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Departments of 1 Kinesiology and 2 Physics, University of Waterloo, Waterloo N2L 3G1; and 3 Department of Surgery, University of Toronto, Toronto, Ontario, Canada M5S 1A1
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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In this study, we employed an in vivo model of
prolonged ischemia in rat skeletal muscle to investigate the
hypothesis that structural modifications to the sarcoplasmic reticulum
(SR) Ca2+-ATPase can explain the alterations in
Ca2+-ATPase activity that occur with ischemia. To
induce total ischemia, a tourniquet was placed around the upper
hindlimb in 27 female Sprague-Dawley rats weighing 256 ± 6.7 g (mean ± SE) and was inflated to 350 mmHg for 4 h. The
contralateral limb served as control (C) to the ischemic limb
(I), and the limbs of animals killed immediately after anesthetization
served as a double control (CC). Mixed gastrocnemius and tibialis
anterior muscles were sampled and used for SR vesicle preparation.
Maximal Ca2+-ATPase activity (µmol · g
protein
1 · min1) of C (15,802 ± 1,246) and I (11,609 ± 1,029) was 90 and 73% (P < 0.05) of CC (17,562 ± 1,682), respectively.
No differences were found between groups in either the Hill coefficient
or the free Ca2+ at half-maximal activity. The fluorescent
probes, FITC and
N-cyclohexyl-N'-(dimethylamino-
-naphthyl) carbodiimide, used to assess structural alterations in the
regions of the ATP binding site and the Ca2+ binding sites
of the Ca2+-ATPase, respectively, indicated a 26%
reduction (P < 0.05) in FITC binding capacity
(absolute units) in I (0.22 ± 0.01) compared with CC (0.29 ± 0.02) and C (0.29 ± 0.03). Our results suggest that the
reduction in maximal SR Ca2+-ATPase activity in SR vesicles
with ischemia is related to structural modification in the
region of the nucleotide binding domain by mechanisms that are as yet unclear.
muscle; sarcoplasmic reticulum
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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THE CA2+-ATPASE OF SARCOPLASMIC RETICULUM (SR) catalyzes the ATP-dependent translocation of Ca2+ from the cytoplasm into the lumen of the SR and maintains the resting cytoplasmic free Ca2+ ([Ca2+]f) at levels below 100 nM. In skeletal muscle, the SR Ca2+-ATPase plays an important role in excitation-contraction coupling by replenishing SR Ca2+ stores and allowing Ca2+ to be available for release on repeated activation.
The Ca2+-ATPase is a 110-kDa polypeptide chain with known sequence and structure of 997 amino acid residues (20, 37). The large cytoplasmic extramembrane portion of the enzyme (headpiece) contains the phosphate acceptor Asp-351 residue (1, 20) and the binding site for ATP (36). Other functionally important residues for binding and translocation of Ca2+ are oriented in two sites among transmembrane helixes M4, M5, and M6 (28). The Ca2+-ATPase contains 24 cysteine residues (1). Consequently, the SR Ca2+- ATPase may be a principal target for modulation of muscle function by reactive oxygen species (16). Inactivation of the SR Ca2+-ATPase as a result of free radical formation has been demonstrated in numerous in vitro studies (23, 33, 40, 41). Free radicals may cause protein denaturation and damage involving the ATP binding site (41), enhanced lipid peroxidation (15, 23), and increased protein oxidation, leading to both a reduced sulfhydryl group content and increased protein aggregation (23, 33, 40).
It is well established that free radical formation plays a primary role in the etiology of ischemia-induced damage in skeletal muscle (30). With prolonged muscle ischemia, a significant loss of ATP and total adenine nucleotides occurs (2, 12, 29, 35). This leads to elevations in substrates for the enzyme xanthine oxidase, which catalyzes the reaction where both superoxide radicals and hydrogen peroxide are formed in muscle (25).
Although free radical formation would be expected during extended ischemia, it remains unclear whether the disturbance in Ca2+ regulation occurs during the ischemic period per se or whether ischemia simply predisposes the muscle, with the actual changes becoming manifest during reperfusion. Unexpectedly, we have found a time-dependent increase in maximal Ca2+-ATPase activity with ischemia in both rat soleus and extensor digitorum longus muscle (8). Because the effects were only demonstrated in homogenate preparations, it is unclear what is happening at the level of enriched SR vesicle preparations, which are free from the potential contaminating effects of other proteins and cellular ATPases. Interestingly, reductions in Ca2+-ATPase activity have been found after ischemia in vesicle preparations from cardiac muscle (27).
Studies of ischemia-reperfusion in cardiac muscle, and more recently in skeletal muscle, have shown that impaired SR function and Ca2+ homeostasis may also be involved in the etiology of ischemia-reperfusion injury (9, 14, 19). In one study, pretreatment with the oxygen free radical scavengers superoxide dismutase and catalase maintained higher Ca2+ uptake by the SR of skeletal muscle after 3 h of ischemia and 19 h of reperfusion in rat hindlimb (19). Thus free radical formation is likely a mechanism for impaired SR function with ischemia and reperfusion.
Because measurement of SR function in ischemia studies is generally done in vitro, under optimal conditions, ischemia-induced reductions in Ca2+-ATPase activity and Ca2+ uptake are probably due to structural alterations to the Ca2+-ATPase protein and/or the SR membrane. However, the nature or precise location of altered structure on the SR Ca2+-ATPase has not been determined in skeletal muscle samples harvested from tissue that was made ischemic in vivo.
In this study, we employed a 4-h hindlimb ischemia model in
rats to characterize the alterations in SR Ca2+-ATPase
activity and structure that occur with prolonged periods of skeletal
muscle ischemia. To assess the structural alterations to the
Ca2+-ATPase, the fluorescent probes FITC and
N-cyclohexyl-N'-(dimethylamino--naphthyl)carbodiimide (NCD-4) were used to measure changes in the regions of the ATP binding
site and the Ca2+ binding sites of the
Ca2+-ATPase, respectively. We hypothesized that
Ca2+-ATPase activity would be lower in ischemic SR
compared with control and that the lower Ca2+-ATPase would
be accompanied by a reduction in FITC binding, indicative of structural
alterations to the ATP binding site.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Animal Description and Care
Adult female Sprague-Dawley rats weighing 256 ± 6.7 g (mean ± SE) were housed in an environmentally controlled room (temperature 22-24°C, 40-60% relative humidity) with reversed light-dark cycles. Animals were fed ad libitum on laboratory chow and water until the time of the experiment. All experiments were initiated at approximately the same time each day to avoid large diurnal variations in muscle glycogen (5). Experimental protocols were approved by the Animal Care Committee of the University of Waterloo.Experimental Protocol
To investigate the effects of complete ischemia on SR Ca2+-ATPase structure and function, animals were randomly assigned to a control control (CC) group (n = 9) to be killed immediately after anesthetization or to experimental (E) (n = 27) groups. For each E animal, the experimental condition, 4 h of total ischemia, was randomly assigned to one hindlimb (I) while the contralateral limb served as a control limb (C). Due to tissue requirements for the isolation procedure used to obtain SR vesicles, experiments were conducted on one CC and three E animals each day. Ischemia was induced by placing a tourniquet around the upper hindlimb and proximal to the knee joint. To ensure total occlusion of blood flow to the hindlimb, a 350-mmHg pressure was employed (7). Total ischemia was confirmed on the basis of almost total depletion of muscle phosphocreatine and ATP after 4 h of ischemia (see Table 1).
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Before the induction of ischemia, the rats were weighed and anesthetized. Anesthesia was initially accomplished by using an intraperitoneal injection of pentobarbital sodium (6 mg/100 g body wt) and then was maintained by using supplementary intraperitoneal injections as required. To prevent dehydration, experimental rats were administered 2 ml of saline by injection just under the skin before the induction of ischemia. Throughout the ischemic periods, body temperature was maintained between 37 and 39°C by having the rats lay in a prone position on a warm heating pad. At the end of each of the ischemic periods, a small piece of white gastrocnemius (G) muscle was rapidly sampled from each of the I and C limbs and frozen in liquid nitrogen for later analysis of muscle metabolites. The remainder of the G muscle (both red and white portions) and the entire tibialis anterior (TA) muscle were excised and placed in ice-cold buffer to be used for SR isolation by differential centrifugation. The hindlimbs were not reperfused before muscle sampling. The G and TA muscles from the CC animal were sampled and excised in the same manner immediately after anesthetization.
Analytic Procedures
Sample preparation for SR assessment in vitro.
Ischemic and control muscles were prepared according to
Heilmann et al. (11). Mixed G and TA muscles were diluted
~1:5 (wt/vol) in ice-cold homogenizing buffer containing (in mM) 5 HEPES (pH 7.5), 250 sucrose, 0.2% sodium azide, and 0.2 phenylmethylsulfonyl fluoride (PMSF) and mechanically homogenized with
a polytron homogenizer (PT 3,100) at 16,500 rpm, for two 30-s bursts.
An aliquot of this sample was quick frozen in liquid nitrogen, stored
at 
70° to 80°C and used for homogenate determinations of
Ca2+-ATPase activity. To obtain an enriched SR membrane
fraction, a combination of two SR isolation protocols was used
(6, 11). The homogenate was centrifuged at 5,500 g for 10 min to remove cellular debris, and the supernatant
was filtered through four layers of gauze to remove as much fat as
possible. The supernatant was then transferred to clean tubes and
centrifuged at 12,500 g for 18 min. These pellets were
discarded, and the spin was repeated. Again, the supernatant was
transferred to clean tubes and centrifuged at 50,000 g for
52 min. These pellets were resuspended in 10 ml homogenizing buffer
plus 600 mM KCl and allowed to incubate at 4°C for 30 min. This
suspension was then centrifuged at 15,000 g for 10 min to
pellet all the mitochondria. The supernatant was centrifuged at 50,000 g for 52 min. The final pellet, enriched in SR membranes (no
sucrose cushion), was resuspended in homogenizing buffer at a protein
concentration of 2-6 mg/ml. SR isolation was carried out by
differential centrifugation by use of a Beckmann ultracentrifuge with a
70.1 Ti fixed-angle rotor. The SR membrane fraction was used for
measurements of Ca2+-ATPase activity and isoform
composition and to examine structural alterations to the enzyme. All
homogenates and SR membrane isolations were made with only PMSF as a
proteolytic inhibitor.
SR Ca2+-ATPase activity
measurements.
Spectrophotometric (Schimadzu UV 160U) measurement of SR
Ca2+-ATPase activity was performed on homogenates by using
procedures developed by Simonides and van Hardeveld (34)
and SR samples analyzed according to methods of Leberer et al.
(18) with minor modifications. Total
(Mg2+-activated)-ATPase activity was measured in the
presence of the Ca2+ ionophore A-23187, across a range of
CaCl2 concentrations. Basal activity was measured in the
presence of 40 µM cyclopiazonic acid, which completely inhibits SR
Ca2+-ATPase activity (32). The difference
between total and basal activities represents the
Ca2+-activated ATPase activity. Maximal activity and the
Ca2+ dependency of Ca2+-ATPase activity were
assessed by adding 1-11 µl of 100 mM CaCl2 in
0.5-µl additions. Ca2+-ATPase activity increases with
[Ca2+]f until a plateau occurs, once maximal
activity is reached. The [Ca2+]f
corresponding to each CaCl2 addition was assessed
separately, on a different SR aliquot, by using dual-wavelength
spectrofluorometry and the Ca2+-fluorescent dye indo 1. Ca2+-ATPase activity was then plotted against the negative
logarithm of [Ca2+]f (pCa), and the Hill
coefficient and the [Ca2+]f that gives
half-maximal activity (Ca50) were determined. These properties were measured through nonlinear regression with computer software (Graph Pad Software) using the following sigmoidal
dose-response equation
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SDS-PAGE and Western blotting. A suspension of 0.5 mg/ml SR protein in either 40 µl reducing buffer [1.25 M sucrose, 0.1 M dithiothreitol (DTT), 0.25 M Tris · HCl, pH 6.8, 5% SDS, 0.01% bromophenol] or nonreducing buffer (1.25 M sucrose, 0.25 M Tris · HCl, pH 6.8, 5% SDS, 0.01% bromophenol) brought to 200 µl by distilled water was heated for 10 min at 100°C, and solid DTT was added to the sample in reducing buffer to raise the final concentration of DTT to 100 mM. All samples were then sonicated for 10 s in a probe sonicator, and 5 µg of each sample was analyzed in duplicate on separate 7% polyacrylamide SDS gels (BIO-RAD Mini-PROTEAN II) with a 3.75% stacking gel.
After SDS-PAGE and a 15 min equilibration in cold transfer buffer (25 mM Tris, 192 mM glycine, and 20% vol/vol methanol), the proteins were transferred to a polyvinylidene difluoride membrane (Bio-Rad) by placing the gel in transfer buffer and applying a high voltage (100 V) for 45 min (Trans-Blot Cell, Bio-Rad). Nonspecific binding sites were blocked with 10% skim milk powder in Tris-buffered saline (pH 7.5), applied overnight at room temperature. Immunoblotting was performed with use of the primary monoclonal antibody IIH11 specific for rat (Affinity Bioreagents) for determination of SERCA1 protein and the aggregation state of SERCA1. Incubation with the primary antibodies was performed for 60 min at room temperature. After washing, a secondary antibody (anti-mouse IgG1 conjugated to horseradish peroxidase) was applied for 60 min at room temperature. Protein quantification was performed by using densitometry and an enhanced chemiluminescence immunodetection procedure (Amersham-ECL-RPN2106P1). After exposure to photographic film (Kodak Hyperfilm-ECL), the blot was developed for 90 s in Kodak GBX developing solution and fixed in Kodak GBX fixer. Relative SERCA1 protein levels were determined by scanning densitometry, and values were expressed as a percentage of the CC value.Fluorescence measurements.
Fluorescence measurements were made on an SLM-4800S spectrofluorometer
(SLM Instruments, Urbana, IL) according to Lalonde et al.
(17). FITC (Sigma Chemical) and NCD-4 (Molecular Probes) were stored at a concentration of 5 mM in ethanol at 20°C. FITC emission spectra (500-550 nm) were collected by exciting samples at 490 nm (see Fig. 3A). FITC labeling was done by washing
the SR samples once in wash buffer (homogenizing buffer without
sucrose) with no DTT, then resuspending the samples in FITC labeling
buffer (wash buffer plus 2.5 µM FITC, pH 8.8) and vortexing gently in darkness for 20 min at 25°C. The SR samples were then washed again in
wash buffer to remove unbound label. NCD-4 emission spectra were
collected by exciting samples at 340 nm and scanning the emission
intensity from 400 to 430 nm at 1-nm increments. NCD-4 labeling was
done by washing the SR samples once in wash buffer with no DTT, then
resuspending in NCD-4 labeling buffer (wash buffer plus 150 µM NCD-4,
pH 6.2) and incubating in darkness for 3 h at 25°C. As before,
the sample was washed to remove unbound label.
Muscle metabolites.
Muscle metabolites were measured on samples of stored tissues
(80°C) that were freeze dried and cleared of visible connective tissue and blood. After extraction of the metabolites by perchloric acid (0.5 M) and neutralization, the contents of phosphocreatine (PCr),
creatine, and lactate were assessed by using fluorometric procedures
according to techniques previously published by our laboratory
(10). A portion of the extract was also used for the
determination of ATP, ADP, AMP, IMP, inosine, and hypoxanthine by using
ion-pair, reversed-phase HPLC techniques (13) as described earlier (10).
Statistical Analysis
For all measurements, a one-way ANOVA was used to test for differences between means. When significant differences were found, Tukey's post hoc tests were used to compare specific means. For all comparisons, statistical significance was accepted at P < 0.05. All data are expressed as means ± SE.| |
RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Ca2+-ATPase Activity
Maximal Ca2+-ATPase activity (µmol · g protein1 · min1) measured in
homogenates between the ischemic muscle (970 ± 54) and
contralateral control (907 ± 70) was not different. Similarly,
there were no differences between these muscles and the muscles from
nonischemic animals (826 ± 46). In enriched SR vesicles,
maximal Ca2+-ATPase activity, which occurred at a
[Ca2+]f of ~6-10 µM in all groups
(data not shown), was 73% (P < 0.05) and 90%
(P < 0.05) of CC compared with I and C, respectively
(Table 1). There was no difference between CC and C. However, although maximal activity was depressed after ischemia, there was no
effect on enzyme kinetics (Table 1; Fig.
1). Kinetic analysis of the Ca2+-ATPase activity-pCa curves showed that both the Hill
coefficient and the Ca50 were not different between groups.
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Electrophoresis and Western Blot Analysis
Total SR Ca2+-ATPase protein contents were compared between groups by Western blot analysis. Total protein was only analyzed on SR samples subjected to reducing conditions (with DTT) SDS-PAGE, because all of the Ca2+-ATPase protein should be in the monomer form under these conditions and easily detected by the monoclonal antibody IIH11 (22). Six discrete bands were present under these conditions, corresponding to the monomer form of SERCA1 and smaller molecular weight SERCA1 products (Fig. 2B). No discrete bands corresponding to dimers or higher molecular weight aggregates were observed. Relative total protein content was taken as the sum intensity of all six bands and was expressed relative to CC. There was no difference between groups in total SERCA1 protein content. Compared with CC, the values for C and I groups were 94.8 ± 8.9 and 104 ± 10.3%, respectively.
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To determine whether prolonged ischemia results in SERCA1
protein oxidation and protein aggregation, SR samples from all groups were subjected to nonreducing (no DTT) and reducing (DTT) SDS-PAGE. Under nonreducing conditions, only two main bands were detected, corresponding to the monomer form of SERCA1 (110 kDa) and a smaller molecular weight (~70 kDa) SERCA1 product (Fig. 2A). Under
these conditions, the intensity of the band corresponding to the
monomer form of SERCA1 was lower (P < 0.05) in I
relative to CC but not to C (Fig.
3A). There were no differences
between CC and C. No differences were found in relative intensity of
the 70-kDa bands between groups (Fig. 3B). Similarly, when
the same two bands were analyzed for relative intensity under reducing
conditions, there were no differences for either band between groups.
This finding suggests that higher molecular weight aggregates were
present in ischemic SR, leading to a lower intensity of the
monomer form of SERCA1 under nonreducing conditions but not under
reducing conditions.
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Fluorescence Measurements
FITC and NCD-4 binding were used as a method to assess the structure of the nucleotide binding domain and the Ca2+ binding domain of the Ca2+-ATPase after prolonged ischemia, respectively. FITC covalently labels Lys515, which is close to the ATP binding site and competitively inhibits ATP binding (26). Similarly, the label NCD-4 binds near the two Ca2+ binding sites in addition to some nonspecific labeling, inhibiting binding of Ca2+ without inhibiting the binding of ATP (3).A sample emission spectrum of FITC from each group is shown in
Fig. 4A. The average maximum
intensity, which occurs at 520 nm, was 26% lower in I
(P < 0.05) compared with both CC and C (Fig.
4B). There was no difference between CC and C. The maximum emission intensity of NCD-4 was 0.36 ± 0.2, 0.36 ± 0.2, and
0.34 ± 0.2 for the CC, C, and I groups, respectively. No
differences were found between any of the groups.
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Ischemia resulted in extensive changes in the metabolic
status of the muscle (Table 2). For the
metabolites measured, ischemia induced near-complete depletion
of ATP and PCr. These changes were accompanied by large relative
increases in IMP, inosine, and hypoxanthine. In contrast, ADP, but not
AMP, was reduced with ischemia. Total creatine was not
different in any of the groups. In addition, lactate content was
elevated ~12-fold over control muscles. No differences were found for
any of the metabolites between the CC and C groups.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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In summary, we have found that 4 h of ischemia resulted in a reduction in maximal Ca2+-ATPase activity in SR vesicles that was accompanied by a reduction in FITC but not NCD-4 binding. The reduction in maximal Ca2+-ATPase activity was not accompanied by changes in either the Hill coefficient or pCa50. Interestingly, no changes in maximal Ca2+-ATPase activity were observed with ischemia in homogenates.
Differences Between Homogenates and SR Fractions
A key concern is why the effects of ischemia on Ca2+-ATPase activity were observed only in the SR vesicles and not in the homogenates. Interestingly, we have previously observed increases in maximal activity in homogenates with shorter periods of ischemia (8). It is possible that ischemia is without effect on homogenates and that the reductions in Ca2+-ATPase activity in SR vesicles simply reflect a selective discard of undamaged SR during the isolation procedure. This has been observed previously in ischemic hearts (27). On the other hand, the failure to find reductions in Ca2+-ATPase activity in homogenates could be due to activation of other cellular ATPases, masking the effects of the inhibiting agents or recruitment of additional enzyme by covalent modification, leading to phosphorylation or production of an activator substance during ischemia, which binds to the Ca2+- ATPase and activates it (8). It is possible that these changes become lost during the vesicle isolation process. Regardless of the mechanism, the overall effect would be to minimize the inactivation of the pool of enzymes that occurs during ischemia. This finding is potentially very important because isolation artifact could conceivably explain much of the existing controversy in the literature regarding ischemic effects on SR function (24).Structural Changes in Ca2+-ATPase
In this study, we attempted to elucidate the structural alterations that occur to the SR Ca2+-ATPase in vivo with prolonged ischemia in rat skeletal muscle, which could explain the predicted reduction in Ca2+-ATPase activity that occurs with ischemia. Our results for the SR vesicles are consistent with our hypothesis, namely that the reductions in Ca2+-ATPase activity are accompanied by alterations in the region of the nucleotide binding site on the enzyme.The reductions in maximal Ca2+-ATPase activity that we observed in this study in ischemic SR compared with CC and C paralleled the reductions in FITC binding that occurred with ischemia. On the other hand, kinetic analysis of Ca2+-ATPase activity shows that both the Hill coefficient and sensitivity of the enzyme to Ca2+ (Ca50) were unaffected. These results are consistent with a problem in binding ATP, but only in a selected population of Ca2+ pumps. A similar effect has been postulated to occur in rabbit muscle after chronic muscle activity (18). The reduction in FITC binding is not due to reductions in Ca2+-ATPase protein as determined by Western blot analysis. Rather, it appears that a reduction in the number of FITC binding sites per Ca2+-ATPase protein occurred in response to the prolonged ischemia.
We did probe for structural alterations in the region of the Ca2+ binding domain of the Ca2+-ATPase, by using the fluorescent probe NCD-4. We found that ischemia had no effect on the maximum binding capacity of NCD-4, suggesting that the structure of the Ca2+ binding domain was unaltered after prolonged ischemia. This is in close agreement with our kinetic analysis of ATPase activity because the Hill coefficient, which theoretically represents the number of Ca2+ binding sites, was not different between groups. However, it must be emphasized that the NCD-4 probe not only binds near to Ca2+ binding sites but displays some nonspecific binding as well (3).
Potential Role of Free Radicals
Although several mechanisms may be involved, our metabolic data indicate a strong possibility that free radical production, mediated during the 4 h of ischemia, is involved. The ischemic period resulted in massive reductions in the high-energy phosphates ATP and PCr in ischemic muscle but not in control muscles. As a consequence, large elevations in hypoxanthine and xanthine, which are substrates for the enzyme xanthine oxidase, occurred, as would be expected (29). The enzyme catalyzes the reduction of O2, leading to the formation of superoxide and H2O2, and it has been proposed as a central mechanism of oxidative injury (21). Therefore, although we did not directly measure free radical production in this study, it can be assumed that there was significant free radical production in the ischemic muscle compared with control.Our results indicate that the structural changes in Ca2+-ATPase with ischemia are similar to those reported after exposure of the Ca2+-ATPase to oxidizing conditions in vitro. In the in vitro study, it was found that exposure of the Ca2+-ATPase to levels of hydroxyl radicals similar to that measured during postischemic reperfusion denatures the Ca2+-ATPase and inhibits ATPase activity by directly attacking the ATP binding site without damaging the primary structure of the enzyme (41). This would suggest that prolonged ischemia also leads to structural reorganization of the region of the nucleotide binding domain, which would likely impair ATP binding and ATPase activity.
In the in vitro study, it was also found that presaturation of the active site with ATP completely protected both cardiac and skeletal muscle SR Ca2+-ATPase function from hydroxyl radical-induced inhibition. This suggests that depletion of cellular ATP, in the region of the enzyme, induces the structural alteration to the nucleotide binding domain of the Ca2+-ATPase. In our study, depletion of muscle ATP stores, as observed with prolonged periods of skeletal muscle ischemia, not only suggests formation of free radicals in skeletal muscle but may also indicate the susceptibility of SR Ca2+-ATPase to free radical-induced damage, specifically to the nucleotide binding domain.
The precise nature of the structural modification to the nucleotide binding domain in ischemic SR, which resulted in a reduced FITC binding capacity, cannot be directly ascertained from this study. However, several in vitro studies have helped to characterize the free radical-induced molecular modification of the SR Ca2+-ATPase that is correlated with its functional properties (33, 39). Viner et al. (39) employed a peroxyl radical-generating system by using the free radical initiator 2,2'-azobis(2-amidinopropane) dihydrochloride to examine and identify oxidation-sensitive peptides within the SR Ca2+-ATPase of fast-twitch rabbit skeletal muscle. They identified six oxidatively sensitive peptides on the cytoplasmic side of the SR membrane. One of these peptide segments (Glu551-Arg604) is located in the nucleotide binding domain and was found to participate in the formation of intermolecular bityrosine cross-links with the identical Glu551-Arg604 peptide from a neighboring Ca2+-ATPase polypeptide chain. Although this peptide does not contain the FITC binding site Lys515 (4) or the actual ATP binding site around Arg604 (36), cross-linking and aggregation in this region may interfere with both FITC and ATP binding. Whether cysteine residues are affected by prolonged ischemia, as might be expected if aggregation occurred, was not assessed in this study.
As reported, we detected smaller molecular weight SERCA1 fragments by using reducing SDS-PAGE and Western blot analysis. However, the relative amount of each fragment was not different between groups (data not shown). Likely, the appearance of these products was due to proteolytic activity and/or oxidative fragmentation that took place during homogenization and preparation of SR vesicles, and this should be the same for all groups. Our homogenization buffer only included one proteolytic inhibitor (PMSF) and did not include the sulfhydryl reducing agent, DTT. The decision not to use DTT was purposeful because we have reported that even 5 mM DTT in the homogenization buffer can alter the effects of 4 h ischemia on SR Ca2+-ATPase activity (38).
Although aggregation of Ca2+-ATPase in ischemic SR compared with control is suggested, as indicated by the lower relative monomer form of the protein in I, the gels were not supportive. The difference in monomer levels was corrected in reducing gels. This suggests that aggregation did occur with ischemia and was due to disulfide cross-links. A similar finding was reported by Senisterra et al. (33), with exposure of the SR Ca2+-ATPase to the thiol-specific reagents diamide and arsenite.
In the present study, we used an ischemia model in rat skeletal muscle known to lead to elevations in oxygen free radical production and reductions in SR Ca2+-ATPase activity to assess the structural alterations associated with in vivo oxidation of the SR Ca2+-ATPase. We have shown that prolonged ischemia leads to reductions in FITC binding capacity in isolated SR preparations, which is associated with reductions in maximal Ca2+-ATPase activity. We suggest that the molecular mechanism is likely oxidation of one or more of the cysteine residues within the nucleotide binding domain of the Ca2+-ATPase by xanthine oxidase-produced superoxide and/or H2O2. Whether these structural alterations are manifested in vivo remains to be demonstrated.
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ACKNOWLEDGEMENTS |
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This research was supported by grants from the Medical Research Council (Canada) and the Natural Sciences and Engineering Research Council (Canada).
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FOOTNOTES |
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Address for reprint requests and other correspondence: H. J. Green, Dept. of Kinesiology, Univ. of Waterloo, Waterloo, ON, Canada N2L 3G1 (E-mail: green{at}healthy.uwaterloo.ca).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 7 December 2000; accepted in final form 29 June 2001.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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1.
Brandl, CJ,
Green NM,
Korczak B,
and
MacLennan DH.
Ca-ATPase genes. Homologies and mechanistic implications of reduced amino acid sequences.
Cell Motil Cytoskeleton
44:
597-607,
1986.
2.
Carvalho, AJ,
McKee NH,
and
Green HJ.
Metabolic and contractile responses of fast and slow twitch rat skeletal muscle to ischemia and reperfusion.
Plast Reconstr Surg
99:
163-171,
1997[ISI][Medline].
3.
Chadwick, CC,
and
Thomas EW.
Inactivation of sarcoplasmic reticulum (Ca2+ + Mg2+)-ATPase by N-cyclohexyl-N'-(4-dimethylamino--naphthyl) carbodimide.
Biochim Biophys Acta
730:
201-206,
1983[Medline].
4.
Champeil, PS,
Riollet S,
Orlowski F,
Guillain CJ,
and
Seebergst DB.
ATP regulation of SR Ca-ATPase, metal-free ATP and 8-bromo ATP binding with high affinity to the catalytic site of phosphorylated ATPase and accelerated dephosphorylation.
J Biol Chem
263:
12288-12294,
1988
5.
Conlee, RK,
Rennie MJ,
and
Winder WW.
Skeletal muscle glycogen content: diurnal variation and effects of fasting.
Am J Physiol
231:
614-618,
1976.
6.
Eletr, S,
and
Inesi B.
Phospholipid orientation in sarcoplasmic membranes: spin-label ESR and proton MNR studies.
Biochim Biophys Acta
282:
174-179,
1972[Medline].
7.
Fish, JS,
McKee NH,
Kuzon B, Jr,
and
Plyley MJ.
The effect of hypothermia on changes in isometric contractile function in skeletal muscle after tourniquet ischemia.
J Hand Surg [Am]
18:
210-217,
1993[Medline].
8.
Green, HJ,
McKee NH,
Carvalho AJ,
and
Dossett-Mercer JD.
Ischemia induced alterations in sarcoplasmic reticulum Ca2+-ATPase activity in rat soleus and EDL.
Am J Physiol Cell Physiol
271:
C1942-C1948,
1996
9.
Green, HJ,
McKee NH,
Carvalho AJ,
and
Phillips SM.
Reductions in sarcoplasmic reticulum Ca2+ ATPase activity in rat skeletal muscles of different fibre composition with ischemia and reperfusion.
Can J Physiol Pharmacol
75:
78-82,
1997[ISI][Medline].
10.
Green, HJ,
Sutton J,
Young P,
Cymerman A,
and
Houston CS.
Operation Everest II: muscle energetics during maximal exhaustive exercise.
J Appl Physiol
66:
142-150,
1989
11.
Heilmann, C,
Brdiczka D,
Nickel E,
and
Pette D.
ATPase activities, Ca++ transport and phosphoprotein formation in sarcoplasmic reticulum subfractions of fast and slow muscles.
Eur J Biochem
81:
211-221,
1977[ISI][Medline].
12.
Idström, JP,
Soussi B,
Elander A,
and
Bylund-Fellenius AC.
Purine metabolism after in vivo ischemia and reperfusion in rat skeletal muscle.
Am J Physiol Heart Circ Physiol
258:
H1668-H1673,
1990
13.
Ingebretsen, DC,
Bakken AM,
Segadal L,
and
Farstad M.
Determination of adenine nucleotides and inosine in human myocardium by ion pair reversed phase high performance liquid chromatography.
J Chromatogr A
242:
119-126,
1982.
14.
Kaplan, P,
Hendrikx M,
Mattheussen M,
Mubagwa K,
and
Flameng W.
Effect of ischemia and reperfusion on sarcoplasmic reticulum calcium uptake.
Circ Res
71:
1123-1130,
1992
15.
Kourie, JI.
Interaction of reactive oxygen species with ion transport mechanisms.
Am J Physiol Cell Physiol
275:
C1-C24,
1998
16.
Kukreja, RG,
Okabe E,
Schrier GM,
and
Hess M.
Oxygen radical-mediated lipid peroxidation and inhibition of Ca2+- ATPase activity of cardiac sarcoplasmic reticulum.
Arch Biochem Biophys
261:
447-457,
1988[ISI][Medline].
17.
Lalonde, RJ,
Lepock JR,
and
Kruuv J.
Site of freeze-thaw damage and cryoprotection by amino acids of the calcium ATPase of sarcoplasmic reticulum.
Biochim Biophys Acta
1079:
128-138,
1991[Medline].
18.
Leberer, E,
Härtner KT,
and
Pette D.
Reversible inhibition of sarcoplasmic reticulum Ca-ATPase by altered neuromuscular activity in rabbit fast-twitch muscle.
Eur J Biochem
162:
555-561,
1987[ISI][Medline].
19.
Lee, KR,
Cronenwett JL,
Shlafer M,
Corpron C,
and
Zelenock GB.
Effect of superoxide dismutase plus catalase on Ca2+ transport in ischemic and reperfused skeletal muscle.
J Surg Res
42:
24-32,
1987[ISI][Medline].
20.
MacLennan, DH,
Brandl CJ,
Korczak B,
and
Green NM.
Amino acid sequence of a Ca-Mg-dependent ATPase from rabbit muscle sarcoplasmic reticulum deduced from its complementary DNA sequence.
Nature
316:
696-700,
1985[Medline].
21.
McCord, JM.
Oxygen-derived free radicals in postischemic tissue injury.
N Engl J Med
312:
159-163,
1985[Abstract].
22.
Molnar, E,
Seidler NW,
Jona I,
and
Martonosi AN.
The binding of monoclonal and polyclonal antibodies to the Ca2+-ATPase of sarcoplasmic reticulum: effects on interactions between ATPase molecules.
Biochim Biophys Acta
1023:
147-167,
1990[Medline].
23.
Morris, TE,
and
Sulakhe PV.
Sarcoplasmic reticulum Ca2+-pump dysfunction in rat cardiomyocytes briefly exposed to hydroxyl radicals.
Free Radic Biol Med
22:
37-47,
1997[ISI][Medline].
24.
Mubagwa, K.
Sarcoplasmic reticulum function during myocardial ischemia and reperfusion.
Cardiovasc Res
30:
166-175,
1995[ISI][Medline].
25.
Parks, DA,
and
Granger DN.
Xanthine oxidase: biochemistry, distribution and physiology.
Acta Physiol Scand Suppl
548:
87-99,
1986.
26.
Pick, U,
and
Karlish SJD
Indications for an oligomeric structure and for conformational changes in sarcoplasmic reticulum Ca2+-ATPase labelled selectively with fluorescein.
Biochim Biophys Acta
626:
255-261,
1980[Medline].
27.
Rapundalo, ST,
Briggs FN,
and
Feher JJ.
Effects of ischemia on the isolation and function of canine cardiac sarcoplasmic reticulum.
J Mol Cell Cardiol
18:
837-851,
1986[ISI][Medline].
28.
Rice, WJ,
Green NM,
and
MacLennan DH.
Site-directed disulfide mapping of helices M4 and M6 in the Ca2+ binding domain of SERCA 1a, the Ca2+ ATPase of fast twitch skeletal muscle sarcoplasmic reticulum.
J Biol Chem
272:
31412-31419,
1997
29.
Rubin, BB,
Liauw S,
Tittley J,
Romaschin AD,
and
Walker PM.
Prolonged adenine nucleotide re-synthesis and reperfusion injury in post-ischemic skeletal muscle.
Am J Physiol Heart Circ Physiol
262:
H1538-H1547,
1992
30.
Rubin, BB,
Romaschin A,
Walker PM,
Gute DC,
and
Korthuis RT.
Mechanisms of postischemic injury in skeletal muscle: intervention strategies.
J Appl Physiol
80:
369-387,
1996
31.
Schacterle, GR,
and
Pollock RL.
A simplified method for the quantitative assay of small amounts of protein in biologic material.
Anal Biochem
51:
654-655,
1973[ISI][Medline].
32.
Seidler, NW,
Jona I,
Vegh M,
and
Martonosi A.
Cyclopiazonic acid is a specific inhibitor of the Ca2+-ATPase of sarcoplasmic reticulum.
J Biol Chem
264:
17816-17823,
1989
33.
Senisterra, GA,
Huntley SA,
Escaravage M,
Sekhar ML,
Freeman ML,
Borrelli M,
and
Lepock JR.
Destabilization of the Ca2+-ATPase of sarcoplasmic reticulum by thiol-specific, heat shock inducers results in thermal denaturation at 37°C.
Biochemistry
36:
11002-11011,
1997[Medline].
34.
Simonides, WS,
and
van Hardeveld C.
An assay for sarcoplasmic reticulum Ca2+-ATPase activity in muscle homogenates.
Anal Biochem
191:
321-331,
1990[ISI][Medline].
35.
Soussi, B,
Lagerwall K,
Idström JP,
and
Schersten T.
Purine metabolic pathways in rat hindlimb perfusion model during ischemia and reperfusion.
Am J Physiol Heart Circ Physiol
265:
H1074-H1081,
1993
36.
Taylor, WR,
and
Green NM.
The predicted secondary structure of the nucleotide binding sites of six cation-transporting ATPases lead to a probable tertiary fold.
Eur J Biochem
179:
241-248,
1989[ISI][Medline].
37.
Toyoshima, C,
Sasabe H,
and
Stokes DL.
Three-dimensional cryo-electron microscopy of the calcium ion pump in the sarcoplasmic reticulum membrane.
Nature
362:
467-471,
1993[Medline].
38.
Tupling, R,
Green H,
and
McKee N.
The effects of ischemia on sarcoplasmic reticulum Ca2+-ATPase activity are altered in rat skeletal muscle prepared with DTT (Abstract).
Med Sci Sports Exerc Suppl
31:
S166,
1999.
39.
Viner, RI,
Krainev AG,
Williams TD,
Schöneich C,
and
Bigelow DJ.
Identification of oxidation-sensitive peptides within the cytoplasmic domain of the sarcoplasmic reticulum Ca2+-ATPase.
Biochemistry
36:
7706-7716,
1997[Medline].
40.
Viner, RI,
Williams TD,
and
Schöneich C.
Peroxynitrite modification of protein thiols: oxidation, nitrosylation, and S-glutathiolation of functionally important cysteine residue(s) in the sarcoplasmic reticulum Ca-ATPase.
Biochemistry
38:
12408-12415,
1999[Medline].
41.
Xu, KY,
Zweier JL,
and
Becker LC.
Hydroxyl radical inhibits sarcoplasmic reticulum Ca2+-ATPase function by direct attack on the ATP binding site.
Circ Res
80:
76-81,
1997
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), control (C, 
), and ischemic
(I, 
) sarcoplasmic reticulum (SR) vesicles prepared
from mixed gastrocnemius and tibialis anterior muscles. Curves were fit
by nonlinear regression by using the average values of the Hill
coefficient and cytoplasmic free Ca2+ that gives
half-maximal activity (Ca50) from Table 
), C (