Functional imaging in muscular diseases.

OBJECTIVE: The development of morphological and functional imaging techniques has improved the diagnosis of muscular disorders.
METHODS: With the use of whole-body magnetic resonance imaging (MRI) the possibility of imaging the entire body has been introduced. In patients with suspected myositis, oedematous and inflammatory changed muscles can be sufficiently depicted and therefore biopsies become more precise.
RESULTS: Functional MR methods visualise different aspects of muscular (patho)physiology: muscular sodium (Na(+)) homeostasis can be monitored with (23)Na MRI; the muscular energy and lipid metabolism can be monitored using (31)P and (1)H MR spectroscopy. (23)Na MRI has reached an acceptable value in the diagnosis and follow-up of patients with muscular Na(+) channelopathies that are characterised by myocellular Na(+) overload and consecutive muscle weakness. Besides MRI, low mechanical index contrast-enhanced ultrasound (CEUS) methods have also been introduced. For evaluation of myositis, CEUS is more efficient in the diagnostic work-up than usual b-mode ultrasound, because CEUS can detect the inflammatory-induced muscular hyperperfusion in acute myositis. Moreover, the arterial perfusion reserve in peripheral arterial disease can be adequately examined using CEUS.
CONCLUSION: Modern muscular imaging techniques offer deeper insights in muscular (patho)physiology than just illustrating unspecific myopathic manifestations like oedematous or lipomatous changes, hypertrophy or atrophy.

Introduction

Various causes, like neurogenic, metabolic, dystrophic or inflammatory mechanisms, as well as muscular channelopathies leading to disorders of the muscle cell membrane, may potentially cause muscular diseases. Although muscular diseases are a heterogeneous group, in most cases of progressive disease, the result is a focal or general muscular weakness. Unfortunately, muscular weakness is a very unspecific symptom that often does not allow conclusions to be drawn about the origin of the paresis. Standard neuromuscular literature suggests that radiological imaging would play only an inferior role because of absent pathognomonic findings [1]. Why does radiological imaging hold such a low significance in the case of muscular diseases? Routine protocols of magnetic resonance imaging (MRI) only show morphology and demonstrate oedematous or lipomatous changes, atrophy or hypertrophy (Fig. 1). However, these morphological changes are not very disease-specific [2-6]. Apparent changes like consecutive muscular haematoma after blunt trauma can be nicely verified, but the huge and heterogeneous group of myopathies based upon different origins cannot be further differentiated because the underlying (patho)physiology is not demonstrated. The following short review introduces examples of modern functional imaging methods for the evaluation of muscular diseases with emphasis on pathophysiological fundamentals.

Fig. 1

Typical pathological changes in muscular tissue shown in standard proton (1H) MRI

Whole-body MRI

Whole-body MRI allows the entire human body to be investigated within one single examination. It is necessary for the patient to be completely covered with coils (Fig. 2a). The examination lasts up to approximately 60 min, but the duration depends on the protocol and sequence design used; for example, turbo-spin-echo and gradient echo sequences require comparatively less time than spin-echo sequences. For the diagnosis of muscular disorders, axial and coronal T1-weighted sequences as well as axial and coronal short-tau inversion recovery (STIR) sequences are useful (Fig. 2b, c). Contrast media are not needed in most cases. One of the main advantages of whole-body MRI in the field of muscular disorders is biopsy targeting: when a biopsy is planned, adequate targets can regularly be found using MRI as oedematous muscular changes, e.g. in suspected dermatositis or polymyositis [7]. The diseases have to be diagnosed quickly, because they can be treated successfully with immunosuppressive therapy, contrary to many other muscular diseases. Unfortunately, they lead to irreversible muscular weakness when the diagnosis is missed. A central problem is that the muscles may be affected focally, and false-negative biopsy findings are found in up to 25% in random biopsies instead of image guidance. Common findings in MRI of an active inflammatory process are oedematous changes of the muscular tissue that can be—more reliably than with clinical examination or electromyography—identified and mapped using whole-body MRI [8, 9]. With a combination of fat-suppressed T2-weighted sequences and T1-weighted sequences, fatty degenerated muscular tissue can be nicely differentiated from oedematous affected muscular tissue as a hint for acute inflammation. These muscle regions showing oedematous changes, which are potentially caused by inflammation, should be targeted. Therefore, biopsy results will be improved when performing biopsy with imaging guidance.

Fig. 2

a Example of a completely covered patient during a whole-body MRI examination. b Whole-body MRI of a 67-year-old patient with sarcoidosis-associated chronic myositis. The arrow clearly shows oedematous changes within the enlarged image of the left fibularis muscle using fat-saturated sequences. c Whole-body MRI of the same patient as in b: standard T1-weighted sequences clearly show lipomatous changes. The arrow within the enlarged image indicates lipomatous degeneration of the right semimembranosus muscle

However, the pathological changes of muscular tissue are less specific. For example, rhabdomyolysis, muscular dystrophy or acute neuromuscular denervation may appear with muscular oedematous changes, too. Generally, oedematous changes give a hint for an acute process, whereas lipomatous degeneration is observed in chronic stages of disease.

Another advantage of whole-body MRI is its potential to show patterns of muscle involvement that are in favour of a specific myopathy. Also, better than with clinical examination, e.g. by using the Medical Research Council (MRC) score for paresis, subtle involvement of muscle groups can be detected [10].

For several forms of cancer, whole-body MRI is regularly used for the detection or control of metastases. For example, in patients with multiple myeloma, metastases involving connective tissue or muscle can regularly be identified (Fig. 3)

Fig. 3

Whole-body MRI of a 45-year-old patient with multiple myeloma. The STIR sequence clearly shows a bone metastasis located in the left os ilium and the perifocal muscular reaction depicted as oedematous changes

23Na MRI

Conventional MRI uses the gyration of protons (1H), basically of water and carbohydrate compounds, for image acquisition. Innovative techniques like 23Na MRI offer the possibility of detecting sodium ions (Na+). In a healthy muscle cell, the Na/K-ATPase moves Na+ out of the cytoplasm and K+ into the cytoplasm and thus contributes to maintaining a constant membrane potential and an Na+ concentration gradient. In healthy tissue, the extracellular sodium concentration ([Na+]ex = 145 mM) is about tenfold higher than the intracellular concentration ([Na+]in = 10–15 mM) [11]. 23Na MRI allows volume- and relaxation-weighted measurements of these Na+ compartments, non-invasively. The membrane potential is necessary to allow for a contraction of muscle cells. Muscular Na+ channels within the cell membrane provide auxiliary control of Na+ homeostasis. In several groups of muscle diseases, the muscular sodium channelopathies, patients are affected from an incomplete inactivation of these muscular Na+ channels. The resulting Na+ leak leads to an inward Na+ current that causes an ongoing depolarisation of muscle fibres and an increase in the intracellular Na+ concentration. This leads to an elevated total Na+ concentration compared with healthy muscle tissue. 23Na MRI is able to non-invasively measure this pathological increase in the Na+ concentration. However, 23Na MRI is associated with several challenges. First, the physical NMR sensitivity of 23Na is only about 9% of the sensitivity of 1H. Considering a 1,000- to 5,000-fold lower in vivo concentration compared with 1H, this leads to an 11,000- to 55,000-fold lower 23Na signal. Second, the 23Na signal in vivo decays bi-exponentially, with a fast (0.5–3.0 ms) and a slow (15–30 ms) component. To measure the total 23Na signal, sequences with ultra-short echo times are necessary [12]. Furthermore, acquisition techniques that combine both short echo times and high signal-to-noise ratio efficiency, such as twisted projection imaging [13] or density-adapted sampling [14] are favourable for 23Na MRI. Moreover, specific hardware and software are needed; for example, double resonant coils that are able to work with the resonance frequency both of sodium nuclei (16.8 MHz at 1.5 Tesla; 78.6 MHz at 7 Tesla) and protons (63.6 MHz at 1.5 Tesla; 300 MHz at 7 Tesla). It is a further challenge to discriminate between the intracellular and extracellular amount of sodium via non-invasive techniques like MRI. Paramagnetic shift reagents allow for a clear separation between intracellular and extracellular sodium [15]. Unfortunately, they cannot be applied in humans because of their toxicity. Current research in 23Na MRI demonstrated the possibility of reducing the signal from extracellular sodium compartments, such as in vasogenic oedema. A 23Na inversion recovery sequence was developed to reduce the 23Na signal received from vasogenic oedema to achieve a weighting of the intracellular 23Na amount [16]. 23Na MRI has effectively achieved value in the radiological management of muscular sodium channel diseases [17, 18]. In the affected patients, an autosomal-dominant bequeathed defect of muscular Na+ channels leads to a pathological Na+ influx that causes intermittent or permanent muscular paresis as well as muscular stiffness (Fig. 4a) [19]. Typical triggers are exposure to cold or ingestion of potassium-rich food. The diseases appear rarely, examples would be hyperkalaemic and hypokalaemic periodic paralysis or paramyotonia congenita. 23Na MRI is able to depict an intracellular muscular sodium accumulation simultaneous to development of muscular paresis or muscular stiffness (Fig. 4b). The sodium accumulation correlates well with the grade of paresis and is reproducible [18, 20]. Additionally, 23Na MRI allows for therapy monitoring; for example, mexiletine reduces myoplasmic sodium overload in patients with paramyotonia congenita. With 23Na MRI, the decrease in myoplasmic Na+ content becomes visible non-invasively. Another example is hypokalaemic periodic paralysis that goes along with intramuscular Na+ accumulation. The sodium overload causes muscle oedema and weakness in these patients, and it now can be treated specifically with acetazolamide [17]. The muscular oedema as well as the muscular weakness will decrease under treatment, and the muscular strength will improve. Recently, the development of 23Na MRI at field strengths of 3–7 Tesla (standard are 1.5-Tesla devices) allows for a more precise quantification of intracellular 23Na homeostasis. In addition, 23Na homeostasis may be examined more precisely in healthy volunteers as well as in patients, because initial findings indicate the high potential of 23Na MRI at 7 Tesla (Fig. 5) [21].

Fig. 4

a In muscular sodium channel diseases, a defective sodium channel within the muscular cell membrane leads to a pathological influx of Na+ after provocation with typical triggers, e.g. exposition to cold. Results are muscular weakness or muscular stiffness. b STIR weighted 1H imaging shows elevated signal in the lower leg muscles of this patient suffering from hypokalaemic periodic paralysis type 1. The intracellular Na+ accumulation can be visualised nicely with 23Na (arrows). Observe the reference tubes: 0.3% NaCl solution in the middle, 0.3% NaCl bound with agarose gel on the left-hand side, 0.6% NaCl solution on the right-hand side

Fig. 5

23Na MRI at 3 T (TE = 0.2 ms) and 7 T (TE = 0.55 ms). Transverse and coronal slices of the lower legs in a healthy volunteer. Observe the significantly improved signal-to-noise ratio at 7 T

31P-magnetic resonance spectroscopy

31P-magnetic resonance (MR) spectroscopy was introduced in the 1980s with the aim of evaluating the energy metabolism of muscular tissue. The phosphorous MR spectrum demonstrates several peaks of specific energy metabolites, like phosphocreatine, that mirrors a typical short-time energy deliverer, as well as anorganic phosphate that is a degradation product [22]. Moreover, adenosine-5′-triphosphate, which is necessary for muscular contraction, as well as phosphodiester, can be extrapolated from the spectrum and quantified (Fig. 6a). When the chemical shift of anorganic phosphate to phosphocreatine is analysed, the intracellular pH value can be calculated. These techniques can be used successfully in vivo during muscular exercise and can depict a decrease in phosphocreatine during physical trials [23]. The technique offers a useful diagnostic tool; for example, in patients suffering from the glycogenosis McArdle’s disease, the muscular glycolysis is disturbed, and the physiological decrease of pH value due to lactate production does not take place. This can reliably be demonstrated in patients with glycogenosis/McArdle’s disease using 31P-MR spectroscopy [24, 25]. Several research groups tried to find a specific pattern using 31P-MR spectroscopy, but the muscular degeneration finally leads to lipomatous conversion and consecutive loss of high-energy phosphates within the spectrum that can finally be observed in all chronic myopathies. Moreover, the cross-sectional area of muscular fibres correlates with the amount of phosphocreatine and adenosine-5′-triphosphate. This correlation makes sense, as both metabolites are necessary for muscular contraction. Further developed 31P-MR spectroscopy-related imaging techniques allow for a spatial illustration of the phosphocreatine signal received and thus a two-dimensional illustration of the muscular energy level [26].

Fig. 6

Typical metabolites in the muscular 31phosphorous MR spectrum (a) and muscular 1H-MR spectrum (b)

Proton (1H) MR spectroscopy

This method delivers the opportunity to quantify intramyocellular lipids [27]. Further interesting metabolites are phosphocreatine, choline as a marker for the rebuilding of the cell membrane, or extramyocellular lipids that are present within the lipomatous intermuscular connection tissue and the subcutis and are regarded as a contaminator of the intramyocellular lipids in a spectrum (Fig. 6b). But intramyocellular lipids show a highly inter-individual variability and it is obvious that different physical conditions of muscles obtain different concentrations of this lipid fraction. Therefore, it sounds a paradox that athletes show a high level of intramyocellular lipids and a high insulin sensitiveness of their muscular tissue. However, the intramyocellular lipids serve as energy donators for the muscular mitochondria. Physical work leads to a decrease in intramyocellular lipids. Interestingly, untrained patients suffering from type-2 diabetes with peripheral muscular insulin resistance show a high level of intramyocellular lipids too [28, 29]. In the end, many parameters influence the level of intramyocellular lipids, e.g. dietary nutrition, sex, gender, body mass index and the oxygen content of tissue. Additionally, modern spectroscopic techniques deliver the possibility of spatially visualising the evaluated resonance peaks with the aid of parametric colour maps. Several groups are researching 13C-MR spectroscopy. The nucleus plays an important part in muscle physiology and pathophysiology [30, 31]. A central problem is that the MRI need special equipment like broadband transmitters and receivers to allow for 13C-MR spectroscopy. Nevertheless, a further development of this technique may be expected in the future.

Blood oxygen level-dependent MRI

Blood oxygen level-dependent (BOLD) MRI mirrors the local ratio of oxyhaemoglobin and deoxyhaemoglobin. T2*-weighted functional MRI sequences are in common use for BOLD MRI. The signal acquisition is based upon susceptibility effects and subsequent MRI signal changes in muscular tissue, caused by the paramagnetic effect of deoxyhaemoglobin. Oxyhaemoglobin, in turn, is diamagnetic. For muscular tissue, in particular, the signal is influenced by the microvascular density, blood flow and volume, and oxygen extraction rate [32-36]. Experiments evaluating the BOLD response of muscular tissue during post-occlusive reactive hyperaemia showed a steep increase in the T2* signal, followed by a non-linear signal decrease. In patients with peripheral arterial disease (PAD), the T2* signal increase during post-occlusive reactive hyperaemia is a lesser step and delayed. Moreover, a significant age-dependent difference in the rate, intensity and recovery of the post-occlusive muscle BOLD signal was revealed [37, 38].

Arterial spin labelling MRI

Arterial spin labelling (ASL) is based upon magnetic labelling of moving blood particles of a certain slice by an inversion pulse at the first step, and read-out of the labelled blood particles during arrival in the slice of interest (for example, the capillary bed) at the second step [39]. Before acquisition of the image with labelled blood particles, an image of the same region without labelled blood particles is acquired and serves as a control. The difference between the labelled and the control image yield the perfusion-weighted image (Fig. 7). The received signal increases linearly proportional to the underlying tissue perfusion [40, 41]. An advantage is the illustration of local perfusion without the need for contrast media. A disadvantage is the comparatively long examination time. The technique has reached a level of clinical acceptance for quantification of muscular perfusion with MRI [39, 41]. Moreover, the development of arterial spin labelling techniques at ultra-high field MRI showed that the signal-to-noise ratio and thus image quality is enhanced with an increase in field strength [42]—which will additionally improve the frequency of clinical implementation.

Fig. 7

Description of arterial spin labelling. Previously inverted magnetisation enters the slice of interest and is exchanged with normal tissue magnetisation. The resulting image intensity is a measure of local tissue perfusion

MR elastography

With MR elastography (MRE) a quantitative measure of mechanical elasticity of tissue and muscles is possible. The technique allows for visualisation of disturbed fibre characteristics due to pathological changes within the tissue. For example, cancer, inflammation and fibrosis may change the local tissue elasticity. Image acquisition obtains several steps. First, shear waves within the examined tissue are generated. Second, the propagation of the induced waves is depicted with MRI. Third, a postprocessing of the depicted shear wave images is performed and quantitative maps of tissue elasticity are produced. For skeletal muscle, several approaches in MRE exist. For example, MRE showed that neuromuscular diseases (i.e. childhood poliomyelitis, spastic and flaccid paraplegia) have an influence on muscle elasticity [43]. Moreover, MRE can be used for quantification of muscle stiffness caused by immobilisation [44] and thus has the potential to visualise effects of rehabilitation in patients with loss of mobility. In conclusion, MRE delivers important information about the local or general fibre physiology and pathology; it can be predicted that MRE will reach a higher level of clinical acceptance in the future.

Diffusion-weighted imaging and diffusion tensor imaging

With diffusion-weighted imaging (DWI) the mobility of water molecules (and therefore the mobility of 1H protons) can be visualised. The fundamental hypothesis is that the mobility of water molecules within diseased tissue (for example, cancer-involved or inflammatory tissue) differs from that of normal tissue. For image acquisition, the spins of 1H protons are activated and the resulting echo is recorded. In diseased tissue with decreased ability of diffusion, the activated 1H protons obtain decreased mobility and thus remain at almost the same place. The result is a high intensity of regions with disturbed diffusion on DWI images. The potential of DWI for brain and stroke imaging has already been well demonstrated [45-47]. Diffusion tensor imaging (DTI) is a further development of DWI, where the direction of diffusion is captured. As a benefit, tractographies, for example, of neuronal structures like nerve fibres, can be reconstructed. Development of DWI and DTI for examination of the musculoskeletal system is still just beginning, but the first results are promising [48, 49]. Physiological and impaired muscle function can be sufficiently examined by using diffusion tensor imaging. As DTI values are related to the state of muscle contraction, the technique allows for a non-invasive measure of muscle elasticity and its capability of contraction [50]. A precise quantification of muscular DTI seems to be reproducible even in different individuals, as age or gender has no effect on water diffusivity values [51]. With an emphasis on in vivo MR tractography, the anatomical structure and micro-architecture of muscle fibres can be visualised [52]. DTI offers the opportunity to qualitatively determine the impacting force vectors. For example, in patients with lateral patellar dislocation, the visualisation of force vectors delivers important information about the static and dynamic constitution of the knee joint [53]. Not only muscles, but also nerves are visualised by functional MRI. Recent research in neuro-imaging attested DTI to be an excellent tool for detecting injuries or entrapments of peripheral nerves and their recovery after trauma [54]. The deranged and recovered micro-architecture of the peripheral nerves itself becomes visible, whereas conventional sequences like STIR only provide secondary information, such as consecutive oedema.

Real-time ultrasound elastography

With ultrasound elastography, the relative tissue rigidness can be visualised. Therefore, the technique allows for a more objective quantification of the findings gained from conventional palpation by the physician. Analogous to the duplex ultrasound, the colour-coded map that mirrors the tissue rigidness is overlaid on the B-mode ultrasound image. The performance of ultrasound elastography for detection of suspicious breast lesions, pancreatic lesions or suspicious lymphatic nodules had been approved before [55-57]. In the case of muscular diseases, ultrasound elastography delivers additional information about the local condition of the muscle, because the local muscle rigidness may be disturbed in several muscular diseases. Moreover, the technique can be used to localise parts of diseased muscle and thus alleviate muscle biopsies.

Contrast-enhanced ultrasound (CEUS)

Usually, B-mode ultrasound is the first practiced and the most frequently used examination to evaluate muscular disorders. The outcome of sports accidents like ruptures of muscular fibres, haematomas, ruptures of ligaments or extrusion can be well demonstrated [58]. The development of ultrasound over the last few years has made it possible to visualise (patho)physiological information about muscular microcirculation. Ultrasound contrast media are stabilised microbubbles that stay within the vasculature and thus can be used to evaluate the capillary muscular perfusion.

Ultrasound contrast media of the first generation consist of microbubbles that are burst with the use of high-energy ultrasound pulses. During the burst, an ultrasound signal is emitted, a so-called stimulated acoustic emission (SAE), and can be received. A disadvantage of first-generation ultrasound contrast media was that an evaluation of local perfusion in real time was not possible. For example, examination during muscular exercise could not be performed.

Second-generation ultrasound contrast media like SonoVue (Bracco Imaging, Milan, Italy) are not destroyed by ultrasound waves but are put into oscillation. Using this technique, increased muscular tissue perfusion in correlation with an increased number of capillaries can be evaluated in real time. For example, endurance-trained athletes obtain an increased muscular tissue perfusion during rest in combination with a high density of capillaries compared with non-trained volunteers. Moreover, the quantified local blood volume within the selected ultrasound slice correlates with the aerobic capacity and with the perfusion evaluated with venous occlusion plethysmography [59]. Also, changes in the micro-circulation of skeletal muscle during isometric exercise have become visible in real time [60]. This information allows for a better understanding of the physiological adaption of skeletal muscle due to physical strain or inflammation, and has the potential to improve exercise testing and prescription. In the case of confirmed dermatomyositis or polymyositis, a significantly higher muscular perfusion compared with healthy volunteers was shown [61]. Additionally, the oedematous muscular changes visible in B-mode ultrasound underline the suspicion of acute myositis. In the case of confirmed polymyositis, immunosuppressive therapy causes an increased muscular strength, a reduction in the creatinine kinase level and decreased muscular perfusion at rest.

Special ultrasound techniques allow for the detection of oscillating microbubbles, separation from muscular tissue and deliver the opportunity to assess muscular tissue perfusion in real time. Depending on the grade of isometric physical exercise, reduced perfusion due to compression of muscular venules can be observed. At the end of physical exercise, an increased ultrasound signal can be detected because of reactive hyperperfusion. These findings showed that the resulting hyperperfusion depended on the grade of muscular exercise [59]. Moreover, the arterial perfusion reserve can be adequately examined with CEUS in combination with transient arterial occlusion. Initial findings showed that the arterial perfusion reserve in patients suffering from PAD is reduced in comparison to that of healthy volunteers (Fig. 8). Further prospective studies are required to evaluate if this technique is sufficient for use in monitoring pro-angiogenic therapy in patients with PAD.

Fig. 8

Examples of typical signal-intensity-over-time curves of the dynamic CEUS examination. a A rapid increase in the measured CEUS signal was observed after release of arterial occlusion in a healthy volunteer, while the time–intensity curve of a patient with peripheral arterial disease (walking distance, 100 m) increased more slowly with a delayed and less high maximum after provocation (b)

Conclusion

Muscular diseases and their pathological features are complex. Ultrasound and MRI allow for much more than a simple evaluation of lipomatous, oedematous, hypertrophic or hypotrophic changes within muscular tissue. Pathophysiological surrogate parameters such as muscular microcirculation, sodium homeostasis, energy and lipid metabolism or muscular tissue elasticity can be examined. We expect a much higher level of acceptance of these new techniques in the near future.