Integrated preassembled system that performs imaging and sequence library preparation at the same time

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Stanford Reference: 16-007 Abstract Researchers at Stanford University have developed ATAC-see (Assay of Transposase-Accessible Chromatin with visualization), a one-step strategy to image and sequence regulatory DNA. Eukaryotic genomes are generally compacted into chromatin except for the active regulatory elements that control gene activity. The spatial organization of these accessible elements is linked to gene expression, replication and DNA repair, however the in situ organization is largely unknown. To overcome this, the inventors have developed the ATAC-see method. It uses a novel bifunctional enzyme complex. When the complex is placed on cell samples it simultaneously makes the active regulatory DNA fluorescent and ready for sequencing. This method enables direct imaging of the accessible genome in situ, cell sorting, and deep sequencing to reveal the identity of the imaged elements. ATAC-see provides a combination of spatial and epigenomic information for a molecular portrait of the cell. Stage of research The ATAC-see method has been used to examine the spatial organization of the accessible genome in its native context for a variety of cell types, including five human cell types. Applications Research Single cell analysis Morphological identification of diseased cells Prospective sorting of cells based on regulatory DNA status Identification of regulatory DNA by imaging and sequencing Advantages New method to: Capture spatial information on regulatory DNA in intact cell Sort cells based on status of regulatory DNA Image and sequence DNA from the same sample Allows identification of epigenomic information from formalin-fixed cells, including clinical samples Integrated preassembled system that performs imaging and sequence library preparation at the same time Easy quality control for DNA sequencing libraries Labeling strategy is compatible with different fluorophores and chemical tags Compatible with multimodal imaging of landmark proteins  

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