(Received for publication, January 21, 1997)
From the Department of Pharmacology, Faculty of Medicine, The University of Tokyo and CREST, Japan Science and Technology Corporation, Hongo 7-3-1, Bunkyo-ku, Tokyo 113, Japan
Ca2+ release mediated by the ryanodine receptor (RyR) regulates many important cell functions including excitation-contraction (E-C) coupling in skeletal muscle, by which membrane depolarization controls the opening of RyR via the dihydropyridine receptor. Among the three RyR subtypes, RyR-1 mediates skeletal muscle E-C coupling, whereas RyR-2 and RyR-3 cannot substitute for RyR-1. We carried out expression experiments using cultured mutant skeletal myocytes not having intrinsic intracellular Ca2+ release channels to study the structure-function relationship of amino acid residues 1303-1406 in RyR-1 (D2 region). In this region the amino acid sequences are highly divergent between RyR-1 and RyR-2, and the corresponding sequence is lacking in RyR-3. Expression of RyR-1 but not of RyR-2 rescued E-C coupling in the mutant cells. Deletion of either the entire D2 region or its N-terminal half from RyR-1 preserved the function of RyR-1 as a Ca2+ release channel but resulted in the loss of E-C coupling. Substitution of the D2 region for the corresponding sequence of RyR-2 had no effect on the function of RyR-1. These results indicate that the presence of the D2 region is critical for E-C coupling in skeletal muscle, although the D2 region alone cannot determine the functional difference between RyR-1 and RyR-2.
The ryanodine receptors (RyRs)1 are a family of channels that mediate the release of intracellular Ca2+ stores and comprise three subtypes derived from distinct genes (1-3). The function of RyRs was first recognized and most extensively studied in skeletal muscle, although the study of RyRs has been expanded to cardiac and smooth muscle cells, nerve cells, and certain nonexcitable cells. In skeletal muscle excitation-contraction (E-C) coupling, membrane depolarization reaches the interior of the cell through the transverse tubules (T-tubules), where the arrival of membrane depolarization is sensed by the dihydropyridine receptor (DHPR). A still unknown signal is then transmitted from the DHPR located on the T-tubule membrane to the RyR, which constitutes the foot structure forming a bridge between the T-tubules and the SR membrane (4, 5). Upon receipt of the signal from the DHPR, the RyR induces release of Ca2+ from the SR (6-8). One of the characteristic features of this coupling mechanism is that it does not require the presence of extracellular Ca2+ (9).
Two RyR subtypes, type 1 (RyR-1) and type 3 (RyR-3), are expressed in skeletal muscle cells. RyR-1 is the dominant subtype and mediates E-C coupling, whereas RyR-3 is the minor component the functions of which are still poorly understood. Indeed, targeted disruption of the gene encoding RyR-1 resulted in the loss of E-C coupling (10), whereas skeletal muscle cells in RyR-3-deficient mice show normal E-C coupling (11). Although all subtypes of RyR mediate Ca2+-induced Ca2+ release (CICR), neither RyR-2 nor RyR-3 is capable of substituting for RyR-1 in skeletal muscle E-C coupling (12, 13). Thus, the three subtypes of RyR have clear functional differences. Although the overall amino acid sequence identity among the RyR subtypes is 67-70% (14), there are several regions where the amino acid sequences significantly diverge. These regions are referred to as D1, D2, and D3 (15). It is an interesting possibility, therefore, that these divergence regions may correspond to the different functions of the RyR subtypes.
Among the divergence regions of the RyRs, the D2 region of RyR-1 (amino acid residues 1342-1403) is contained within the stretch of amino acid residues 1303-1406, the corresponding sequence of which is entirely absent in RyR-3 (14). In this study, we refer to the residues 1303-1406 of RyR-1 as the D2 region and examine its functional significance. First we cultured skeletal myocytes from mutant mice lacking both RyR-1 and RyR-3. The cells were then transfected with expression plasmids carrying mutated RyR-1 cDNAs with deletions or substituted with the region of RyR-2 corresponding to the D2 region to examine if the mutated RyR-1 can mediate E-C coupling. The results obtained indicate that the presence of the D2 region in RyR-1 is essential for E-C coupling in skeletal muscle but is not for the CICR per se.
The method of generation of mice carrying the disrupted RyR-1 or RyR-3 gene is described elsewhere (10, 11). Neonates simultaneously homozygous for both mutations were obtained by mating double heterozygotes. The genotypes of all the neonates used in the present experiments were determined by polymerase chain reaction analysis (10, 11). Primary cultured myocytes were prepared from newborn mice, and expression plasmids were co-transfected with the green fluorescent protein (GFP) expression plasmid (Life Technologies, Inc.) using LipofectAMINE (Life Technologies, Inc.) as described previously (13). After 3-5 days of culture in differentiation medium, myocytes were used in the experiments. Successfully transfected myocytes were identified by the fluorescence of GFP.
Intracellular Ca2+ MeasurementsCultured cells were incubated in a physiological salt solution (13) containing 20 µM Fura-2 for 30-35 min. The fluorescence intensity of Ca2+ indicator-loaded cultured cells was imaged using a cooled CCD camera (Photometrics) attached to an inverted Olympus IX70 microscope with a 40× (UPlanApo) objective. The excitation wavelength was 470 nm for GFP and 340 nm for Fura-2. Two-dimensional images composed of 128 × 128 pixels were acquired every 0.2 or 0.5 s (13).
Construction of Expression PlasmidsThe plasmid pCAGGS (16)
was digested with HindIII, blunted using Klenow fragment,
and self-ligated to delete the HindIII site. The resulting
plasmid was cleaved with EcoRI and ligated to a synthetic
polylinker carrying EcoRI, XhoI,
HindIII, NotI, and NheI sites to
generate the expression plasmid pCAGPL. The expression plasmid pYT-1
was constructed by inserting the 15-kilobase pair HindIII
fragment from pRRS11 (17), containing the entire coding sequence of the
rabbit RyR-1, into the HindIII site of pCAGPL in the same
orientation with respect to the -actin promoter. The plasmid pYT-2
was generated by deleting nucleotide residues 3907-4218 of the RyR-1
cDNA (see Ref. 18 for the residue numbers) from pYT-1; to generate
the ApaLI site in pYT-2, a base conversion, T to A at
position 4221, was introduced that causes no amino acid substitution.
The plasmids pYT-3 and pYT-4 were generated by deleting residues
3907-4101 and 4069-4218 from pYT-1, respectively; base substitutions
T to A at position 4104 in pYT-3, G to T at position 4068, and T to A
at position 4221 in pYT-4 cause no amino acid changes. The plasmid
pYT-5 was generated by inserting the fragment 3946-4200 of RyR-2
cDNA (see Ref. 19 for the residue numbers) into the
ApaLI site of pYT-2.
Myocytes isolated from the skeletal muscle of
wild-type, RyR-1-deficient, and RyR-3-deficient mice as well as from
double mutant mice lacking both RyR-1 and RyR-3 were cultured. The
cultured cells from the wild-type and RyR-3-deficient mice responded
with an intracellular Ca2+ concentration
([Ca2+]i) increase to electrical stimulation even
in the absence of extracellular Ca2+ (Fig.
1, A and B) in accordance with the
results obtained in intact muscle bundles (11). However, electrical
stimuli were unable to induce an increase in
[Ca2+]i in RyR-1-deficient and double mutant
myocytes in the absence of extracellular Ca2+ (not shown).
These results confirm that RyR-1 is required for skeletal muscle E-C
coupling.
Upon application of 25 mM caffeine, a [Ca2+]i increase was observed in control, RyR-1-deficient, and RyR-3-deficient myocytes (Fig. 1, A, B, and C). However, no caffeine-induced [Ca2+]i increase was observed in double mutant myocytes (Fig. 1D). When cyclopiazonic acid, an inhibitor of SR Ca2+-ATPase (20), was applied to the double mutant myocytes, a [Ca2+]i increase was observed in the absence of extracellular Ca2+ (not shown). Therefore, even though Ca2+ was stored in the SR, caffeine failed to induce Ca2+ release in double mutant myocytes. Caffeine has been shown to induce Ca2+ release through activation of one of the RyR subtypes (12, 21). Hence, the results obtained indicate that no RyR is expressed in the double mutant myocytes.
In our previous studies we showed that RyR-1-deficient myocytes responded with a slow [Ca2+]i increase of long duration to electrical stimulation in the presence of 10 mM Ca2+ and 10 µM Bay K-8644, a Ca2+ channel agonist, in the extracellular solution (10, 12). However, it was not determined whether this [Ca2+]i increase was due solely to an influx of Ca2+ or to CICR from the SR secondary to the Ca2+ influx. Here we show that upon electrical stimulation, a [Ca2+]i increase that was similar in size and kinetics to that of RyR-1-deficient myocytes was induced in double mutant myocytes in the presence of the high concentration of extracellular Ca2+ and Bay K-8644 (Fig. 1, C and D). The peak height of the Fura-2 fluorescence intensity increase relative to the resting fluorescence and the time to reach 50% of the peak height were 1.13 ± 0.02 and 0.32 ± 0.12 s for RyR-1-deficient myocytes and 1.13 ± 0.02 and 0.39 ± 0.14 s for double mutant myocytes (mean ± S.E., n = 8 for both cell types). There was no statistically significant difference in the [Ca2+]i increase between the two types of mutant myocytes (p > 0.3, t test). These observations suggest that the electrically evoked [Ca2+]i increase observed in RyR-1-deficient myocytes was due to an influx of Ca2+ and was independent of CICR through RyR-3, the activation of which requires a relatively high Ca2+ concentration (12).
Ca2+ Response in Myocytes Transfected with Mutated RyR-1 cDNAIn double mutant myocytes transfected with RyR-1
cDNA, a [Ca2+]i increase was observed in
response to electrical stimulation in the absence of extracellular
Ca2+ (see Fig. 3A). When RyR-2 cDNA was
transfected in place of RyR-1, the myocytes failed to respond to
electrical stimulation, although they showed spontaneous
Ca2+ oscillations (not shown). These results are in
accordance with previous results obtained using RyR-1-deficient
myocytes (13, 22).
To determine whether the D2 region is responsible for the functional
difference among the RyR subtypes, we constructed four different
expression plasmids (pYT-2, -3, -4, and -5) carrying mutated RyR-1
cDNAs. The entire D2 region (amino acid residues 1303-1406) was
deleted in pYT-2, whereas either the N-terminal half (1303-1367) or
the C-terminal half (1357-1406) of D2 was deleted in pYT-3 and pYT-4,
respectively (Fig. 2). In pYT-5 the entire D2 region was
replaced by the corresponding sequence of RyR-2 (1316-1400).
In all double mutant myocytes transfected with any of the mutated RyR-1 cDNAs, the [Ca2+]i response to caffeine was recovered (Fig. 3, B-E). Therefore, the mutations in the D2 region had no obvious effect on the Ca2+ release function and responsiveness to caffeine. Double mutant myocytes transfected with either pYT-4 or pYT-5 responded with a [Ca2+]i increase to electrical stimulation even in the absence of extracellular Ca2+ (Fig. 3, D and E). However, electrical stimulation could not induce a [Ca2+]i increase in myocytes transfected with pYT-2 and pYT-3 (Fig. 3, B and C). These results suggest that the presence of the D2 region in RyR-1, especially the C-terminal half of this region (amino acid residues 1303-1356), is indispensable for skeletal muscle E-C coupling. The lack of this region in RyR-3 could be one of the reasons for the inability of RyR-3 to mediate E-C coupling in skeletal muscle. The double mutant myocytes transfected with RyR-2 cDNA did not exhibit E-C coupling and showed Ca2+ oscillations as in the equivalent experiment in RyR-1-deficient myocytes (13). However, E-C coupling in skeletal muscle was recovered when the double mutant myocytes were transfected with mutated RyR-1 cDNA carrying the sequence of the D2 region of RyR-2 (pYT-5). Therefore, the D2 region alone does not determine the functional difference between RyR-1 and RyR-2 in terms of E-C coupling.
In skeletal muscle E-C coupling, direct intermolecular coupling between the DHPR and RyR-1 is assumed to mediate the transmission of signal from the T-tubule to the SR, although the presence of an intervening molecule cannot be excluded at present. The D2 region is relatively hydrophilic (18) and overlaps with one of the protease-sensitive regions (amino acid residues 1220-1360) in RyR-1 (23). Furthermore, it has been shown that cleavage of RyR-1 within the D2 region by calpain results in enhancement of CICR activity (24-26). Therefore, the D2 region seems to be located on the cytoplasmic surface and may have important roles in the control of channel activity. Four negatively charged amino acid residues appear at every other position within the critical site of the D2 region (amino acid residues 1327-1333 in RyR-1) and are conserved between RyR-1 and RyR-2. It is an interesting possibility that the acidic region may participate in the protein-protein interaction in E-C coupling.