Abstract
Some genetic disorders caused by mutations in genes encoding components of the transcriptional machinery as well as proteins involved in epigenetic modification of the genome share many overlapping features, such as facial dysmorphisms, growth problems and developmental delay/intellectual disability. As a basis for some shared phenotypic characteristics in these syndromes, a similar transcriptome disturbance, characterized by global transcriptional dysregulation, is believed to play a major role. In this review article, a general overview of gene transcription is provided, and the current knowledge of the mechanisms underlying some disorders of transcriptional regulation, such as Rubinstein- Taybi, Coffin-Siris, Cornelia de Lange, and CHOPS syndromes, are discussed.
Human multiple malformation syndromes can serve as useful models to deepen the understanding of embryogenesis, since such malformation syndromes arise as a consequence of abnormal embryonic development. Human embryogenesis is intricately regulated by the spatiotemporal expression of many genes, and dysregulation of gene transcription is a known cause of many developmental syndromes. Hence, novel insights into human embryogenesis can be obtained from multiple malformation syndrome research.
The recent introduction of next-generation sequencing (NGS) technology has accelerated the pace of multiple malformation syndrome studies. NGS technology provides several advantages including high-throughput sequencing capability and precise quantification of nucleotides. By taking advantage of technology, our understanding of multiple malformation syndromes has been deepened, and the significant contribution of transcriptional disturbance in the pathogenesis of these syndromes has been revealed. In this review article, multiple malformation syndromes characterized by primary disruption of transcriptional regulation and categorized as ‘disorders of transcriptional regulation' are discussed.
An Overview of Gene Transcription
The human genome contains ∼20,000 protein-coding genes [Ezkurdia et al., 2014]. According to the central dogma, genes are typically transcribed into mRNAs and then translated into proteins. The gene transcription process is initiated by the binding of DNA-binding transcription factors to enhancer and promoter regions. Such transcription factors facilitate the binding of transcriptional co-activators such as histone modification enzymes and chromatin remodelers, and then the transcriptional machinery initiates gene transcription to produce mRNA.
The human genome is composed of over 3 billion bp. To pack such enormous stretches of genomic DNA into a small cellular nucleus, DNA is wrapped around histones. The histone core is an octamer composed of H2A, H2B, H3, and H4. Altogether, DNA and histones form a nucleosome. During gene transcription, since gene transcriptional machinery needs access to the genomic DNA, the nucleosome structure can become a physical barrier. Therefore, the unwrapping of the DNA from the histone proteins is required for active gene transcription. This unwrapping process is controlled by histone modification and chromatin remodeling (fig. 1).
Histone Modification and Chromatin Remodeling
The N-terminal domain of histones undergoes post-translational modifications such as acetylation and methylation [Swygert and Peterson, 2014]. These modifications affect the binding of chromatin remodeler proteins. For example, acetyl-lysine modifications of histones can be recognized by a bromodomain, which is a vital region of many DNA-associated proteins including the SWI/SNF family of chromatin remodeling enzymes. Likewise, methyl-lysine modifications of histones can be recognized by plant homeodomain finger-containing and chromodomain-containing chromatin remodeler proteins [Swygert and Peterson, 2014]. By affecting the attraction of these chromatin remodelers, these so-called ‘histone codes' play important roles in gene transcription regulation. Not only histone modifications, but also histone variants, DNA sequence and structure, RNA molecules, and transcription factors influence the genomic binding of chromatin remodelers [Längst and Manelyte, 2015]. Histone remodelers mobilize nucleosomes using ATP-dependent enzymatic reactions and unwrap the genomic DNA from the histones [Längst and Manelyte, 2015]. Such chromatin remodeling occurs both at regulatory elements, such as enhancers, and promoter regions. As a result, transcriptional machinery is enabled to initiate gene transcription.
Transcriptional Initiation
Protein-coding genes are transcribed by RNA polymerase II (RNAP2) (fig. 2). For transcriptional initiation, RNAP2 assembles general transcription factor complexes including TFIIA, TFIIB, TFIID, TFIIE, TFIIF, and TFIIH at gene promoter regions and forms the pre-initiation complex [Cler et al., 2009; Sainsbury et al., 2015]. Each general transcription factor complex plays a different role during transcriptional initiation. For example, TFIID, composed of 14 TAF proteins (TAF1-TAF14) is important for gene promoter binding of general transcription factor complexes [Vermeulen et al., 2007]. The TFIIH complex contains CDK7, which phosphorylates the C-terminal domain of RNAP2 [Sainsbury et al., 2015]. A 7-amino acid repeat exists in this domain. Phosphorylation of this heptad repeat controls the transitions between various transcription stages from transcriptional initiation, pausing to elongation. CDK7 of TFIIH phosphorylates the serine 5 residue of the heptad repeat during transcriptional initiation. Furthermore, the Mediator complex is also required for the pre-initiation complex assembly [Allen and Taatjes, 2015]. This Mediator complex is comprised of multiple subunits and has various roles throughout gene transcription, including the organization of chromatin architecture, transcriptional initiation, pausing, and elongation. The Mediator complex can interact with different transcriptional regulators, such as DNA-binding transcription factors and RNAP2, and regulate multiple aspects of gene transcription [Allen and Taatjes, 2015].
Transcriptional Pausing and Elongation
After transcriptional initiation, gene transcription is transiently paused by the recruitment of pausing factors such as the negative elongation factor and the DRB sensitivity-inducing factor [Jonkers and Lis, 2015]. To release the pause and transition into active transcriptional elongation, the positive transcription elongation factor b (P-TEFb), comprising cyclin T1 and CDK9, is required [Jonkers and Lis, 2015]. P-TEFb is a component of the super elongation complex (SEC). CDK9 phosphorylates the negative elongation factor and the DRB sensitivity-inducing factor as well as the serine 2 residue of the heptad repeat in RNAP2. Consequently, RNAP2 is released from the promoter-proximal pausing site, and the transcriptional elongation continues [Jonkers and Lis, 2015]. The Mediator complex interacts with SEC and regulates transcriptional elongation as well.
Enhancer-Promoter Looping
The pre-initiation complex and transcription elongation factors are present not only at gene-body regions, but also at gene-enhancer regions [Heinz et al., 2015]. To produce transcriptional activation, the looping of the genomic DNA is required to bring enhancer elements closer to promoter regions [Heinz et al., 2015]. As a result, the amount of transcriptional machinery at gene promoter regions increases, and successful gene transcription occurs. This process is facilitated by the cohesin and Mediator complexes. The cohesin complex forms a ring structure and embraces the DNA looping to maintain enhancer-promoter interactions [Ball et al., 2014]. The roles of the Mediator complex include the organization of the genomic DNA into topological domains and mediation of DNA looping as well as in transcriptional initiation and elongation [Kagey et al., 2010; Allen and Taatjes, 2015]. Cooperative interactions among cohesin and Mediator complexes appear to play a major role in maintaining enhancer-promoter looping.
An Overview of Disorders of Transcriptional Regulation
In this review, disorders characterized by global transcriptional dysregulation are discussed. In this group of disorders, multiple malformation syndromes caused by mutations in genes encoding transcriptional machineries, chromatin remodeler, and histone modification enzymes should be included. Genetic conditions due to mutations in genes encoding DNA-binding transcription factors, such as the GATA family of transcription factors, are not included in the disorders of transcriptional regulation because the associated clinical symptoms appear to be somewhat different from those of the above-mentioned category. Interestingly, genetic disorders caused by mutations in genes encoding components of the transcriptional machinery as well as in proteins involved in epigenetic modification of the genome share many overlapping features, e.g., the Rubinstein-Taybi, Coffin-Siris, Cornelia de Lange, and CHOPS syndromes. As a basis for some shared phenotypic characteristics in these syndromes, a similar transcriptome disturbance is believed to play a major role. Therefore, the current knowledge of the mechanisms underlying these disorders will be discussed herein.
Rubinstein-Taybi Syndrome: A Disorder of Histone Modifications
Rubinstein-Taybi syndrome (RSTS; MIM 180849 and 613684) is characterized by facial dysmorphisms, including downslanting palpebral fissures, broad thumbs and halluces, developmental delay/intellectual disability, and short stature (fig. 3a) [Hennekam, 2006]. RSTS is caused by heterozygous mutations in the CBP and EP300 genes [Roelfsema et al., 2005]. In about 55% of the RSTS cases, mutations are found in CBP, whereas mutations in EP300 have been identified only in up to 8% of the cases [Roelfsema et al., 2005; Hennekam, 2006; Negri et al., 2015]. Mutations in CBP cause the most typical RSTS phenotype, and although EP300 mutations can be found in typical RSTS cases, a wider phenotypic spectrum is seen in individuals with EP300 mutations [Roelfsema et al., 2005; Bartholdi et al., 2007; Negri et al., 2015]. Given the genomic deletions of CBP or EP300 causing the typical phenotype of RSTS, haploinsufficiency of either CBP or EP300 is suggested as the disease mechanism of RSTS [Roelfsema et al., 2005; Bartholdi et al., 2007; Tsai et al., 2011; Negri et al., 2015, 2016; Rusconi et al., 2015]. These genes encode transcriptional coactivators with lysine acetyltransferase activity (fig. 3b) [Kasper et al., 2014].
Pathogenesis of Rubinstein-Taybi Syndrome
CBP encodes the CREB-binding protein, and EP300 encodes the p300 protein. These proteins have high sequence similarity, including a bromodomain and a histone acetyltransferase domain. The acetylation of histone lysines is the hallmark of a transcriptionally active chromatin region. CREB-binding protein and p300 are the primary acetyltransferases to mark H3K18 and H3K27 acetylation [Kasper et al., 2014]. H3K27 acetylation is known as an active enhancer and promoter histone mark. Consistent with the concept that RSTS is caused by defective histone acetylation, lymphoblastoid cell lines obtained from individuals with RSTS showed a reduction of histone H2B and H2A acetylation [Lopez-Atalaya et al., 2012]. Therefore, the molecular mechanism of RSTS appears to be a global transcriptional disturbance due to an altered genome-wide histone modification. Recently, in an individual with features of Cornelia de Lange syndrome (CdLS), an EP300 mutation was identified, suggesting a similar transcriptome disturbance between RSTS and CdLS [Woods et al., 2014].
Coffin-Siris Syndrome: A Disorder of Chromatin Remodeling
Coffin-Siris syndrome (CSS; MIM 135900) is characterized by facial dysmorphisms, such as thick eyebrows, periorbital fullness, a wide mouth with full lips, and coarse facial features as well as fifth fingernail hypoplasia, absence of terminal phalanges, hypertrichosis, developmental delay/intellectual disability, and short stature [Vergano and Deardorff, 2014]. CSS is caused by heterozygous germline mutations in genes encoding a component of BAF (BRG1/hBRM-associated factors) complex, which belongs to the SWI/SNF chromatin remodeler complex family [Santen et al., 2012; Tsurusaki et al., 2012]. In individuals with CSS, mutations have been found in ARID1A(encoding BAF250a), ARID1B(encoding BAF250b), SMARCA4(encoding BRG1), SMARCB1(encoding BAF47), and SMARCE1(encoding BAF57). Mutations in SMARCA2(encoding BRM) have been reported in Nicolaides-Baraitser syndrome (NCBRS), which has phenotypic overlap with CSS (see below) [Santen et al., 2012; Tsurusaki et al., 2012; Van Houdt et al., 2012]. All of the encoded proteins are components of the BAF complex (fig. 4a). BRM and BRG1 possess an ATPase domain, and only one of these proteins exists per BAF complex. Likewise, BAF250a and BAF250b are mutually exclusive in the BAF complex [Kadoch and Crabtree, 2015].
Mutations in one of these genes can be found in about 60-70% of the patients with CSS [Santen et al., 2013; Wieczorek et al., 2013]. ARID1B mutations are found most frequently and are associated with relatively milder phenotypes compared to CSS due to mutations in other genes [Santen et al., 2013; Wieczorek et al., 2013; Tsurusaki et al., 2014]. Since loss-of-function mutations in ARID1B and ARID1A were found in individuals with CSS, the disease mechanism appears to be haploinsufficiency of ARID1Aand ARID1B[Santen et al., 2013; Wieczorek et al., 2013; Tsurusaki et al., 2014]. On the other hand, mutations in SMARCA4, SMARCB1, and SMARCE1 were mainly missense or in-frame deletions [Santen et al., 2013; Tsurusaki et al., 2014].
NCBRS (MIM 601358) is also caused by mutations in the BAF complex protein-encoding SMARCA2 gene [Van Houdt et al., 2012]. The clinical phenotype of NCBRS highly overlaps with that of CSS and is characterized by facial dysmorphisms, sparse hair, short stature, microcephaly, and intellectual disability [Van Houdt et al., 2012]. As a distinguishing feature, NCBRS patients have interphalangeal joint swelling, and they do not show hypoplasia of digits, which is typically associated with CSS. The main SMARCA2 mutations identified in NCBRS were missense; therefore, the molecular mechanism resulting from SMARCA2 mutation may not be a simple loss of function [Van Houdt et al., 2012]. In addition to SMARCA2, ARID1B mutations were found to be associated with NCBRS clinical features [Wieczorek et al., 2013]. Given the clinical similarities and molecular overlap between CSS and NCBRS, a similar molecular pathogenesis of CSS and NCBRS might be considered.
Pathogenesis of Coffin-Siris Syndrome and Nicolaides-Baraitser Syndrome
Since SWI/SNF complex remodelers alter chromatin conformation by their ATPase enzymatic activity, mutations in BAF complex protein-coding genes are expected to cause transcriptional disturbance due to modifications in the chromatin accessibility. A previous study, using chromatin immunoprecipitation followed by massive parallel sequencing, demonstrated a combinatorial regulation of gene expression achieved by distinct BAF complexes with different components [Raab et al., 2015]. Although ARID1A-encoded BAF250a and ARID1B-encoded BAF250b proteins do not coexist in a single complex, they bind to similar genomic locations. BAF250a and BAF250b both bind close to transcriptional start sites of genes, as well as gene enhancer regions, suggesting the importance of the BAF complex in remodeling the promoter and enhancer regions of the chromatin structure (fig. 4b) [Raab et al., 2015]. However, the mechanism by which the BAF complex chromatin remodeler controls gene transcription remains to be fully understood. Given the role of the BAF complex in transcriptional regulation, global transcriptional disturbance probably underlies the molecular mechanism of CSS and NCBRS.
Cornelia de Lange Syndrome: A Disorder of the Cohesin Complex
CdLS (MIM 122470) is characterized by craniofacial dysmorphisms, such as synophrys, high-arched eyebrows and a thin downturned upper lip, hirsutism, intellectual disability, microcephaly, growth retardation, limb anomalies, such as micromelia, phocomelia and oligodactyly as well as several other systemic abnormalities (fig. 5a) [Liu and Krantz, 2009]. CdLS is caused by germline mutations in genes encoding the structural and regulatory components of the cohesin complex. Mutations have been found in NIPBL, HDAC8, SMC1A, and SMC3 in CdLS [Krantz et al., 2004; Tonkin et al., 2004; Musio et al., 2006; Deardorff et al., 2007, 2012a]. A CdLS-like phenotype was also observed in individuals with RAD21mutations [Deardorff et al., 2012b].The cohesin complex is composed of SMC1A, SMC3, RAD21,and STAG1or STAG2(fig. 5b).The cohesin complex has a ring-like structure and ‘embraces' the genomic DNA. NIPBLencodes a protein that controls the cohesin complex genome loading. The SMC3 component of the cohesin complex becomes acetylated once loaded onto the genome and is subsequently deacetylated by HDAC8 for cohesin protein recycling.
NIPBL mutations can be found in ∼50% of the individuals with CdLS, and in general, more severely (or ‘classically') affected individuals are much more likely to harbor a mutation in NIPBL, with loss-of-function mutations causing a severe phenotype [Mannini et al., 2013]. Mutations in SMC1A, SMC3, and HDAC8 can be found in a small percentage of the individuals with CdLS. In individuals with NIPBL mutations, the disease mechanism is due to haploinsufficiency of NIPBL [Pehlivan et al., 2012; Mannini et al., 2013]. Although both HDAC8and SMC1A are located in the X chromosome, affected females with heterozygous HDAC8 or SMC1A mutations have been reported [Deardorff et al., 2007; Kaiser et al., 2014]. Most mutations in HDAC8 are missense and de novo. In general, males with HDAC8 mutations tend to show more severe manifestations compared to females. Although heterozygous females with HDAC8 mutations can be asymptomatic, affected heterozygous females were also reported, depending on the skewing level of X inactivation [Kaiser et al., 2014]. HDAC8 mutations produce loss of function in the acetyltransferase activity [Deardorff et al., 2012a; Kaiser et al., 2014]. SMC1A escapes X inactivation and shows a biallelic expression pattern. Interestingly, female CdLS probands with an SMC1A mutation tend to show a more severe phenotype compared to males with SMC1A mutations [Deardorff et al., 2007]. SMC1A and SMC3 mutations found in individuals with CdLS were missense mutations or in-frame deletions [Deardorff et al., 2007; Gil-Rodríguez et al., 2015]. Recently, female probands with heterozygous loss-of-function mutations in SMC1A were found in association with seizures and intellectual disability without a clear CdLS phenotype [Goldstein et al., 2015; Lebrun et al., 2015; Jansen et al., 2016]. Therefore, the disease mechanism of SMC1A and SMC3 mutations in CdLS is unlikely to be a mere loss-of-function effect, and a dominant-negative effect is suspected.
Pathogenesis of Cornelia de Lange Syndrome
The cohesin complex was originally identified with a critical role in preventing premature sister chromatid separation during mitosis [Ball et al., 2014]. Therefore, when NIPBL was identified as a causative gene for CdLS, it was originally thought that sister chromatid separation defects might underlie the disease mechanism of CdLS. However, cell lines obtained from patients with CdLS did not show an increased frequency of premature sister chromatid separation, suggesting that disruption of cohesin's canonical role was unlikely to be the underlying mechanism causing the CdLS phenotype [Kaur et al., 2005; Castronovo et al., 2009]. Instead, animal model studies, including drosophila, zebrafish, and mice as well as patient-derived cell line studies demonstrated a clear role for cohesin in transcriptional regulation [Kawauchi et al., 2009; Liu et al., 2009; Muto et al., 2014; Wu et al., 2015].
There are 2 proposed mechanisms regarding the transcriptional regulatory mechanism of cohesin (fig. 5c) [Ball et al., 2014; Izumi et al., 2015]. The first suggests that the cohesin complex facilitates gene promoter-enhancer interactions, whereas the second indicates a direct role in transcriptional regulation by interacting with RNAP2. By using its ring structure, cohesin is known to promote DNA looping, allowing physical interactions between distal regulatory elements and promoter regions [Ball et al., 2014]. A direct transcriptional regulatory role of cohesin is supported by the observation that RNAP2, as well as the SEC, interacts with cohesin, specifically STAG1-cohesin [Izumi et al., 2015]. Furthermore, cohesin-binding sites were enriched within the promoter regions of CdLS dysregulated genes, suggesting its role in transcriptional initiation or elongation control [Liu et al., 2009].
NIPBL forms a heterodimer complex with MAU2, and functions as a cohesin loader. In yeast, RSC chromatin remodeler complex, yeast ortholog of BAF complex, was shown to play a major role in cohesin loaders (SCC2/SCC4) genome binding, and cohesin loaders and RSC remodeler cooperatively maintain nucleosome-free regions [Lopez-Serra et al., 2014]. Furthermore, transcriptional similarities were established between the cohesin component inactivation and the RSC complex inactivation in the yeast model [Lopez-Serra et al., 2014]. Therefore, the derangements of nucleosome positioning might cause transcriptional disturbances not only in CSS but also in CdLS.
Recently, mutations in TAF1 and TAF6 were shown to be associated with a CdLS-like phenotype [O'Rawe et al., 2015; Yuan et al., 2015]. TAF1 and TAF6 encode components of the TFIID complex, which plays a major role in transcriptional initiation. Therefore, disruption of transcriptional initiation or transition from transcriptional initiation to the elongation phase may be the steps affected in CdLS.
CHOPS Syndrome: A Disorder of Transcriptional Elongation
CHOPS syndrome (MIM 616368) is a multisystem developmental disorder characterized by coarse facial features, cognitive impairment, heart defects, obesity, pulmonary symptoms, skeletal defects, and short stature (fig. 6a) [Izumi et al., 2015]. CHOPS syndrome probands were originally suspected to have CdLS, although they lacked several typical features of CdLS, such as microcephaly. CHOPS syndrome is caused by gain-of-function mutations in AFF4, which encodes a key component of the SEC (fig. 6b) [Izumi et al., 2015].
Pathogenesis of CHOPS Syndrome
SEC includes P-TEFb, which plays important roles in RNAP2 pausing release. Other components of the SEC are AFF1, AFF4, AF9, ENL, and ELL protein families. AFF4 is a scaffolding protein located at the center of the SEC, which does not exist if AFF4 is knocked down [Lin et al., 2010]. All the mutations found in CHOPS syndrome probands were missense and were located within the ALF homology domain of the AFF4 protein [Izumi et al., 2015]. The AFF4 protein is degraded by ubiquitination-dependent proteasomal degradation. For AFF4 to be transported to the proteasome, AFF4 is ubiquitinated by E3 ubiquitin ligase, SIAH1. SIAH1 binds to AFF4 by recognizing the SIAH1-binding motif located within the ALF domain [Oliver et al., 2004]. In CHOPS syndrome, missense mutations hamper the binding of SIAH1, causing a less efficient proteasomal degradation of AFF4. As a result, the AFF4 protein accumulates in the cells of CHOPS syndrome probands [Izumi et al., 2015].
The effect of the accumulation of AFF4 proteins is transcriptional overactivation of genes, whose expression is controlled by transcriptional elongation, such as MYC(fig. 6c). Chromatin immunoprecipitation followed by massive parallel sequencing demonstrated accumulation of the AFF4 protein around transcription start sites in genes in which expression is activated in CHOPS syndrome [Izumi et al., 2015]. Furthermore, the elongating form of RNAP2 (RNAP2 Ser2ph) was accumulated around gene bodies of overexpressed genes in CHOPS syndrome. Combining these observations, the transcriptional disturbance of CHOPS syndrome results from an overactivation of the transcriptional elongation system.
Transcriptome comparison between CHOPS syndrome and CdLS showed similar transcriptome profiles [Izumi et al., 2015]. Thus, disruption of molecular interactions of cohesin, SEC, and RNAP2 would lead to similar transcriptional disturbances by altering transcriptional elongation. Since CHOPS syndrome probands have clinical features that overlap those seen in CdLS, a part of the CdLS disease mechanism could be explained by excessive transcriptional elongation, similar to that seen in CHOPS syndrome.
Other Disorders of Transcriptional Regulation
In recent years, an increasing number of genetic disorders, due to mutations in genes encoding histone modifiers and chromatin remodeler proteins, have been identified (table 1). These disorders include: CHARGE syndrome due to CHD7 mutations, Wiedemann-Steiner syndrome due to KMT2A mutations, Kabuki syndrome due to KMT2D and KDM6A mutations, and Say-Barber-Biesecker/Young-Simpson syndrome due to KAT6B mutations [Vissers et al., 2004; Ng et al., 2010; Clayton-Smith et al., 2011; Jones et al., 2012; Lederer et al., 2012]. CHD7 is a chromatin remodeler protein with a chromodomain histone-modification recognition motif. KMT2A, KMT2D, KDM6A, and KAT6Bencode histone modification enzymes. KBG syndrome may also be categorized in this group of disorders because the causative gene for KBG syndrome, ANKRD11, encodes Ankyrin repeat domain 11 protein, known to regulate histone acetylation via functioning with HDAC3 [Sirmaci et al., 2011; Gallagher et al., 2015]. Mutations in genes encoding the mediator complex proteins have also been reported. MED23 and MED25 mutations were found in individuals with intellectual disability, and MED12 mutations have been found in individuals with FG syndrome and X-linked Ohdo syndrome [Risheg et al., 2007; Hashimoto et al., 2011; Vulto-van Silfhout et al., 2013; Basel-Vanagaite et al., 2015; Figueiredo et al., 2015]. There are clinical features that allow astute clinicians to distinguish between typical cases of these syndromes. However, in their atypical presentations, a clinical distinction may not be feasible. The use of exome sequencing in clinical practice has allowed for an expansion of the phenotypic spectrum of these Mendelian disorders. We recently reported a case of an RSTS patient who had overlapping features with CHARGE syndrome [Masuda et al., 2015]. Likewise, mutations in the ANKRD11 gene, whose mutations cause KBG syndrome, are identified in CdLS-overlapping phenotype patients [Parenti et al., 2016]. As illustrated by these cases with overlapping phenotypes among various disorders of transcriptional regulation, unbiased genome screening, by either exome or genome sequencing, may obscure the clinical distinction among disorders of transcriptional regulation.
Conclusion
Similarities between the clinical phenotypes of diverse syndromic diagnoses facilitate the identification of common molecular mechanisms linking these diverse diagnoses on a pathogenetic level. Such insights have contributed significantly not only to deepening our understanding of the etiologies of these malformation syndromes, but also in shedding light on the mechanism of fundamental cellular processes such as gene transcription. Due to the increasing use of NGS-based technologies in the clinical and research fields, novel gene discovery will continue to provide insights into the molecular controls of transcription and will further our understanding of a growing class of diagnoses - the disorders of transcriptional regulation. Elucidation of the mechanisms of transcriptional abnormalities underlying disorders of transcriptional regulation will contribute to the advancement of both clinical genetics and molecular cell biology.
Acknowledgments
The author thanks Ian D. Krantz and Katsuhiko Shirahige for their support and mentorship. He also thanks Masashige Bando, Kazuhiro Akiyama and Matthew A Deardorff for fruitful discussion. The author's research is supported by a Grant-in-Aid for Scientific Research from the Mochida Memorial Foundation for Medical and Pharmaceutical Research and a Research grant from the Takeda Science Foundation.
Disclosure Statement
The author has no conflict of interest to declare.