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DOI: 10.1055/a-1859-0800
Recognizable Pattern of Arthrogryposis and Congenital Myopathy Caused by the Recurrent TTN Metatranscript-only c.39974-11T > G Splice Variant
Abstract
Introduction Arthrogryposis is characterized by the presence of multiple contractures at birth and can be caused by pathogenic variants in TTN (Titin). Exons and variants that are not expressed in one of the three major isoforms of titin are referred to as “metatranscript-only” and have been considered to be only expressed during fetal development. Recently, the metatranscript-only variant (c.39974–11T > G) in TTN with a second truncating TTN variant has been linked to arthrogryposis multiplex congenita and myopathy.
Methods Via exome sequencing we identified the TTN c.39974–11T > G splice variant in trans with one of three truncating variants (p.Arg8922*, p.Lys32998Asnfs*63, p.Tyr10345*) in five individuals from three families. Clinical presentation and muscle ultrasound as well as MRI images were analyzed.
Results All five patients presented with generalized muscular hypotonia, reduced muscle bulk, and congenital contractures most prominently affecting the upper limbs and distal joints. Muscular hypotonia persisted and contractures improved over time. One individual, the recipient twin in the setting of twin-to-twin transfusion syndrome, died from severe cardiac hypertrophy 1 day after birth. Ultrasound and MRI imaging studies revealed a recognizable pattern of muscle involvement with striking fibrofatty involvement of the hamstrings and calves, and relative sparing of the femoral adductors and anterior segment of the thighs.
Conclusion The recurrent TTN c.39974–11T > G variant consistently causes congenital arthrogryposis and persisting myopathy providing evidence that the metatranscript-only 213 to 217 exons impact muscle elasticity during early development and beyond. There is a recognizable pattern of muscle involvement, which is distinct from other myopathies and provides valuable clues for diagnostic work-up.
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Introduction
Arthrogryposis is characterized by congenital non-progressive contractures involving more than one joint. Arthrogryposis is attributed to variable conditions, which all cause decreased fetal movements.[1] The disease spectrum includes disorders of the peripheral (i.e., neuropathies), or central nervous system, congenital myopathies, myasthenic syndromes, metabolic diseases, and inherited disorders of the connective tissue, mirroring the broad clinical spectrum.[2]
Pathogenic variants in TTN, encoding the sarcomeric protein titin, account for a heterogenous group of muscular diseases including cardiomyopathy, congenital myopathies, and other skeletal myopathies such as autosomal dominant tibial muscular dystrophy and limb-girdle muscular dystrophy.[3] TTN is the most common gene causing autosomal dominant dilated cardiomyopathy (DCM) in adulthood.[4] [5] [6]
Titin, along with myosin and actin, is one of the three major structural proteins in the sarcomere. Titin elastically connects myosin to the Z-disk of the sarcomere, thereby holding myosin in position, mediating passive elasticity, and preventing overstretching of the sarcomere. Titin is an extraordinarily large (approximately 3 megadalton) protein spanning over a distance of 1 to 2 µm (Z- to M-line) and consisting of up to 34,000 amino acids.[7] TTN undergoes extensive differential splicing and many alternatively spliced and differentially expressed isoforms have been identified, making TTN a very complex gene and a challenge for genetic diagnostics.[8] [9] The N2B TTN isoform containing the N2B element is cardiac specific, while the N2A isoform containing N2A elements is primarily expressed in skeletal muscle. The larger N2BA isoforms include both the N2B and N2A elements and are expressed in the heart, with a maximal expression during fetal development.[10] The theoretical, inferred isoform that includes all exons is referred to as metatranscript (NM_001267550.1). Many of the metatranscript-only exons were formerly thought to be only expressed during fetal development.[9]
First, recessive TTN splice variants predicted to affect all three major isoforms N2A, N2B, N2BA and were reported to cause congenital arthrogryposis with cardiac involvement including left ventricular non-compaction and DCM.[11] Later, metatranscript-only variants were reported in association with congenital arthrogryposis without cardiac involvement.[12] [13]
Recently, a metratranscript-only intronic variant (c.39974–11T > G) in TTN inherited in trans with a second truncating TTN variant was identified to cause arthrogryposis multiplex congenita and myopathy.[14] Individuals presented with variable congenital contractures and muscular hypotonia, but none of the patients was noted to have cardiac involvement.
Here, we report five additional patients from three families with congenital arthrogryposis and myopathy harboring the recurrent intronic variant c.39974–11T > G (NM_001267550.1:c.39974–11T > G) in TTN (designated “TTN-11”) and a second truncating variant in trans. One individual, the recipient twin in the setting of twin-to-twin transfusion syndrome, died from severe cardiac hypertrophy 1 day after birth suggesting that TTN-11-arthrogryposis might be associated with cardiomyopathy under specific circumstances. This series confirms the distinct presentation of TTN-11-associated myopathy and reveals a recognizable pattern of muscle involvement on MRI and ultrasound images.
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Methods
Study Design and Patients Recruitment
The study is designed as an observational case series. From March 2020 to March 2021, five patients with arthrogryposis and congenital myopathies were identified newly in-hospital and were enrolled for further analyses. The legal guardians gave informed consent. Ethical approval was obtained from the institutional ethical review boards in Düsseldorf and the NIH (Bethesda, Maryland).
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Exome Sequencing, Clinical Investigation, Radiographic Analyses
Exome sequencing was performed at two centers: Tübingen (Family A + B) and Genomics Platform at the Broad Institute of MIT and Harvard (Family C) ([Supplementary Material], available in the online version). Clinical information, including natural histories of clinical symptoms, evalutation of cardiac and pulmonary function, serum creatine levels were reviewed. Muscle biopsies and autopsy samples were prepared for sectioning and staining using standard protocols and evaluated by pathologists (A.S.J.). Ultrasound scans were assessed according to standard protocol ([Supplementary Material], available in the online version). Axial and coronal muscle MR images of the legs were acquired in conventional T1-weighted and short T1 inversion recovery sequences. Fatty infiltration and edema were evaluated by radiologists and neurologists (S.S.).
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Results
Clinical History of Patients AII-1, AII-2, BII-1, CII-1, and CII-2
BII-1 is a 3-year-old girl, and CII-1 and CII-2- are 11-year-old and 4-year-old boys, respectively. AII-1 and AII-2 are monozygotic monochorionic-diamniotic twins and their pregnancy was complicated by twin-to-twin transfusion syndrome. The recipient twin AII-1 died of cardiac failure at day 1 after birth.
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Perinatal and Neonatal Period
During pregnancy slightly reduced fetal movements were noted in all patients.
All reported patients were born by C-section (causes are listed in [Table 1]). Except for the twins (AII-1 and AII-2), who had twin-to-twin transfusion syndrome, the auxological data were within normal range. All patients (5/5) presented with congenital onset muscular hypotonia with frog-leg position and weakness with abnormal positioning of extremities and fixed contractures ([Fig. 1B]-i + ii; [Supplementary Table S1], available in the online version). Four patients (⅘) had fractures of the upper extremities. All patients had a weak cry and suck and some had feeding difficulties. AII-1 required nasogastric tube feeding for 2 weeks. CII-1 had severe dysphagia and aspiration requiring G-tube placement and intensive care during the first 3 months of life. AII-1 and BII-1 required respiratory support (continuous positive airway pressure [CPAP]) during their first weeks of life.
Abbreviations: D, day; Mos, months; w; weeks; yr(s), year(s).
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Neuromuscular and Motor Development
In all patients, the muscular weakness presented at birth. Contractures showed a consistent interindividual pattern and were most evident in the upper extremities. Elbows were most severely affected. All patients had a recognizable ulnar abduction and extension of wrist ([Fig. 1B]). In all patients, flexion contractures improved over time. For example, the degree of reduced elbow extension improved from 110 degrees (1 month) to 40 degrees (12 months) ([Fig. 1C]). The degree of knee flexion contracture was only mild (5–10 degrees). Most patients had adduced thumbs (3/5), flexed fingers including distal interphalangeal joints (5/5), clubfeet (3/5), and second toes overlapping first toes (3/4). Torticollis (3/5) or scoliosis (2/5) was mild ([Fig. 1B]-vi + vii) (details are provided in [Supplementary Table S1], available in the online version).
Muscular weakness was proximal more pronounced than distal in both upper and lower extremities and was stable, non-progressive. Pulmonary function tests in CII only showed mildly decreased forced vital capacity. While language and cognitive development were unremarkable, all patients had motor delay. At 10 months of age, AII-1 was not able to lift the upper arms against gravity, and elevation of legs was incomplete. BII-1 and CII-1 learned walking (at 3 years and 5 years of age, respectively), but required assist devices for ambulation and walking. C-II required a wheelchair for mobility. There was generalized hyporeflexia in all patients. Serum creatinine kinase was within normal range (5/5). The neuromuscular phenotype significantly overlaps with the clinical description of the nine patients with the recurrent TTN-11 splice variant reported by Bryen et al ([Table 1]).[14]
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Facial Features
Facial features included high arched palates ([Fig. 1B]-vii) (5/5) and retrognathia (3/5) ([Fig. 1B]-iii) and three patients had positional plagiocephaly.
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Muscle Ultrasound
Muscle ultrasound was performed in all patients who survived (4/5) (AII-1: 6 months; BII-1: 1.5 years, CII-2: 4 years, CII-1: 11 years). In all patients, ultrasound imaging revealed moderate to severe involvement of hamstrings muscles with most severe fatty fibrotic changes in semitendinosus (“semitendinosus sign,” [Fig. 2D], [F]). There was a consistent sparing of the adductor muscles and the tibialis anterior and peroneus muscles when compared with the other muscles of the legs ([Fig. 2B], [D], [F]). In all patients, there was mild to moderate involvement of upper extremity muscles, including M. biceps brachii ([Fig. 2D], [F], grading of muscle involvement see [Supplementary Tables S2] and [S3], available in the online version).
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Muscle Magnetic Resonance Imaging (MRI)
Muscle MRI was performed in AII-1 (6 months), CII-2 (4 years), and CII-1 (11 years). MRI of the lower extremity showed generalized reduced muscle bulk and fatty-fibrotic changes throughout (see [Fig. 2A], [C], [E]) and severe involvement of quadriceps and all hamstring muscles. The semitendinosus exhibited the most severe fatty-fibrotic changes, while the adductor muscles (M. sartorius and M. gracilis) were relatively spared. In the lower leg, there was prominent involvement of posterior compartment (M. gastrocnemius) and relative sparing of anterior compartment ([Fig. 2C]).
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Cardiac Involvement
Echocardiography of BII-1 showed a small, apical ventricular septal defect, which was not present anymore at the age of 6 months. Echocardiography of patient BII-1 (3 weeks; 6 months), CII-2 (4 years), and CII-1 (11 years) was unremarkable and there was no dilated or hypertrophic cardiomyopathy.
The twins of family A were subject to twin-to-twin transfusion syndrome and were born preterm (29 weeks of gestation): AII-1 was the donor twin with oligohydramnios (birth weight 730 g; −2.08 SD) and AII-2 was the recipient twin (1,550 g; +0.47 SD) with polyhydramnios requiring repeated amniotic fluid punctures. Echocardiography of the smaller, donor twin showed mildly restricted ejection function on the day of birth and a normal cardiac function on the follow-up examination ([Fig. 3A]). In contrast, echocardiography of the recipient twin (AII-2) revealed severe non-obstructive, global myocardial hypertrophy, moderate pulmonary hypertension (two-thirds of systemic pressure). Chest X-ray depicted pulmonary edema, and invasive inhalation was necessary ([Fig. 3E]). While cardiac function was initially hyperdynamic, pump function rapidly decreased ([Fig. 3B–D], [Videos 1] [2] [3], [Supplementary Tables S4] available in the online version). Fifteen hours after birth, severe bradycardia occurred. Despite cardiac resuscitation and maximal care, the neonate died of low-output cardiac failure. Post-mortem autopsy showed severe myocardial hypertrophy (heart weight, 15 g, reference: 7.2 ± 2.7 g) ([Fig. 3F], [Supplementary Table S4], available in the online version). Histology of the myocardium showed variable muscle fiber size, cardiomyocyte degeneration, and mild immune cell infiltration ([Fig. 3G]).
Video 1 Echocardiography of AII-2 at the first day after birth (short axis).
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Video 2 Echocardiography of AII-2 at the first day after birth (four chambers view).
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Video 3 Echocardiography of AII-2 at the first day after birth (five chambers view).
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Family histories of family A and B were unremarkable with respect to cardiac conditions. In family C, two sisters of the maternal grandmother died of cardiomyopathy at the age of 40 to 50 years and the maternal grandmother's mother died of cardiomyopathy in her 60s.
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Variants and Isoforms
Via exome sequencing, we identified the c.39974–11T > G (TTN-11) extended splice site variant in TTN (reference transcript: NM_001267550.1, ENST00000589042) in the four tested affected patients in compound heterozygosity with a truncating TTN variant. In the monozygotic twin affected by twin-to-twin transfusion syndrome who deceased 1 day after birth (AII-2), no specimen was available for genetic testing; however, given monozygosity and consistent phenotype the same genotype is assumed.
The variant TTN-11 is located in the intron 213 ([Fig. 4A]). It was shown that TTN-11 either causes abnormal exon 214 skipping by removing exon 214 (28 amino-acids) or abnormal use of cryptic 3′splice site resulting in a frameshift and premature termination.[14] TTN-11 is predicted not to impact any of the major skeletal or cardiac isoforms and thus is referred to as a metatranscript-only variant ([Fig. 4B]).
In the previous report, the TTN-11 splice variant was discussed as a potential founder mutation, since it co-segregated with the c.23177C > T, c.45328G > A, c.70969G > C polymorphisms ([Supplementary Table S5], available in the online version).[14] In the three families presented here, the three polymorphisms were present with the TTN-11 variant. Thus, our data confirm a shared haplotype and a common founder pathogenic variant.
All affected patients harbored a second pathogenic or likely pathogenic TTN truncating or splicing variant on the other allele. Parental testing confirmed the inheritance in trans ([Fig. 1A]). The variants were either absent from the population database gnomAD (family A + B) or reported once (family C).
All variants but TTN-11 are predicted to impact the long skeletal N2A isoform ([Fig. 4B], [Supplementary Table S6], available in the online version). While the truncating variants of families A and B were also predicted to impact the longer cardiac isoform N2BA, the variant of family C was predicted to impact, both, the longer cardiac isoform N2BA as well as the short cardiac isoform N2B ([Fig. 4B], [Supplementary Table S6], available in the online version). This is important to notice as in family C, two aunts and one grandmother have died of cardiomyopathy in their forties to sixties.
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Discussion
This study reports on five additional patients with the recurrent intronic pathogenic variant c.39974–11T > G in TTN (TTN-11) presenting with congenital myopathy and confirms the severe, consistent, and recognizable manifestation of this variant.[14]
This variant impacts the near-splice acceptor site of intron 213 and is assumed to alter exclusively the splicing or expression of the metatranscript-only isoform (NM_001267550.1). The metatranscript-only isoform is a hypothetical isoform including all known exons and was formerly thought to be only expressed during fetal development.[9] Based on this, during adulthood one would not expect a clinical significance of genetic alterations in exons 213 or 214 and only minor significance during embryonic development.
However, recent transcript analyses of skeletal muscle in healthy patients revealed that TTN exons 213 to 217 are not only expressed in the fetal muscle, but are also expressed to a lower extent (60%) in adult muscle.[9] [14] [15] In studies dealing with recessive titinopathies, almost all patients with pathogenic metatranscript-only variants clinically presented with arthrogryposis, supporting the notion, that isoforms bearing metatranscript-only exons might be of importance during early prenatal and postnatal development.[13]
Depending on differential splicing, TTN-11 can cause either abnormal in-frame exon 214 skipping by removing exon 214 (28 amino-acids), or abnormal use of a cryptic 3′splice site resulting in the inclusion of intronic bases into the mature messenger RNA, causing a frameshift and premature termination.[14] Transcript analyses of three muscle biopsies from patients with TTN-11 variants via RT-PCR confirmed the presence of both transcripts lacking exon 214 or transcript harboring intronic bases and a frameshift transcript.[14] While a damaging effect can be assumed for the frameshift variants, the interpretation and functional implication of the loss of exon 214 is unclear.
There are three spring elements ([1] proline-glutamine–valine–lysine [PEVK]-,[2] N2B- and the [3] tandem Ig-spring segments that mediate the passive, elastic forces of titin in the I-band region.[15] The PEVK elements account for the majority of the passive tension response of titin. Skeletal muscle and cardiac specific isoforms differ in the number of Ig and PEVK domains.[16] Exon-skipping events of PEVK region were shown to mediate myogenic differentiation resulting in muscle types with unique titin-based elastic properties, e.g., psoas fibers have a higher degree of passive tension than soleus fibers.[16] Exon 214 includes such PEVK repeat units.[9] [16] [17] Based on the function of PEVK repeat region in tension regulation, it can be speculated that loss of exon 214 might reduce muscle elasticity eventually resulting in contractures during early embryonic development. Fetal and neonatal skeletal muscle in mice and rabbits expresses large titin isoforms and additional exons in the PEVK regions, which is accompanied by a lower titin-based passive stiffness of the fetal and neonatal muscle.[17]
During the first year of life the large isoforms are gradually replaced by smaller isoforms.[17] In line with a declining functional importance of the large isoforms during infancy, the contractures of the patients were most pronounced at birth, and showed improvement over time.
None of the previously published individuals with arthrogryposis and the TTN-11 variant were explicitly reported to have cardiac involvement. However, one patient required cardiopulmonary resuscitation in the neonatal period, and one individual died at 26 years of age from unknown cause. Of note, the twins we report here had twin-to-twin transfusion syndrome. Due to intrauterine volume overload, the recipient twin is at increased risk of myocardial hypertrophy.[18] [19]
TTN-11 can cause exon 214 skipping and shortening of PEVK.[14] In a mouse model PEVK knockout resulted in cardiac hypertrophy in line with cardiac hypertrophy being present in AII-2.[20] Former transcript studies showed a relatively low fractional expression of exon 213 and exon 217 in the heart when compared with skeletal muscle (exon 213: fetal skeletal muscle: >95% vs. fetal heart approx. 23%; adult skeletal muscle: approx. 60% vs. adult heart approx. 20%).[9] However, the low level of transcription containing exons 213, 217, and presumably exon 214 in fetal and neonatal heart does not essentially rule out a role in cardiac function and adaptation. Similarly, heterozygous truncating variants in TTN are associated with dilated and hypertrophic cardiomyopathy which might unmask during cardiac stress by volume overload.[21] Whether the recurrent intronic splice variant TTN-11 or the truncating variant in trans contributed to postnatal heart failure is difficult to prove.
Larger sequencing studies of cardiomyopathy cohorts might give further information of functional impact of exons 213, 214, and 217 and TTN-11 on cardiac function.
The variant p.Tyr10345* of family B only affects the long cardiac N2BA isoform. Patient BII-1 had an apical ventricular septal defect at birth which spontaneously resolved. Recessive TTN pathogenic variants have been associated with septal defect, however, the evidence is still sparse.[11]
The variant p.Lys32998Asnfs*63 of family C affects both, the short N2B and the long cardiac N2BA isoforms, and three first degree relatives of CII-1 of the truncating TTN variant (CII-1) passed away from cardiomyopathy before the age of 60 years. This is consistent with studies reporting variants affecting both, the long N2BA and the short N2B cardiac isoforms, but not variants that affect only either of both, are significantly associated with cardiomyopathy.[12] [13]
Three of the ten previous published TTN-11 cases and four of our five patients had fractures affecting the upper extremities. Ten to 25% of individuals with arthrogryposis congenita are reported to have congenital fractures which are suggested to be caused by decreased fetal movement and inactivity-induced osteoporosis of long bones making bones more prone to fractures.[22] [23]
The evaluation of muscle involvement via ultrasound and MRI imaging in our patients with a “metatranscript-only” titinopathy revealed a consistent and recognizable pattern with severe involvement of quadriceps and hamstring muscles with relative sparing of adductors, sartorius, and gracilis in upper thigh. In the lower legs imaging reveals prominent involvement of the posterior compartment muscles and relative sparing of the anterior compartment muscles.[24] Similar findings were recently observed in three patients from two families all harboring biallelic TTN pathogenic variants including one metatranscript-only variant in trans (exon 163, p.Glu11932*; exon 201:, p.Leu12974Trpfs*104).[12] [24] These patients also had a marked calf involvement, clear adductor sparing, and sparing of the anterior compartment of the lower legs.
Taking together, these findings suggest that the distribution of the TTN-11-associated muscle involvement is specific and distinct from other forms of congenital myopathies.[25] [26] [27] The identified pattern enables imaging-based clinical phenotyping, which is especially important for variant interpretation in the current “era of reverse phenotyping after exome or genome sequencing.”
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Conclusion
The assessment of the functional relevance of different TTN transcripts and variants is a challenge for clinical diagnostics. Our findings confirm that the metatranscript-only isoforms including exons 213 to 217 are of importance during early fetal development and beyond, possibly related to its role in mediating higher elasticity and preventing contractures. The lethal cardiac involvement of one patient might point to a potential functional relevance of the variants in the developing heart. There is a distinct pattern of muscle involvement in “metatranscript-only” congenital titinopathy, providing valuable clues for genetic diagnostic work-up and suggesting specific genotype–phenotype correlations in TTN myopathies.
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Conflict of Interest
None declared.
Acknowledgments
The authors acknowledge collaborative support of S.T. Cooper and S.J. Bryen of Kids Neuroscience Centre, The Children's Hospital at Westmead, The University of Sydney, and the Children's Medical Research Institute for their expert opinion and critical review of research data. They thank the patients and their families for participating in our research study and Christopher Mendoza, Christine Jones, Gilberto (“Mike”) Averion, Ying Hu, and Kia Brook for their help in the clinical and research setting.
Full Data Access Statement
The principal author and the senior author take full responsibility for the data, analyses, and interpretation, and the conduct of the research; they have full access to all of the data; and that they have the right to publish any and all data, separate and apart from the guidance of any sponsor.
Data Availability Statement
Data is not provided in the article because of space limitations but may be shared (anonymized) at the request of any qualified investigator for the purpose of replicating procedures and results.
Author Contributions
L.A., F.D., and S.D. contributed toward conceptualization. L.A., S.D., D.H., S.W., S.S., U.L., A.S.J., T.H., D.G., A.R., K.R.C., and S.B.N. contributed toward data acquisition. L.A., S.W., and S.S. did the illustrations. F.D., E.M., and C.G.B. reviewed the manuscript. L.A. and F.D. drafted the manuscript.
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References
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- 2 Kang PB, Lidov HGW, David WS. et al. Diagnostic value of electromyography and muscle biopsy in arthrogryposis multiplex congenita. Ann Neurol 2003; 54 (06) 790-795
- 3 Hackman P, Vihola A, Haravuori H. et al. Tibial muscular dystrophy is a titinopathy caused by mutations in TTN, the gene encoding the giant skeletal-muscle protein titin. Am J Hum Genet 2002; 71 (03) 492-500
- 4 Gerull B, Gramlich M, Atherton J. et al. Mutations of TTN, encoding the giant muscle filament titin, cause familial dilated cardiomyopathy. Nat Genet 2002; 30 (02) 201-204
- 5 Itoh-Satoh M, Hayashi T, Nishi H. et al. Titin mutations as the molecular basis for dilated cardiomyopathy. Biochem Biophys Res Commun 2002; 291 (02) 385-393
- 6 Herman DS, Lam L, Taylor MRG. et al. Truncations of titin causing dilated cardiomyopathy. N Engl J Med 2012; 366 (07) 619-628
- 7 Chauveau C, Rowell J, Ferreiro A. A rising titan: TTN review and mutation update. Hum Mutat 2014; 35 (09) 1046-1059
- 8 Gautel M, Lehtonen E, Pietruschka F. Assembly of the cardiac I-band region of titin/connectin: expression of the cardiac-specific regions and their structural relation to the elastic segments. J Muscle Res Cell Motil 1996; 17 (04) 449-461
- 9 Savarese M, Jonson PH, Huovinen S. et al. The complexity of titin splicing pattern in human adult skeletal muscles. Skelet Muscle 2018; 8 (01) 11
- 10 Opitz CA, Linke WA. Plasticity of cardiac titin/connectin in heart development. J Muscle Res Cell Motil 2005; 26 (6-8): 333-342
- 11 Chauveau C, Bonnemann CG, Julien C. et al. Recessive TTN truncating mutations define novel forms of core myopathy with heart disease. Hum Mol Genet 2014; 23 (04) 980-991
- 12 Oates EC, Jones KJ, Donkervoort S. et al. Congenital titinopathy: comprehensive characterization and pathogenic insights. Ann Neurol 2018; 83 (06) 1105-1124
- 13 Savarese M, Vihola A, Oates EC. et al. Genotype-phenotype correlations in recessive titinopathies. Genet Med 2020; 22 (12) 2029-2040
- 14 Bryen SJ, Ewans LJ, Pinner J. et al. Recurrent TTN metatranscript-only c.39974-11T>G splice variant associated with autosomal recessive arthrogryposis multiplex congenita and myopathy. Hum Mutat 2020; 41 (02) 403-411
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- 16 Freiburg A, Trombitas K, Hell W. et al. Series of exon-skipping events in the elastic spring region of titin as the structural basis for myofibrillar elastic diversity. Circ Res 2000; 86 (11) 1114-1121
- 17 Ottenheijm CAC, Knottnerus AM, Buck D. et al. Tuning passive mechanics through differential splicing of titin during skeletal muscle development. Biophys J 2009; 97 (08) 2277-2286
- 18 Hyodo HM, Unno N, Masuda H, Watanabe T, Kozuma S, Taketani Y. Myocardial hypertrophy of the recipient twins in twin-to-twin transfusion syndrome and cerebral palsy. Int J Gynaecol Obstet 2003; 80 (01) 29-34
- 19 Springer S, Mlczoch E, Krampl-Bettelheim E. et al. Congenital heart disease in monochorionic twins with and without twin-to-twin transfusion syndrome. Prenat Diagn 2014; 34 (10) 994-999
- 20 Granzier HL, Radke MH, Peng J. et al. Truncation of titin's elastic PEVK region leads to cardiomyopathy with diastolic dysfunction. Circ Res 2009; 105 (06) 557-564
- 21 Schafer S, de Marvao A, Adami E. et al. Titin-truncating variants affect heart function in disease cohorts and the general population. Nat Genet 2017; 49 (01) 46-53
- 22 Hall JG, Aldinger KA, Tanaka KI. Amyoplasia revisited. Am J Med Genet A 2014; 164A (03) 700-730
- 23 Diamond LS, Alegado R. Perinatal fractures in arthrogryposis multiplex congenita. J Pediatr Orthop 1981; 1 (02) 189-192
- 24 Yu M, Zhu Y, Xie Z. et al. Novel TTN mutations and muscle imaging characteristics in congenital titinopathy. Ann Clin Transl Neurol 2019; 6 (07) 1311-1318
- 25 Jungbluth H, Davis MR, Müller C. et al. Magnetic resonance imaging of muscle in congenital myopathies associated with RYR1 mutations. Neuromuscul Disord 2004; 14 (12) 785-790
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- 27 Mercuri E, Lampe A, Allsop J. et al. Muscle MRI in Ullrich congenital muscular dystrophy and Bethlem myopathy. Neuromuscul Disord 2005; 15 (04) 303-310
Address for correspondence
Publication History
Received: 07 January 2022
Accepted: 18 May 2022
Accepted Manuscript online:
23 May 2022
Article published online:
02 October 2022
© 2022. Thieme. All rights reserved.
Georg Thieme Verlag KG
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References
- 1 Hall JG, Kimber E, Dieterich K. Classification of arthrogryposis. Am J Med Genet C Semin Med Genet 2019; 181 (03) 300-303
- 2 Kang PB, Lidov HGW, David WS. et al. Diagnostic value of electromyography and muscle biopsy in arthrogryposis multiplex congenita. Ann Neurol 2003; 54 (06) 790-795
- 3 Hackman P, Vihola A, Haravuori H. et al. Tibial muscular dystrophy is a titinopathy caused by mutations in TTN, the gene encoding the giant skeletal-muscle protein titin. Am J Hum Genet 2002; 71 (03) 492-500
- 4 Gerull B, Gramlich M, Atherton J. et al. Mutations of TTN, encoding the giant muscle filament titin, cause familial dilated cardiomyopathy. Nat Genet 2002; 30 (02) 201-204
- 5 Itoh-Satoh M, Hayashi T, Nishi H. et al. Titin mutations as the molecular basis for dilated cardiomyopathy. Biochem Biophys Res Commun 2002; 291 (02) 385-393
- 6 Herman DS, Lam L, Taylor MRG. et al. Truncations of titin causing dilated cardiomyopathy. N Engl J Med 2012; 366 (07) 619-628
- 7 Chauveau C, Rowell J, Ferreiro A. A rising titan: TTN review and mutation update. Hum Mutat 2014; 35 (09) 1046-1059
- 8 Gautel M, Lehtonen E, Pietruschka F. Assembly of the cardiac I-band region of titin/connectin: expression of the cardiac-specific regions and their structural relation to the elastic segments. J Muscle Res Cell Motil 1996; 17 (04) 449-461
- 9 Savarese M, Jonson PH, Huovinen S. et al. The complexity of titin splicing pattern in human adult skeletal muscles. Skelet Muscle 2018; 8 (01) 11
- 10 Opitz CA, Linke WA. Plasticity of cardiac titin/connectin in heart development. J Muscle Res Cell Motil 2005; 26 (6-8): 333-342
- 11 Chauveau C, Bonnemann CG, Julien C. et al. Recessive TTN truncating mutations define novel forms of core myopathy with heart disease. Hum Mol Genet 2014; 23 (04) 980-991
- 12 Oates EC, Jones KJ, Donkervoort S. et al. Congenital titinopathy: comprehensive characterization and pathogenic insights. Ann Neurol 2018; 83 (06) 1105-1124
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