Multiplexed volumetric CLEM enabled by scFvs provides insights into the cytology of cerebellar cortex.
Xiaomeng HanXiaotang LuPeter H LiShuohong WangRichard SchalekYaron MeirovitchZudi LinJason AdhinartaKarl D MurrayLeah M MacNivenDaniel Raimund BergerYuelong WuTao FangElif Sevde MeralShadnan AsrafHidde L PloeghHanspeter PfisterDonglai WeiViren JainJames S TrimmerJeff William LichtmanPublished in: Nature communications (2024)
Mapping neuronal networks is a central focus in neuroscience. While volume electron microscopy (vEM) can reveal the fine structure of neuronal networks (connectomics), it does not provide molecular information to identify cell types or functions. We developed an approach that uses fluorescent single-chain variable fragments (scFvs) to perform multiplexed detergent-free immunolabeling and volumetric-correlated-light-and-electron-microscopy on the same sample. We generated eight fluorescent scFvs targeting brain markers. Six fluorescent probes were imaged in the cerebellum of a female mouse, using confocal microscopy with spectral unmixing, followed by vEM of the same sample. The results provide excellent ultrastructure superimposed with multiple fluorescence channels. Using this approach, we documented a poorly described cell type, two types of mossy fiber terminals, and the subcellular localization of one type of ion channel. Because scFvs can be derived from existing monoclonal antibodies, hundreds of such probes can be generated to enable molecular overlays for connectomic studies.
Keyphrases
- electron microscopy
- living cells
- single molecule
- single cell
- fluorescent probe
- quantum dots
- cerebral ischemia
- label free
- small molecule
- functional connectivity
- high resolution
- resting state
- high grade
- stem cells
- healthcare
- white matter
- cancer therapy
- cell therapy
- mass spectrometry
- energy transfer
- brain injury
- health information
- case control
- high density
- subarachnoid hemorrhage
- bone marrow