Development of a method for large-scale single-molecule analysis of tau proteoforms

  1. James Joly
  2. Vivekananda Budamagunta
  3. Zhengjian Zhang
  4. Brittany Nortman
  5. Maryam Jouzi
  6. Rajat Bhatnagar
  7. Jarrett D Egertson
  8. Michael E Flaster
  9. Robert Grothe
  10. Sanjib Guha
  11. Kota Kaneshige
  12. Kevin McVey
  13. Nick Nelson
  14. Rukshan T Perera
  15. Steven J Tan
  16. David Arnott
  17. Joanna Lipka
  18. Lionel Rouge
  19. Tim Wendorff
  20. Don Kirkpatrick
  21. Alexis Rohou
  22. David C Butler
  23. Steven Lotz
  24. Ana Forton-Juarez
  25. Emily R Sartori
  26. Phil S Brereton
  27. Kevin Chen
  28. Michael A Darcy
  29. Hamid R Golnabi
  30. Ross Hartley
  31. Pierre F Indermuhl
  32. Christina E Inman
  33. Kevin M Jin
  34. Stanislav Katsyuk
  35. Rajesh Kota
  36. Bryant Lowry
  37. Jonathan C Menger
  38. Denise A Miller
  39. Maureen R Newman
  40. Adedeji Ogunyemi
  41. Julia K Robinson
  42. Noah Steiner
  43. Juanfeng Sun
  44. Lisen Wang
  45. Zhiqiang Wang
  46. Sheri K Wilcox
  47. Nautilus Biotechnology
  48. Greg T Kapp
  49. Sujal Patel
  50. Sally Temple
  51. Taylor Bertucci
  52. Joel Blanchard
  53. Andreas Huhmer
  54. Subra Sankar
  55. Kara Juneau
  56. Parag Mallick
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Abstract

Proteins exist as diverse proteoforms resulting from a combination of genetic variation, alternative splicing, and post-translational modifications. Current methods struggle to capture this complexity at the single-molecule level. Here we introduce Iterative Mapping of Proteoforms (IMaP), a method that enables the massively-parallel interrogation of millions to billions of single-protein molecules through iterative probing with fluorescently labeled antibodies. Using 12 site-specific antibodies, the method is capable of measuring 2^12 (4,096) potential proteoform groups. We used IMaP to measure proteoform group profiles of the tau protein, a key player in neurodegenerative diseases, using two pan anti-tau antibodies (Tau-13, Tau-216), three isoform-specific antibodies (Anti-0N, Anti-2N, Anti-4R), and seven phosphosite-specific antibodies (Anti-pT181, Anti-pS202+pT205, Anti-pT205, Anti-pS214, Anti-pT217, Anti-pT231, and Anti-pS396). The method demonstrates high sensitivity (detecting proteoforms at 0.1% abundance), high reproducibility (median CV <5.5%), and broad dynamic range (>3 orders of magnitude), outperforming conventional techniques in resolving closely related proteoform groups. We demonstrated that the method can be used on relevant biological samples by examining various neuronal models (iNeuron cells, organoids, miBrains, and mouse brains) and human samples. This examination revealed 130 distinct tau proteoform groups with as many as six phosphorylation events. The non-random distribution of these phosphorylation events suggests ordered and site-specific modification processes rather than random, stochastic accumulation. Certain combinations of phosphorylation events were more abundant than others; for example, pT217 preferentially co-occurred with pT181. In validating the applicability of the assay to human disease samples, we noted a specific pattern of multiple phosphorylation events in an advanced Alzheimer's disease patient that suggests a sequential pathway of pathological tau modification. Iterative Mapping of Proteoforms provides insights into proteoform complexity at the single-molecule level, with significant implications for understanding protein regulation in neurodegenerative diseases and beyond.

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  1. Version published to 10.1101/2025.06.26.660445v1 on bioRxiv