Biochemistry and Pharmacology - Research Publications

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Author: Compton, Alison × Author: Stroud, David × Author: Thorburn, David × Start date: 2020 × Type: Journal Article ×

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    Integrated multi-omics for rapid rare disease diagnosis on a national scale
    Lunke, S ; Bouffler, SEE ; Patel, CVV ; Sandaradura, SAA ; Wilson, M ; Pinner, J ; Hunter, MFF ; Barnett, CPP ; Wallis, M ; Kamien, B ; Tan, TYY ; Freckmann, M-L ; Chong, B ; Phelan, D ; Francis, D ; Kassahn, KSS ; Ha, T ; Gao, S ; Arts, P ; Jackson, MRSR ; Scott, HSS ; Eggers, S ; Rowley, S ; Boggs, K ; Rakonjac, A ; Brett, GRR ; de Silva, MGG ; Springer, A ; Ward, M ; Stallard, K ; Simons, C ; Conway, T ; Halman, A ; Van Bergen, NJJ ; Sikora, T ; Semcesen, LNN ; Stroud, DAA ; Compton, AGG ; Thorburn, DRR ; Bell, KMM ; Sadedin, S ; North, KNN ; Christodoulou, J ; Stark, Z (NATURE PORTFOLIO, 2023-07)
    Critically ill infants and children with rare diseases need equitable access to rapid and accurate diagnosis to direct clinical management. Over 2 years, the Acute Care Genomics program provided whole-genome sequencing to 290 families whose critically ill infants and children were admitted to hospitals throughout Australia with suspected genetic conditions. The average time to result was 2.9 d and diagnostic yield was 47%. We performed additional bioinformatic analyses and transcriptome sequencing in all patients who remained undiagnosed. Long-read sequencing and functional assays, ranging from clinically accredited enzyme analysis to bespoke quantitative proteomics, were deployed in selected cases. This resulted in an additional 19 diagnoses and an overall diagnostic yield of 54%. Diagnostic variants ranged from structural chromosomal abnormalities through to an intronic retrotransposon, disrupting splicing. Critical care management changed in 120 diagnosed patients (77%). This included major impacts, such as informing precision treatments, surgical and transplant decisions and palliation, in 94 patients (60%). Our results provide preliminary evidence of the clinical utility of integrating multi-omic approaches into mainstream diagnostic practice to fully realize the potential of rare disease genomic testing in a timely manner.
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    Multi-omics identifies large mitoribosomal subunit instability caused by pathogenic MRPL39 variants as a cause of pediatric onset mitochondrial disease
    Amarasekera, SSC ; Hock, DH ; Lake, NJ ; Calvo, SE ; Gronborg, SW ; Krzesinski, E ; Amor, DJ ; Fahey, MC ; Simons, C ; Wibrand, F ; Mootha, VK ; Lek, M ; Lunke, S ; Stark, Z ; ostergaard, E ; Christodoulou, J ; Thorburn, DR ; Stroud, DA ; Compton, AG (OXFORD UNIV PRESS, 2023-07-20)
    MRPL39 encodes one of 52 proteins comprising the large subunit of the mitochondrial ribosome (mitoribosome). In conjunction with 30 proteins in the small subunit, the mitoribosome synthesizes the 13 subunits of the mitochondrial oxidative phosphorylation (OXPHOS) system encoded by mitochondrial Deoxyribonucleic acid (DNA). We used multi-omics and gene matching to identify three unrelated individuals with biallelic variants in MRPL39 presenting with multisystem diseases with severity ranging from lethal, infantile-onset (Leigh syndrome spectrum) to milder with survival into adulthood. Clinical exome sequencing of known disease genes failed to diagnose these patients; however quantitative proteomics identified a specific decrease in the abundance of large but not small mitoribosomal subunits in fibroblasts from the two patients with severe phenotype. Re-analysis of exome sequencing led to the identification of candidate single heterozygous variants in mitoribosomal genes MRPL39 (both patients) and MRPL15. Genome sequencing identified a shared deep intronic MRPL39 variant predicted to generate a cryptic exon, with transcriptomics and targeted studies providing further functional evidence for causation. The patient with the milder disease was homozygous for a missense variant identified through trio exome sequencing. Our study highlights the utility of quantitative proteomics in detecting protein signatures and in characterizing gene-disease associations in exome-unsolved patients. We describe Relative Complex Abundance analysis of proteomics data, a sensitive method that can identify defects in OXPHOS disorders to a similar or greater sensitivity to the traditional enzymology. Relative Complex Abundance has potential utility for functional validation or prioritization in many hundreds of inherited rare diseases where protein complex assembly is disrupted.
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    Deficiency of the mitochondrial ribosomal subunit, MRPL50, causes autosomal recessive syndromic premature ovarian insufficiency
    Bakhshalizadeh, S ; Hock, DHH ; Siddall, NAA ; Kline, BLL ; Sreenivasan, R ; Bell, KMM ; Casagranda, F ; Kamalanathan, S ; Sahoo, J ; Narayanan, N ; Naik, D ; Suryadevara, V ; Compton, AGG ; Amarasekera, SSC ; Kapoor, R ; Jaillard, S ; Simpson, A ; Robevska, G ; van den Bergen, J ; Pachernegg, S ; Ayers, KLL ; Thorburn, DRR ; Stroud, DAA ; Hime, GRR ; Sinclair, AHH ; Tucker, EJJ (SPRINGER, 2023-07)
    Premature ovarian insufficiency (POI) is a common cause of infertility in women, characterised by amenorrhea and elevated FSH under the age of 40 years. In some cases, POI is syndromic in association with other features such as sensorineural hearing loss in Perrault syndrome. POI is a heterogeneous disease with over 80 causative genes known so far; however, these explain only a minority of cases. Using whole-exome sequencing (WES), we identified a MRPL50 homozygous missense variant (c.335T > A; p.Val112Asp) shared by twin sisters presenting with POI, bilateral high-frequency sensorineural hearing loss, kidney and heart dysfunction. MRPL50 encodes a component of the large subunit of the mitochondrial ribosome. Using quantitative proteomics and western blot analysis on patient fibroblasts, we demonstrated a loss of MRPL50 protein and an associated destabilisation of the large subunit of the mitochondrial ribosome whilst the small subunit was preserved. The mitochondrial ribosome is responsible for the translation of subunits of the mitochondrial oxidative phosphorylation machinery, and we found patient fibroblasts have a mild but significant decrease in the abundance of mitochondrial complex I. These data support a biochemical phenotype associated with MRPL50 variants. We validated the association of MRPL50 with the clinical phenotype by knockdown/knockout of mRpL50 in Drosophila, which resulted abnormal ovarian development. In conclusion, we have shown that a MRPL50 missense variant destabilises the mitochondrial ribosome, leading to oxidative phosphorylation deficiency and syndromic POI, highlighting the importance of mitochondrial support in ovarian development and function.
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    Fatal Perinatal Mitochondrial Cardiac Failure Caused by Recurrent De Novo Duplications in the ATAD3 Locus
    Frazier, AE ; Compton, AG ; Kishita, Y ; Hock, DH ; Welch, AE ; Amarasekera, SSC ; Rius, R ; Formosa, LE ; Imai-Okazaki, A ; Francis, D ; Wang, M ; Lake, NJ ; Tregoning, S ; Jabbari, JS ; Lucattini, A ; Nitta, KR ; Ohtake, A ; Murayama, K ; Amor, DJ ; McGillivray, G ; Wong, FY ; van der Knaap, MS ; Vermeulen, RJ ; Wiltshire, EJ ; Fletcher, JM ; Lewis, B ; Baynam, G ; Ellaway, C ; Balasubramaniam, S ; Bhattacharya, K ; Freckmann, M-L ; Arbuckle, S ; Rodriguez, M ; Taft, RJ ; Sadedin, S ; Cowley, MJ ; Minoche, AE ; Calvo, SE ; Mootha, VK ; Ryan, MT ; Okazaki, Y ; Stroud, DA ; Simons, C ; Christodoulou, J ; Thorburn, DR (CELL PRESS, 2021-01-15)
    BACKGROUND: In about half of all patients with a suspected monogenic disease, genomic investigations fail to identify the diagnosis. A contributing factor is the difficulty with repetitive regions of the genome, such as those generated by segmental duplications. The ATAD3 locus is one such region, in which recessive deletions and dominant duplications have recently been reported to cause lethal perinatal mitochondrial diseases characterized by pontocerebellar hypoplasia or cardiomyopathy, respectively. METHODS: Whole exome, whole genome and long-read DNA sequencing techniques combined with studies of RNA and quantitative proteomics were used to investigate 17 subjects from 16 unrelated families with suspected mitochondrial disease. FINDINGS: We report six different de novo duplications in the ATAD3 gene locus causing a distinctive presentation including lethal perinatal cardiomyopathy, persistent hyperlactacidemia, and frequently corneal clouding or cataracts and encephalopathy. The recurrent 68 Kb ATAD3 duplications are identifiable from genome and exome sequencing but usually missed by microarrays. The ATAD3 duplications result in the formation of identical chimeric ATAD3A/ATAD3C proteins, altered ATAD3 complexes and a striking reduction in mitochondrial oxidative phosphorylation complex I and its activity in heart tissue. CONCLUSIONS: ATAD3 duplications appear to act in a dominant-negative manner and the de novo inheritance infers a low recurrence risk for families, unlike most pediatric mitochondrial diseases. More than 350 genes underlie mitochondrial diseases. In our experience the ATAD3 locus is now one of the five most common causes of nuclear-encoded pediatric mitochondrial disease but the repetitive nature of the locus means ATAD3 diagnoses may be frequently missed by current genomic strategies. FUNDING: Australian NHMRC, US Department of Defense, Japanese AMED and JSPS agencies, Australian Genomics Health Alliance and Australian Mito Foundation.
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    HIGD2A is Required for Assembly of the COX3 Module of Human Mitochondrial Complex IV
    Hock, DH ; Reljic, B ; Ang, C-S ; Muellner-Wong, L ; Mountford, HS ; Compton, AG ; Ryan, MT ; Thorburn, DR ; Stroud, DA (American Society for Biochemistry and Molecular Biology, 2020-07-01)
    Assembly factors play a critical role in the biogenesis of mitochondrial respiratory chain complexes I-IV where they assist in the membrane insertion of subunits, attachment of co-factors, and stabilization of assembly intermediates. The major fraction of complexes I, III and IV are present together in large molecular structures known as respiratory chain supercomplexes. Several assembly factors have been proposed as required for supercomplex assembly, including the hypoxia inducible gene 1 domain family member HIGD2A. Using gene-edited human cell lines and extensive steady state, translation and affinity enrichment proteomics techniques we show that loss of HIGD2A leads to defects in the de novo biogenesis of mtDNA-encoded COX3, subsequent accumulation of complex IV intermediates and turnover of COX3 partner proteins. Deletion of HIGD2A also leads to defective complex IV activity. The impact of HIGD2A loss on complex IV was not altered by growth under hypoxic conditions, consistent with its role being in basal complex IV assembly. Although in the absence of HIGD2A we show that mitochondria do contain an altered supercomplex assembly, we demonstrate it to harbor a crippled complex IV lacking COX3. Our results redefine HIGD2A as a classical assembly factor required for building the COX3 module of complex IV.
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    Multiomic analysis elucidates Complex I deficiency caused by a deep intronic variant in NDUFB10
    Helman, G ; Compton, AG ; Hock, DH ; Walkiewicz, M ; Brett, GR ; Pais, L ; Tan, TY ; De Paoli-Iseppi, R ; Clark, MB ; Christodoulou, J ; White, SM ; Thorburn, DR ; Stroud, DA ; Stark, Z ; Simons, C (WILEY-HINDAWI, 2021-01)
    The diagnosis of Mendelian disorders following uninformative exome and genome sequencing remains a challenging and often unmet need. Following uninformative exome and genome sequencing of a family quartet including two siblings with suspected mitochondrial disorder, RNA sequencing (RNAseq) was pursued in one sibling. Long-read amplicon sequencing was used to determine and quantify transcript structure. Immunoblotting studies and quantitative proteomics were performed to demonstrate functional impact. Differential expression analysis of RNAseq data identified significantly decreased expression of the mitochondrial OXPHOS Complex I subunit NDUFB10 associated with a cryptic exon in intron 1 of NDUFB10, that included an in-frame stop codon. The cryptic exon contained a rare intronic variant that was homozygous in both affected siblings. Immunoblot and quantitative proteomic analysis of fibroblasts revealed decreased abundance of Complex I subunits, providing evidence of isolated Complex I deficiency. Through multiomic analysis we present data implicating a deep intronic variant in NDUFB10 as the cause of mitochondrial disease in two individuals, providing further support of the gene-disease association. This study highlights the importance of transcriptomic and proteomic analyses as complementary diagnostic tools in patients undergoing genome-wide diagnostic evaluation.