Functional Electrical Stimulation as a Safe and Effective Treatment for Equine Epaxial Muscle Spasms: Clinical Evaluations and Histochemical Morphometry of Mitochondria in Muscle Biopsies.

Functional Electrical Stimulation (FES) has been used extensively over several decades to reverse muscle atrophy during rehabilitation for spinal cord injury patients. The benefits of the technology are being expanded into other areas, and FES has been recently utilized for injury rehabilitation and performance enhancement in horses. Six retired horses (age from 10 to 17 yrs) that had been previously used mainly for dressage riding were selected for this study. Clinical evaluation found epaxial muscle spasms in all horses with minimal to no pelvic extension when manually palpated. FES treatments were performed on the sacral/lumbar region 3 times per week for a period of 8 weeks, obtaining a total of 22 treatments per horse. The Modified Ashworth Scale for grading muscle spasms found a one grade improvement after approximately four FES treatments, indicating improved functional movement of the sacral/lumbar region, supporting the evidence by clinical palpations that a reduction in epaxial muscle spasms occurred. Skeletal muscle biopsies Pre and Post FES treatments were obtained from the longissimus lumborum muscle. Cryosections were stained with a Hemotoxylin-Eosin (H-E), and nicotinamide adenine dinucleotide tetrazolium reductase reaction (NADH-TR). The eventual size change of the muscle fibers were evaluated by morphometry in the H-E and NADH-TR stained cryosections, while in the NADH-TR slides the histochemical density and distribution of mitochondria were also determined. The main results of the morphometric analyses were: 1) As expected for the type of FES treatment used in this study, only a couple of horses showed significant increases in mean muscle fiber size when Pre- vs Post-FES biopsies were compared; 2) In the older horses, there were sparse (or many in one horse) very atrophic and angulated muscle fibers in both Pre- and Post-FES samples, whose attributes and distribution suggests that they were denervated due to a distal neuropathy; 3) The hypothesis of generalized FES-induced muscle fiber damage during epaxial muscle training is not supported by our data since: 3.1) Denervated muscle fibers were also present in the Pre-FES biopsies and 3.2) Only one horse presented with several long-term denervated muscles fibers Post-FES; 4) Preliminary data indicate an increased density and distribution of mitochondria in Post-FES biopsies, suggesting that the clinical improvements in the FES treated horses may be related to daily increased muscle contraction and perfusion induced by FES training. In conclusion, FES in horses is a safe treatment that provides clinical improvements in equine epaxial muscle spasms.

Functional Electrical Stimulation (FES) has been used extensively over several decades as an effective means to reduce or reverse muscle atrophy and to obtain some functional recovery by rehabilitation strategies for spinal cord injury patients,[1-5] including those paraplegics with permanent and complete denervation of the legs (complete Conus and Cauda Equina Syndrome).[6-23] The benefits of this technology are being expanded into other areas, and FES has been recently utilized for injury rehabilitation and performance enhancement in horses.[24-27]

The ability of FES to obtain precise, controlled functional movement, when compared to other electrotherapy approaches, is intriguing. FES has the flexibility to obtain minimal movement during the early stages of rehabilitation, as well as more aggressive movement during the later stages. Currently, research is being performed on the use of FES for inducing muscular exercise in populations that are either noncompliant to exercise, or are not physically able to exercise (e.g., balance disruption). In one study to determine the training effect of FES, healthy adults were placed on a training program (29 treatments over 6 wk) to obtain a cardiovascular exercise response without loading the limbs or joints. A treadmill test determined that a significant increase in peak aerobic capacity and quadriceps muscle strength occurred, suggesting that electrical muscle stimulation can be used in sedentary adults to improve physical fitness.[28] An expanding list of studies are indicating that the application of FES on healthy muscle can elicit some of the same metabolic benefits as voluntary muscle active exercise.[29-31]

The purpose of this study was to confirm that FES is an effective and safe means to reduce chronic muscle spasms in the top line of horses. The present study will add objective histological evidence to previous clinical findings,[27] through the evaluation of equine epaxial muscle biopsies harvested before and after 8 weeks of FES treatments.

Material and Methods

Horse demography

Six retired horses were selected for the study and ranged in age from 10-17 years of age (Table 1). The horses had been all clinically evaluated by veterinarians for axial musculoskeletal pathologies and none had been noted. The horses had no known myogenic or neurogenic disorders and had not been tested for those pathologies. The horses had not been ridden for at least 1 year and were not ridden during the study. The horses were placed in a free paddock for self exercise 1-6 hr daily, depending on weather conditions, and were stalled at night. The horses were used mainly for dressage riding and one horse had been used for some driving. All horses were evaluated by the owners and/or trainers as being uncomfortable and tight in the back muscles and difficult to ride, and therefore had been retired from riding. No nutritional or other management changes occurred during the period of the study.

Table 1.

Demography of the horses

Number	Age	Discipline	Breed	Sex
7003	10	Dressage	Holsteiner/Arabian/Saddlebred	Male (Gelding)
7004	13	Dressage	Trakenhner	Female
7005	15	Dressage	Trakenhner	Female
7006	12	Driving/Dressage	Friesian/Arabian/Saddlebred	Female
7007	14	Dressage	Dutch Warmblood	Female
7008	17	Dressage	Trakenhner	Male (Gelding)

Clinical examination of the horses

Clinical examination of the horses found epaxial muscle spasms in all horses, with minimal to no pelvic extension when manually palpated. The Modified Ashworth Scale (MAS) was used to determine the initial level of muscle spasm and to grade the changes observed during the FES treatments (Table 2).[32] The MAS scale is widely used to objectively evaluate the rehabilitation progress for humans, and has been shown to have a 86.7% (p<.001) interrater reliability.[33] The “catch” referred to in the MAS designates the “jerk” felt by the practitioner at the moment the muscle releases to the steady pressure applied to obtain joint movement. A “catch” is not desirable because the movement of the joint should be smooth.

Table 2.

Modified Ashworth Scale for grading muscle spasm. * ROM (range of motion)

Modified Ashworth Scale
Grade	Description
0	No increase in muscle tone
1	Slight increase in muscle tone, manifested by a catch and release or by minimal resistance at the end of the range of motion when the affected part(s) is moved in flexion or extension
1+	Slight increase in muscle tone, manifested by a catch, followed by minimal resistance throughout the remainder (less than half) of the ROM*
2	More marked increase in muscle tone through most of the ROM, but affected part(s) easily moved
3	Considerable increase in muscle tone, passive movement difficult
4	Affected part(s) rigid in flexion or extension

Functional Electrical Stimulation Treatments

FES treatments were performed 3 times per week for a period of 8 weeks, yielding a total of 22 treatments. The first two treatments were given during the initial 24 hours and the remaining treatments were between 2-4 days apart to obtain 3 treatments per week. The first 2 treatments were given within 24 hours to better assist in obtaining an initial reduction in the muscle spasm. The FES system used was a 16-bit digital micro controller and provided a pulsed, biphasic, rectangular waveform at 60Hz, with a 0 net charge (FES310, EquiNew LLC, River Falls, WI, USA). The signal was pulsed at a rate of 2 seconds on and 2 seconds off.

Three channels, with 6 electrodes paired in an astrick design, were used to transfer the signal to the horse for a treatment time of 35 minutes. The electrodes were placed in a pad, which was centered over the biopsy site of each horse. The skin was sponged with water and ultrasound gel was used between the pad and the skin to reduce impedance. The voltage applied to elicit functional movement ranged from 7.6 to 15.8 volts. Twenty-two FES treatments were performed on the epaxial muscles of the horses including the superficial and middle gluteals and the dorsal edge of the biceps femoris muscle. During the FES treatments, the voltage was increased until pelvic extension was obtained. The pelvic extension ranged from approximately 5-15 degrees. Every 7-9 days, the grade of muscle spasm was determined thorough palpation of the epaxial muscles approximately 10 cm ventral to the dorsal spinal processes, together with palpation over the dorsal spinal processes. Three palpations were performed using the clinician’s fingers on both sides of the horse. The same clinician performed all of the palpations and performed all of the grading of the muscle spasms based on the Modified Ashworth Scale for consistency.

Muscle Biopsies

Muscle biopsies were harvested from the longissimus lumborum muscle at the beginning of the study and then approximately 8 weeks later (54 days) at the end of the study. The biopsies were taken approximately 72 hours prior to the first FES treatments and 72 hours after the last FES treatment. Biopsy specimens were obtained on the same side of the horse for both the Pre-FES and Post-FES samples. A 6 mm diameter Bergstrom biopsy needle was used at a depth of 3 cm to obtain the muscle specimens. Two cc of the local anesthetic lidocaine was given subcutaneous and a 1 cm incision was made over the right longissimus lumborum muscle. The pre treatment longissimus lumborum muscle specimens were obtained 20 cm cranial to the tuber sacrale and 3 cm lateral to the midline. The post treatment longissimus lumborum muscle specimens were obtained 18 cm cranial to the tuber sacrale and 3 cm lateral from the midline. Muscle specimens were approximately 2 cm long. One suture was used after the muscle sample was taken and the suture was removed at 10 days. Biopsy specimens were placed on saline moistened gauze in a plastic container and taken on ice to the laboratory within 2 hours of sampling. Fresh muscle samples were frozen in isopentane chilled in liquid nitrogen upon arrival at the laboratory.[34-37] Thick sections of about 10 μm were stained with Hemotoxylin-Eosin (H-E) and nicotinamide adenine dinucleotide tetrazolium reductase reaction (NADH-TR).[38] Hematoxilin-Eosin and NADH-TR stained slides were photographed and morphometry was performed on random-selected fields in the Translational Myology Lab of the Interdepartmental Research Center (CIR-Myo) of the University of Padova, Italy. Muscle fiber size before and after FES was determined in H-E and NADH-TR stained samples as described in Rossini et al. 2002.[8] Quantitative analyses of mitochondrial density and distribution in the myofiber were determined on microphotographs taken at medium magnification (20x) of NADH-TR stained sections. The staining dots were defined well enough to discriminate larger muscle fibers with a low content of stain-dots (Type 2, glycolytic muscle fibers), from the smaller muscle fibers rich in staining (Type 1, oxidative muscle fibers). In the Type 1 oxidative muscle fibers, the stained dots are typically distributed in a central area with a relatively low-density of intermyofibrillar stain dots (similar to those found in the glycolytic muscle fibers), which are distributed at a higher density in a subsarcolemmal coronal area. Furthermore, some of the oxidative muscle fibers will display 3-9 patches of very high-density subsarcolemmal mitochondria. The intensity of the NADH-TR reaction and the presence or absence of the subsarcolemmal ring of high-density mitochondria, can also distinguish oxidative (Type 1) from glycolytic-oxidative (Type 2A) muscle fibers (Fig. 1).

Fig 1.

NADH-TR reaction identifies mitochondria distribution and density in horse muscle biopsies.

A, a typical Type 2, large, glycolytic muscle fiber, low-density mitochondria is depicted; B and D, typical Type 1, smaller, oxidative muscle fibers are depicted; C, beside a typical Type 1 muscle fiber, a typical Type 2A glycolytic-oxidative muscle fibers is present. Arrows point to subsarcolemmal mitochondrial patches. In panel D the circle defines the central intermyofibrillar mitochondrial area. Magnification = 20 X

Statistical Analysis

The observed percentage of change between pre- and post-FES for equine epaxial muscle spasms treatment were analyzed by two-sided t tests and significance was determined at p<0.05.[39-41]

Results

Clinical Analysis

Palpation by the same clinician was used to determine the grade of the muscle spasm during the initial observation before the first FES treatment (Table 3). The spasm grading was based on the Modified Ashworth Scale (Table 2). Improvements were defined as a change in the spasm scale to a lower grade, indicating reduced muscle spasms. These evaluations were performed by palpation of each horse’s back initially before the first FES treatment, and before each subsequent FES treatment.

Table 3.

Initial grading of horse muscle spasms based on Modified Ashworth Score (MAS), treatments required to obtain 1 grade change in MAS and average voltage of all FES treatments

Number	Age	Sex	MAS Initial grade	Tx* to obtain MAS grade change of 1	Average Voltage
7003	10	Male (Gelding)	3	5	12.06
7006	12	Female	3	8	11.3
7004	13	Female	2	5	10.07
7007	14	Female	3	4	12.2
7005	15	Female	3	4	10.7
7008	17	Male (Gelding)	3	6	13.3

*Tx = treatments

The majority of the horses (5/6) were initially rated at Grade 3, indicating a high level of muscle spasm making spinal movement by hand manipulation impossible. A spasm grade of 2 was found in 1 out of the 6 horses, indicating that although muscle tone was greater than normal, some joint movement was possible with manipulation. The number of treatments necessary to change from a grade 3 or 2 to a grade 1 spasm, varied from 4 treatments in two horses, 5 treatments in two horses, 6 treatments in one horse and 8 treatments in one horse (Table 3). A comparison of the average voltage used during the 22-treatment period for each horse are found in Table 3. When the treatment notes were evaluated, there was a clear pattern of increasing acceptance by the horses of a higher voltage, as the treatment period progressed, together with an associated increase in the degree of pelvic movement. The higher the voltage the deeper the electrical field reaches into the muscle tissue.

Histological and histochemical analyses of muscle biopsies

While the majority of the cryosections of muscle biopsies, stained with H-E, presented with the normal aspects of mammal adult muscles, (Fig 2) some samples displayed a higher variability in size than normal. Table 4 shows changes in the overall muscle fiber diameter when Pre- vs Post-FES biopsies are compared. Two of the younger horses presented with an increased muscle fiber size (with one change being significant p<0.05), whereas the other 4 horses had a statistically significant decrease when muscle fiber size means were compared Pre- and Post-FES. The means of the pooled fiber data of all horses shows a 11% decrease in fiber size, which is also statistically significant (p<0.05).

Table 4.

Mean size (diameter, μm) and percentage of change Pre- and Post-FES of equine muscle fibers in cryosections stained by H-E. T test, significance set to p < 0.05. *SD = Standard deviation

HORSE	AGE	Pre-FESSample Mean Fiber Diameter	Post-FESSample Mean Fiber Diameter		Δ%
7003	10	58.59SD*=21.07	61.67SD=22.83		5.26% (p=.1239)
7006	12	65.44SD=18.91	54.18SD=12.80		-17.20% (p<.001)
7004	13	57.18SD=19.66	66.61SD=15.41		16.48% (p<.001)
7007	14	59.57SD=18.28	44.47SD=15.22		-25.35% (p<.001)
7005	15	55.31SD=17.17	40.41SD=17.04		-26.95% (p<.001)
7008	17	63.25SD=18.91	52.17SD=15.41		-17.52% (p<.001)
Total(pooled fibers)		59.38n=1461SD=19.04	52.57n=1643SD=18.51		-11.46% (p<.001)

Morphometry and topography of the NADH-TR stained cryosections were used to identify and count poor-reacting, large, glycolytic muscle fibers (fast-contracting, Type 2B) and highly-reacting, small, oxidative muscle fibers (slow contracting, Type 1) and the intermediate oxidative-glycolytic muscle fibers (fast-contracting Type 2A) (Table 5). The changes in mean muscle fiber size determined by NADH-TR stain (Table 5), when Pre-FES data are compared to Post-FES data, are in agreement with the values obtained in Table 4. As expected, the Type 2B (glycolytic) muscle fibers were substantially larger than the Type 1 (oxidative) muscle fibers. An evaluation of the Type 1 fibers, showed significant changes in mean muscle fiber size (either increases or decreases) in four horses. Type 2 fibers, showed significant changes in mean muscle fiber size (either increases or decreases) in 2 horses with a borderline significance in a third horse. The pooled data for both Type 1 and Type 2 muscle fibers showed significant decreases in mean muscle fiber sizes when Pre-FES fiber size means were compared to Post-FES fiber size means (Table 5). In all horses, and in both the H-E and NADH-TR stained cryosections, there were scanty very small muscle fibers found in the three younger horses, and focal groups of angulated small muscle fibers in the 3 older horses (encircled in Figs. 2, 3 and 4). In addition, the histogram in Fig. 5 shows that denervation is more pronounced in the three older horses as seen by the number of fibers 30 microns in size and smaller, with horse 7005 (15 yr) showing the largest number of Pre-and Post-FES very atrophic (i.e., denervated) muscle fibers. When evaluating the Pre-FES and Post-FES cryosections of horse 7005, these very small, angulated muscle fibers most likely contribute to the smaller Pre-and Post-FES mean muscle fiber sizes for this horse (Table 4). Based on the NADH-TR staining, the mean percentual content of Type 1, oxidative muscle fibers seemed to increase with age at the expense of Type 2, glycolytic muscle fibers (Table 6). When comparing the absolute changes in the percentage of fibers Pre- to Post-FES for all horses, there is no significant difference for both Type 1 or Type 2 muscle fibers (p=0.6442). When an increase in the percentage of Type 1 muscle fibers for one horse increases there is an associated decrease in the Type 2 muscle fibers for that same horse. The percentual content of oxidative muscle fibers, when comparing Pre-FES to post-FES, increases in 3 of the horses, however, one of those values is minimal (0.54%). When comparing the absolute changes in the percentage of fibers Pre- to Post-FES for all horses, there is no significant difference for both Type 1 or Type 2 muscle fibers (p=0.9853). Further, preliminary analyses of the NADH–TR stained cryosections (not shown) suggest a positive effect of FES on the mean mitochondrial density and distribution. The mean mitochondrial density seemed to increase for both NADH-TR high-positive fibers (Type 1, oxidative) and Low positive fibers (Type 2, glycolytic) in the Post-FES muscle fibers when compared to the Pre-FES muscle fibers (Barbara Ravara, personal observation).

Table 5.

Mean size (diameter, μm) and percentage of change Pre- and Post-FES of Type 1 (oxidative) and Type 2 (glycolytic) for equine muscle fibers in cryo sections stained by Mitochondrial NADH-TR. T test, significance set to p < 0.05. * SD = Standard deviation.

Type 1 (oxidative)
Horse	AGE	Pre-FES	Post-FES	Δ%
7003	10	77.36SD*=14.32	62.96SD=17.98	-18.62%(p<0.001)
7006	12	64.41SD=13.17	64.89SD=13.76	0.74%(p=0.830)
7004	13	62.71SD=16.00	72.82SD=17.78	16.13%(p<0.001)
7007	14	64.81SD=22.66	48.86SD=17.62	-24.61%(p<0.001)
7005	15	69.51SD=23.78	65.50SD=14.68	-5.76%(p.223)
7008	17	66.57SD=19.00	55.26SD=16.66	-16.99%(p<0.001)
Total(pooled fibers)		67.06n=482SD=19.26	60.19n=530SD=18.55	-10.25%(p<0.001)
Type 2 (glycolitic)	AGE	Pre-FES	Post-FES	Δ%
7003	10	108.10SD=30.28	84.85SD=21.48	-21.50%(p<0.001)
7006	12	78.71SD=15.72	85.94SD=22.63	9.19%(p=0.0529)
7004	13	83.31SD=19.56	90.37SD=23.53	8.47%(p=.084)
7007	14	90.52SD=22.65	76.10SD=25.05	-15.93%(p=0.016
7005	15	83.33SD=29.71	81.82SD=22.54	-1.81%(p=.782)
7008	17	101.09SD=23.12	79.29SD=16.32	-21.57%(p<0.001)
Total(pooled fibers)		73.94n=714SD=23.81	67.69n=778SD=22.98	-8.45%(p<0.001)

Fig 2.

H-E stain of Pre- (A) and Post- (B) FES muscle biopsies from horse 7003 (10 yr) and 7005 (15 yr). In A and B, arrows point to atrophic, angulated (denervated) muscle fibers. Arrowheads in B point to muscle fiber with central nuclei. Note that B is a magnified image. Bar, 100 μm

Fig 3.

NADH-TR reaction of muscle fibers of Post- (A) and Pre- (B) FES. Circles indicate groups of very atrophic muscle fibers present in the horse 7005 (15 yr). Magnification = 20 x

Fig 4.

A, H-E stain Post-FES, B, NADH-TR reaction Post-FES of muscle fibers harvested from horse 7005 (15 yr). Groups of severely atrophic muscle fibers, whit distribution suggestive of an axonopathy. Magnification = 20 x

Fig 5.

Histogram of contents of severely atrophic denervated muscle fibers versus the horse age

Table 6.

Percentual content of Type 1, oxidative and Type 2, glycolytic muscle fibers in equine muscle biopsies stained by NADH-TR reaction. z test of proportions, significance set to p < 0.05.

Horse	Pre-FES% of Type 1 (oxidative)	Post-FES% of Type 1 (oxidative)	Absolute change in %	p value
7003	58.65%	51.82%	-6.83%	0.3857
7006	60.48%	61.02%	0.54%	1
7004	63.50%	63.36%	-0.14%	1
7007	67.69%	73.96%	6.27%	0.2733
7005	62.20%	64.08%	1.88%	0.8473
7008	71.32%	62.96%	-8.36%	0.1893
Total (pooled fibers)	64.18%	64.01%	-0.17%	0.9853
	Pre-FES % of Type 2 (glycolytic)	Post-FES% of Type 2 (glycolytic)	Absolute change in %	p value
7003	41.35%	48.18%	6.83%	0.3857
7006	39.52%	38.98%	-0.54%	1
7004	36.50%	36.64%	0.14%	1
7007	32.31%	26.04%	-6.27%	0.2733
7005	37.80%	35.92%	-1.88%	0.8473
7008	28.68%	37.04%	8.36%	0.1893
Total (pooled fibers)	35.82%	35.99%	0.17%	0.9853

Discussion.

In this study muscle biopsies were harvested from 6 horses before and after 22 FES treatments over 8 weeks. The horses that were sampled had all been retired from competition due to epaxial muscle spasms and had not been ridden for at least one year. All of the horses had been examined previously by veterinarians and no obvious neuromuscular pathologies were found. At the beginning of the study, all horses were clinically evaluated and the epaxial muscle spasms for each horse were graded based on the Modified Ashworth Score (Table 2). A previous study documenting the use of FES for epaxial muscle spasms, found that an improvement by one grade of muscle spasm happened quickly. Almost 80% (193) of the horses improved by one grade of spasm after 2 treatments, and an additional 14% (33) of the horses showed a change in one grade of spasm after 3 treatments.[27] The horses in this study required an average of 4.3 treatments to achieve a one-grade improvement in muscle spasm. Therefore these horses appeared to have a somewhat higher level of epaxial muscle spasms than the typical population of horses that receive FES treatments.

An evaluation of the H-E stain cryosections found evidence of an overall decrease in the mean size of the muscle fibers Post-FES when compared to Pre-FES mean muscle fiber size (Table 4). Morphometry of the muscle fibers size and type was also performed for the cryosections stained for mitochondrial NADH-TR reaction. This evaluation analyzed the fiber sizes of the smaller Type 1 (oxidative) separate from the larger Type 2 (glycolytic) muscle fibers (Table 5). Quantitative analyses of the NADH-TR cryosections confirmed the H-E stain results showed that there was an overall significant decrease in the mean fiber size of both Type 1 and Type 2 muscle fibers in both Pre- and Post-FES biopsies. However, in both stainings, some of the younger horses in the study (10-13 yr) presented with an increase in muscle fiber diameters.

A decrease in size of muscle fibers are described as an apparently paradoxically effect of electrical muscle stimulation when endurance protocols are applied to the muscle.[42] This reduction in muscle fiber size (physiological in nature) is related to amelioration of the oxygen diffusion from the capillaries to the core of the muscle fibers, when a fast to slow transformation of fiber types is wanted and obtained. FES treatments may, thus, produce in the muscle an increased resistance to fatigue accompanied with related fiber typing changes of the muscle seen initially by the decrease in muscle fiber size noted in this study.

Very small muscle fibers were found in both the Pre-FES and Post-FES muscle biopsies, in both the H-E and NADH-TR stained cryosections and in the majority of horses. These very small muscle fibers were absent or observed rarely in the three youngest horses, which have a mean age of 11 years (7003, 7004 and 7006). The mean age of 16 years of the group of horses (7005, 7007 and 7008) that displayed a large number of “denervated” muscle fibers is not that much older than the mean age of the group of younger horses. However, most sport horses begin to decline in sports performance after the age of 13. Only one horse (7005, 15 yr) had groups of very small muscle fibers Post-FES. In all samples, there were no inflammatory cells infiltrating the tissue surrounding the small, angulated muscle fibers (evidence of absence of inflammatory reaction or myositis). These observations are evidence that there are areas of muscle fiber denervation in both Pre- and Post-FES muscle biopsies. Therefore, the conclusion can be made that these very small muscle fibers are not the result of the FES, otherwise all post FES muscle fiber samples would show a similar level of very small, angulated (denervated) muscle fibers since all the horses were exposed to the same series of FES treatments. Further, in the horse 7005 the severely atrophic muscle fibers are also present in groups suggesting that they are the result of a peripheral nerve disorder. In addition the horse 7005 received one of the lowest average voltage levels of all 6 horses at 10.7 volts. The reason for the appearance of denervated muscle fibers in both Pre-and Post-FES muscle specimens could be a “subclinical” peripheral neuromuscular disorder that resulted in retirement of the horses from competitions due to “being difficult to ride” and/or being “sore in the back”. Indeed, all horses used in this study were retired due to the fact that they were difficult to ride and had consistently sore backs. Some horses had more denervated fibers than others, but all horses were found to have some very small muscle fibers in Pre- and/or Post-FES samples, which were harvested from different areas of the longissimus lumborum muscle. In summary, the fact that there is no generalized FES-induced muscle damage during epaxial muscle FES treatments is supported by our data since: 1) Only one horse (7005, 15 yr) presented with a high numbers of long-term denervated muscles Post-FES; 2) Individual muscle fibers or groups of small-diameter muscle fibers are also present in the Pre-FES biopsies and 3) Angulated myofibers with a diameter of less than 30 microns are taken as denervated myofibers that cannot respond to electrical stimulation, therefore it is not surprising that they remain atrophic.[9,12,15-17] In addition, FES has also been shown to be safe in reducing atrophy and improving muscle strength in even the most fragile muscle tissue, the long-term denervated muscle.[11]

It seems that it is not by chance that the majority of the denervated muscle fibers are present in the Pre-FES biopsies from the older group of horses. Indeed, the histologic features of aging muscle in humans suggest that denervation contributes to atrophy, that immobility accelerates the process, and that routine exercise may protect against loss of motor units and muscle tissue.[29] Based on the NADH-TR staining, the mean percentual content of oxidative muscle fibers seems to increase with age at the expense of glycolytic muscle fibers (Table 6). Most importantly though, when comparing the absolute changes in the percentage of fibers Pre- to Post-FES, there is no significant difference for either Type 1 or Type 2 for any of the horses. Therefore, the FES treatment protocol used in this study does not appear to change the percentage of Type 1 or Type 2 fibers when Pre- and Post-FES data is compared. This suggests, again, that the overall significant decrease in the mean muscle fiber size Post-FES, when compared to Pre-FES, which was noted in both the H-E and NADH-TR stainings, are not enough to change fiber typing. Preliminary data (not reported) suggest a positive effect of FES on mitochondrial density and distribution (Barbara Ravara, personal observation) by the NADH-TR reaction is interesting and worthy of confirmation by additional analyses. These changes in Post-FES muscle biopsies may be related to an increased number of contractions due to the FES stimulation,[43] and to the related increase in blood perfusion in FES treated muscles. This seems to be a retained effect due to the fact that the muscle biopsies were harvested 72 hours after the last stimulation session. The increases in mitochondrial density and distribution could be the result of the adaptive mechanisms of the muscle fibers to the increased number of contractions per week and of the associated increase in muscle perfusion.[6,7]

In conclusion, the present data from the histological evaluation of the equine longissimus lumborum muscle pre and post 22 treatments of FES over a period of 8 weeks shows that: 1) As expected for the type of FES treatment used in this study, only a couple of horses showed significant increases in mean muscle fiber size when Pre- vs Post-FES biopsies were compared; 2) In the older horses, there were sparse (or many in one horse) very atrophic and angulated muscle fibers in both Pre- and Post-FES samples, whose attributes and distribution suggests that they were denervated due to a distal neuropathy; 3) The hypothesis of generalized FES-induced muscle fiber damage during epaxial muscle training is not supported by our data since: 3.1) Denervated muscle fibers were also present in the Pre-FES biopsies and 3.2) Only one horse presented many long-term denervated muscles fibers Post-FES; 4) Preliminary data indicate an increased density and distribution of mitochondria in Post-FES biopsies, suggesting that the clinical improvements in the FES treated horses may be related to daily increased muscle contraction and perfusion induced by FES training. Finally, we stress that FES treatment, as here provided, is a safe rehabilitation strategy in the management of equine epaxial muscle spasms and provides clinical improvements and some structural changes of the muscle tissue at the histological level.