2019
DOI: 10.1186/s13072-019-0294-5
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The DNA repair protein SHPRH is a nucleosome-stimulated ATPase and a nucleosome-E3 ubiquitin ligase

Abstract: Background Maintenance of genome integrity during DNA replication is crucial to the perpetuation of all organisms. In eukaryotes, the bypass of DNA lesions by the replication machinery prevents prolonged stalling of the replication fork, which could otherwise lead to greater damages such as gross chromosomal rearrangements. Bypassing DNA lesions and subsequent repair are accomplished by the activation of DNA damage tolerance pathways such as the template switching (TS) pathway. In yeast, the RAD5 … Show more

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Cited by 22 publications
(14 citation statements)
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References 74 publications
(72 reference statements)
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“…2a ), and with the fact that the HSS mutation is not at a lysine or arginine residue, both of which were shown to be important for DNA binding by SANT-SLIDE modules 7 . To exclude that additional DNA binding modules in CHD6, like its chromodomains 48 , 49 , might compensate for the I1600M mutation, we purified and tested the second putative CHD6 SANT-SLIDE module alone in EMSAs. Again, wild-type and mutant CHD6 SANT-SLIDE modules did bind DNA and nucleosomes with similar efficiencies (Supplementary Fig.…”
Section: Resultsmentioning
confidence: 99%
See 1 more Smart Citation
“…2a ), and with the fact that the HSS mutation is not at a lysine or arginine residue, both of which were shown to be important for DNA binding by SANT-SLIDE modules 7 . To exclude that additional DNA binding modules in CHD6, like its chromodomains 48 , 49 , might compensate for the I1600M mutation, we purified and tested the second putative CHD6 SANT-SLIDE module alone in EMSAs. Again, wild-type and mutant CHD6 SANT-SLIDE modules did bind DNA and nucleosomes with similar efficiencies (Supplementary Fig.…”
Section: Resultsmentioning
confidence: 99%
“…Steps from cloning to protein expression and purification were carried out as described previously 48 . In brief, WT and mutant I1600M CHD6-HA cDNAs were cloned into pFastBac1 and the HA tag was replaced by a FLAG tag using PCR and Gibson assembly.…”
Section: Methodsmentioning
confidence: 99%
“…How SHPRH knockdown reduces CHK2 activation is elusive. The reduced CHK2 activation could possibly be caused by lack of the ubiquitin ligase activity of SHPRH and increased stability of other ubiquitin ligases responsible for CHK2 turnover e.g., via SIAH2 [36], or by the recently suggested role of SHPRH as a nucleosome-E3 ubiquitin ligase, which could possibly change the gene expression level of CHK2 [37]. The ubiquitin ligase activity of SHPRH could also regulate degradation of proteins involved in activation of origin firing leading to increased origin firing independent of CHK2.…”
Section: Reduced Phosphorylation Of Chk2 and Mcm2 In Cells Lacking Shprhmentioning
confidence: 99%
“…Steps from cloning to protein expression and purification were carried out as described previously 80 .…”
Section: Chd6 Protein Expression and Purification And In Vitro Assaysmentioning
confidence: 99%
“…All baculoviruses were produced according to the Bac-to-Bac Baculovirus Expression Systems manual (Life Technologies) and CHD6-FLAG protein constructs were next purified from ~4 L of Sf9 insect cell cultures. Purified proteins were used in electrophoretic mobility shift assays (EMSA), as well as in nucleosome mobilization/sliding and restriction enzyme accessibility (REA) assays using DNA and nucleosome substrates as described previously 80 . Detection and quantification of non-radioactive substrates was achieved following staining with SYBR Gold Nucleic Acid Gel Stain (ThermoFisher).…”
Section: Chd6 Protein Expression and Purification And In Vitro Assaysmentioning
confidence: 99%