The Genetic Determinants and Genomic Consequences of Non-Leukemogenic Somatic Point Mutations

  1. Joshua S. Weinstock
  2. Sharjeel A. Chaudhry
  3. Maria Ioannou
  4. Maria Viskadourou
  5. Paula Reventun
  6. Yasminka A. Jakubek
  7. L. Alexander Liggett
  8. Cecelia Laurie
  9. Jai G. Broome
  10. Alyna Khan
  11. Kent D. Taylor
  12. Xiuqing Guo
  13. Patricia A. Peyser
  14. Eric Boerwinkle
  15. Nathalie Chami
  16. Eimear E. Kenny
  17. Ruth J. Loos
  18. Bruce M. Psaty
  19. Tracy P. Russell
  20. Jennifer A. Brody
  21. Jeong H. Yun
  22. Michael H. Cho
  23. Ramachandran S. Vasan
  24. Sharon L. Kardia
  25. Jennifer A. Smith
  26. Laura M. Raffield
  27. Aurelian Bidulescu
  28. Emily O’Brien
  29. Mariza de Andrade
  30. Jerome I. Rotter
  31. Stephen S. Rich
  32. Russell P. Tracy
  33. Yii Der Ida Chen
  34. C. Charles Gu
  35. Chao A. Hsiung
  36. Charles Kooperberg
  37. Bernhard Haring
  38. Rami Nassir
  39. Rasika Mathias
  40. Alex Reiner
  41. Vijay Sankaran
  42. Charles J. Lowenstein
  43. Thomas W. Blackwell
  44. Goncalo R. Abecasis
  45. Albert V. Smith
  46. Hyun M. Kang
  47. Pradeep Natarajan
  48. Siddhartha Jaiswal
  49. Alexander Bick
  50. Wendy S. Post
  51. Paul Scheet
  52. Paul Auer
  53. Theodoros Karantanos
  54. Alexis Battle
  55. Marios Arvanitis
Read the full article See related articles

Listed in

This article is not in any list yet, why not save it to one of your lists.
Log in to save this article

Abstract

Clonal hematopoiesis (CH) is defined by the expansion of a lineage of genetically identical cells in blood. Genetic lesions that confer a fitness advantage, such as point mutations or mosaic chromosomal alterations (mCAs) in genes associated with hematologic malignancy, are frequent mediators of CH. However, recent analyses of both single cell-derived colonies of hematopoietic cells and population sequencing cohorts have revealed CH frequently occurs in the absence of known driver genetic lesions. To characterize CH without known driver genetic lesions, we used 51,399 deeply sequenced whole genomes from the NHLBI TOPMed sequencing initiative to perform simultaneous germline and somatic mutation analyses among individuals without leukemogenic point mutations (LPM), which we term CH-LPMneg. We quantified CH by estimating the total mutation burden. Because estimating somatic mutation burden without a paired-tissue sample is challenging, we developed a novel statistical method, the Genomic and Epigenomic informed Mutation (GEM) rate, that uses external genomic and epigenomic data sources to distinguish artifactual signals from true somatic mutations. We performed a genome-wide association study of GEM to discover the germline determinants of CH-LPMneg. After fine-mapping and variant-to-gene analyses, we identified seven genes associated with CH-LPMneg ( TCL1A, TERT, SMC4, NRIP1, PRDM16 , MSRA , SCARB1 ), and one locus associated with a sex-associated mutation pathway ( SRGAP2C) . We performed a secondary analysis excluding individuals with mCAs, finding that the genetic architecture was largely unaffected by their inclusion. Functional analyses of SMC4 and NRIP1 implicated altered HSC self-renewal and proliferation as the primary mediator of mutation burden in blood. We then performed comprehensive multi-tissue transcriptomic analyses, finding that the expression levels of 404 genes are associated with GEM. Finally, we performed phenotypic association meta-analyses across four cohorts, finding that GEM is associated with increased white blood cell count and increased risk for incident peripheral artery disease, but is not significantly associated with incident stroke or coronary disease events. Overall, we develop GEM for quantifying mutation burden from WGS without a paired-tissue sample and use GEM to discover the genetic, genomic, and phenotypic correlates of CH-LPMneg.

Article activity feed

  1. Version published to 10.1101/2024.08.22.24312319v2 on medRxiv
  2. Version published to 10.1101/2024.08.22.24312319v1 on medRxiv