[
Methods Cell Biol,
1995]
Both the localization and distribution of nucleic acid sequences in genomes and in cells can be visualized by hybridization of labeled probe DNAs to cytological preparations of chromosomes or tissues. With the introduction of nonisotopically labeled nucleotides that could be incorporated into cloned DNAs by enzymatic methods in vitro, it became possible to detect the site of hybridization quickly using antibodies that recognized the modifying group on the nucleotides incorporated into the probe DNA. More recently, nucleotides labeled with a fluorescent molecule have been incorporated into probes by invitro enzymatic reactions and the site of hybridization can then be visualized directly. As fluorescence in situ hybridization provides a rapid and high-resolution method for mapping genes, it is being sued increasingly for mapping cloned DNAs to chromosomes and for the ordering of clones in large-scale genome projects. On the other hand, physically mapped clones can also be used to label chromosomes for analysis of such biological processes as chromosome segregation, pairing in meiosis, and interphase nuclear order. Nonisotopic methods of hybridization are also ideally suited to visualization of mRNA distributions in tissues, because the signal can be detected in thick specimens, in contrast to isotopic methods that require thin specimens for detection by autoradiography...
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Orphanet J Rare Dis,
2020]
BACKGROUND: Pathogenic variations in the gene encoding the skeletal muscle ryanodine receptor (RyR1) are associated with malignant hyperthermia (MH) susceptibility, a life-threatening hypermetabolic condition and RYR1-related myopathies (RYR1-RM), a spectrum of rare neuromuscular disorders. In RYR1-RM, intracellular calcium dysregulation, post-translational modifications, and decreased protein expression lead to a heterogenous clinical presentation including proximal muscle weakness, contractures, scoliosis, respiratory insufficiency, and ophthalmoplegia. Preclinical model systems of RYR1-RM and MH have been developed to better understand underlying pathomechanisms and test potential therapeutics. METHODS: We conducted a comprehensive scoping review of scientific literature pertaining to RYR1-RM and MH preclinical model systems in accordance with the PRISMA Scoping Reviews Checklist and the framework proposed by Arksey and O'Malley. Two major electronic databases (PubMed and EMBASE) were searched without language restriction for articles and abstracts published between January 1, 1990 and July 3, 2019. RESULTS: Our search yielded 5049 publications from which 262 were included in this review. A majority of variants tested in RYR1 preclinical models were localized to established MH/central core disease (MH/CCD) hot spots. A total of 250 unique RYR1 variations were reported in human/rodent/porcine models with 95% being missense substitutions. The most frequently reported RYR1 variant was R614C/R615C (human/porcine total n=39), followed by Y523S/Y524S (rabbit/mouse total n=30), I4898T/I4897T/I4895T (human/rabbit/mouse total n=20), and R163C/R165C (human/mouse total n=18). The dyspedic mouse was utilized by 47% of publications in the rodent category and its RyR1-null (1B5) myotubes were transfected in 23% of publications in the cellular model category. In studies of transfected HEK-293 cells, 57% of RYR1 variations affected the RyR1 channel and activation core domain. A total of 15 RYR1 mutant mouse strains were identified of which ten were heterozygous, three were compound heterozygous, and a further two were knockout. Porcine, avian, zebrafish, C. elegans, canine, equine, and drosophila model systems were also reported. CONCLUSIONS: Over the past 30years, there were 262 publications on MH and RYR1-RM preclinical model systems featuring more than 200 unique RYR1 variations tested in a broad range of species. Findings from these studies have set the foundation for therapeutic development for MH and RYR1-RM.