50 % of the length of the repair tissue | 5 |
>50 % of the length of the repair tissue | 0 |
Surface of the repair tissue | Surface intact (lamina splendens intact) | 10 |
Surface damaged (fibrillations, fissures, and ulcerations) |
<50 % of repair tissue depth | 5 |
>50 % of repair tissue depth or total degeneration | 0 |
Structure of the repair tissue | Homogeneous | 5 |
Inhomogeneous or cleft formation | 0 |
Signal intensity of the repair tissue | Isointense | 30 |
Moderately hyperintense | 10 |
Markedly hyperintense | 0 |
Subchondral lamina | Intact | 5 |
Not intact | 0 |
Subchondral bone | Intact | 5 |
Edema, granulation tissue, cysts, sclerosis | 0 |
Adhesions | No | 5 |
Yes | 0 |
Effusion | No effusion | 5 |
Effusion | 0 |
Maximum score | | 100 |
Statistical analysis
To compare the LKS and other clinical scores, as well as the above MRI-related scores, the relationships between the respective scores obtained at PP, EP I, and EP II were statistically analyzed.
Multiple linear regression was used to statistically analyze the evaluations of the LKS and MRI scores, and Wilcoxon’s signed rank test was used to analyze the effects at each evaluation time (PP, EP I, EP II) for the MRI scores. Differences were considered significant at p < 0.05.
Discussion
In this research, we obtained excellent results after implanting three-dimensionally cultured human chondrocytes grown in atelocollagen gel, which were prepared according to the method described by Ochi et al. To date, the findings have suggested that post-implantation formation of cartilage-like tissue is excellent, similar to the results obtained for autologous cartilage implantation (ACI) prepared in monolayer culture, as described by Brittberg et al
. [
1], although the histological findings of the repaired tissues were not examined in the present study to avoid damaging the repaired tissues. Furthermore, during our 6-year post-implantation evaluation period, no patients required further surgery. According to the comparative evaluation by Knutsen et al. [
3], further surgery was required in 23 % of patients at 60 months after both ACI and microfracture treatment. During follow-up to 37 months described by Saris et al. [
24], further surgery was required in 3.9 % of patients receiving characterized chondrocyte implants and 11.5 % of patients receiving microfracture surgery. Given these published results, it is clear that the results of long-term follow-up for our method were excellent, and compare favorably to those in previous reports on ACI.
By contrast, post-approval surveillance data for ACI in the United States show that adverse events were reported in 294 patients (497 events) in the period from 1996 to 2003. The most common adverse event was graft failure, reported in 73 patients (24.8 %), followed by delamination in 65 patients (22.1 %), tissue hypertrophy in 52 patients (17.7 %), and local infection in 21 patients (7.1 %) [
5]. As there was no record of the total number of implantations, the incidence of adverse events cannot be calculated. Nevertheless, the adverse events that occurred were mainly associated with delamination or hypertrophy, and while the number of events was low, infection was also reported. In the report by Peterson et al. [
21] describing research in which 94 patients were followed for 2–9 years after undergoing ACI, similar results were also obtained, with hypertrophy reported in 26 patients (27.6 %) and graft failure in 7 patients (7.4 %). In the earlier report of our research results, graft failure was reported in 2 of 31 subjects up to 1 year post-implantation. Of these 2 cases of graft failure, excessive flexion was forced in 1 case, and a hypertrophied portion became delaminated in the other. These findings were similar to many other case reports. Fortunately, transient pain was subsequently reported by only 2 patients up to the end of the present evaluation period, no patients required revision surgery during our follow-up, and no obvious adverse events were reported.
Usually, when evaluating treatment methods such as those described in this report, it is preferable to conduct a comparative study such as a randomized controlled trial (RCT). A number of reports describe efficacy evaluations of ACI made via RCTs [
24,
25]. Unfortunately, for reasons associated with health insurance and other considerations, it would be difficult to conduct a complete RCT in Japan, and we were also unable to use such a design in the present clinical study. In brief, the reasons for not conducting an RCT included the following key ethical concerns. (1) Because implantation of tissue-engineered cartilage involves tissue being harvested for culture, it necessitates a different protocol from that of microfracture surgery alone, and the element of blinding is therefore lost. (2) Post-implantation follow-up would also require unnecessary arthroscopic examination to be conducted routinely in the control group of patients. (3) Patients who are seeking treatment with tissue-engineered cartilage would not be able to receive their desired treatment. (4) Minas et al. [
26] reported problems with the prognosis for patients who were scheduled to undergo ACI if they had already received microfracture surgery beforehand. Hence, by using an MRI evaluation (given its relatively low level of invasiveness) in this study, we sought to ascertain the superiority of the treatment by observing changes from 1 to 6 years post-implantation, in addition to long-term follow-up for 6 years.
Quantifying joint cartilage defects or the state of their repair is difficult with MRI scans, and there have been almost no routinely established methods. To address this situation, Domayer et al. proposed a scoring system (MOCART score) that aimed to produce an objective evaluation using MRI scans [
23]. Their method encompasses a comprehensive point score for examining MRI scans in post-implantation evaluation of repaired cartilage. This scoring system includes the height and signal intensity of the repaired cartilage, the state of integration with the surrounding tissue, the condition of the surface, and the state of formation of subchondral bone, which we believed was also the most appropriate indicator in our research. However, since an MRI imaging procedure for obtaining all of these evaluations was unavailable at the start of our study, we modified the method to comprise one type of imaging sequence to assess the signal intensity of the repair tissue.
As previously noted, our research is a comparison of the conditions at 1 year and 6 years post-implantation against that before implantation. Hence, as mentioned above, we were unable to use the results of our research to directly determine its superiority over other treatment methods. However, we were able to obtain findings that were not seen in earlier reports, such as temporal changes in MRI findings at each evaluation visit. The statistical analysis revealed no significant differences between the MRI findings at 1 year post-implantation and those at 6 years post-implantation, suggesting that the therapeutic benefit had been maintained. Although there were no statistically significant differences between the MOCART scores in EP I and EP II, we found a tendency for the scores to improve. Of course, we cannot draw any definitive conclusions from this study alone, and there is the possibility that this may be a characteristic of tissue-engineered cartilage implantation, because its condition after conventional cartilage repair procedure is anticipated to worsen. We definitely need more patients with a longer follow-up in the future to clarify this issue.
It could be claimed that the number of patients was not especially large and that the follow-up period was relatively short in the present study. Moreover, a retrospective approach was used for the MOCART score. Since the images required for the original method were unavailable, it was not possible to faithfully adhere to the original method, and hence a modified method was employed. To further improve the technique of implantation of tissue-engineered cartilage, it will now be necessary to accumulate more cases, and to conduct comparative analyses of variables such as MRI findings and various patient characteristics, severity of disease, and post-implantation management.
In our study, no patients required revision surgery after implantation, and the therapeutic outcomes were relatively stable from 1 year to about 6 years after implantation. These results could be attributed to the fact that the surgeons involved in the diagnosis and surgical procedure were well versed in this treatment method, and that the conditions of the operative procedure were adequately controlled. Moreover, the tissue-engineered cartilage used in our study was prepared at a rigorously controlled cell processing center, and was only supplied to the study after assuring quality via post-culture tests. To achieve clearance in relation to various biohazards and to minimize immunogenicity, a recommended rinsing step with residual serum was performed and a specified value for bovine serum albumin was imposed to assure safety. Moreover, standards for glycosaminoglycans (GAG) and type II collagen as well as the viable cell rate together with other variables were also used to assure efficacy. Under this control framework, the implanted tissue used in this research met all of the predetermined specification values. To stabilize the clinical outcomes achieved using this cultured cartilage in the future, it will be critically important to not only improve the surgical techniques and diagnostic capability of the surgeons and the safety of the cultured tissue used in implantation, but also to identify the efficacy parameters that can be used to establish performance.
In conclusion, although some patients showed deteriorations in their Lysholm and original knee scores between 1 year post-implantation and the final follow-up, we confirmed that the average clinical scores and MRI findings after implantation of tissue-engineered cartilage were improved at 1 year after implantation and were maintained until 6 years after implantation, indicating that our procedure has mid-term longevity.