RESUMO
Cryogenic electron microscopy (cryo-EM) has now been widely used for determining multi-chain protein complexes. However, modeling a complex structure is challenging particularly when the map resolution is low, typically in the intermediate resolution range of 5 to 10 Å. Within this resolution range, even accurate structure fitting is difficult, let alone de novo modeling. To address this challenge, here we present DiffModeler, a fully automated method for modeling protein complex structures. DiffModeler employs a diffusion model for backbone tracing and integrates AlphaFold2-predicted single-chain structures for structure fitting. Extensive testing on cryo-EM maps at intermediate resolutions demonstrates the exceptional accuracy of DiffModeler in structure modeling, achieving an average TM-Score of 0.92, surpassing existing methodologies significantly. Notably, DiffModeler successfully modeled a protein complex composed of 47 chains and 13,462 residues, achieving a high TM-Score of 0.94. Further benchmarking at low resolutions (10-20 Å confirms its versatility, demonstrating plausible performance. Moreover, when coupled with CryoREAD, DiffModeler excels in constructing protein-DNA/RNA complex structures for near-atomic resolution maps (0-5 Å), showcasing state-of-the-art performance with average TM-Scores of 0.88 and 0.91 across two datasets.
RESUMO
Despite ferritin's critical role in regulating cellular and systemic iron levels, our understanding of the structure and assembly mechanism of isoferritins, discovered over eight decades ago, remains limited. Unveiling how the composition and molecular architecture of hetero-oligomeric ferritins confer distinct functionality to isoferritins is essential to understanding how the structural intricacies of H and L subunits influence their interactions with cellular machinery. In this study, ferritin heteropolymers with specific H to L subunit ratios were synthesized using a uniquely engineered plasmid design, followed by high-resolution cryo-electron microscopy analysis and deep learning-based amino acid modeling. Our structural examination revealed unique architectural features during the self-assembly mechanism of heteropolymer ferritins and demonstrated a significant preference for H-L heterodimer formation over H-H or L-L homodimers. Unexpectedly, while dimers seem essential building blocks in the protein self-assembly process, the overall mechanism of ferritin self-assembly is observed to proceed randomly through diverse pathways. The physiological significance of these findings is discussed including how ferritin microheterogeneity could represent a tissue-specific adaptation process that imparts distinctive tissue-specific functions to isoferritins.
Assuntos
Ferritinas , Multimerização Proteica , Humanos , Ferritinas/química , Ferritinas/metabolismo , Ferritinas/genética , Modelos Moleculares , Microscopia CrioeletrônicaRESUMO
The three-dimensional structure of a protein plays a fundamental role in determining its function and has an essential impact on understanding biological processes. Despite significant progress in protein structure prediction, such as AlphaFold2, challenges remain on those hard targets that Alphafold2 does not often perform well due to the complex folding of protein and a large number of possible conformations. Here we present a modified version of the AlphaFold2, called Distance-AF, which aims to improve the performance of AlphaFold2 by including distance constraints as input information. Distance-AF uses AlphaFold2's predicted structure as a starting point and incorporates distance constraints between amino acids to adjust folding of the protein structure until it meets the constraints. Distance-AF can correct the domain orientation on challenging targets, leading to more accurate structures with a lower root mean square deviation (RMSD). The ability of Distance-AF is also useful in fitting protein structures into cryo-electron microscopy maps.