Long CTG·CAG Repeats from Myotonic Dystrophy Are Preferred Sites for Intermolecular Recombination

Pluciennik, Anna; Iyer, Ravi; Напиерала, Марек; Larson, Jacquelynn E.; Filutowicz, Marcin; Wells, Robert D.

doi:10.1074/jbc.m202127200

Cited by 43 publications

(65 citation statements)

References 83 publications

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“…Oligonucleotide Model Studies: Enzymatic Probing-Two oligonucleotides, d(CAGG) 26 and d(CCTG) 26 , were chemically synthesized to study their structural properties as related to the behavior of unpaired regions of the (CCTG⅐CAGG) repeats during replication and related processes that unwind the duplex. d(CAGG) 26 and d(CCTG) 26 were purified and labeled ("Experimental Procedures").…”

Section: Resultsmentioning

confidence: 99%

“…The individual oligonucleotides (Genosys), d(CCTG) 26 and d(CAGG) 26 , were purified on a 6% denaturing polyacrylamide gel containing 7.5 M urea in glycerol tolerant gel buffer (U. S. Biochemical Corp.). The purified oligonucleotides were labeled at the 5Ј end with 15 units of T4 polynucleotide kinase (U. S. Biochemical Corp.) and [␥-32 P]ATP at 37°C for 1 h. The labeled oligonucleotides were purified on a 6% denaturing polyacrylamide gel.…”

Section: Substrate Preparation For Chemical Modification and Enzymaticmentioning

confidence: 99%

“…Chemical Modifications and Enzymatic Probing-Three chemical probes, osmium tetraoxide (OsO 4 ) (Aldrich), potassium permanganate (KMnO 4 ) (Fisher), and diethyl pyrocarbonate (DEPC) (Sigma), each were used to modify the d(CCTG) 26 oligonucleotide, whereas the latter two chemicals were used to modify the d(CAGG) 26 oligonucleotide. The purified and labeled oligonucleotides (4 -5 ϫ 10 5 cpm/reaction) in 10 mM Tris, 40 mM NaCl, and 10 mM MgCl 2 were denatured by heating at 80°C for 5 min followed by renaturation by gradually decreasing the temperature (2°C/min) to the indicated reaction temperature (61).…”

Section: Substrate Preparation For Chemical Modification and Enzymaticmentioning

confidence: 99%

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Hairpin Structure-forming Propensity of the (CCTG·CAGG) Tetranucleotide Repeats Contributes to the Genetic Instability Associated with Myotonic Dystrophy Type 2

Dere

Напиерала

Ranum

et al. 2004

Journal of Biological Chemistry

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The genetic instabilities of (CCTG⅐CAGG) n tetranucleotide repeats were investigated to evaluate the molecular mechanisms responsible for the massive expansions found in myotonic dystrophy type 2 (DM2) patients. DM2 is caused by an expansion of the repeat from the normal allele of 26 to as many as 11,000 repeats. Genetic expansions and deletions were monitored in an African green monkey kidney cell culture system (COS-7 cells) as a function of the length (30, 114, or 200 repeats), orientation, or proximity of the repeat tracts to the origin (SV40) of replication. As found for CTG⅐CAG repeats related to DM1, the instabilities were greater for the longer tetranucleotide repeat tracts. Also, the expansions and deletions predominated when cloned in orientation II (CAGG on the leading strand template) rather than I and when cloned proximal rather than distal to the replication origin. Biochemical studies on synthetic d(CAGG) 26 and d(CCTG) 26 as models of unpaired regions of the replication fork revealed that d(CAGG) 26 has a marked propensity to adopt a defined base paired hairpin structure, whereas the complementary d(CCTG) 26 lacks this capacity. The effect of orientation described above differs from all previous results with three triplet repeat sequences (including CTG⅐CAG), which are also involved in the etiologies of other hereditary neurological diseases. However, similar to the triplet repeat sequences, the ability of one of the two strands to form a more stable folded structure, in our case the CAGG strand, explains this unorthodox "reversed" behavior.

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Section: Resultsmentioning

confidence: 99%

Section: Substrate Preparation For Chemical Modification and Enzymaticmentioning

confidence: 99%

Section: Substrate Preparation For Chemical Modification and Enzymaticmentioning

confidence: 99%

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Hairpin Structure-forming Propensity of the (CCTG·CAGG) Tetranucleotide Repeats Contributes to the Genetic Instability Associated with Myotonic Dystrophy Type 2

Dere

Напиерала

Ranum

et al. 2004

Journal of Biological Chemistry

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“…Strains and Plasmids-Escherichia coli strain ECF001 contains a chromosomal copy of the pir gene under an arabinose-inducible promoter, Para BAD (22). Construction of plasmids pFW25 (23) and pRK1 (20) was previously described.…”

Section: Methodsmentioning

confidence: 99%

“…5. To conduct our experiments, we used an E. coli strain (ECF001) that carried an arabinose-inducible pir gene on its chromosome (22); it also harbored the ␥ ori containing plasmid, pFW25. In this strain, the replication rate of plasmid pFW25 rises with increasing levels of supplied arabinose (and then levels off).…”

Section: /Iteron Major and Minor Groove Contacts Detected By Methylatmentioning

confidence: 99%

Binding Modes of the Initiator and Inhibitor Forms of the Replication Protein π to the γ ori Iteron of Plasmid R6K

Kunnimalaiyaan

Krüger

Ross

et al. 2004

Journal of Biological Chemistry

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Discerning the interactions between initiator protein and the origin of replication should provide insights into the mechanism of DNA replication initiation. In the ␥ origin of plasmid R6K, the Rep protein, , is distinctive in that it can bind the seven 22-bp iterons in two forms; monomers activate replication, whereas dimers act as inhibitors. In this work, we used wild type and variants of the protein with altered monomer/dimer ratios to study iteron/ interactions. High resolution contact mapping was conducted using multiple techniques (missing base contact probing, methylation protection, base modification, and hydroxyl radical footprinting), and the electrophoretic separation of nucleoprotein complexes allowed us to discriminate between contact patterns produced by monomers and dimers. We also isolated iteron mutants that affected the binding of monomers (only) or both monomers and dimers. The mutational studies and footprinting analyses revealed that, when binding DNA, monomers interact with nucleotides spanning the entire length of the iteron. In contrast, dimers interact with only the left half of the iteron; however, the retained interactions are strikingly similar to those seen with monomers. These results support a model in which Rep protein dimerization disturbs one of two DNA binding domains important for monomer/iteron interaction; the dimer/iteron interaction utilizes only one DNA binding domain.

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Giant SCA8 alleles in nine children whose mother has two moderately large ones

Corral

Genı́s

Banchs

et al. 2005

Annals of Neurology

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We report here a family in which each of nine children has inherited giant SCA8 CTG expansions from a homozygous mother who has two moderately large SCA8 CTG alleles. In contrast, three homozygous male individuals and a case of coexistence of two expansions of the FRDA gene and one of SCA8, all of them with moderately large alleles, have transmitted their respective SCA8 expanded alleles with minor changes, as usually occurs in heterozygous male transmissions.

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Long CTG·CAG Repeats from Myotonic Dystrophy Are Preferred Sites for Intermolecular Recombination

Cited by 43 publications

References 83 publications

Hairpin Structure-forming Propensity of the (CCTG·CAGG) Tetranucleotide Repeats Contributes to the Genetic Instability Associated with Myotonic Dystrophy Type 2

Hairpin Structure-forming Propensity of the (CCTG·CAGG) Tetranucleotide Repeats Contributes to the Genetic Instability Associated with Myotonic Dystrophy Type 2

Binding Modes of the Initiator and Inhibitor Forms of the Replication Protein π to the γ ori Iteron of Plasmid R6K

Giant SCA8 alleles in nine children whose mother has two moderately large ones

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