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Structural and molecular interrogation of intact biological systems

2013; Nature Portfolio; Volume: 497; Issue: 7449 Linguagem: Inglês

10.1038/nature12107

1476-4687

Kwanghun Chung, Jenelle L. Wallace, Sung‐Yon Kim, Sandhiya Kalyanasundaram, Aaron S. Andalman, Thomas J. Davidson, Julie J. Mirzabekov, Kelly A. Zalocusky, Joanna Mattis, Aleksandra K. Denisin, Sally Pak, Hannah L. Bernstein, Charu Ramakrishnan, Logan Grosenick, Viviana Gradinaru, Karl Deisseroth,

Cell Image Analysis Techniques

Obtaining high-resolution information from a complex system, while maintaining the global perspective needed to understand system function, represents a key challenge in biology. Here we address this challenge with a method (termed CLARITY) for the transformation of intact tissue into a nanoporous hydrogel-hybridized form (crosslinked to a three-dimensional network of hydrophilic polymers) that is fully assembled but optically transparent and macromolecule-permeable. Using mouse brains, we show intact-tissue imaging of long-range projections, local circuit wiring, cellular relationships, subcellular structures, protein complexes, nucleic acids and neurotransmitters. CLARITY also enables intact-tissue in situ hybridization, immunohistochemistry with multiple rounds of staining and de-staining in non-sectioned tissue, and antibody labelling throughout the intact adult mouse brain. Finally, we show that CLARITY enables fine structural analysis of clinical samples, including non-sectioned human tissue from a neuropsychiatric-disease setting, establishing a path for the transmutation of human tissue into a stable, intact and accessible form suitable for probing structural and molecular underpinnings of physiological function and disease. High-resolution imaging has traditionally required thin sectioning, a process that disrupts long-range connectivity in the case of brains: here, intact mouse brains and human brain samples have been made fully transparent and macromolecule permeable using a new method termed CLARITY, which allows for intact-tissue imaging as well as repeated antibody labelling and in situ hybridization of non-sectioned tissue. High-resolution imaging of biological tissue has traditionally required sectioning, which for tissues like the brain means the loss of long-range connectivity. Now Karl Deisseroth and colleagues have developed a way of making full, intact organs optically transparent and macromolecule-permeable by building a hydrogel-based infrastructure from within the tissue that allows subsequent removal of light-scattering lipids, resulting in a transparent brain. The method, termed CLARITY, also allows repeated antibody labelling of proteins, and in situ hybridization of nucleic acids in non-sectioned tissue, such as full mouse brains or human clinical samples stored in formalin for many years.