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MITOCIRCLE

MITOCIRCLE. WP 3.2: Positional cloning of the gene defect Maastricht L. van den Heuvel. Gene hunting in human OXPHOS deficiency. Positional gene cloning (1) Candidate gene approach (2) Positional candidate gene approach (3). Positional cloning (1):.

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MITOCIRCLE

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  1. MITOCIRCLE • WP 3.2: Positional cloning of the gene defect Maastricht L. van den Heuvel

  2. Gene hunting in human OXPHOS deficiency • Positional gene cloning (1) • Candidate gene approach (2) • Positional candidate gene approach (3)

  3. Positional cloning (1): • Large families for total genome scan with linkage analysis are rarely available. Linkage analysis: cosegregation between disease phenotype and microsatellite markers

  4. Candidate gene approach (2): • Candidate genes obtained from biochemical diagnostics

  5. Respiratory chain enzyme activities in different tissues of patient N. Fibroblast (control range) Muscle Liver Complex I 0.067 (0.10-0.24) 8.83 (4.7-29) 7.15 Complex II + III 0.25 (0.21-0.33) 11.4 (4-28) 30.8 Complex IV 146 (128-250) 52.1 (52-186) 72.9 Citrate synthase 158 (140-257) 84.6 (48-162) 34.2 Enzyme activities are expressed in mU/mg protein.

  6. mitochondrial donor denucleation rho 0 mitochondrial donor mix and fuse hybrid transmitochondrial recipient rho 0 Rho zero test

  7. Case report • Leigh Syndrome • 4-months-old male Spanish infant with a negative family history • Normal enzymatic activities of respiratory chain complexes in muscle and liver • Low complex I activity in fibroblasts (67%) • No mutations found in nuclear CI subunits

  8. Mutation in ND6 T14487C (M63V) ” CONTROL PATIENT

  9. 156 CONTROL TspRI 23 133 PATIENT C1 C2 C3 ♀ M L F 175 102 80 24% 65% 65% 86% mutant mtDNA Heteroplasmy of ND6 (T14487C) mutation

  10. Features of the mutation (ND6): M63V • Localized in the most • conserved region of ND6 • Transmembrane segment • ND6 mutations: • Hot spot gene for LHON mutations (A14484G → M64V) • Mutation in MELAS (G14453A) • Mutation in LHON/dystonia or Leigh Syndrome (G14459A)

  11. Assembly in a ND6 patient • Role of ND6: • Essential for the assembly of CI • - affects assembly of membrane arm and respiratory function in a mouse cell line with a frameshift mutation in ND6 • (Bai & Attardi, EMBO J., 1998) • - absence of intact ND6 prevents assembly of CI in Chlamydomonas (Cardol et al., JMB, 2002)

  12. Co 1 Pat Co 2 1D 880 kD 2D 440 kD Assembly in a ND6 patient CI V NDUFA9 (39 kD) CONTROL PATIENT Low levels of fully-assembled CI Detection of a lower MW subcomplex

  13. Candidate gene approach (2): • Evolutionary conserved genes.

  14. Complex IV vs Complex I

  15. Evolutionary building blocks of Complex I T Friedrich J. Bioenerg. Biomembr. 2001

  16. Human complex I NDUFA1 NDUFA2 NDUFA3 NDUFA4 NDUFA6 NDUFA7 NDUFA8 NDUFA9 NDUFA10 NDUFAB1 NDUFB1 NDUFB2 NDUFB3 NDUFB4 NDUFB5 NDUFB6 NDUFB7 NDUFB8 NDUFB9 NDUFB10 NDUFC1 NDUFC2 NDUFS7 NDUFS8 17.2 kDa ? ND1 ND2 ND3 ND4L ND4 ND5 ND6 ? NADH NAD+ +H+ e- NDUFV1 NDUFV2 NDUFV3 FMN FP Fe-S NDUFS1 NDUFS2 NDUFS3 NDUFS4 NDUFS5 NDUFS6 NDUFA5 e- Fe-S Fe-S e- Matrix IP Fe-S H+ Ubiquinone e- e- Fe-S HP HP H+ Ims

  17. Candidate gene approach (3): • Candidate genes obtained from recognized protein function (for example function in complex I assembly).

  18. Nijmegen Center for Mitochondrial Disorders International Center for Clinical Care, Diagnostics and Research of Patients with disturbed Mitochondrial Energy Metabolism BIO INFORMATICS

  19. Human CIA30 genomic structure • Chromosomal location: 15q13.3 • Promoter region: TATA box CG box NRF-2 site CpG elements • Gene length: ~ 15 kb • Gene composition: 5 exons (75 to 654 bp) 4 introns (0.8 to 6.3 kb) • mRNA sequence: 1436 bp encoding 327 amino acids • Predicted mitochondrial targeting sequence of the first 24 amino acids

  20. Tissue distribution of CIA30 mRNA • CIA30 expression is ubiquitous • There is a slightly higher expression in the various heart tissues, kidney, lung, and liver

  21. CIA30: Results and Further Studies • Mutational detection: 13 patients • Five polymorphisms: 4/5 resulting in amino acid substitutions (frequent in ESTs) - Probably other Complex I assembly factors are involved in complex I deficiency

  22. Positional candidate geneapproach (3): • Chromosome transfer in combination with linkage analyses and/or candidate gene approach. * OXPHOS defect is expressed in fibroblasts. * Fibroblast are immortalized.

  23. Chromosome transfer: • Cloning of the SURF1 gene in COX deficient Leigh patients. • Map the gene for combined OXPHOS deficiency.

  24. Regulation of COX assembly • Identified assembly intermediates • Part of the assembly route could be identified. • In COX deficient patients (e.g. SURF1 mutants) give a disturbed assembly

  25. SurfI affects this step in the assembly of COX

  26. Nuclear gene defects in OXPHOS deficiency: • Complex I: NDUFS1, -S2, -S3, -S4, -S6,-S7, -S8 NDUFV1, -V2 • Complex II: SDHA, -B, -C, -D • Complex III: BCS1L and UQCRB • Complex IV: SURF1, SCO1, SCO2, COX10, COX15, LRPPC • MtDNA replication/maintenance: TP, ANT1, C10 ORF 2, DGUOK, TK2, DNC, THTR-1, SLC19A2, SPG7, FRDA, OPA1, TAZ.

  27. MITOCIRCLE • WP 3.2: Positional cloning of the gene defect

  28. Objectives: • 1.)The identification of the disease locus in cohorts of patients belonging to the same complementation group by linkage analysis or functional complementation. • 2.)The characterization of the causative gene defect.

  29. Description of work: • 1.)The discovery of new genes involved in the defects of complex I, complex IV, or both. - The identification of the disease locus in cohorts of patients belonging to the same complementation group by: • * linkage analysis on informative families. • * functional complementation strategies based on chromosome transfer. • 2.)Screening of candidate genes, identified by bioinformatics tools, for mutations.

  30. Deliverables: • 1.)A list of candidate loci for CI, CIV and CI+IV deficiency. • 2.)A list of new genes involved in these deficiencies and OXPHOS dysfunction. • 3.)A list of new pathogenic mutations causing these deficiencies. • 4.)Diagnostic protocols to screen the genes involved for mutations.

  31. Discussion(1): • 1.)Who is going to deliver the bioinformatics support? • 2.)Which patients (+biochemical and genetic characteristics) are available for these studies? • - complex I • - complex IV • - complex I+IV • - individual cases/ informative families • - Known genetic defects have been screened for?

  32. Discussion(2): • 4.)Are complementation groups available? • 5.)Which are the candidate genes for the different patient groups? • 6.)Which group is going to study specific patients groups?

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