Taro Matsuzaki1, Shinya Yoshida2, Satoshi Kojima3, Masanori Watanabe4, Masahiro Hoso1. 1. Division of Health Science, Kanazawa University Graduate School of Medical Science, Japan. 2. Kanazawa University Hospital, Japan. 3. Department of Medical Health Science, Kinjo University, Japan. 4. Department of Rehabilitation Science, Nagoya Gakuin University, Japan.
Abstract
[Purpose] The aim of this study was to clarify the effects of the ROM exercise on joint components according to histopathological analysis. [Subjects and Methods] In total, twenty-six 9-week-old adult male Wistar rats were used in this study. The rats were randomly divided into three groups, the immobilization group (n=10), exercise group (n=10), and control group (n=6). The immobilization group and exercise group were anaesthetized and operated on under sterile conditions. The right knee joints in the immobilization group and exercise group were immobilized with external fixation at 120 degrees of flexion. Range of motion exercise was started from the day after immobilization. ROM exercise was performed in the exercise group once a day for 3 minutes, 6 days a week, for 2 weeks. [Result] The joint capsule in the immobilization group and exercise group showed narrowing of the collagen bundles in interstitial spaces but was less dense in the control group. In the immobilized group, a hyperplastic reaction was associated with infiltration into the articular cavity and adhesion to the surface of the articular cartilage. Conversely, in the exercise group, hyperplasia of tissue was localized to the synovial membrane. [Conclusion] This finding may suggest that ROM exercise induces some changes within the joint components and tissue metabolism.
[Purpose] The aim of this study was to clarify the effects of the ROM exercise on joint components according to histopathological analysis. [Subjects and Methods] In total, twenty-six 9-week-old adult male Wistar rats were used in this study. The rats were randomly divided into three groups, the immobilization group (n=10), exercise group (n=10), and control group (n=6). The immobilization group and exercise group were anaesthetized and operated on under sterile conditions. The right knee joints in the immobilization group and exercise group were immobilized with external fixation at 120 degrees of flexion. Range of motion exercise was started from the day after immobilization. ROM exercise was performed in the exercise group once a day for 3 minutes, 6 days a week, for 2 weeks. [Result] The joint capsule in the immobilization group and exercise group showed narrowing of the collagen bundles in interstitial spaces but was less dense in the control group. In the immobilized group, a hyperplastic reaction was associated with infiltration into the articular cavity and adhesion to the surface of the articular cartilage. Conversely, in the exercise group, hyperplasia of tissue was localized to the synovial membrane. [Conclusion] This finding may suggest that ROM exercise induces some changes within the joint components and tissue metabolism.
Entities:
Keywords:
Contracture; Joint immobilization; ROM exercise
Prolonged immobilization reduces passive range of motion of joints, creating joint
contractures1,2,3,4,5,6). This may cause inconveniences with regard to activities of daily
living; thus physiotherapy is often used to treat problems related to joint movement
limitation. In previous studies, we have reported the histopathological changes that occur
in the rat knee joint components during immobilization; however, the changes have not been
fully clarified. In addition, controversies still remain regarding the pathosis of joint
contracture. Joint immobilization induces muscle atrophy, articular cartilage loss, and
proliferation of connective tissue within the joint space1, 7). Immobilization of joints
surrounded by edematous soft tissue often produces joint stiffness more quickly and more
severely than immobilization of nonedematous extremities8). After two weeks of joint immobilization, the number of synoviocytes
in the posterior synovial intima was increased compared with a control group9). Watanabe reported atrophy of fat cells,
proliferation of fibroblasts, and narrowing of the spaces between collagen fibers in the rat
knee joint after immobilization10). Some
studies reported changes in joint components caused by remobilization after
immobilization8, 11,12,13,14,15). The range of motion of rat knees immobilized for 8 weeks remained
substantially reduced after a 4-week period of unassisted remobilization16). But histopathological findings of the
joint components were not described in that study. In the precedent studies,
histopathological changes in joint components after remobilization and/or reloading during
joint contracture were observed. The purpose of these studies was to observe the healing
process. But studies about prevention of joint contracture have not been performed. A few
studies have reported the effect of exercise during an immobilization period17, 18). Tatsuta related that exercise during immobilization periods did not
improve range of motion but also that granulation tissue did not infiltrate into the
articular cavity19). In this study, we
used external fixation in order to immobilize the joint and subjected the rats to exercise
during the immobilization period. Thereafter, we observed the influence of ROM exercise on
the immobilized joint. The purpose of this study was to clarify the effects of the ROM
exercise on joint components according to histopathological analysis.
SUBJECTS AND METHODS
The protocol for these experiments were approved by the Animal Care Committee and
Institutional Ethics Committee of Kanazawa University, and all procedures for animal care
and treatment were performed in accordance with the Guidelines for the Care and Use of
Laboratory Animals at Kanazawa University. In total, twenty-six 9-week-old adult male Wistar
rats (weighing 250–275 g) were used in this study. The rats were randomly divided into three
groups, the immobilization group (n=10), exercise group (n=10), and control group (n=6). The
animals were kept under normal conditions for one week before the start of experiments in
order to acclimatize them to the environment. They were housed, 1 per cage, in a room
maintained under a 12-hour light-dark cycle. Food and water were given ad libitum.The immobilization group and exercise group were anaesthetized (pentobarbital sodium,
40 mg/kg bw, ip) and operated on under sterile conditions. The right knee joints of the rats
in the immobilization group and exercise group were immobilized with external fixation at
120 degrees of flexion. A 2-mm longitudinal incision was made in the right hind thigh skin;
the right femur and tibia were pierced by Kirschner wire with a diameter of 0.8 mm, and the
wire was then bent (Fig. 1). Kirschner wires were fixed outside the wounds in a knee flexion posture with screw
(4 mm diameter) and nuts. The instruments for external fixation weighed 6 to 7 g. The rat’s
knee flexion angle (120 degrees) was determined by the method described in our previous
studys13, 21, 22). This immobilization
method is low cost, and immobilization can be reversed to perform exercise and then
reestablished easily. Although the right hindlimb knee joint was immobilized, the rats were
able to move freely without restriction in their respective cages and had free access to
food and water.
Fig. 1.
The right femur and tibia were pierced by Kirschner wire with a diameter of 0.8 mm,
and the wire was then bent (X-ray).
The right femur and tibia were pierced by Kirschner wire with a diameter of 0.8 mm,
and the wire was then bent (X-ray).Range of motion exercise (ROM Ex) was started from the day after immobilization. ROM Ex was
performed in the exercise group once a day for 3 minutes, 6 days a week, for 2 weeks. ROM Ex
was performed in the left lateral decubitus position under anaesthesia. The mean torque
necessary for the rat to passively extend the knee joint was 1 N, and this value was adopted
as the strength during the ROM Ex. The exercise consisted in 18 cycles of 10 seconds of
exercise (a total of 3 minutes). The exercise time was determinate according to the results
of a preliminary experiment. In the first 5 seconds of the exercise cycle, the rat’s right
hind limb was maintained in 120 degrees of hip flexion, and in the next 5 seconds, the limb
was pulled in the caudal direction with 1 N force applied by a manual force gauge. The ROM
exercise intensity was controlled using a force gauge continuously during the 3 minutes.
After each exercise, the rat knee was re-immobilized by external fixation at 120 degrees of
knee flexion. The control group did not undergo surgery and was not subjected to
exercises.After 2 weeks of intervention, the ROMs of all rat knees (extension limitation) were
measured under anaesthesia. In the rats in the immobilization and exercise groups, the
external fixation was removed, and shortly after the tight hind limbs of the rats were later
pulled with 1 N force in the caudal direction. The knee angles were measured using a
goniometer for human fingers. After angle measurement, the knees of the rats were
re-immobilized at 120 degrees of flexion by external fixation. Later, the rats were
sacrificed by intraperitoneal injection of an overdose of pentobarbital sodium. Immediately
after euthanasia, their right hind limbs were disarticulated and dissected out from the hip
joint for histopathological study. The right knees of the rats were fixed in 10% buffered
formalin and decalcified. After decalcification, they knees were cut in the sagittal plane
at the level of the anterior and posterior cruciate ligament. Following neutralization with
5% sodium sulfate solution, the specimens were fixed, decalcified, and neutralized at 4 °C
for 72 hours. The specimens were embedded in paraffin, sectioned at 3 μm, and mounted on
microscope slides. All sections were stained with hematoxylin and eosin and toluidine blue
stains and used for observation in a histopathological examination. Histopathological
analysis was performed by examining the synovial membrane, the joint capsule, and the joint
cartilage.Knee limitation data were statistically analyzed using IBM SPSS Statistics for Windows
(version 19.0.1, IBM Corp., Armonk, NY, USA). ROM was analyzed using one-factor analysis of
variance (ANOVA) with Bonferroni post-hoc multiple comparisons. A value of p<0.05 was
accepted as statistically significant. All results are reported as mean±SD values.
RESULTS
All animals survived the experimental period. The histopathological analysis showed no
swelling or signs of infection in the knees as a result of the intervention.The mean values of knee ROM (extension limitation angle) were 19.3±3.0 degrees, 77.3±7.4
degrees, and 51.0±4.9 degrees in the control group, immobilization group, and exercise
group, respectively, and each groups showed a statistically significant difference
(p<0.05). The mean body weights were 326.0±8.8 g, 310.6±16.6 g, and 304.5±7.7 g in the
control group, immobilization group, and exercise group, respectively. There were
statistically significant differences (p<0.05) between the control group and other
groups.In the control group, the joint capsule was typically composed of coarse and relatively
loose fibrous connective tissues. The joint capsule in the immobilization group and exercise
group showed narrowing of the collagen bundles in interstitial spaces but was less dense in
the control group (Fig. 2). The surface of the articular cartilage in animals of the control group was smooth,
and the hyaline cartilage was directly exposed to the articular cavity (Fig. 3). Chondrocytes were observed in the outer layer of the joint cartilage. The cartilage
matrix of the hyaline cartilage was stained with toluidine blue. In the immobilized group,
proliferation of granulation-like tissue connecting with synovial tissue was observed. The
articular cartilages were covered with the proliferating tissue composed of fibroblast-like
spindle-shaped cells (Fig. 4). Negative stain of the proliferating tissue areas were illustrated by toluidine blue
stain. Conversely, in the exercise group, hyperplasia of membrane-like tissue was localized
to the synovial membrane, and the infiltration of fibroblast-like spindle-shaped cells was
localized to the articular cavity (Fig. 5). Notably, the presence of erythrocytes that had leaked into the articular cavity was
observed in some exercise group animals (n=6), suggesting the presence of hemorrhage after
ROM Ex.
Fig. 2.
The joint capsule in the control group was typically composed of coarse and
relatively loose fibrous connective tissues, but those in the immobilization group and
exercise group showed narrowing of the collagen bundles of interstitial spaces; the
joint capsule was less dense in the control group. A, control group; B, immobilization
group; C, exercise group. HE stain ×200
Fig. 3.
The surface of the articular cartilage in the control group. The surface of the
articular cartilage was smooth, and the hyaline cartilage was directly exposed to the
articular cavity (A); the cartilage matrix of the hyaline cartilage was stained with
toluidine blue (B). F, femur; T, tibia; M, meniscus. HE stain ×200
Fig. 4.
Hyperplastic tissues infiltrated into the articular cavity and adhered to the
surface of the articular cartilage (white arrow head), and infiltration of vessels
(black arrows) was observed. HE stain (A), toluidine blue stain (B) ×200
Fig. 5.
Hyperplasia of tissue was localized to the meniscus (black arrows), and the surface
of the articular cartilage was smooth (A). HE stain ×100. The cartilage matrix of the
hyaline cartilage was stained with toluidine blue (B). Toluidine blue stain ×200
The joint capsule in the control group was typically composed of coarse and
relatively loose fibrous connective tissues, but those in the immobilization group and
exercise group showed narrowing of the collagen bundles of interstitial spaces; the
joint capsule was less dense in the control group. A, control group; B, immobilization
group; C, exercise group. HE stain ×200The surface of the articular cartilage in the control group. The surface of the
articular cartilage was smooth, and the hyaline cartilage was directly exposed to the
articular cavity (A); the cartilage matrix of the hyaline cartilage was stained with
toluidine blue (B). F, femur; T, tibia; M, meniscus. HE stain ×200Hyperplastic tissues infiltrated into the articular cavity and adhered to the
surface of the articular cartilage (white arrow head), and infiltration of vessels
(black arrows) was observed. HE stain (A), toluidine blue stain (B) ×200Hyperplasia of tissue was localized to the meniscus (black arrows), and the surface
of the articular cartilage was smooth (A). HE stain ×100. The cartilage matrix of the
hyaline cartilage was stained with toluidine blue (B). Toluidine blue stain ×200
DISCUSSION
It is well known that immobilization causes joint contracture and articular cartilage
degeneration. There have been many reports concerning joint components changing after
immobilization. Proliferation of intracapsular connective tissue and the formation of
adhesions are primary responses to limitation of motion5). In this study, we observed the presence of granulation tissue-like
organization and infiltration in the joint cavity after two weeks of knee immobilization in
rats. The cartilage appeared to be more or less confluent with the overlying connective
tissue20). These findings are consistent
with those reported in our previous study21, 22). During the first two weeks of
immobilization, ROM limitation caused damage in the myogenic component, and after two weeks,
the arthrogenic component constituted more than 80% of the total restriction in ROM20). This suggests that in our contracture
model, the myogenic factor was stronger than the arthrogenic factor for ROM limitation. ROM
limitation was significantly decreased by exercise, presumably due to its property that
contributes to the maintenance of muscle extensibility. However, changes were found not only
in the muscular component but also in the joint component. Proliferation of intracapsular
connective tissue and the formation of adhesions are primary responses to limitation of
motion20). In the present study, there
were clearly differences between the immobilization group and the exercise group. Extensive
hyperplasia of fibroblasts was observed in all animals in the immobilization group, but it
was less severe and was focally distributed in the animals in the exercise group. This
finding may suggest that ROM exercise induces some change within the joint components and
tissue metabolism. Connective-tissue proliferation was present in all three of the knees
immobilized for fifteen days, and it was well established at thirty days20). The changes in the joint capsule were
observed from the early period, and there were no important differences between the
immobilized group and exercised group. In our model, we did not observe a significant
influence of exercise on the joint capsule; however we cannot rule out that some changes may
be observe in response to other exercise methods. We observed slight intra-articular
hemorrhage, which indicates that the exercises used in this study might cause laceration of
granulation tissue and adhesion. In this study, it was clarified that ROM Ex maintains range
of motion and reduces the changes in the joint components. But the effective frequency and
strength were not investigated. Therefore, it is necessary to examine several kinds of
frequency and the exercise strength in a future study. A number of studies have performed
remobilization following a joint immobilization period, and some have subjected animals to
exercise during an immobilization period. These reported studies were still controversial.
We necessary to find for effective ROM exercise method.
Authors: Cathryn D Peltz; Joseph J Sarver; Leann M Dourte; Carola C Würgler-Hauri; Gerald R Williams; Louis J Soslowsky Journal: J Orthop Res Date: 2010-07 Impact factor: 3.494
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