Broad segmental progeroid changes in short-lived <i>Ercc1</i> <sup>−/Δ7</sup> mice

Dollé, Martijn E.T.; Kuiper, Raoul V.; Roodbergen, Marianne; Robinson, Joke; Vlugt, Sisca de; Wijnhoven, Susan; Beems, Rudolf B.; Fonteyne, Liset de la; Pluijm, Ingrid van der; Niedernhofer, Laura J.; Hasty, Paul; Vijg, Jan; Hoeijmakers, Jan H.J.; Steeg, Harry van

doi:10.3402/pba.v1i0.7219

Cited by 87 publications

(157 citation statements)

References 26 publications

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“…To verify the presence of an 8-oxoG and abasic site (THF residue) in the loop region of the substrates, we initially probed the formation of hairpins in the CAG repeat tract of the substrates using ssDNA-specific nucleases, Mung Bean Nuclease and S1 Nuclease. We found that Mung Bean Nuclease cleavage on the (CAG) 7 14 -THF hairpin substrate, the nuclease cleavage led to production of products with 45, 48 and 52 nt (Figure 2.3, lanes 7-9), whereas S1 Nuclease cleavage on the (CAG) 14 -8-oxoG and (CAG) 14 -THF hairpin substrates resulted in products with 45, 49, 51 and 54 nt (Figure 2.2 and 2.4, lanes 7-9). This indicates that the substrates contained a hairpin with a (CAG) 4 loop with an 8-oxoG or THF residue and 10 CAG repeats in the stem region.…”

Section: A Dna Base Lesion Located In a Cag Repeat Hairpin Loop Can Bmentioning

confidence: 88%

“…Substrates containing a (CAG) 7 or (CAG) 14 hairpin with an 8-oxoG or a tetrahydrofuran (THF), an abasic site analog (used to represent an oxidized sugar in this study), located in the hairpin loop region were designed to mimic a TNR hairpin with a base lesion in the hairpin loop region. Substrates were constructed by annealing the damaged strands that contained (CAG) 13 or (CAG) 20 repeats to their template strand containing (CTG) 7 repeats at a molar ratio of 1:1.…”

Section: Oligonucleotide Substratesmentioning

confidence: 99%

“…In vitro BER of an 8-oxoG or oxidized abasic site (THF) in the loop region of CAG repeat hairpins with varying sizes was performed by incubating 25 nM substrates containing a (CAG) 7 or (CAG) 14 Substrates and products were separated by 15% urea-denaturing polyacrylamide gel electrophoresis and detected by a Pharos FX Plus PhosphorImager from Bio-Rad.…”

Section: In Vitro Ber Reconstituted With Purified Enzymesmentioning

confidence: 99%

“…The enzyme removes an 8-oxoG in a CAG hairpin loop that is detached from duplex DNA 700-fold slower than it does in duplex DNA (204). To determine if OGG1 can remove an 8-oxoG in a CAG hairpin loop that is located in duplex DNA, we examined OGG1 cleavage of an 8-oxoG in the loop region of a (CAG) 7 or (CAG) 14 hairpin in a CAG repeat tract. To verify the presence of an 8-oxoG and abasic site (THF residue) in the loop region of the substrates, we initially probed the formation of hairpins in the CAG repeat tract of the substrates using ssDNA-specific nucleases, Mung Bean Nuclease and S1 Nuclease.…”

Section: A Dna Base Lesion Located In a Cag Repeat Hairpin Loop Can Bmentioning

confidence: 99%

“…To determine if removal of an 8-oxoG and an abasic lesion located at a CAG repeat hairpin may result in any repaired product, we reconstituted BER for removing a base lesion in the loop region of a (CAG) 7 or (CAG) 14 hairpin substrate. Surprisingly, we found that BER in the small (CAG) 7 hairpin loop generated a product with the same length as the template strand.…”

Section: Ber Of a Base Lesion In The Loop Region Of A Cag Repeat Hairmentioning

confidence: 99%

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Oxidative DNA Damage Modulates Trinucleotide Repeat Instability Via DNA Base Excision Repair

Xu¹

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Section: A Dna Base Lesion Located In a Cag Repeat Hairpin Loop Can Bmentioning

confidence: 88%

Section: Oligonucleotide Substratesmentioning

confidence: 99%

Section: In Vitro Ber Reconstituted With Purified Enzymesmentioning

confidence: 99%

Section: A Dna Base Lesion Located In a Cag Repeat Hairpin Loop Can Bmentioning

confidence: 99%

Section: Ber Of a Base Lesion In The Loop Region Of A Cag Repeat Hairmentioning

confidence: 99%

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Oxidative DNA Damage Modulates Trinucleotide Repeat Instability Via DNA Base Excision Repair

Xu¹

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Nucleotide Excision Repair and Transcription‐Associated Genome Instability

et al. 2019

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Transcription is a potential threat to genome integrity, and transcription‐associated DNA damage must be repaired for proper messenger RNA (mRNA) synthesis and for cells to transmit their genome intact into progeny. For a wide range of structurally diverse DNA lesions, cells employ the highly conserved nucleotide excision repair (NER) pathway to restore their genome back to its native form. Recent evidence suggests that NER factors function, in addition to the canonical DNA repair mechanism, in processes that facilitate mRNA synthesis or shape the 3D chromatin architecture. Here, these findings are critically discussed and a working model that explains the puzzling clinical heterogeneity of NER syndromes highlighting the relevance of physiological, transcription‐associated DNA damage to mammalian development and disease is proposed.

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Intrinsic DNA damage repair deficiency results in progressive microglia loss and replacement

Zhang

Heng

Kooistra

et al. 2020

Glia

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The DNA excision repair protein Ercc1 is important for nucleotide excision, double strand DNA break, and interstrand DNA crosslink repair. In constitutive Ercc1‐knockout mice, microglia display increased phagocytosis, proliferation and an enhanced responsiveness to lipopolysaccharide (LPS)‐induced peripheral inflammation. However, the intrinsic effects of Ercc1‐deficiency on microglia are unclear. In this study, Ercc1 was specifically deleted from Cx3cr1‐expressing cells and changes in microglia morphology and immune responses at different times after deletion were determined. Microglia numbers were reduced with approximately 50% at 2–12 months after Ercc1 deletion. Larger and more ramified microglia were observed following Ercc1 deletion both in vivo and in organotypic hippocampal slice cultures. Ercc1‐deficient microglia were progressively lost, and during this period, microglia proliferation was transiently increased. Ercc1‐deficient microglia were gradually replaced by nondeficient microglia carrying a functional Ercc1 allele. In contrast to constitutive Ercc1‐deficient mice, microglia‐specific deletion of Ercc1 did not induce microglia activation or increase their responsiveness to a systemic LPS challenge. Gene expression analysis suggested that Ercc1 deletion in microglia induced a transient aging signature, which was different from a priming or disease‐associated microglia gene expression profile.

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Broad segmental progeroid changes in short-lived Ercc1 ^−/Δ7 mice

Cited by 87 publications

References 26 publications

Oxidative DNA Damage Modulates Trinucleotide Repeat Instability Via DNA Base Excision Repair

Oxidative DNA Damage Modulates Trinucleotide Repeat Instability Via DNA Base Excision Repair

Nucleotide Excision Repair and Transcription‐Associated Genome Instability

Intrinsic DNA damage repair deficiency results in progressive microglia loss and replacement

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Broad segmental progeroid changes in short-lived Ercc1 −/Δ7 mice

Cited by 87 publications

References 26 publications

Oxidative DNA Damage Modulates Trinucleotide Repeat Instability Via DNA Base Excision Repair

Oxidative DNA Damage Modulates Trinucleotide Repeat Instability Via DNA Base Excision Repair

Nucleotide Excision Repair and Transcription‐Associated Genome Instability

Intrinsic DNA damage repair deficiency results in progressive microglia loss and replacement

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Broad segmental progeroid changes in short-lived Ercc1 ^−/Δ7 mice