Regina Groisman scite author profile

It is well known that histone acetylases are important chromatin modifiers and that they play a central role in chromatin transcription. Here, we present evidence for novel roles of histone acetylases. The TIP60 histone acetylase purifies as a multimeric protein complex. Besides histone acetylase activity on chromatin, the TIP60 complex possesses ATPase, DNA helicase, and structural DNA binding activities. Ectopic expression of mutated TIP60 lacking histone acetylase activity results in cells with defective double-strand DNA break repair. Importantly, the resulting cells lose their apoptotic competence, suggesting a defect in the cells' ability to signal the existence of DNA damage to the apoptotic machinery. These results indicate that the histone acetylase TIP60-containing complex plays a role in DNA repair and apoptosis.

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The Ubiquitin Ligase Activity in the DDB2 and CSA Complexes Is Differentially Regulated by the COP9 Signalosome in Response to DNA Damage

Groisman

Polanowska

Kuraoka

et al. 2003

Cell

664

738

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Nucleotide excision repair (NER) is a major cellular defense against the carcinogenic effects of ultraviolet light from the sun. Mutational inactivation of NER proteins, like DDB and CSA, leads to hereditary diseases such as xeroderma pigmentosum (XP) and Cockayne syndrome (CS). Here, we show that DDB2 and CSA are each integrated into nearly identical complexes via interaction with DDB1. Both complexes contain cullin 4A and Roc1 and display ubiquitin ligase activity. They also contain the COP9 signalosome (CSN), a known regulator of cullin-based ubiquitin ligases. Strikingly, CSN differentially regulates ubiquitin ligase activity of the DDB2 and CSA complexes in response to UV irradiation. Knockdown of CSN with RNA interference leads to defects in NER. These results suggest that the distinct UV response of the DDB2 and CSA complexes is involved in diverse mechanisms of NER.

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Retinoblastoma protein represses transcription by recruiting a histone deacetylase

Magnaghi-Jaulin

Groisman

Naguibneva

et al. 1998

Nature

863

657

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The retinoblastoma tumour-suppressor protein Rb inhibits cell proliferation by repressing a subset of genes that are controlled by the E2F family of transcription factors and which are involved in progression from the G1 to the S phase of the cell cycle. Rb, which is recruited to target promoters by E2F1, represses transcription by masking the E2F1 transactivation domain and by inhibiting surrounding enhancer elements, an active repression that could be crucial for the proper control of progression through the cell cycle. Some transcriptional regulators act by acetylating or deacetylating the tails protruding from the core histones, thereby modulating the local structure of chromatin: for example, some transcriptional repressors function through the recruitment of histone deacetylases. We show here that the histone deacetylase HDAC1 physically interacts and cooperates with Rb. In HDAC1, the sequence involved is an LXCXE motif, similar to that used by viral transforming proteins to contact Rb. Our results strongly suggest that the Rb/HDAC1 complex is a key element in the control of cell proliferation and differentiation and that it is a likely target for transforming viruses.

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Structural Basis of UV DNA-Damage Recognition by the DDB1–DDB2 Complex

Scrima

Koníčková

Czyzewski

et al. 2008

Cell

378

429

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Ultraviolet (UV) light-induced pyrimidine photodimers are repaired by the nucleotide excision repair pathway. Photolesions have biophysical parameters closely resembling undamaged DNA, impeding discovery through damage surveillance proteins. The DDB1-DDB2 complex serves in the initial detection of UV lesions in vivo. Here we present the structures of the DDB1-DDB2 complex alone and bound to DNA containing either a 6-4 pyrimidine-pyrimidone photodimer (6-4PP) lesion or an abasic site. The structure shows that the lesion is held exclusively by the WD40 domain of DDB2. A DDB2 hairpin inserts into the minor groove, extrudes the photodimer into a binding pocket, and kinks the duplex by approximately 40 degrees. The tightly localized probing of the photolesions, combined with proofreading in the photodimer pocket, enables DDB2 to detect lesions refractory to detection by other damage surveillance proteins. The structure provides insights into damage recognition in chromatin and suggests a mechanism by which the DDB1-associated CUL4 ubiquitin ligase targets proteins surrounding the site of damage.

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The microRNA miR-181 targets the homeobox protein Hox-A11 during mammalian myoblast differentiation

Naguibneva¹,

Ameyar-Zazoua²,

Polesskaya³

et al. 2006

Nat Cell Biol

542

399

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Deciphering the mechanisms underlying skeletal muscle-cell differentiation in mammals is an important challenge. Cell differentiation involves complex pathways regulated at both transcriptional and post-transcriptional levels. Recent observations have revealed the importance of small (20-25 base pair) non-coding RNAs (microRNAs or miRNAs) that are expressed in both lower organisms and in mammals. miRNAs modulate gene expression by affecting mRNA translation or stability. In lower organisms, miRNAs are essential for cell differentiation during development; some miRNAs are involved in maintenance of the differentiated state. Here, we show that miR-181, a microRNA that is strongly upregulated during differentiation, participates in establishing the muscle phenotype. Moreover, our results suggest that miR-181 downregulates the homeobox protein Hox-A11 (a repressor of the differentiation process), thus establishing a functional link between miR-181 and the complex process of mammalian skeletal-muscle differentiation. Therefore, miRNAs can be involved in the establishment of a differentiated phenotype - even when they are not expressed in the corresponding fully differentiated tissue.

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CSA-dependent degradation of CSB by the ubiquitin–proteasome pathway establishes a link between complementation factors of the Cockayne syndrome

Groisman¹,

Kuraoka²,

Chevallier³

et al. 2006

Genes Dev.

221

180

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Mutations in the CSA or CSB complementation genes cause the Cockayne syndrome, a severe genetic disorder that results in patients' death in early adulthood. CSA and CSB act in a transcription-coupled repair (TCR) pathway, but their functional relationship is not understood. We have previously shown that CSA is a subunit of an E3 ubiquitin ligase complex. Here we demonstrate that CSB is a substrate of this ligase: Following UV irradiation, CSB is degraded at a late stage of the repair process in a proteasome-and CSA-dependent manner. Moreover, we demonstrate the importance of CSB degradation for post-TCR recovery of transcription and for the Cockayne syndrome. Our results unravel for the first time the functional relationship between CSA and CSB. DNA damage represents a major threat for the maintenance of genomic integrity, and a variety of cellular pathways recognize and repair defects in DNA structure. Repair of UV-light-induced pyrimidine dimers or of adducts created by cisplatin is carried out by the nucleotide excision repair (NER) pathway. This pathway is impaired in several diseases such as Xeroderma pigmentosum (XP), Cockayne syndrome (CS), trichothiodystrophy (TTD), and the mild ultraviolet (UV)-light-sensitive syndrome (Bootsma et al. 1998).NER proceeds via two alternative pathways: The global genome repair (GGR) is involved in the repair of any sequence in the genome regardless of its transcriptional status; the transcription-coupled repair (TCR) is only involved in the repair of actively transcribed DNA strands. TCR occurs at a higher rate than GGR, but the reason for this difference is not fully understood. Most of the events of the two pathways are identical; in both cases, DNA unwinding is followed by excision of a 27-30-nucleotide oligonucleotide fragment containing the photoproduct of the damaged DNA strand and its replacement by de novo synthesis using the opposite, untouched, DNA strand as the template. Thus, the major difference between GGR and TCR occurs at the level of recognition of the DNA damage. In the GGR pathway, the damage is initially recognized via a direct interaction of NER proteins XPE and XPC-HR23B with damaged DNA. In contrast, in TCR, damages appear to be signaled via the stalling of RNA polymerase II (Pol II). The release of RNA polymerase involves two proteins, CSA and CSB, but their mode of action is unknown (Friedberg et al. 1995;Svejstrup 2002).CSA and CSB are TCR factors, the mutation of which causes the Cockayne syndrome. CSB is a member of the SWI2/SNF2 family of ATP-dependent chromatin remodeling factors and has the activities of SWI2/SNF2 proteins (Troelstra et al. 1992): DNA-dependent ATPase (but not classical helicase) (Selby and Sancar 1997b;Citterio et al. 1998), nucleosome remodeling, and interaction with core histones . In addition, CSB locally influences the DNA conformation, likely by wrapping the DNA around itself (Beerens et al. 2005), thereby modifying the interface between stalled RNA polymerase II and DNA. This modification promotes DNA repair or allows ...

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The secreted glycoprotein CREG enhances differentiation of NTERA-2 human embryonal carcinoma cells

et al. 2000

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Translational control of TWIST1 expression in MCF-10A cell lines recapitulating breast cancer progression

Vislovukh

Meng

et al. 2012

Oncogene

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TWIST1 is a highly conserved basic helix-loop-helix transcription factor that promotes epithelial --mesenchymal transition (EMT). Its misregulation has been observed in various types of tumors. Using the MCF-10A-series of cell lines that recapitulate the early stages of breast cancer formation and EMT, we found TWIST1 to be upregulated during EMT and downregulated early in carcinogenesis. The TWIST1 3 0 UTR contains putative regulatory elements, including miRNA target sites and two cytoplasmic polyadenylation elements (CPE). We found that miR-580, CPEB1, and CPEB2 act as negative regulators of TWIST1 expression in a sequence-specific and additive/cooperative manner.

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Regina Groisman

Involvement of the TIP60 Histone Acetylase Complex in DNA Repair and Apoptosis

The Ubiquitin Ligase Activity in the DDB2 and CSA Complexes Is Differentially Regulated by the COP9 Signalosome in Response to DNA Damage

Retinoblastoma protein represses transcription by recruiting a histone deacetylase

Structural Basis of UV DNA-Damage Recognition by the DDB1–DDB2 Complex

The microRNA miR-181 targets the homeobox protein Hox-A11 during mammalian myoblast differentiation

CSA-dependent degradation of CSB by the ubiquitin–proteasome pathway establishes a link between complementation factors of the Cockayne syndrome

The secreted glycoprotein CREG enhances differentiation of NTERA-2 human embryonal carcinoma cells

Translational control of TWIST1 expression in MCF-10A cell lines recapitulating breast cancer progression

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