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Query: UNIPROT:P21817 (
RyR1
)
1,154
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The skeletal isoform of Ca2+ release channel,
RyR1
, plays a central role in activation of skeletal muscle contraction. Another isoform,
RyR3
, has been observed recently in some mammalian skeletal muscles, but whether it participates in regulating skeletal muscle contraction is not known. The expression of
RyR3
in skeletal muscles was studied in mice from late fetal stages to adult life.
RyR3
was found to be expressed widely in murine skeletal muscles during the post-natal phase of muscle development, but was not detectable in muscles of adult mice, with the exception of the diaphragm and soleus muscles.
RyR3
knockout mice were generated, and it was shown that skeletal muscle contraction in these mice was impaired during the first weeks after birth. In skeletal muscles isolated from newborn
RyR3
(-/- )mice, but not in those from adult mice, the twitch elicited by electrical stimulation and the contracture induced by caffeine were strongly depressed. These results provide the first evidence that
RyR3
has a physiological role in excitation-contraction coupling of neonatal skeletal muscles. The disproportion between the low amount of
RyR3
and the large impact of the
RyR3
knockout suggests that this isoform contributes to the amplification of Ca2+ released by the existing population of ryanodine receptors (
RyR1
).
...
PMID:Requirement for the ryanodine receptor type 3 for efficient contraction in neonatal skeletal muscles. 938 75
Skeletal muscle contraction is triggered by the release of Ca2+ from the sarcoplasmic reticulum through the type 1 ryanodine receptor (
RyR1
). Recently it has been shown that also the type 3 isoform of ryanodine receptor (
RyR3
), which is expressed in some mammalian skeletal muscles, may participate in the regulation of skeletal muscle contraction. Here we report the generation and the characterization of double mutant mice carrying a targeted disruption of both the
RyR1
and the
RyR3
genes (
RyR1
-/-;
RyR3
-/-). Skeletal muscles from mice homozygous for both mutations are unable to contract in response to caffeine and to ryanodine. In addition, they show a very poor capability to develop tension when directly activated with micromolar [Ca2+]i after membrane permeabilization which indicates either poor development or degeneration of the myofibrils. This was confirmed by biochemical analysis of contractile proteins. Electron microscopy confirms small size of myofibrils and shows complete absence of feet (RyRs) in the junctional SR.
...
PMID:Contractile impairment and structural alterations of skeletal muscles from knockout mice lacking type 1 and type 3 ryanodine receptors. 948 97
Single-channel analysis of sarcoplasmic reticulum vesicles prepared from diaphragm muscle, which contains both
RyR1
and
RyR3
isoforms, revealed the presence of two functionally distinct ryanodine receptor calcium release channels. In addition to channels with properties typical of
RyR1
channels, a second population of ryanodine-sensitive channels with properties distinct from those of
RyR1
channels was observed. The novel channels displayed close-to-zero open-probability at nanomolar Ca2+ concentrations in the presence of 1 mM ATP, but were shifted to the open conformation by increasing Ca2+ to micromolar levels and were not inhibited at higher Ca2+ concentrations. These novel channels were sensitive to the stimulatory effects of cyclic adenosine 5'-diphosphoribose (cADPR). Detection of this second population of RyR channels in lipid bilayers was always associated with the presence of the
RyR3
isoform in muscle preparations used for single-channel measurements and was abrogated by the knockout of the
RyR3
gene in mice. Based on the above, we associated the novel population of channels with the
RyR3
isoform of Ca2+ release channels. The functional properties of the
RyR3
channels are in agreement with a potential qualitative contribution of this channel to Ca2+ release in skeletal muscle and in other tissues.
...
PMID:Functional properties of the ryanodine receptor type 3 (RyR3) Ca2+ release channel. 958 72
Ryanodine receptors (RyRs), which form Ca2+ channels in the membrane of the endoplasmic reticulum, consist of three subtypes (
RyR1
, RyR2, and
RyR3
). The RyRs release Ca2+ from the endoplasmic reticulum into the cytoplasm and thus play an important role, especially in the contraction of skeletal and cardiac muscle cells. The genes of these RyRs are also expressed in many non-muscle tissues, but the role played by RyRs in non-muscle cells is not fully understood. In the present study, we examined the morphological changes in such cells caused by a deficiency of RyRs genes using three mutant mice lacking
RyR1
,
RyR3
, or both
RyR1
and
RyR3
. The results showed morphological abnormalities in the adrenal cortical cells in all three mutant mice. In addition, an excessive accumulation of glycogen granules in hepatic cells, and a hypertrophy of the liver were both present in those mutant mice lacking both
RyR1
and
RyR3
. We discuss the relationship between the morphological abnormalities of the adrenal cortex and liver induced by a deficiency of RyRs, and the possible causes of these abnormalities.
...
PMID:Morphological abnormalities of adrenal gland and hypertrophy of liver in mutant mice lacking ryanodine receptors. 979 64
The role of intracellular Ca2+ release in the activation of human bladder smooth muscle is controversial. We have measured the expression of mRNA encoding for the ryanodine receptor (RyR) isoforms (
RyR1
, RyR2 and
RyR3
) in isolated human detrusor smooth muscle. mRNA for RyR2 was detected in all samples but no mRNA for
RyR1
or
RyR3
could be found. Human bladder smooth muscle cells in culture are unresponsive to caffeine, suggesting the absence of a functional RyR system. However, mRNA encoding for RyR2 was detected in these cells. Using saponin-permeabilized cells, a Ruthenium Red-sensitive Ca(2+)-dependent 45Ca2+ release could be demonstrated from the sarcoplasmic reticulum (SR). These data confirm the functional presence of Ca(2+)-induced Ca2+ release (CICR) in cells and suggest that the properties of the RyR2 isoform in human detrusor may change when the cells are maintained in culture. The implications of these observations to detrusor smooth muscle function are discussed.
...
PMID:Ryanodine receptors in human bladder smooth muscle. 1008 5
We characterized type 3 ryanodine receptor (
RyR3
) purified from rabbit diaphragm by immunoaffinity chromatography using a specific antibody. The purified receptor was free from 12-kDa FK506-binding protein, although it retained the ability to bind 12-kDa FK506-binding protein. Negatively stained images of
RyR3
show a characteristic rectangular structure that was indistinguishable from
RyR1
. The location of the D2 segment, which exists uniquely in the
RyR1
isoform, was determined as the region around domain 9 close to the corner of the square-shaped assembly, with use of D2-directed antibody as a probe. The
RyR3
homotetramer had a single class of high affinity [3H]ryanodine-binding sites with a stoichiometry of 1 mol/mol. In planar lipid bilayers,
RyR3
displayed cation channel activity that was modulated by several ligands including Ca2+, Mg2+, caffeine, and ATP, which is consistent with [3H]ryanodine binding activity.
RyR3
showed a slightly larger unit conductance and a longer mean open time than
RyR1
. Whereas
RyR1
showed two classes of channel activity with distinct open probabilities (Po),
RyR3
displayed a homogeneous and steeply Ca2+-dependent activity with Po approximately 1.
RyR3
was more steeply affected in the channel activity by sulfhydryl-oxidizing and -reducing reagents than
RyR1
, suggesting that the channel activity of
RyR3
may be transformed more precipitously by the redox state. This is also a likely explanation for the difference in the Ca2+ dependence of
RyR3
between [3H]ryanodine binding and channel activity.
...
PMID:Further characterization of the type 3 ryanodine receptor (RyR3) purified from rabbit diaphragm. 1035 90
The type 3 ryanodine receptor (
RyR3
) is a ubiquitous calcium release channel that has recently been found in mammalian skeletal muscles. However, in contrast to the skeletal muscle isoform (
RyR1
), neither the subcellular distribution nor the physiological role of
RyR3
are known. Here, we used isoform-specific antibodies to localize
RyR3
in muscles of normal and RyR knockout mice. In normal hind limb and diaphragm muscles of young mice,
RyR3
was expressed in all fibers where it was codistributed with
RyR1
and with the skeletal muscle dihydropyridine receptor. This distribution pattern indicates that
RyR3
is localized in the triadic junctions between the transverse tubules and the sarcoplasmic reticulum. During development,
RyR3
expression declined rapidly in some fibers whereas other fibers maintained expression of
RyR3
into adulthood. Comparing the distribution of
RyR3
-containing fibers with that of known fiber types did not show a direct correlation. Targeted deletion of the
RyR1
or
RyR3
gene resulted in the expected loss of the targeted isoform, but had no adverse effects on the expression and localization of the respective other RyR isoform. The localization of
RyR3
in skeletal muscle triads, together with
RyR1
, is consistent with an accessory function of
RyR3
in skeletal muscle excitation-contraction coupling.
...
PMID:Type 3 and type 1 ryanodine receptors are localized in triads of the same mammalian skeletal muscle fibers. 1044 70
Three genomically distinct isoforms of RyR are now known.
RyR1
homologue is the primary isoform in skeletal muscles, whereas in cardiac muscles it is RyR2 homologue.
RyR3
homologue occurs ubiquitously in many cells, but the biological function is little known, partly because of its minuscule amount in mammalian cells. The difference among RyR isoforms may not be so great in CICR activity, in other words, in the interaction of RyR isoforms with Ca2+, adenine nucleotides and caffeine. Species specificity among
RyR1
homologues may be more important in the apparent difference between
RyR1
and
RyR3
homologues. CICR is likely to be the dominant underlying mechanism for E-C coupling in the cardiac muscle and probably in cells other than the skeletal muscle where the significance of CICR is controversial in physiological contraction. In E-C coupling of skeletal muscle (DICR), the reciprocal tight interactions between DHPR and
RyR1
are critically required. The alpha 1 subunit of DHPR was only the main target of our current interests in the interaction with
RyR1
; the involvement of auxiliary subunits of alpha 2/delta and beta subunits and their mutual interactions, however, are also important. DICR and CICR in
RyR1
share common properties of stimulation by concentrated solutes and modulation by luminal calcium or Ca2+, suggesting that the main difference between the two Ca2+ release mechanisms may be in the gating mechanism of the channel. Further investigations are required to understand molecular interactions during E-C coupling.
...
PMID:Ryanodine receptor isoforms in excitation-contraction coupling. 1046 72
Skeletal muscle expresses at least two isoforms of the calcium release channel in the sarcoplasmic reticulum (
RyR1
and
RyR3
). Whereas the function of
RyR1
is well defined, the physiological significance of
RyR3
is unclear. Some authors have suggested that
RyR3
participates in excitation-contraction coupling and that
RyR3
may specifically confer resistance to fatigue. To test this hypothesis, we measured contractile function of diaphragm strips from adult
RyR3
-deficient mice (exon 2-targeted mutation) and their heterozygous and wild-type littermates. In unfatigued diaphragm, there were no differences in isometric contractile properties (twitch characteristics, force-frequency relationships, maximal force) among the three groups. Our fatigue protocol (30 Hz, 0.25 duty cycle, 37 degrees C) depressed force to 25% of the initial force; however, lack of
RyR3
did not accelerate the decline in force production. The force-frequency relationship was shifted to higher frequencies and was depressed in fatigued diaphragm; lack of
RyR3
did not exaggerate these changes. We therefore provide evidence that
RyR3
deficiency does not alter contractile function of adult muscle before, during, or after fatigue.
...
PMID:Contractile function is unaltered in diaphragm from mice lacking calcium release channel isoform 3. 1051 63
Amyotrophic lateral sclerosis is characterized by motoneuron degeneration, in which glutamate-induced cell death is thought to play a pathogenic role. This excitotoxic process is mediated by cytosolic Ca2+ overload. The glutamatergic ionotropic channel molecules, which constitute a major route of Ca2+ entry, were present on cultured spinal motoneurons. Using ratio RT-PCR, the relative presence in isolated motoneurons of the GluR subunits of the alpha-amino-3-hydroxy-5-methyl-4-isoxazole-propionic acid (AMPA) receptor was evaluated. GluR1 and GluR2 mRNAs were present abundantly, while GluR3 and GluR4 mRNAs were much less abundant. The relative amount of mRNAs encoding the different protein isoforms responsible for Ca2+ uptake into the internal stores and for controlled release of Ca2+ from these stores was also determined. For the sarco/endoplasmic reticulum Ca2+ ATPases (SERCAs), only the SERCA2b class 4 splice variant was found. The inositol 1,4,5-trisphosphate receptor (IP3R) mRNAs were mainly transcribed from the IP3RI and IP3RII genes. Heterogeneity was also observed for the ryanodine receptors (RyR) as the
RyR1
, RyR2 and
RyR3
mRNAs were present.
...
PMID:Calcium handling proteins in isolated spinal motoneurons. 1057 26
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