HMGB1 interacts with XPA to facilitate the processing of DNA interstrand crosslinks in human cells

Mukherjee, Anirban; Vásquez, Karen M.

doi:10.1093/nar/gkv1183

Cited by 25 publications

(37 citation statements)

References 47 publications

(71 reference statements)

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“…The recruitment of NER proteins to ICLs has been directly demonstrated in G1 cells, lending support to the studies conducted with reporter plasmids [32]. In addition to NER factors, mismatch repair (MMR) and HMG proteins have been shown to interact with NER proteins at ICLs and may therefore also contribute to replication-independent repair of ICLs [33, 34]. …”

Section: Replication-independent Icl Repairmentioning

confidence: 79%

Involvement of translesion synthesis DNA polymerases in DNA interstrand crosslink repair

Roy

Schärer

2016

DNA Repair

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DNA interstrand crosslinks (ICLs) covalently join the two strands of a DNA duplex and block essential processes such as DNA replication and transcription. Several important anti-tumor drugs such as cisplatin and nitrogen mustards exert their cytotoxicity by forming ICLs. However, multiple complex pathways repair ICLs and these are thought to contribute to the development of resistance towards ICL-inducing agents. While the understanding of many aspects of ICL repair is still rudimentary, studies in recent years have provided significant insights into the pathways of ICL repair. In this perspective we review the recent advances made in elucidating the mechanism of ICL repair with a focus on the role of TLS polymerases. We describe the emerging models for how these enzymes contribute to and are regulated in ICL repair, discuss the key open questions and examine the implications for this pathway in anti-cancer therapy.

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Section: Replication-independent Icl Repairmentioning

confidence: 79%

Involvement of translesion synthesis DNA polymerases in DNA interstrand crosslink repair

Roy

Schärer

2016

DNA Repair

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“…Cell culture and determination of cisplatin LD 50 values Cells were purchased from ATCC where they perform short tandem repeat profiling for cell line authentication. Cells were cultured as described previously (11). Cells were grown to 80%-90% confluency and were passaged at least three times after thawing before any experiments were performed and were cultured for a period of 6 months to perform all the experiments and repetitions.…”

Section: Methodsmentioning

confidence: 99%

“…We have previously demonstrated that the high-mobility group box 1 (HMGB1) protein binds with high affinity to ICLs and acts as an NER cofactor in human cells (10,11). Other members of the HMGB family, HMGB2 and HMGB3, share sequence and structural similarities with HMGB1 and possess two box domains, boxes A and B; where box A binds DNA and box B bends DNA, and acidic C-terminal tails.…”

Section: Introductionmentioning

confidence: 99%

Targeting the High-Mobility Group Box 3 Protein Sensitizes Chemoresistant Ovarian Cancer Cells to Cisplatin

et al. 2019

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Chemotherapeutic regimens for ovarian cancer often include the use of DNA interstrand crosslink-inducing agents (e.g., platinum drugs) or DNA double-strand break-inducing agents. Unfortunately, the majority of patients fail to maintain a durable response to treatment, in part, due to drug resistance, contributing to a poor survival rate. In this study, we report that cisplatin sensitivity can be restored in cisplatin-resistant ovarian cancer cells by targeting the chromatin-associated high-mobility group box 3 (HMGB3) protein. HMGB proteins have been implicated in the pathogenesis and prognosis of ovarian cancer, and HMGB3 is often upregulated in cancer cells, making it a potential selective target for therapeutic intervention. Depletion of HMGB3 in cisplatin-sensitive and cisplatin-resistant cells resulted in transcriptional downregu-lation of the kinases ATR and CHK1, which attenuated the ATR/CHK1/p-CHK1 DNA damage signaling pathway. HMGB3 was associated with the promoter regions of ATR and CHK1, suggesting a new role for HMGB3 in transcriptional regulation. Furthermore, HMGB3 depletion significantly increased apoptosis in cisplatin-resistant A2780/CP70 cells after cisplatin treatment. Taken together, our results indicate that targeted depletion of HMGB3 attenuates cisplatin resistance in human ovarian cancer cells, increasing tumor cell sensitivity to platinum drugs.Significance: This study shows that targeting HMGB3 is a potential therapeutic strategy to overcome chemoresistance in ovarian cancer.

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“…The functional consequences of HMGB1 binding to damaged DNA have been alternately suggested to be a shielding of the lesion from the repair machinery or enhanced recognition of the damaged site (99,101,102). For example, HMGB1 has been reported to sensitize cells to cisplatin by impeding repair, perhaps influenced by the cellular redox state (103,104); conversely, human HMGB1 has been reported to facilitate nucleotide excision repair (NER) by recruiting the NER protein XPA to interstrand cross-links (105). Interestingly, the recruitment of XPA to nondamaged sites was increased in HMGB1-depleted cells, suggesting that HMGB1 not only promotes NER but also facilitates the specificity of XPA-mediated damage recognition.…”

Section: High Mobility Group Proteinsmentioning

confidence: 99%

Yeast HMO1: Linker Histone Reinvented

Panday

Grove

2017

Microbiol Mol Biol Rev

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SUMMARY Eukaryotic genomes are packaged in chromatin. The higher-order organization of nucleosome core particles is controlled by the association of the intervening linker DNA with either the linker histone H1 or high mobility group box (HMGB) proteins. While H1 is thought to stabilize the nucleosome by preventing DNA unwrapping, the DNA bending imposed by HMGB may propagate to the nucleosome to destabilize chromatin. For metazoan H1, chromatin compaction requires its lysine-rich C-terminal domain, a domain that is buried between globular domains in the previously characterized yeast Saccharomyces cerevisiae linker histone Hho1p. Here, we discuss the functions of S. cerevisiae HMO1, an HMGB family protein unique in containing a terminal lysine-rich domain and in stabilizing genomic DNA. On ribosomal DNA (rDNA) and genes encoding ribosomal proteins, HMO1 appears to exert its role primarily by stabilizing nucleosome-free regions or “fragile” nucleosomes. During replication, HMO1 likewise appears to ensure low nucleosome density at DNA junctions associated with the DNA damage response or the need for topoisomerases to resolve catenanes. Notably, HMO1 shares with the mammalian linker histone H1 the ability to stabilize chromatin, as evidenced by the absence of HMO1 creating a more dynamic chromatin environment that is more sensitive to nuclease digestion and in which chromatin-remodeling events associated with DNA double-strand break repair occur faster; such chromatin stabilization requires the lysine-rich extension of HMO1. Thus, HMO1 appears to have evolved a unique linker histone-like function involving the ability to stabilize both conventional nucleosome arrays as well as DNA regions characterized by low nucleosome density or the presence of noncanonical nucleosomes.

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HMGB1 interacts with XPA to facilitate the processing of DNA interstrand crosslinks in human cells

Cited by 25 publications

References 47 publications

Involvement of translesion synthesis DNA polymerases in DNA interstrand crosslink repair

Involvement of translesion synthesis DNA polymerases in DNA interstrand crosslink repair

Targeting the High-Mobility Group Box 3 Protein Sensitizes Chemoresistant Ovarian Cancer Cells to Cisplatin

Yeast HMO1: Linker Histone Reinvented

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