Function and Regulation of Nuclear DNA Sensors During Viral Infection and Tumorigenesis

IFI16, hnRNPA2B1, and nuclear cGAS are nuclear-located DNA sensors that play important roles in initiating host antiviral immunity and modulating tumorigenesis. IFI16 triggers innate antiviral immunity, inflammasome, and suppresses tumorigenesis by recognizing double-stranded DNA (dsDNA), single-stranded DNA (ssDNA), damaged nuclear DNA, or cooperatively interacting with multiple tumor suppressors such as p53 and BRCA1. hnRNPA2B1 initiates interferon (IFN)-α/β production and enhances STING-dependent cytosolic antiviral signaling by directly binding viral dsDNA from invaded viruses and facilitating N6-methyladenosine (m6A) modification of cGAS, IFI16, and STING mRNAs. Nuclear cGAS is recruited to double-stranded breaks (DSBs), suppresses DNA repair, and promotes tumorigenesis. This review briefly describes the nuclear functions of IFI16, hnRNPA2B1, and cGAS, and summarizes the transcriptional, post-transcriptional, and post-translational regulation of these nuclear DNA sensors.


INTRODUCTION
The first line of host defense against pathogenic threats is orchestrated by the innate immune system, which relies on the ability of immune cells to recognize the presence of extracellular or intracellular pathogen-associated molecular patterns (PAMPs) through germline-encoded pattern recognition receptors (PRRs) (1). Viral nucleic acids are the main PAMPs generated during viral infection. Once infected, the interactions between PRRs and viral nucleic acids evoke a series of signaling transduction cascades that lead to the initiation of cell defense to eliminate viruses. For instance, recognition of viral DNA by cytosolic DNA sensors like cyclic GMP-AMP synthase (cGAS) elicits the activation of the adaptor protein stimulator of interferon genes (STING), which further recruits and activates TANK-binding kinase 1 (TBK1) and interferon-regulatory factor 3 (IRF3) (2)(3)(4). STING also activates the transcription factor nuclear factor-kB (NF-kB), which subsequently collaborates with IRF3 to promote the expression of type I IFNs (IFN-Is) and proinflammatory cytokines (5)(6)(7). Additionally, cytosolic DNA binds to the receptor absent in melanoma 2 (AIM2), leading to the recruitment of the apoptosis-associated speck-like protein containing CARD (ASC) and pro-caspase-1 to assemble a multi-protein complex termed inflammasome, which constitutes a group of PRRs and plays essential roles in response to viral infection (8). Once assembled, the AIM2 inflammasome complex further promotes the proteolytic maturation and secretion of proinflammatory cytokines, including interleukin 1 beta (IL-1b) and IL-18, thereby initiating the inflammatory cascade (9).
Although the stimulation of cytosolic nucleic acid sensors by viral nucleic acids is critical for host antiviral defense, multiple viruses replicate in the nucleus with much less or no opportunities for cytosolic engagement of viral nucleic acids.
In the past few years, accumulating evidence has demonstrated that nuclear DNA sensors, such as IFN-g-inducible protein 16 (IFI16), heterogeneous nuclear ribonucleoprotein A2/B1 (hnRNPA2B1), and nuclear cGAS, also exert critical roles in initiating host antiviral immunity (10). However, compared to the wealth of knowledge about cytosolic DNA sensors and the other PRRs, studies for the roles and underlying mechanisms of nuclear DNA sensors are only just emerging (11)(12)(13). Recent evidence indicates that nuclear DNA sensors are also involved in tumor development beyond pathogenic DNA recognition. Aberrant or damaged self-DNA species generated due to genomic instability serve as ligands to engage these nuclear DNA sensors during tumorigenesis.
This review focuses on the latest findings to provide a more comprehensive understanding of the functions of nuclear DNA sensors during viral infection and tumorigenesis. It also summarizes the regulation of these nuclear DNA sensors, including transcriptional, post-transcriptional, and posttranslational regulation during viral infection and tumorigenesis.

NUCLEAR DNA SENSORS FACILITATE ANTIVIRAL IMMUNITY
IFI16 is a member of the pyrin and HIN200 domain-containing protein family (PYHIN) that contains a pyrin domain and two DNA-binding HIN domains. It has been identified as a nuclear DNA sensor that mediates the induction of IFN-Is (14). Upon detecting viral DNA in the nucleus, IFI16 translocates to the cytoplasm where it oligomerizes and relays signals through adaptor molecule STING, engaging the TBK1-IRF3 axis and the NF-kB pathway to induce the transcription of IFN-Is (2,15,16). IFI16 has also been shown to interact with Kaposi's sarcomaassociated herpesvirus (KSHV) genomic DNA in the nucleus, leading to the formation of a functional inflammasome. Different from the cytosolic AIM2 inflammasome, the IFI16 inflammasome complex is initially assembled in the nucleus and subsequently translocates to the cytoplasm, suggesting a nucleus-associated inflammasome sensor component against KSHV infection (17,18). The overexpression of IFI16 with other inflammasome components in HEK293T cells is of note as it exhibits a lowlevel production of IL-1b. When these cells are infected by KSHV, an elevated level of IL-1b is observed, implying that the IFI16 inflammasome requires additional cofactors for optimal activation. The work of Brunette et al. further supports this notion that IFI16 and its mouse homolog p204 are poor activators of either STING-dependent IFNs or ASCinflammasome, while AIM2 robustly activates both IFNs and the inflammasome in an experimental overexpression system (19). hnRNPA2B1 is a member of the hnRNP family and has been recently identified as a nuclear DNA sensor (12). Upon sensing viral DNA in the nucleus, hnRNPA2B1 dimerizes and is demethylated by arginine demethylase JMJD6, which results in the cytoplasmic translocation of hnRNPA2B1. The cytoplasmic hnRNPA2B1 dimers interact with STING and activate the TBK1-IRF3 signal transduction cascade to facilitate the transcription of downstream IFN-Is. Moreover, hnRNPA2B1 can disassociate with fat mass and obesity-associated protein (FTO) after virus infection, leading to the promotion of N 6methyladenosine (m 6 A) modification, nucleocytoplasmic trafficking, and translation of cGAS, STING, and IFI16 mRNAs to amplify the activation of IFN-Is in antiviral innate immune response (20). A recent study shows that hnRNPA2B1 plays a vital role in transporting herpes simplex virus 1 (HSV-1) from the envelopment site to the extracellular environment (21). Interestingly, hnRNPA2B1 facilitates the replication of hepatitis E virus (HEV), an ssRNA virus, though hnRNPA2B1 is initially identified as a DNA sensor (22).
cGAS is a member of the nucleotidyltransferase family, the binding of cytoplasmic pathogenic DNA to cGAS induces a phase transition to liquid-like droplets, promoting the production of the secondary messenger cyclic guanosine monophosphate-adenosine monophosphate (cGAMP) and subsequent induction of IFN-Is through the STING-TBK1-IRF3 signaling axis (23,24). cGAS mainly localizes in the cytoplasm, yet cGAS expresses in interphase and may translocate to the nucleus due to nuclear envelope rupture or mitosis (24,25). Nuclear cGAS usually maintains a suppressed state by chromatin tethering to limit reactivity against self-DNA (26,27). A recent study reveals that upon nuclear entry of the human immunodeficiency virus (HIV), NONO, an innate immune sensor of the viral capsid proteins is associated with cGAS in the nucleus and is required to retain cGAS in the nucleus but has no impact on the cytosolic pool of cGAS. The crosstalk between NONO and cGAS in the nucleus enables the sensing of DNA intermediate during HIV infection. The detection of the nuclear viral capsid by NONO promotes DNA sensing by cGAS and reveals an innate strategy of distinguishing viruses from self in the nucleus (28).

IFI16 SUPPRESSES VIRAL REPLICATION AS A TRANSCRIPTIONAL REPRESSOR
Several studies have reported that IFI16 functions as a transcriptional repressor (29). For instance, IFI16 has been described as a restriction factor for human cytomegalovirus (HCMV) replication on account of suppressing the transcriptional activity of the viral DNA polymerase gene (UL54) (30). Besides, IFI16 transcriptionally represses HSV-1 gene expression such as the immediate-early proteins (ICP0 and ICP4), the early proteins (ICP8 and TK), and the late proteins (GB and Us11), and limits viral replicative capacity (31,32). IFI16 has also been demonstrated to function as a restriction factor for human papillomavirus 18 (HPV18) replication through histone modifications (33). A recent study shows that IFI16 limits HIV-1 transcription and latency reactivation by targeting the transcription factor Sp1 (34). Overall, these data identify IFI16 as a transcriptional repressor for various DNA viruses in the nucleus, of which the mechanisms still need deeper investigation.
Most studies suggest that IFI16 modulates transcription mainly through association with transcription factors or promoters. As mentioned above, IFI16 binds to the transcription factor Sp1 to suppress HIV-1 transcription (34). Similarly, Cristea et al. show that IFI16 interacts with the major immediate-early promoter (MIEP), and participates in controlling the viral immediate-early gene transcription by HCMV virion protein pUL83 (35). In addition to associating with transcription factors or promoters directly, IFI16 prevents transcription factors from interacting with their promoters. For instance, IFI16 has been shown to inhibit the association of some transcription factors such as Sp1 with the HCMV promoter (30).
Additionally, a study shows that IFI16 blocks the interaction of transcription factors, TATA-binding protein (TBP), and Octamer-Binding Transcription Factor 1 (Oct 1), with HSV-1 promoters (31). Meanwhile, the study also suggests that IFI16 may facilitate global histone modifications by modulating the formation of heterochromatin and euchromatin for both viral and cellular genes. Consequently, IFI16 may modulate transcription through chromatin modification. Another study also suggests that IFI16 promotes the addition of heterochromatin marks and the reduction of euchromatin marks on viral chromatin, thereby inhibiting viral gene expression and replication (36). Furthermore, IFI16 promotes the assembly of heterochromatin on HPV DNA, thus reducing both viral replication and transcription (33). Altogether, IFI16 is involved in transcriptional repression through association with transcription factors or promoters, preventing transcription factors from binding to their promoters and inducing changes in chromatin markers.

NUCLEAR DNA SENSORS REGULATE TUMORIGENESIS
Despite the essential roles of nuclear DNA sensors in the host antiviral defense, studies on these PRRs have also been well documented in the absence of infection. IFI16 acts as a DNA damage amplifier by interacting with p53 through its C-terminal domain and consequently promotes the accumulation and activation of p53 caused by DNA damage (37,38). Increased levels of IFI16 promote the transcription of known p53 target genes, such as the cell cycle kinase inhibitor p21 and the proapoptotic Bcl-2 family member Bax, inducing p53-mediated cell cycle arrest and apoptosis in human cancer cells (38,39). Decreased IFI16 mRNA expression is observed in numerous breast cell lines, which results in dysfunction of p53-mediated apoptosis and leads to cancer development (38). Subsequently, Lin et al. show that IFI16 functions as a tumor suppressor in hepatocellular carcinoma (HCC) by activating the p53 signaling pathway and inflammasome (40). In turn, functional activation of p53 stimulates the transcription of IFI16 through associating with the regulatory region of the IFI16 gene in the cells treated with DNA-damaging agents, suggesting a positive feedback loop between p53 and IFI16 (41). A recent research indicates that IFI16 positively regulates programmed cell death 1 ligand 1 (PD-L1) in cervical cancer cells by activating the STING-TBK1-NF-kB pathway, which can interact with the proximal region of the PD-L1 promoter to facilitate PD-L1 expression, and promoting the progression of cervical cancer (42).
Studies have also provided evidence that hnRNPA2B1 functions as a putative proto-oncogene in some cancers such as glioblastoma, pancreatic cancer, liver cancer, and pancreatic ductal adenocarcinoma (PDAC) (43)(44)(45)(46). The upregulated expression of hnRNPA2B1 facilitates the malignant phenotypes of cancer cells by modulating many downstream target genes. hnRNPA2B1 is also overexpressed in a variety of other tumors. For instance, the expression of hnRNPA2B1 in human ovarian cancer tissues is significantly higher than that in normal ovarian epithelium tissues, and increased hnRNPA2B1 level is related to the poor prognosis of ovarian cancer patients (47). hnRNPA2B1 also serves as a diagnostic marker for the early detection of lung cancer (48)(49)(50).
Another recent study by Liu et al. confirms that DNA damage triggers nuclear translocation of cGAS and leads to the recruitment of cGAS to the site of double-stranded breaks, suppressing homologous recombination DNA repair (HR) and increasing genomic instability and, consequently, tumorigenesis (51). This observation is further supported by a study by Jiang et al., which found that nuclear cGAS inhibits HR in a STINGindependent manner (52). These findings suggest that nuclear cGAS is a tumor enhancer by modulating the DNA damage response and influencing genome stability, indicating potential implications for inhibitors that block the nuclear translocation of cGAS for cancer intervention. The above studies suggest that nuclear DNA sensors play critical roles in tumorigenesis and might be a valuable prognostic marker for malignancy development and patient survival.
The functions of nuclear DNA sensors in regulating antiviral immunity, inflammasome activation, transcriptional repression, and tumorigenesis are summarized in Figure 1. Due to their important functions, the expression and cellular location of nuclear DNA sensors are tightly regulated ( Figure 2).

TRANSCRIPTIONAL REGULATION OF NUCLEAR DNA SENSORS
IFI16 mRNA is induced by both IFN-I (IFN-a and IFN-b) and IFN-II (IFN-g) in multiple human cell lines such as human myeloid leukemia cells and fibrosarcoma cells (53,54). IFNs are key molecules that contribute to the pathogenesis of systemic lupus erythematosus (SLE), and overproduction of IFN-I is always observed in patients with SLE (55)(56)(57). Consistently, the IFI16 transcripts in peripheral blood monocytes (PBMCs) of patients with SLE are significantly higher than that of healthy people (58). Infection with DNA viruses such as vaccinia virus (VACV), HSV-1, and human T-lymphotropic virus type 1 (HTLV-1) induces IFI16 expression dramatically (15,20,59,60). IFI16 mRNA expression is correlated with high viral load and low CD4 + T cell counts in HIV patients (61). IFI16 epigenetically suppresses hepatitis B virus (HBV) covalently closed circular DNA (cccDNA) by targeting an interferonsensitive response element (ISRE) located in cccDNA. However, HBV infection downregulates the mRNA expression of IFI16 in the hepatocytes and liver tissues of patients with chronic hepatitis B (62). In addition to being tightly controlled transcriptionally during viral infection, IFI16 expression is precisely regulated during tumorigenesis. For instance, as mentioned above, IFI16 directly binds to the C-terminal region of p53 and enhances p53mediated transcriptional activation (37,38). Moreover, p53 also facilitates IFI16 transcription by directly binding to the promoter region of IFI16 and thus provides positive feedback regulation of p53 signaling (41). The IL-6/JAK/STAT3 pathway plays a key role in the growth and development of many human cancers (63). IL-6 treatment induces STAT3 phosphorylation and drives IFI16 transcription in a STAT3-dependent manner in human adenocarcinoma cell lines (64). The oncogene ZNF217 acts as a transcriptional repressor and plays an important role during FIGURE 1 | Major functions of nuclear DNA sensors. Upon detecting nuclear viral DNA, IFI16 is transported to the cytoplasm to activate the STING signaling cascade, inducing IFN-Is expression through the TBK1-IRF3 and NF-kB axis. IFI16 also activates inflammasome to promote IL-1b and IL-18 maturation. Additionally, IFI16 functions as a transcriptional repressor to restrict viral replication by associating with transcription factors or promoters, preventing transcription factors from binding to promoters, and inducing chromatin marker changes. Nuclear hnRNPA2B1 dimerizes and is demethylated by JMJD6 after binding to viral dsDNA, resulting in the cytoplasmic translocation of hnRNPA2B1. The cytoplasmic hnRNPA2B1 activates the STING-TBK1-IRF3 signal to facilitate the transcription of IFN-Is. Moreover, demethylated hnRNPA2B1 enhances nucleocytoplasmic trafficking and translates cGAS, STING, and IFI16 mRNAs to amplify the antiviral immune response. Besides, the roles of nuclear DNA sensors during tumorigenesis have also been investigated. IFI16 is shown to act as a tumor suppressor in several types of cancers by interacting with p53 and enhancing p53-mediated transcriptional activation. In turn, functional activation of p53 stimulate the transcription of IFI16 through associating with the regulatory region of the IFI16 promoter. DNA damage triggers nuclear translocation of cGAS. Nuclear cGAS promotes tumorigenesis by modulating the DNA damage response and increasing genomic instability. ASC, apoptosis-associated speck-like protein containing a CARD; STING, stimulator of interferon genes; TBK1, TANK-binding kinase 1; IKK, IkB kinase; IRF3, interferon regulatory factor 3; IFN-I, type I interferon; A2B1, hnRNPA2B1; JMJD6, jumonji domain containing 6; Me, methylation; m 6 A, N 6 -Methyladenosine; FTO, fat mass and obesity-associated protein; KPNA, karyopherin alpha; PARP1, Poly (ADP-Ribose) Polymerase 1. gH2AX, phosphorylated H2A histone family member X (H2AX) on serine 139. neoplastic transformation (65)(66)(67). Consistent with its oncogenic role, ZNF217 represses the transcription of IFI16 (68). hnRNPA2B1 mRNA levels are constitutively expressed during viral infection (20). By contrast, it is overexpressed in various malignant tumor tissues and cancer cell lines (69)(70)(71)(72). For example, increased mRNA level of hnRNPA2B1 has been found in breast cancer cell lines deficient for breast cancer susceptibility gene 1 (BRCA1) expression. The restoration of BRCA1 expression reverts hnRNPA2B1 upregulation, implying the involvement of BRCA1 in the regulation of hnRNPA2B1 (73). Long non-coding RNA (lncRNA) CACNA1G-AS1 promotes the expression of hnRNPA2B1 in non-small cell lung cancer (NSCLC) cell lines, inducing malignant cell invasion, migration, and epithelial-mesenchymal transformation (EMT) (74). cGAS is an interferon-stimulated gene (ISG), and two adjacent ISREs in the promoter region of cGAS mediate the induction of cGAS by IFN-Is (75). The cGAS mRNA is upregulated in the PBMCs from patients with SLE (76). Both HSV-1 infection and IFN-a treatment induce cGAS mRNA expression in neonatal PBMCs from 1-month-old infants (77). facilitates IFI16 transcription by directly binding to the promoter region of IFI16, and IL-6 drives IFI16 transcription in a STAT3-dependent manner. Post-transcriptional regulation also involves modulating the expression of nuclear DNA sensors. During DNA virus infection, hnRNPA2B1 functions as an m 6 A modulator to promote nucleocytoplasmic trafficking of cGAS and IFI16 mRNAs. UL41 from HSV-1 significantly reduces the expression of cGAS and IFI16 by degrading their transcripts. Furthermore, PTMs, particularly the phosphorylation, ubiquitination, acetylation, and methylation, play critical roles in regulating the activity and stability of nuclear DNA sensors. Phosphorylation of IFI16 controls its subcellular localization, and related antiviral immunity and BLK-mediated phosphorylation of cGAS facilitates its cytosolic retention. ICP0 from HSV-1 induces the ubiquitination and proteasome-dependent degradation of IFI16 and thus suppresses inflammasome activation. STING promotes IFI16 degradation via the ubiquitin-proteasome system by TRIM21. The acetyltransferase p300 mediates acetylation of IFI16 during HSV-1 infection, an essential step for inflammasome assembly and cytoplasmic translocation, activation of cytoplasmic STING signaling, and downstream IFN-b production. The sensing ability of IFI16 is modulated by acetylation of Lys99 and Lys128 within its NLS, and this PTM of IFI16 promotes the cytoplasmic translocation of IFI16, whereas HDACs promotes its nuclear import. hnRNPA2B1 is demethylated by JMJD6 in the HSV-1-infected cells, which consequently initiates IFN-a/b production and enhances STING-dependent cytoplasmic antiviral signaling. BLK, B-lymphoid tyrosine kinase; MVB, multivesicular bodies; ICP0, human HSV-1 infected cell polypeptide 0; TRIM21, tripartite motif-containing protein 21; Ub, Ubiquitination; Ac, Acetylation; Me, Methylation; STAT3, signal transducer and activator of transcription 3; NLS, nuclear localization signal; HDAC, histone deacetylase; PRMT5, protein arginine N-methyltransferase 5.
LncRNA NEAT1 epigenetically inhibits cGAS expression to regulate the malignant phenotype of cancer cells and cytotoxic T cell infiltration in lung cancer (78).

POST-TRANSCRIPTIONAL REGULATION OF NUCLEAR DNA SENSORS
Post-transcriptional regulation also plays a key role in modulating the expression of nuclear DNA sensors and related host antiviral immunity and tumorigenesis. Three isoforms of IFI16, isoform-A, B, and C, are widely detected in multiple cell lines and primary cells due to IFI16 pre-mRNA alternative splicing (79,80). The spliceosome-associated factor, CTNNBL1, regulates the expression and alternative splicing of IFI16 and promotes proliferation and invasion in ovarian cancer (81). A novel transcript isoform of IFI16, which contains two HIN domains but lacks the PYD domain, interacts with AIM2 to impede the formation of a functional AIM2-ASC complex and inhibits AIM2 inflammasome (82). hnRNPA2B1 is a nuclear m 6 A reader and mediates m 6 A-dependent primary microRNA processing events (83). During DNA virus infection, hnRNPA2B1 functions as an m 6 A modulator to promote the m 6 A modification and nucleocytoplasmic trafficking of cGAS and IFI16 mRNAs after viral DNA recognition by hnRNPA2B1 (20). In addition to alternative splicing and m 6 A modification, viral proteins control IFI16 and cGAS mRNAs stability. UL41 from HSV-1 significantly degrades cGAS mRNA in HSV-1infected human foreskin fibroblast (HFF) cells abrogating cGAS-STING-mediated IFN-I production dependent on its RNase activity (84). UL41 also reduces the expression of IFI16 by degrading its transcripts (85).

POST-TRANSLATIONAL MODIFICATION OF NUCLEAR DNA SENSORS
Post-translational modifications (PTMs) play important roles in regulating the activity, stability, and folding of targeted proteins by inducing their covalent linkage to new functional groups, such as phosphate, methyl group, and acetate (86). PTMs including phosphorylation, ubiquitination, methylation, and acetylation have been shown to influence PRR-dependent antiviral immunity and inflammatory responses by targeting the innate sensors and downstream signaling molecules, including receptors, adaptors, enzymes, and transcription factors (1,86,87). Moreover, PTMs dynamically change the compartmentalization, trafficking, and physical interaction of key molecules that control immunological processes. Here, this review summarizes the PTMs involved in the positive and negative regulation of the nuclear DNA sensors during viral infection and tumorigenesis, and a summary of the posttranslational modifications of nuclear DNA sensors are listed in Table 1.
Phosphorylation is the most extensively investigated PTM type in antiviral innate immunity (87,94). IFI16 contains a CcN motif that targets a heterologous protein to the nucleus and subsequently undergoes phosphorylation, particularly by the CcN-motif-phosphorylating protein kinase (CK2). The IFI16 CK2 phosphorylation site enhances nuclear import by facilitating binding to a nuclear component, and the nuclearimport characteristics of the IFI16 CcN motif were consistent with those of the HIV-1 Tat nuclear target signal (95). The viral protein kinase pUL97 of HCMV, which binds and phosphorylates nuclear IFI16, contributes to the nucleocytoplasmic translocation of IFI16 to overcome the restriction activity of IFI16 (88). These studies indicate that the phosphorylation of IFI16 controls IFI16 cellular location and relates antiviral immunity. Up until recently, there was no direct evidence indicating that IFI16 can be phosphorylated at specific sites upon inflammasome assembly.
Although IFI16 is required for the maximal phosphorylation and activation of p53 induced by ionizing radiation (38), it is unclear whether phosphorylation of IFI16 is also critical for its pro-apoptosis and antitumor role during tumorigenesis. DNA damage induces the nuclear translocation of cGAS, which suppresses DNA repair and promotes tumorigenesis by interacting with PARP (51). However, the B-lymphoid tyrosine kinase (BLK)-mediated phosphorylation of cGAS at Tyr215 facilitates the cytosolic retention of cGAS, which may be important for its antiviral role as a cytosolic DNA sensor (51).
Ubiquitination is also a key regulatory mechanism for nuclear DNA sensors, particularly for IFI16. The protein ubiquitination of target substrates involves a stepwise catalyzation by three enzymes, ubiquitin-activating enzyme (E1), ubiquitin- Demethylation hnRNPA2B1 is demethylated by JMJD6 in the HSV-1-infected cells, which initiates IFN-I production (20) conjugating enzyme (E2), and ubiquitin ligase (E3) (96,97), resulting in mono-ubiquitination. Ubiquitin can be further conjugated to additional ubiquitin moieties via the same threestep process, yielding polyubiquitin chains. Ubiquitin undergoes ubiquitination itself at its seven lysine residues (K6/K11/K27/ K29/K33/K48/K63) or its amino-terminal methionine, which generates different types of ubiquitin chains with distinct functions (98). For instance, the K48-linked ubiquitin chain often induces the proteasomal degradation of targeted proteins, while the K63-linked ubiquitin chain is involved in the transduction of signaling pathways (99,100). In addition to inducing IFN-I production as a DNA sensor, IFI16 induces the assembly of inflammasome complexes in response to DNA viruses, which is essential in immune protection against viral infections (17,101). To counter IFI16-triggered antiviral immune responses, HSV-1 expresses an immediate-early protein, infected cell protein 0 (ICP0), an E3 ubiquitin ligase. After HSV-1 infection, ICP0 promotes the ubiquitination and proteasome-dependent degradation of IFI16 and suppresses inflammasome activation (89). Moreover, a previous study showed that the viral ICP0 protein leads to nuclear relocalization and the degradation of IFI16, resulting in the downstream inhibition of IRF3 signaling during HSV-1 infection (102). However, another study indicates that ICP0 is neither sufficient nor necessary for the degradation of IFI16 during HSV-1 infection (103). Due to these controversial results, the role of IFI16 ubiquitination mediated by ICP0 in antiviral immunity needs to be further clarified. Furthermore, it was recently found that STING facilitates ubiquitination on the first three lysines in the N-terminal region of IFI16 and promotes IFI16 degradation via the ubiquitin-proteasome pathway by recruiting the ubiquitin E3 ligase TRIM21 and restricting IFN-I overproduction during host antiviral immunity (90). The acetylation of lysine residues, which is inversely regulated by acetyltransferases and deacetylases, occurs commonly in the proteome and plays an important role in numerous biological processes, such as chromatin remodeling, nuclear transport, and innate immunity (104). The sensing ability of IFI16 is modulated by acetylation of Lys99 and Lys128 within its nuclear localization signal (NLS), and the PTM of IFI16 promotes the translocation of IFI16 from the nucleus to the cytoplasm, whereas histone deacetylases (HDACs) promotes its nuclear import (91). The acetyltransferase p300 mediates acetylation of IFI16 during HSV-1 infection, which is essential for IFI16-inflammasome assembly in the nucleus and cytoplasmic translocation, activation of STING in the cytoplasm, and IFN-b production (92). Another relevant study also reported that IFI16 in complex with BRCA1-H2B or with BRCA1 recognizes the viral genome, leading to BRCA1 mediated p300 recruitment, interaction with IFI16, acetylation of IFI16 and H2B by p300, and the cytoplasmic transport of acetylated IFI16-H2B-BRCA1 via Ran GTP during KSHV or HSV-1 infection (105).
The methylation of lysine or arginine residues, which is inversely regulated by methyltransferases and demethylases, plays an important role in innate immune responses (106). A recent study demonstrated that IFI16 is methylated by protein arginine methyltransferase 5 (PRMT5) and suppresses the activation of the STING pathway (93). Moreover, a newly identified nuclear DNA sensor, hnRNPA2B1, is methylated in the resting cells. However, hnRNPA2B1 is demethylated by JMJD6 in the HSV-1-infected cells. Demethylated hnRNPA2B1 initiates IFN-a/b production and enhances STING-dependent cytoplasmic antiviral signaling (20).
Together, PTMs, particularly the phosphorylation, ubiquitination, acetylation, and methylation of nuclear DNA sensors, play a vital role in controlling antiviral immunity and tumorigenesis.

CONCLUSION AND FUTURE PERSPECTIVES
Despite rapid advances in understanding of the functions and mechanisms of cytosolic DNA sensors in regulating host antiviral and antitumor immunity, studies that identify novel key nuclear DNA sensors and elucidate these functions are only just emerging. Given the important roles of nuclear DNA sensors during viral infection and tumorigenesis, it is critical to control expression. In this review, we briefly describe the nuclear functions of IFI16, hnRNPA2B1, and cGAS, and summarize the transcriptional, post-transcriptional, and post-translational regulation of these nuclear DNA sensors. However, several intriguing and important topics require further investigation.
The cytosolic DNA sensor, cGAS, has been found to translocate to the nucleus and is recruited to chromatin double-stranded breaks after DNA damage, where it suppresses homologous-recombination-mediated repair and promotes tumor growth (51,52). Similarly, DNA-dependent protein kinase (DNA-PK) plays a critical role in the nucleus, where it is necessary for non-homologous end joining (NHEJ) and repairing double-strand DNA breaks. DNA-PK was recently identified as a cytosolic DNA sensor that activates a STINGindependent DNA sensing pathway (107)(108)(109). These studies show that DNA-PK functions as a DNA sensor in the cytoplasm. However, considering that it predominantly localizes in the nucleus, it may also sense viral DNA in the nucleus and trigger an antiviral immune response like that of nuclear DNA sensors. Since all the three nuclear DNA sensors IFI16, hnRNPA2B1, and cGAS shuttle between cytoplasm and nucleus, all of them are involved in regulating both IFN-I-dependent antiviral immunity and tumorigenesis and newly identified nuclear DNA sensors may possess functions both in cytoplasm and nucleus.
The presence of host self-DNA generally in the nucleus was believed to be an immune-privileged cellular compartment. It is essential to understand how nuclear DNA sensors escape self-DNA-triggered activation in the immune response. cGAS has been reported to maintain an inhibitory state in the nucleus by binding nucleosome tighter to prevent autoreactivity to self-DNA (27,(110)(111)(112). A circular RNA named cia-cGAS has been identified to suppress nuclear cGAS by blocking its enzymatic activity, thereby preventing cGAS from sensing self-DNA to maintain host homeostasis (113). The multiple layers of regulation of nuclear DNA sensors may participate in avoiding inappropriate sensing self-DNA.
Invaded HSV-1 regulates IFI16 at multiple levels. HSV-1 infection-triggered IFN-I production induces IFI16 transcription (15,20,59,60). UL41 protein from HSV-1 degrades IFI16 mRNA via its RNase activity and suppresses IFI16 expression posttranscriptionally (85). The ICP0 protein of HSV-1 degrades IFI16 post-translationally (89). HBV infection also downregulates the IFI16 mRNA level, which is worthy of further investigation (62). Several models have been proposed for the HBV-mediated inhibition of IFI16 expression: 1) HBV may suppress IFI16 transcription by promoting hypermethylation of IFI16 promoters; 2) HBV may stimulate the production of some non-coding RNAs to directly degrade the IFI16 mRNA or target the cellular factors responsible for IFI16 transcription; 3) HBV may actively suppress some innate immune signaling, which is important for IFI16 expression (62). There is always a race between host antiviral innate immunity and the immune evasion strategies of viruses (114). The novel regulation mechanism of nuclear DNA sensors by viral components will be an interesting focus in future studies.
PTMs, including phosphorylation, ubiquitination, methylation, and acetylation, have been shown to regulate the expression and activity of nuclear DNA sensors. Other PTMs, such as glutamylation, SUMOylation, and lactylation, also potentially regulate nuclear DNA sensors during antiviral immunity and tumorigenesis. Hence, three main aspects should be extensively investigated in the next few years: 1) the identification of more important nuclear DNA sensors; 2) elucidation of the novel strategies used by invaded viruses to inhibit the expression and function of nuclear DNA sensors; and, 3) the observation of more PTMs of nuclear DNA sensors and elucidation of related mechanisms.