1. Introduction
Chromatin consists of the DNA and all proteins involved in organizing and regulating DNA structure. The building block of chromatin is the nucleosome, which is composed of 146 base pairs of DNA and a core histone octamer. The core histone oactomer is composed of two heterodimers of histone H2A and histone H2B and a tetramer of histone H3 and histone H4 [1]. The overall chromatin structure is very dynamic in response to diverse biological events. Regulation of chromatin structure is achieved by two major mechanisms. The first is posttranslational modification (PTM) of histones and other chromatin proteins via phosphorylation, methylation, acetylation, ubiquitination and sumoylation [2, 3]. The second is through ATP-dependent nucleosome structure alteration. Cooperation between histone PTMs and chromatin remodelers allows chromatin remodeling to regulate diverse biological events including transcription, chromosome segregation, DNA replication, and DNA repair. In this chapter, we summarize how chromatin structure is regulated during DNA damage response (DDR), focusing particularly on three PTMs: phosphorylation, Poly(ADP-ribosyl)ation (PARylation) and sumoylation. We discuss the DDR in a highly compacted chromatic structure, heterochromatin, as well as the interplay between chromatin remodeling, DNA damage and human aging.
2. DNA damage response
2.1. Sources leading to DNA damage
In order to maintain DNA fidelity, cells must overcome multiple challenges that threaten genome stability. Cues cause DNA damages can be divided into spontaneous and environment-induced. Spontaneous DNA damages are usually caused by intracellular metabolism stress, or formed during genetically programmed processes such as V (variable), D (diversity), and J (joining) (V(D)J) recombination in developing vertebrate lymphocytes or meiotic recombination in germ cells [4, 5]. The major types of damage include aberrant conformations of DNA, chemical instability of DNA, free radicals of oxygen, endogenous mutagens and errors in DNA replications [6]. Environmental DNA damages generally refer to exposure of cells to various genotoxic agents. These agents contain both physical factors, such as ultraviolet (UV), visible light and ionizing radiation; as well as chemical factors, such as alkylating agents, benzopyrene, aflatoxins and cis-Platinum. These DNA damages can lead to single base mutation or more deleterious chromosomal lesion.
2.2. DDR pathway
To maintain genome stability, cells have developed a global signaling network, known as the DNA damage response (DDR), to sense different types of genotoxic stress, to modulate cell cycle transitions and transcriptional process, and to stimulate DNA repair. Mechanistically, proteins involved in the DDR signaling network can be grouped into three major classes: 1) Sensors, acting at the upstream of DDR by recognizing the DNA damage and initiating DDR; 2) Transducers, proteins that pass and amplify DNA damage signals to downstream effectors. Notably, among diverse transducers, ATM (Ataxia Telangiectasia Mutated) and ATR (ATM and Rad3 Related) are central to the entire DDR; 3) Effector, proteins determine the physiological outcome of DNA damage response. Depending on the context of DNA damage, effectors can regulate cell cycle, transcription or cell apoptosis. Nevertheless, we need to point out that although DDR is often referred to as a signaling pathway, it is more accurately described as a network of interacting pathways that coordinate the damage response.
2.3. DNA damage repair
The various types of DNA damage include aberrant base or nucleotide modifications, single strand DNA (ssDNA) breaks, and chromosomal lesions caused by double strand breaks (DSBs). Among these, DSBs are regarded as the most cytotoxic. If left unrepaired, DSBs will affect genome integrity by causing mutations, chromosome deletions or translocations, because there is no intact complimentary template to repair the damaged strand. In this chapter, we will use DSBs as a model lesion.
DSBs can be repaired by two principle mechanisms, the non-homologous end joining (NHEJ) and homologous recombination (HR) [7]. These two pathways differ in their functional enzymes, the repair efficiency and also the cell cycle phases where they are active (Figure 1).
Molecular Basis of NHEJ. In the process of NHEJ, DSBs are repaired by direct ligation of the exposed ends regardless of their DNA sequences. Enzymes involved specifically in NHEJ capture both ends of the broken DNA molecule, bringing them together to form a DNA-protein complex to repair the break. Therefore NHEJ is a very efficient but error-prone way to repair damaged DNA, and it occurs in all phases of the cell cycle [8]. In NHEJ pathway, the Ku70/80 heterodimer initiates NHEJ by binding to both ends of the broken DNA molecule, which creates a scaffold for the assembly of other NHEJ enzymes. After association of Ku70/80, the DNA-dependent protein kinase catalytic subunit (DNA-PKcs) is recruited to the DSB, forming a synaptic complex that brings the broken DNA ends together. Once the DNA ends have been captured and tethered, non-ligatable DNA termini must be processed (single strand fill in) or removed by nucleases and polymerases. Lastly, the processed DNA ends are joint by ligase IV/XRCC4 complex [9]. It was demonstrated that in higher eukaryotes, and especially in mammals, NHEJ is the preferred pathway for DNA DSB repair [10].
Molecular Basis of HR. HR is an error-free, template-dependent strategy to repair DNA DSBs. It occurs during the S and G2 phases, when the sister chromatids are more easily available [11]. The key reactions in HR are homology search and DNA strand invasion, which are catalyzed by the RecA homolog Rad51 [12]. Principally, HR can be divided into three steps: 1) Presynapsis. During this process, DSB ends are recognized and processed to a single-stranded tail with a 3’-OH ending. This ssDNA is then bound by the eukaryotic ssDNA binding protein RPA (replication protein A). 2) Synapsis. With aid of cofactors, such as Rad 52 and Rad 55-57 complexes [13, 14], Rad51 binds to RPA-coated ssDNA, forming Rad51-DNA filament. After this, DNA strand invasion by the Rad51-ssDNA filament generates a D-loop intermediate. 3) Postsynapsis. In DSBs repair, both ends of the DSB are engaged, leading to double Holliday junction formation. Finally, following the actions of polymerases, nucleases and helicases, DNA ligation and substrate resolution occur.
How cells choose between NHEJ or HR to repair the DSBs is unclear. As mentioned above, HR is initiated by ssDNA resection and requires sequence homology, but NHEJ requires neither resection at initiation nor a homologous template. Thus, resection appears to be a pivotal step in DSB repair initiation that determines whether HR or NHEJ occurs. However, an alternative end-joining (A-EJ) pathway, which is also initiated by ssDNA resection but does not require a homologous partner, was recently identified. It is proposed that the presence of ssDNA resection will determine the selection among canonical NHEJ, A-EJ or HR; the size of the resection, which is associated with the cell cycle phase, will then direct the DSB repair to either HR or A-EJ [15].
3. Chromatin remodeling during DNA damage
In 1998, functions of phosphorylation at the Serine139 residue of a histone variant, H2AX, were first discovered in DDR [16]. Since then, extensive studies regarding how chromatin alters its structures in response of DNA damage were made. It is now recognized that small DNA lesion can lead to global chromatin remodeling, with changes including histone modifications, nucleosome positioning and higher-order folding of the chromatin fiber. Furthermore, if the DDR-induced chromatin remodeling is not properly restored, then the epigenetic changes can be heritable and contribute to terminal cell fate, such as transformation, cell senescence and cell apoptosis [17, 18]. In this part, we will discuss recent progress made about chromatin structures regulations in the detecting and repairing process of DNA damage. Specifically, we will focus on H2AX phosphorylation regulation, Poly (ADP-ribosyl)ation, and sumoylation in DDR.
3.1. H2AX phosphorylation
One of the key events that initiates DDR is phosphorylation at the Ser139 of histone H2AX, a chromatin-bound histone variant compromising up to 25% of the H2A [16]. This phosphorylation process is catalyzed by the master regulator of DDR, ATM and ATR. Phosphorylation of H2AX at Ser139 is very rapid and this phosphorylated H2AX (γH2AX) serves as a platform, directly recruiting Mdc1 (mediator of DNA-damage checkpoint 1), and additional factors such as 53BP1, RNF8, and the BRCA1A complex to affected sites [19].
Although γH2AX is a well-recognized marker for DNA damage, its precise role in chromatin remodeling is only just becoming clear. It was recently found that phosphorylation at a tyrosine site, Tyr142, plays a pivotal role in regulating H2AX functions in DDR [20]. Basal phosphorylation of H2AX at Tyr142 was carried out by WSTF (Williams syndrome transcription factor), a component of the WICH ATP-dependent chromatin remodeling complex [20]. At the early stage of DDR (<1hr), inhibition of phosphorylation at Tyr142 by knocking down WICH did not affect γH2AX foci formation, but during the later recovery stages, γH2AX foci was greatly reduced[20]. So it seems that in the absence of Tyr142 phosphorylation, the kinetics of the phosphorylation/dephosphorylation cycle of γ-H2AX may be altered. Following this finding, the phosphatase EYA (eye absent) responsible for dephosphorylating H2AX at Tyr142 was identified [21]. Dephosphorylation of Tyr142 was suggested to be a prerequisite for γH2AX to be recognized by damage repair proteins. When persistent phosphorylation at Tyr142 happens during DNA damage, MDC1-dependent binding of DNA repair factors is inhibited, but recruitment of pro-apoptotic factors, such as JNK1, is promoted [21]. A more recent study demonstrated that the doubly phosphorylated H2AX interact with Microcephalin (MCPH1), an early DNA damage response protein [22]. Although the exact functions of such interaction is still unknown, we speculate that the precise regulation of γH2AX will be an area of great potential for future DNA damage studies.
3.2. Poly(ADP-ribosyl)ation
In addition to H2AX-dependent recruitment, several additional pathways have also been shown to direct the recruitment of various proteins to DNA lesion. Poly(ADP-ribosyl)ation (PARylation) is one of the early events in DDR [2]. Poly(ADP-ribose) polymerases-1 (PARP-1), the founding member of PARP family, sense DNA break through its zinc-finger domain. Structural studies also showed that engaging into the damaged DNA causes PARP-1 conformation change and increases the dynamics of its catalytic domain [23]. In this way, the occurrence of a DNA break is immediately translated into a posttranslational modification of histones H1 and H2B leading to chromatin structure change [24]. Two waves of accumulation of PARP-1 were observed in living cells. The initial recruitment of PARP-1 activates and locates poly(ADP-ribose) synthesis, which in turn generates binding sites for a second wave of PARP-1 recruitment and other DDR proteins [25]. Recently, it was found that polycomb group (PcG) members and nucleosome remodeling and deacetylase (NuRD) complex are recruited by PARP-1 and -2 to DNA lesions [26]. Both PcG and NuRD are negative regulators of gene transcription, and indeed, rapid loss of nascent RNA and elongating RNA polymerase were observed at DNA damage sites. This finding suggests that part of PARP’s regulatory role in DDR involves repression of transcription.
3.3. Sumoylation
Sumoylation, the covalent attachment of the small proteins known as SUMO (small ubiquitin modifier) to protein substrate, is a very dynamic and reversible PTM [27]. Compared to ubiquitination, knowledge about sumoylation in DDR is relative rudimentary. In 2009, two papers demonstrated the importance of this ubiquitin-like protein modification in DDR [28, 29]. A series of immunofluorescence and live-cell image experiments showed that components in the sumoylation pathway, including enzymes E1 (SAE1), E2 (Ubc9), two of the diverse E3 enzymes (PIAS1 and PIAS4) and the conjugates SUMO1, 2 and 3, are rapidly recruited to DNA damage sites. Functionally, sumoylation of BRCA1 is necessary for its ubiquitin ligase activity. While association of 53BP1, BRCA1 and RNF168 with the DNA damage sites requires accumulation of PIAS1 and PIAS4 to the damaged sites [29].
Several more studies have further revealed that sumoylation and ubiquitination signaling pathways are integrated in the cellular response to DNA damage. For example, two groups showed that the human RNF4, a SUMO-targeted ubiquitin E3 ligase, was recruited to DSBs depending on its SUMO interacting motifs [30, 31] Depletion of RNF4 impairs ubiquitin adduct formation at DSB sites, causes persistent histone H2AX phosphorylation [30] and affects the clearance of 53BP1, RNF8, and RNF168 from DNA damage foci [31]. It is proposed that through physical interaction with the SUMO moiety, RNF4 promotes DNA repair by mediating ubiquitylation of sumoylated DDR components at sites of DNA damage.
The role of sumoylation in DNA repair is emphasized by modification of the RPA (replication protein A) complex [32]. RPA was found to physically associate with a SUMO specific protease, SENP6, to maintain its desumoylation status in normal conditions [32]. Under DNA damage, such as those caused by campothecin or IR, the 70 kD subunit of RPA is sumoylated, which in turn recruits Rad51 to DNA lesions, initiating DNA repair through HR. In addition to the specific study of RPA, a recent study in yeast identified a large group of proteins participating in DNA repair and undergoing sumoylation. They showed that defective sumoylation results in failure to complete replication of a damaged genome and impaired DNA end processing, highlighting the importance of sumoylation in maintaining genome stability [33].
4. DNA damage processed in heterochromatin
4.1. The heterochromatin feature
Chromatin can be divided into euchromatin and heterochromatin, on the basis of differential compaction at interphase. Euchromatin is loosely compacted, more accessible to transcriptional machinery and thus usually actively transcribed. Heterochromatin is typically densely packed, and was previously thought to be inaccessible to the transcription components [34]. Molecularly, heterochromatin is featured with specific histone modifications, such as di- or tri-methylation of histone H3 at lysine 9, and the subsequent recruitment of chromatin association protein such as heterochromatin protein1 (Hp1) [35]. Heterochromatin can be further divided into two groups. First is the constitutive heterochromatin, which contains a high density of repetitive DNA elements, such as satellite sequences and transposable elements. They remain condensed throughout the cell cycle. A second group is facultative heterochromatin, which is dynamic chromosomal loci, condensation of which is regulated by cellular and environmental signals [36].
4.2. The functions of heterochromatin
The major function of heterochromatin is to repress transcription and recombination of the embedded repetitive DNA sequences. Disruption of heterochromatin increases the occurrence of spontaneous DSBs, leads to the expansion of DNA repeat arrays, and is correlated with chromosomal defects, such as translocations and loss of heterozygosity [37]. Mechanistically, methylated H3 at Lysine9 (H3K9me) and the chromatin-bound Hp1 serve as a platform, recruiting various proteins to maintain the highly compact feature of heterochromatin. For example, the HDAC Clr3 is recruited to heterochromatic domains by the yeast Hp1 homolog Swi6. Deacytylation by Clr3 stabilizes H3 tri-methylation, increase chromatin condensation and precludes access of Polymerase II [38]. In addition to physically preventing the access of transcription machinery, heterochromatin structure also promotes the post-transcriptional silencing of repetitive sequences. This function is achieved by preferentially targeting the RNA interference components, such as RITS (RNA-induced transcriptional gene silencing) and RDRC (RNA-directed RNA polymerase complex) through H3K9me and Hp1 [39] [40, 41]. On the other side, the recruited RNAi machinery can also contribute to the heterochromatic architecture. In mammalian and drosophila cells, Hp1 shows RNA binding activity, which is required for assembling of condensed chromatin [42, 43]. It is proposed that the RNA derived from repetitive DNA sequence might function as a glue to promote folding or clustering of dispersed heterochromatic loci [36, 41].
4.3. Detection of DSBs in heterochromatin: focusing on γH2A foci
With the realization of heterochromatin structure and functions, the question is how DNA damages in heterochromatin are detected and repaired. In the following sections, we will discuss the recent understanding about these issues.
Abundant reports suggest that heterochromatin is refractory to γH2A foci formation upon ionizing radiation [44-46]. However, it remains to be determined whether this phenomenon is due to inaccessible to phosphorylation of H2AX, or heterochromatin is more resistant to DNA damage. Particularly, following DNA damage, chromatin in the vicinity of damaged sites are rapidly de-condensed, which makes the idea that γH2A foci is absent in highly packed chromatin a topic of debate [46-48]. On the other side, a recent study utilizing fluorescence in situ hybridization found that the high amount of proteins bound to heterochromatin, including Hp1, acts as a protective layer that prevents access to the DNA. Therefore, it seems that heterochromatin may internally act as an isolator to inhibit DNA damage [49].
However, those thoughts were revisited by a recent study conducted in drosophila cells. In 2011, Chiolo
4.4. DSBs repair in heterochromatin
The next question is how cell repairs the DSBs in heterochromatin. Two issues are raised when considering repair of DNA lesions in heterochromatin. The first is that chromatin compaction in heterochromatin might restrict the access of DDR proteins to damaged sites. Indeed, it was found that DSB repair occurs with slower kinetics and is less effective in heterochromatin [51]. Furthermore, a delay in repair of heterochromatic DSBs was observed in human cells [52]. To overcome the challenge given by tightly compacted chromatin, it was found that the cell can employ the ATM signaling pathway to relax chromatin [51]. Goodarzi
The second issue regarding repair of DSBs in heterochromatin is whether NHEJ or HR pathway occurs. In the presence of the closely clustered repeats, HR might produce dicentric and acentric chromosomes, which are known to contribute to human diseases such as cancer and infertility [55]. In this sense, it would be very risky for cells to choose HR to repair the DSBs, since this may lead to abnormal genome rearrangements. In other words, NHEJ repair seems less problematic because small deletions or mutations generally do not affect the function of tandem repeats as severely as genes. However, reports form Chiolo
Together, multiple mechanisms exist to guarantee proper DDR in heterochromatin to repair the damaged DNA without compromising genome stability. With improvements in live-cell imaging, we speculate that more details, like the process of DNA damage-induced heterochromatin expansion and reunion of the repaired heterochromatic region, will be revealed.
5. Human aging and chromatin remodeling
Aging is a complex process that has been long thought to be a consequence of unprogrammed deleterious events and accumulation of random gene mutation. However, with extensive studies in yeast, worm and mouse, and with the research in premature human aging disease, novel insights have been gained into the molecular mechanisms underlying aging. In this section, we will focus on recent understanding about the contributions that chromatin defects and DNA damage have on human aging.
5.1. Heterochromatin defects in human aging
Through studying the premature aging disorder Hutchinson–Gilford Progeria Syndrome (HGPS), the molecular mechanisms leading to chromatin defects in aging are being uncovered. HGPS is an extremely rare genetic disease caused by a point mutation in the
One hallmark of human aging, and also in the aging process of other species, is global change in chromatin structure [62, 63].Particularly, loss of heterochromatin structure, loss of heterochromatin proteins and altered patterns of histone modifications, such as decreased H3K9me3, are found in both physiological and premature aging [61, 64-67]. Furthermore, more open chromatin structure, as indicated by tri-methylation at histone3 lysine4, is implicated in shorter lifespan in worm [68, 69].
5.2. Molecular mechanisms underlying heterochromatin loss and aging
The above evidence suggests that heterochromatin maintenance is critical for longevity. Now the question is how such densely compacted chromatin structure regulates human aging. Unfortunately, due to the complex nature of the aging process and hence experimentally intractability, it is hard to find a direct causal-effect relationship. But recent studies do shed light on the heterochromatic sequence transcription and human aging. Shumaker
5.3. DNA damage and human aging
Persistent DNA damage is another hallmark in human aging. Most human premature aging syndromes are caused by various types of DNA damage, and in particular, DSBs [73, 74]. There is no doubt that chromatin defects and DNA damage are major contributors to human aging. The question is which one comes first? Do the DNA damage and the DDR lead to chromatin defects and thus human aging? Or it is that loss of chromatin structure makes the cell more susceptible to DNA damage, increases genome instability, and therefore promotes human aging? Observations made by Pegoraro
How could aberrant chromatin structure cause DNA damage and thus human aging? There might be two mechanisms. 1) The heterochromatic sequences are highly repetitive. Loss of chromatin condensation can leads to abnormal recombination of such sequence and thus genome rearrangement; 2) Heterochromatin confirmation can protect DNA from various insults and repair the damaged lesion with specific mechanisms, as mentioned above.
The next question is how DNA damage leads to human aging? Numerous studies showed that DNA damage and mutations accumulate in human aging. In aged human cells, cytogenetically visible lesions such as translocations, insertions, dicentrics, and acentric fragments are frequently detected [77]. Several signaling pathways linking DNA damage and aging are also proposed, such as the ATM-p53 axis [77] and the BRCA1 dependent aging process [78].However, in addition to being a driver in the accumulation of mutation, recent reports imply that DNA damage-induced RNA transcription change might be a novel mechanism leading human aging. The involvement of RNA processing components in DNA repair strengthens the role of DNA damage in global gene expression changes. For example, a proteomic screen for mediators of DDR showed that enrichment for RNA processing factors, such as splicing-regulator phosphatase PPM1G [79]. Furthermore, the deregulation of gene expression induced by DNA damage resembles increased transcription heterogeneity seen in aged heart tissue [80]. Specifically, Francia
6. Conclusions
Since discovery of the function of γH2AX in DDR, dynamic regulation of chromatin in response to DNA damage has received great attention during these past decades. In this chapter, we have discussed the contribution of three posttranslational modifications: phosphorylation, PPAR and sumoylation in DDR. We also discussed the current understanding about heterochromatin changes during DDR and how it regulates human aging. We emphasize the function of heterochromatin in DDR because this condensed chromatin structure is particularly involved in human aging. Emerging evidence suggests that heterochromatin is not refractory to DNA damage, but utilize a different downstream mechanism to repair the damaged sites and thus prevent unwanted genome recombination. DNA damage may change the heterochromatin structure by abnormal generation of non-coding RNA at the damaged locus, which could titrate the RNA-binding heterochromatin proteins (such as Hp1) and lead to subsequent abnormal heterochromatin structure. The integrity of the transcriptome can also be affected by DNA damage and regulate human aging. We speculate that the pathways regarding DNA damage repair in heterochromatin and the interplay between heterochromatic sequence transcription and human aging will be a hot area for future research (Figure 3).
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