Efficacy of Carcass Electrical Stimulation in Meat Quality Enhancement: A Review

Article information

Asian-Australas J Anim Sci. 2014;27(3):447-456
1Department of Animal Science, Faculty of Agriculture, Universiti Putra Malaysia, 43400 UPM Serdang, Selangor D.E., Malaysia
2Halal Products Research Institute, Universiti Putra Malaysia, 43400 UPM Serdang, Selangor D.E., Malaysia.
3Department of Animal Production, University of Ilorin, PMB 1515, Ilorin Nigeria.
*Corresponding Author: Awis Qurni Sazili. Tel: +60-3-89474870, Fax: +60-3-89381024, E-mail: awisqurni@gmail.com
Received 2013 August 01; Revised 2013 November 01; Accepted 2013 October 09.

Abstract

The use of electrical stimulation (ES) as a management tool to improve meat quality and efficiency of meat processing is reviewed. The basis of the efficacy of ES is its ability to fast track postmortem glycolysis, which in turn stimulates myriad histological, physical, biochemical, biophysical and physiological changes in the postmortem muscle. Electrical stimulation hastens the onset and resolution of rigor mortis thereby reducing processing time and labor and plays a vital role in improving meat tenderness and other meat quality traits. However, ES may have negative impacts on some meat quality traits such as color stability and water holding capacity in some animals. Electrical stimulation is not an end in itself. In order to achieve the desired benefits from its application, the technique must be properly used in conjunction with various intricate antemortem, perimortem and postmortem management practices. Despite extensive research on ES, the fundamental mechanisms and the appropriate commercial applications remained obscured. In addition, muscles differ in their response to ES. Thus, elementary knowledge of the various alterations with respect to muscle type is needed in order to optimize the effectiveness of ES in the improvement of meat quality.

INTRODUCTION

Changing trends in the meat industry are crucial factors influencing various interventions to improve or maintain product quality. Recently, the meat industry has transformed from commodity-based to consumer-driven (Troy, 2006). Nowadays, consumers demand convenience, health, safety, taste, uniformity, nutritive value, good appearance and variety of meat and meat products. The need to satisfy consumers’ demand necessitates improved research and product development. At postmortem, one of the major interventions adopted in the meat industry for enhancing meat quality traits is carcass electrical stimulation (ES), a practice whereby an electric current is transmitted through the carcass of animals that are freshly slaughtered and eviscerated. In the course of postmortem glycolysis, the muscle undergoes rigor development marked by series of histological, physical and biochemical processes. Therefore, modification of one or more of the processes could eventually alter meat quality traits. The need to curb variability in meat quality traits and to enhance sensory properties of meat necessitate the application of ES. However, it must be realized that the beneficial effects of ES can only be achieved if there is sufficient muscle glycogen before an animal is exsanguinated. This is evident from the study conducted by Dutson et al. (1982) which showed that ES does not affect postmortem pH, color, tenderness and other sensory traits in ante-mortem stressed beef. There are discrepancies among various reports on the influence of ES on meat quality. While some authors reported positive effects (Mckenna et al., 2003; Cetin and Topcu, 2009; Nazli et al., 2010), others reported no effect (Wiklund et al., 2001; Botha et al., 2009; Kim et al., 2013) or in some cases deleterious effects (Hector et al., 1992; den Hertog-Meischke et al., 1997; Simmons et al., 2008) of ES on meat quality. These ostensible paradoxes have not been fully resolved in spite of partial insights given by recent reports. Because of this, there is a need to appraise various reports with a view to create a balance in the effective application of ES to optimize meat quality and other merits. Thus, the objective of this review was to assess the roles and applications of ES as a management tool in meat quality enhancement.

Brief history of electrical stimulation

In 1749, Benjamin Franklin discovered that the flesh of the turkey was tenderized on applying ES shortly postmortem (Lawrie and Ledward, 2006). Some studies had been conducted on ES in the United States during the 1940s. However, such studies failed to yield significant success (Mota-Rojas et al., 2012). Significant application of ES for meat processing took place in the 1950s (Sams, 1999). Thereafter, Harsham and Deatherage filed a patent in 1951 for meat tenderization using ES (Troy, 2006). Harsham and Deatherage (1951) reported that the main effect of ES is to hasten postmortem glycolysis and the basic goal is to swiftly reduce postmortem pH. ES was commercially used in early 1970s to preclude cold shortening and thus enhance meat tenderness (Juarez et al., 2012). The procedure has been commercially used in various livestock to improve tenderness and other meat quality traits. Electrical stimulation regarded as a step in modifying meat quality traits, has been reported to improve meat sensory properties such as color (Taylor and Martoccia, 1995; Mckenna et al., 2003; Cetin and Topcu, 2009; Nazli et al., 2010), tenderness, flavor and odor (Soria and Corva, 2004; Castaneda et al., 2005; Mota-Rojas et al., 2012).

Types of electrical stimulation

Presently, there are three major types of ES. These are the extra low-voltage electrical stimulation (ELVES), low-voltage electrical stimulation (LVES) and high-voltage electrical stimulation (HVES). The ELVES is carried out at voltage of <100 V while HVES is carried out at >110 V. Low voltage electrical stimulation is carried out between 100–110 V and is often regarded as medium-voltage electrical stimulation (MVES). For the purpose of simplicity, two major types of ES (low and high) are often used in most literature with clear definition of the voltage applied. Except the voltage which is somewhat fixed for the major types of ES, high variability exists in the amperage, impulse frequency, duration of application, type and position of electrode, pathways (through direct or nerve) and delay time between slaughtering and stimulation. The variability in the aforementioned factors accounts for discrepancies in reports regarding the efficacy of ES. In addition, variation in reports could be due to differences in animal age, species, breed, management and handling. Both ES methods yield effective stimulation and have merits and demerits. The ideal method depends on the cost, type of animal, existing slaughter floor restraints and throughput.

Low voltage electrical stimulation is mostly used when there is short delay time (10 to 20 min) between bleeding and stimulation. It is often applied before de-hiding (up to 10 min after bleeding) in compliance with the time constraint. The initial cost is very low and it is safer in the work place. The major demerit of LVES is that it is labor intensive since the electrode needs to be manually applied. Although, LVES is safer, its consistency in effect is lesser than HVES (500–1,000 V or more) (Bendall, 1980; Bouton et al., 1980). High voltage electrical stimulation gives room for longer delay time between bleeding and stimulation (up to 60 min after exsanguination). However, it requires huge capital outlay and adequate precaution needs to be taken to ensure the safety of workers. Hwang and Thompson (2001) reported that irrespective of the type of voltage used, when ES is applied to a carcass at about 3 min postmortem, its tenderizing effect would be relatively less than when it is applied at about 40 min postmortem. The authors attributed this to the initial reduction in calpain activity immediately after slaughter. Contrarily, Bendall (1976) suggested that the response of bovine to ES decreases significantly after 50 min postmortem and sooner for lamb carcass. The authors concluded that it is ideal to carry out ES at about 30 min after bleeding. However, in recent time, carcasses are often subject to ES immediately after postmortem. This has been reported to aid bleeding and enhance meat tenderness (MLA and AMPC, 2011).

Mckeith et al. (1981) compared the effectiveness of HVES and LVES at different periods using a total of 390 calves and young bullocks. Carcasses were stimulated at 5 min after exsanguination, 20 and 30 min after evisceration. Carcasses were subjected to 550 V or 150 V for 1 or 2 min at 16 pulses/min and compared against non-stimulated ones and the impulses took place for 1.8 s with an interval of 1.8 s between them. The result showed no improvement for flavor when ES was applied for 1 or 2 min. Nevertheless, carcasses stimulated with 550 V had more tender, brightly colored, better flavored and leaner meat than those stimulated with 150 V. It was concluded that HVES (550 V) and short time (1 min) is ideal for improvement of meat palatability. The report of Roeber et al. (2000) revealed that duration and voltage intensity of ES affected beef color and tenderness. The right halves of beef carcasses were stimulated while the left halves were non-stimulated. High voltage (HV) (300 V) was compared against medium voltage (MV) (100 V). High duration (HD) (16 cps) and medium duration (MD) (11 cps) at 60 Hz were also compared. The result showed that all ES treatments yielded more tender and brighter colored beef than non-stimulated sides. For carcasses whose non-stimulated sides had Warner-Bratzler Shear (WBS) values higher than 4.5 kg, corresponding sides treated with HVHD, HVMD, MVHD, and MVMD had shear force values less than 4.5 kg at 60%, 75%, 88%, and 50% of the time, respectively. Morton and Newbold (1982) reported that time taken for postmortem ATP to decline to half of the initial control in sheep was about 20 min, 2 to 3 h and 5 to 6 h in the HVES (240 V, 14.3 s−1, 10 ms, 50 Hz), LVES (45 V, 14.3 s−1,10 ms, 50 Hz) and the control carcasses, respectively.

Practical application of ES

Recently, ES is often used for other purposes in addition to meat quality improvement. In some abattoirs especially in Australia and New Zealand, ES is applied immediately after stunning before slaughtering, immediately after slaughter and/or during de-hiding. When applied after stunning prior slaughtering, it is aimed at ensuring occupational health (workers’ safety) to prevent shaking of the hind legs when the animal is being exsanguinated. Electrical stimulation applied immediately after slaughter is aimed at increasing the efficiency of bleeding out and to promote blood collection (Craig et al., 1999; MLA and AMPC, 2011). This procedure has been reported to enhance tenderness because the low voltage ES reduces muscle ATP, making it unavailable for muscle contraction during cold storage. In addition, depletion of ATP by ES could lower the frozen storage time necessary to deplete ATP. When applied during de-hiding (especially when a downward hide puller is used) it is aimed at stiffening the animal’s backbone to prevent breakage of spinal cord (MLA and AMPC, 2011). However, it is recommended to reduce all forms of ES on carcasses to prevent heat toughening which could occur during pre-rigor due to rapid decline in muscle pH while muscle temperature is still high (MLA and AMPC, 2011).

In evaluating the efficacy of ES, it is necessary to realize that concurrently with the need to improve meat quality and the efficiency of abattoir operations, there is increasing propensity for abattoirs to engage in integrated preparation of prepackaged cuts (Lawrie and Ledward, 2006). This is due to the rapidly changing consumption patterns that necessitate individual smaller cuts. In addition, hot carcass deboning followed by vacuum packaging of the warm cuts further substantiates the propensities all of which lower exudative and evaporative losses. Given the relatively small proportions of individual cuts, it might be useful to electrically stimulate the cuts or whole carcass to avoid cold shortening since the former would readily be induced under the high rate of cooling accompanying them. Rapid cooling of carcass lowers microbial proliferation, which could occur especially in individual cuts having large surface to volume ratio. Although, cold shortening is prevented, these conditions could avert the tenderizing effect of ES by creating conditions (in vivo temperature and low pH) favorable for quick conditioning. The aforementioned problem could be solved by subjecting various joints or cuts to different cooling regimes following their removal from hot carcass. However, this is somewhat complicated considering the complex nature of muscles and variation in their response to ES and conditioning processes. Different muscles in carcass differ in their rate of cooling. Muscles close to the surface of carcass chill quickly since they have low depth. Conversely, deep muscles situated in the centre of carcass chill more slowly. Thus, it can be inferred that efficacy of ES depends on the nature and duration of cold storage after stimulation. This corroborates the report of Wiklund et al. (2001) who studied the effect of ES on red venison. Their result indicated that through the prevention of cold shortening, ES improved the tenderness of stimulated carcasses compared to non-stimulated ones. However, the tenderizing effect of ES was lost during subsequent ageing at −1.5°C. This implied that ES is not beneficial for products stored for long term at chill temperature.

In some tropical countries, hot deboning could expose the meat to a temperature of 30°C to 40°C. Under this condition, during the onset of rigor mortis, early muscle excision could cause contraction and toughening (Locker et al., 1985). Thus, assessing the effect of ES in such situations will be of prime interest. Babiker and Lawrie (1983) reported that when exposed to temperature of 30°C to 40°C, bovine Longissimus dorsi M. exhibited pronounced tenderness compared to non-stimulated ones. However, at 40°C and in contrast to the observations at 30°C, there was intense loss of water holding capacity accompanied with marked microbial proliferation; besides, the tenderness of electrically stimulated samples decrease proportionately. This observation inferred that the favorable effects of high temperature in enhancing proteolysis were overshadowed by increased protein degradation of the enzymes responsible for the breakdown of proteins.

Role of ES on postmortem glycolysis

The mode of action of ES lies on its ability to accelerate postmortem glycolysis resulting in pH decline via rapid depletion of muscle glycogen (Hwang et al., 2003; Simmons et al., 2008; Castigliego et al., 2012). The application of ES results in extensive contraction of skeletal muscles whereby, the fibers become extended preventing additional contraction thus preventing shortening (Simmons et al., 2008; Mota-Rojas et al., 2012). Besides, myofibrillar matrix is physically disrupted thus accelerating proteolysis (Hwang et al., 2003). Two crucial postmortem changes accelerated by ES are the onset of rigor mortis by acceleration of the rate of glycolysis and pH decline to values less than 6.4. On applying ES, the rate of the aforementioned processes increases significantly but decreases on its cessation (Bendall, 1980). Furthermore, ES precludes thaw rigor in hot carcass frozen prior the onset of rigor mortis and rigor resolution. Based on this, the major merit of ES is the prevention of cold shortening that could arise during postmortem refrigeration due to a swift decline in temperature. Cross (1979) identified several factors that could be responsible for the tenderizing effect of ES. These include the accelerated depletion of ATP, which results in the prevention of cold shortening and rapid decline in postmortem muscle pH amidst high muscle temperature (30°C to 32°C) which enhances the activity of proteolytic enzymes or degradation of muscle fibers.

The biochemical and physiological basis of ES

Electrical stimulation accelerates postmortem glycolysis resulting in a pH decline via rapid depletion of muscle glycogen (Hwang et al., 2003; Simmons et al., 2008; Castigliego et al., 2012). Physiologically, the mechanisms of action of ES for improving meat tenderness occur by the release of calcium ion (Ca2+) from sarcoplasmic reticulum (calcium ion pump). Muscle contraction is promoted by the activation of myosin-ATPase. During muscle contraction, the liberated Ca2+ activates calpain and disrupts the Z-line (Warris, 2010; Mota-Rojas et al., 2012). During this event, the muscle pH and temperature is about 6.5°C and 30°C, respectively (Warris, 2010; Mota-Rojas et al., 2012). This condition favors intense calpain activity. There is also the disruption of lysosomes resulting in the release of cathepsins, which enhance muscle proteolysis (Soria and Corva, 2004; Warris, 2010). On the other hand, when cold shortening occurs that is when hot carcasses are subjected to cold storage (10°C to 15°C) prior the dissipation of body heat, the calcium ion pump is disrupted giving room for massive liberation of Ca2+ from the sarcoplasm amidst the activeness of the myosin-ATPase. Concurrently, the concentration of ATP in muscle is very high thus providing energy needed for contraction. This gives room for severe muscle contraction leading to meat toughening (Warris, 2010). The severity of toughness increases when thaw-rigor occurred. This takes place when pre-rigor meat is subjected to freezing temperature (<−10°C) (Lawrie and Ledward, 2006). Under this condition, ATP has not been depleted; despite the disruption of calcium ion pump by freezing, the Ca2+ remains in the sarcoplasm. Thus, when such meat is thawed in the presence of high concentration of ATP, severe muscle contraction, which leads to shortening takes place. It is therefore not surprising that in countries like Australia and New Zealand where the common practice is to subject carcasses to low voltage electrical stimulation immediately after exsanguination yields tender meat. This is because the low voltage ES employed depletes muscle ATP, which otherwise would have been used for muscle contraction. Besides, ES could decrease the frozen storage time necessary to deplete ATP. Lawrie and Ledward (2006) reported that during thaw rigor, an excised muscle could undergo shortening up to 30% of its original length. Nevertheless, because of the attachment of muscle to the skeleton, its shortening may be prevented to some extent.

The presence of ATP allows the polymerization of contractile protein from actin and myosin to actomyosin during muscle contraction. Reduction in sarcomere length, which subsequently leads to muscle toughening, is a good indicator of protein polymerization. During the onset of rigor mortis, depletion of adenosine triphosphate (ATP) to adenosine diphosphate (ADP) occurs. ADP further depletes to ionosinmonophosphate (IMP) (Savell et al., 2005). This chemical pathway is incapacitated to provide energy needed for polymerization. Thus, rigor mortis takes place when there is a full conversion of ATP to IMP (Prandl et al., 1994). Electrical stimulation ensures full depletion of ATP to IMP. Therefore, there is no available energy for protein polymerization and this prevents muscle contraction. Under this condition, meat tenderness is not affected by freezing since further polymerization cannot occur (Savell et al., 2005). Kang et al. (1991) while studying the effect of ES (50 mA) in rabbit muscle, reported the polymerization of actin and myosin to form actomyosin complex during contraction. Alterations in myofibrillar proteins were evident. The authors reported that the actomyosin complex is pulled in the direction of meromyosin fraction of the main myosin helix. Nevertheless, ATPase activity is present in meromyosin. The actomyosin complex breaks down into actin and myosin when the complex reaches the meromysin ATPase region. This phenomenon leads to relaxation of muscles. Furthermore, an initial decrease in ATPase activity was reported in ES meat but increased slowly during the 7 d postmortem storage. The authors concluded that changes in actomyosin were minimized by ES.

Variations in response of muscles to electrical stimulation

Muscles differ biochemically. Therefore, their response to cold shortening and conditioning behavior differ. These differences result from inherent differences in muscle fibers, which make up the muscle. Muscle fibers differ in size, densities and physiological and biochemical properties; hence, the variation between and within muscles. Color differences (white and red) between muscle fibers has been used as the basis for classification and elucidating characteristics exhibited by each muscle. However, it has been recognized that muscle fibers are not conspicuously white or red but are a heterogeneous mix of the two. The heterogeneous nature of muscle substantiates the variation and complexity in their response to ES. This could be responsible for the conflict of reports on the efficacy of ES on meat quality improvement. Lawrie and Ledward (2006) reported that the rate at which inorganic phosphate was produced during postmortem glycolysis was substantially higher in white muscle than in red muscle. Hence, in early postmortem, the attainment of relatively high concentration of inorganic phosphate in white muscle could explain its’ lack of cold shortening. Furthermore, Buege and Marsh (1975) reported that pre-rigor red muscles did not exhibit cold shortening when cooled below 15°C provided they are supplied with adequate oxygen. This resistance is terminated by reagents that prevent the usage of oxygen for resynthesis of ATP. The authors concluded that the liberation of Ca2+ in postmortem anaerobic condition and the failure of the sarcotubular system to efficiently reabsorb the Ca2+ at low temperatures were responsible for cold shortening.

One of the modes of action of ES in the improvement of tenderness is avoidance of cold shortening (Cross, 1979; Bouton et al., 1980; Mota-Rojas et al., 2012). Thus, ‘white’ muscles, which are less affected by cold shortening, are greatly influenced by ES while ES has less affect ‘red’ muscles due to their relative susceptibility to cold shortening (Devine et al., 1984). The difference in muscle response to ES could give a clue to the absence of marked exudation in beef as oppose to an intense loss of water holding capacity in PSE pork at low pH and in vivo temperature. Although, den Hertog-Meischke et al. (1997) reported reduction in water holding capacity in beef due to rapid pH decline, the magnitude of decrease in water holding capacity depends on the rate of chilling. It is possible that the rapid fall in pH caused by ES promoted intracellular osmotic pressure to a sufficient level to permit loss of water-holding capacity by the muscle proteins in pork. This corroborates the view of Henderson et al. (1970) that pork generally undergoes greater conditioning alterations than beef and this could raise its’cellular osmotic pressure more than that of beef. It is possible that pork proteins (white muscle) are inherently more susceptible to denaturation than beef muscles (red muscles). Evidence abounds that at post-mortem, white muscles are more readily denatured than red muscles (Lawrie and Ledward, 2006). In addition, George et al. (1980) reported that the sarcolemma of pork muscle is more permeable to water than that of beef. This could further account for the 4–5 fold increase in exudation observed in pork muscle subjected to ES when compared with non stimulated sides as reported by Gigiel and James (1984).

The influence of ES on meat eating quality

Meat eating quality is largely determined by sensory properties. Inability to meet consumers’ expectation with respect to sensory traits would lead to economic loss on the part of the producer. Sensory attributes of meat are influenced by myriad factors that occur at pre and post slaughter stages. Alteration of these factors could further promote quality attributes. Electrical stimulation is one of the approaches for enhancing the sensory characteristics of meat. The effects of ES on meat quality characteristics are highlighted below:

Color

Color plays vital role in influencing consumer acceptability of meat. It is the first quality characteristic that consumers consider and thus act as a powerful tool for selection and identification of meat. It is a good quality indicator of freshness or otherwise of meat. In addition to tenderness, ES has been reported to improve meat color in pork (Taylor and Martoccia, 1995), lambs (Polidori et al., 1999), beef (Mckenna et al., 2003), venison (Wiklund et al., 2001), chevon (Savell et al., 1977; Cetin and Topcu, 2009) and chickens (Birkhold and Sams, 1993; Young et al., 1999). The ability of ES to improve meat color could be due to its capability to reduce metabolites of surviving oxidative pathways in the muscle (Lawrie and Ledward, 2006). It could also result from a fast drop in pH, which causes myofibrillar proteins in the ES carcass to reach their isoelectric point earlier thereby opening up the structure of myofibrillar proteins thus causing the oxidation of myoglobin. This may be responsible for the fast development of brighter color in electrically stimulated than in non-stimulated meat when bloomed for about 12 to 20 h postmortem. However, when muscles are exposed to the atmosphere for about 48 to 72 h postmortem, the difference in color development is not obvious (Lawrie and Ledward, 2006). This occurred because by this time, ultimate pH would have been reached by both electrically stimulated and non-stimulated meat. The myofibrillar proteins of both meat samples would have opened up and the rate of myoglobin oxidation would proceed in the same manner (Lawrie and Ledward, 2006).

Studies conducted by Young et al. (1999) to investigate the effects of ES on color alterations in 96 chicken carcasses showed that ES promoted brighter color but less redness intensity of the Pectoralis major M. accompanied by a rapid decline in pH. The pH of the non-stimulated samples decline to a similar level as that of stimulated samples after 2 h postmortem. This finding corroborates the report of Warris (2010) which stated that the bright color exhibited by electrically stimulated carcass could be due to rapid acidification of muscle caused by denaturation of protein which resulted in higher light reflectance on the surface of meat. In cattle, Nazli et al. (2010) reported that when high voltage (500 to 800 V) electrical stimulation was applied to bovine carcasses, there was a rapid pH decrease coupled with brighter meat color compared to beef carcasses that were not stimulated. Roeber et al. (2000) reported positive influence of ES on beef color, which resulted from decreased time for carcass ripening. The works of Sleper et al. (1983) and Martin et al. (1983) also showed improvements in colour of bovine muscles when subjected to ES. Conversely, Ledward et al. (1986) reported that electrically stimulated bovine Semimembranosus M. exhibited pronounced formation of metmyoglobin, which resulted in color loss. This observation corroborates the report of Hector et al. (1992) which showed that low voltage ES causes pH decrease (<6) in beef which in combination with in vivo temperature was responsible for color loss and this was partly due to myosin denaturation. In sheep, high voltage electrical stimulation increased the yellowness and lightness of Longissimus thoracis M. as well as the redness and yellowness in the Gluteus medius M. of lambs (King et al., 2004). A brighter or more youthful color was observed in electrically stimulated lamb carcasses as compared to non-stimulated ones (Riley et al., 1981; Kerth et al., 1999).

Tenderness

The primary aim of electrical stimulation is to enhance meat tenderness (Aalhus et al., 1994; Simmons et al., 2008; Kemp et al., 2010). Tenderness is the most variable and important meat eating quality parameter. Electrical stimulation has been used extensively to enhance tenderness as well as general meat quality traits (Pospiech, 2003; Warris, 2010). There is no consensus among researchers on how ES is associated with tenderness. Some authors attributed the tenderizing effect of ES to avoidance of cold shortening (Cross, 1979; Bouton et al., 1980; Mota-Rojas et al., 2012) while others opined that it could be due to rapid and intense conditioning alterations resulting from the agglomeration of in vivo temperature and low pH (Bendal, 1980; Dutson et al., 1982). Savell et al. (1977) and Dutson (1980) suggested that when ES is applied, the release of Ca2+ from the calcium ion pump could promote proteolysis by the calpain. In addition, cathepsins may be released due to the disruption of the lysosomes membrane following continuous decline in pH (Dutson et al., 1980; Locker, 1985). Lawrie and Ledward, (2006) further inferred that the observed tenderness in electrically stimulated meat as a factor additional to the prevention of cold shortening could be due to accelerated proteolysis at in vivo temperatures.

In the absence of ES, ultimate pH is reached at about 10 to 12 h postmortem in pigs and ruminants whereas with ES this value could be attained within 1 to 2 h postmortem. ES meat displays severe muscular contractions, which result in a quick rate of glycolysis and pH decline. Nevertheless, this rapid decline in pH impels the occurrence of early rigor mortis, which in turn induce rapid rigor resolution that enhances a fast rate of relaxation (Soria and Corva, 2004; Warris, 2010). Simultaneously, there is rapid liberation of intracellular calcium leading to increased calpain activity as well as increased rate of proteolysis thus enhancing meat tenderness (Elgasim et al., 1981; Ducastaing et al., 1985). Pospiech et al. (2003) reported that the degradation of protein during ripening is responsible for meat tenderness. This according to Hedrick et al. (1994) and Ducastaing et al. (1985), results from behavioral changes in muscle fiber, which can be explained by three major events. Firstly, the impediment of cold shortening by reduction of slow phase of rigor mortis. Secondly, the liberation of calcium by ES, which induces increased calpain activity that causes myofibrillar proteolysis and lastly, the electric current causes severe contractions, which fractures the myofibril. The tenderizing effect of ES as reported by Cross (1979), Honikel et al. (1983) and Davey and Gilbert (1980) could have resulted from the prevention of cold shortening caused by rapid depletion of ATP; rapid pH decline amidst high muscle temperature, which favors increased activity of proteolytic enzymes; physical disruption of muscle fibers. The use of mechanical technique and enzymes in conjunction with ES could also improve meat tenderness by reducing the ripening time as well as produce more tender and brighter colored meat (Yanar and Yetim, 2003). The need to enhance various sensory properties of meat necessitates ripening. Application of ES reduces the ripening time thus enhancing meat quality. The extent of weakening and alterations of myofibrillar proteins determines the ultimate meat tenderness. Takahashi et al. (1987) suggested that tenderizing effect of ES is due to physical damage resulting from tetanizing contractions. The avoidance of cold shortening by ES could be due to non-enzymatic disruption of myofibrillar proteins (Takahashi, 1992) mediated by lysosomal enzymes (Dutson et al., 1980). There is possibility that the tenderizing effect of ES could be modulated by agglomeration of two or more underlying mechanisms.

Structurally, meat is composed of connective tissue and myofibrillar proteins (Warris, 2010). The protein content of the connective tissue varies depending on various factors, which include but not limited to specific muscle activity, animal species, age of animal, muscle type etc. (Pospiech, 2003). Trial conducted by Solomon et al. (1986) revealed that young bovine carcasses when subjected to ES at 1.5 A, 550 V and 20 pulses for 2 s produced more tender meat than non-stimulated carcasses as evaluated by sensory panels. In contrast, Kim et al. (2013) reported that low voltage ES at 90 min after exsanguination had no effect on tenderness development and proteolysis in bovine gracilis M., Longissimus dorsi M. and semimembranosus M. Similarly, studies conducted by Botha et al. (2009) inferred that low voltage ES offered no improvement in the quality attributes of ostrich. Using twenty-two ovine carcasses from castrated Doper weighing 40 to 50 kg, Davel et al. (2003) investigated the influence of electrical stimulation at 20 V, 45 Hz for 45 s on sensory features of mutton. Following, stimulation, carcasses were chilled at 2°C for 24 h. Prior sensory evaluation, Longissimus lumborum and thoracis M. were removed, cut into two, packaged under vacuum and subjected to frozen storage at −30°C. Thereafter, the right half was grilled at 160°C at internal temperature of 73°C. The result revealed that the acceptability of stimulated samples was higher than non-stimulated samples. However, no effect of ES was found on cooking losses related to slaughter weight and carcass fat.

Studies conducted by Guerrero et al. (2004) showed that varying stimulation voltages and times influenced pH of Longissimus dorsi M. of female alpacas. Two voltages (500 V and 600 V) were applied for two periods (30 s and 60 s) and pH was monitored after 1 to 24 h postmortem. A significant difference in pH was observed between the treated and control meat samples. It was reported that 500 V applied for 30 s caused a rapid decline in pH (5.27) compared to the control, which had pH (6.31) after 24 h postmortem. Electrically stimulated meat in general had pH<6.0 while untreated meat had pH>6.0. This observation, according to the authors, could have resulted from amplification of the rate of muscle contraction cycles. This accelerates the depletion of glucose stores and enhanced the production of lactate. Also, there was decline in postmortem muscle pH when carcasses obtained from calves were electrically stimulated and this was explained by accumulation of lactate from glycolysis lowering the pH to 6.56 and 5.48 after 2 and 24 h postmortem, respectively (Bryne et al., 2000).

Electrical stimulation of carcasses obtained from electrically stunned birds has been shown to affect pH decline, blood loss and increase in sarcomere length (Craig et al., 1999). When subjected to 440 V, the onset of rigor mortis was accelerated. This report is in line with the earlier report of Savell et al. (1977) with respect to sarcomere length. Canstaneda et al. (2005) investigated the effect of ES on broiler meat. Fifty-four (54) female broilers weighing 1.5 to 1.6 kg were subjected to ES at 450 mA, 450 V, 2×2 s, 7 pulse/s. The results indicated that ES enhances meat tenderness because of the rapid loss of ATP, pH decline and physical disruption of muscle fiber. It was further reported that rapid cooling of carcass at 4°C did not affect the functionality of protein hence PSE condition was not observed. However, the negative impact of slow cooling after ES was evident in various studies. The findings of Elgasim et al. (1981) showed that slow cooling after ES produced a normal pH (5.9) in meat but with PSE features. Slow cooling could also predispose carcass to pale coloring and reduction in water holding capacity (Mota-Rojas et al., 2012). Zywica and Banach (2003) studied the effect of ES and sex on meat tenderness. The authors used 18-month bulls and heifer and the carcasses were split longitudinally into two halves. The right half served as the control while the left half was subjected to ES of 17 Hz, 330 V and 0.9 pulses for 120 s. Instrumental and sensory analysis of Hemiaponeurotic M. revealed that sex of animals influenced the effect of ES on cooked meat. From their trial, ES heifer carcasses produced a better meat quality. Reports of Locker (1985) and Chrystall and Devine (1985) showed that electrically stimulated beef was rated as 10% to 50% more tender than non-stimulated ones. While investigating the effect of diet type on efficacy of ES, Smith (1985) asserted that sometimes, ES was more effective in grass-fed animals and animals fed grains for a short period than animals fed grains for a long period. He also reported that the efficacy of ES was higher in lower-grade carcasses than higher-grade carcasses.

Juiciness

There are variable reports on the effect of ES on meat juiciness. Some authors reported that ES enhanced beef juiciness (Hwang and Thompson, 2001). However, Ferguson et al. (2000) reported a decrease in juiciness while Jeremiah and Martin (1981) reported no effect. The discrepancies in these reports according to Juarez et al. (2012) could be due to the degree of physical disruption of muscle fiber, the degree to which ultimate pH is affected by ES and the degree to which ES accelerates proteolytic activity. Furthermore, juiciness perception in electrically stimulated meat may be influenced by back fat thickness as well as the amount of intramuscular fat (Juarez et al., 2012). Rapid decline in pH during ES in conjunction with insulating properties of fat could cause decline in water holding capacity and additional degradation of myofibrillar proteins. This corroborates the findings of Ferguson et al. (2000) that showed profound decrease in juiciness of ES meat from feedlot finished cattle compared to ES meat from pasture-finished cattle.

Meat microbiological quality

Food safety is a major concern in the meat industry especially when intervention is applied. Various studies have been conducted on the microbial stability of ES meat. Studies conducted by Guerrero et al. (2004) showed a lower bacterial count in ES meat compared to the control. The authors asserted that the decrease in bacterial load resulted from high content of lactic acid, which brought about rapid decline in pH, which caused unfavorable conditions for microbial proliferation. However, the pH is only bacteriostatic (inactivate microbial activity) but not bactericidal (kill microbes). Ockerman and Szczawinski (1983) reported that ES reduced initial postmortem pH and aerobic plate count of beef tissue inoculated with mixed microflora. However, the microbial count increased significantly during the aerobic product storage at 0 to 2°C up to two weeks. Similarly, Butler et al. (1981) studied pH and microbial populations in ground meat obtained from bovine Infraspinatus and Biceps femoris M. The meat were hitherto inoculated with Pseudomonas spp, Moraxella spp, Lactobacillus spp, Brochothrix thermosphaca, Acinetobacter spp and Erwinia herbicola and subjected to ES at 550 V and 16 pulses at interval of 1.8 s. Both inoculated and non-inoculated meat samples with or without ES were assessed for the same microbial populations. The authors reported pH decrease in ES samples but a significant difference was not found between stimulated and non-stimulated samples.

Ockerman and Szczawinski (1984b) reported that ES did not reduce bacterial counts for non-heated microorganisms but caused an initial decrease in post mortem pH in pork. They further reported that ES slightly reduced the thermo-resistance of Pseudomonas putrefaciens and Lactobacillus plantarum but did not reduce thermo-resistance of Streptococcus faecalis. The relationships among ES, hot or cold deboning, beef cuts, and bacteria counts were studied by Kotula and Emswiler-Rose (1981). The authors concluded that ES and cold or hot deboning did not affect proliferation of aerobic bacteria. Ockerman and Szczawinski (1984a) also studied synergistic effect of ES and meat processing methods on meat microbial stability; no synergistic effect was found between ES and storage at −21°C, between ES and 3% salt and between ES and 3% salt+200 ppm nitrate. However, synergistic effect was found between ES and heating at 60°C. The author also opined that lowered pH was not responsible for decrease in thermo-resistance caused by ES.

CONCLUSION

Myriad studies have shown that ES is an effective technique for enhancing various meat quality traits particularly meat tenderness. Nevertheless, the success of the technique is premised on several multifaceted factors that cut across antemortem, perimortem and postmortem phases of an animal. The core attribute of ES is its ability to hasten postmortem glycolysis. ES accelerates the onset as well as resolution of rigor thus reducing processing time and labor. Electrical stimulation also gives room for other processes to be carried out just immediately after bleeding and cleaning.

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