A robot for high yield electrophysiology and morphology of single neurons in vivo

Lu, Li; Ouellette, Benjamin; Stoy, William; Garren, Emma; Daigle, Tanya L.; Forest, Craig R.; Koch, Christof; Zeng, Hongkui

doi:10.1038/ncomms15604

Cited by 18 publications

(18 citation statements)

References 43 publications

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“…Full reconstruction of a single neuron requires sparse, robust and consistent neuronal labeling. Previous genetic approaches applied to produce sparse or single neuron labeling, including viral delivery (e.g., using sindbis virus or AAV) and in vivo electroporation [22][23][24][26][27][28][29][30][31]37 , often resulted in substantial cell-to-cell and animal-to-animal variations, and were usually restricted to few brain regions. In rare cases, extremely sparse labeling was obtained utilizing the low recombination efficiency of CreER driver lines and a sensitive, alkaline phosphatase-based histochemical reporter 25,41 .…”

Section: Sparse Robust and Consistent Neuronal Labelingmentioning

confidence: 99%

“…Despite its importance, data on single neuron axonal morphologies are currently lacking for most projection neuron types in mammals, in large part because axons often cover large distances and are severed in ex vivo brain slices. Previous efforts have been made in rodents to fully label single neurons with small molecules or fluorescent proteins through in vivo whole-cell patching, in vivo electroporation [22][23][24] , sparse transgenic labeling 25 , or sparse viral labeling with sindbis virus [26][27][28] or adeno-associated virus (AAV) [29][30][31] . Conventionally this is followed by serial sectioning, imaging of each section, and manual reconstruction of the labeled neurons across many consecutive sections.…”

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Brain-wide single neuron reconstruction reveals morphological diversity in molecularly defined striatal, thalamic, cortical and claustral neuron types

Peng

Xie

Liu

et al. 2019

Preprint

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32Ever since the seminal findings of Ramon y Cajal, dendritic and axonal morphology has been 33 recognized as a defining feature of neuronal types and their connectivity. Yet our knowledge 34 about the diversity of neuronal morphology, in particular its distant axonal projections, is still 35 extremely limited. To systematically obtain single neuron full morphology on a brain-wide scale 36in mice, we established a pipeline that encompasses five major components: sparse labeling, 37whole-brain imaging, reconstruction, registration, and classification. We achieved sparse, robust 38and consistent fluorescent labeling of a wide range of neuronal types across the mouse brain in 39 an efficient way by combining transgenic or viral Cre delivery with novel transgenic reporter 40 lines, and generated a large set of high-resolution whole-brain fluorescent imaging datasets 41containing thousands of reconstructable neurons using the fluorescence micro-optical sectioning 42 tomography (fMOST) system. We developed a set of software tools based on the visualization 43 and analysis suite, Vaa3D, for large-volume image data processing and computation-assisted 44 morphological reconstruction. In a proof-of-principle case, we reconstructed full morphologies 45 of 96 neurons from the claustrum and cortex that belong to a single transcriptomically-defined 46 neuronal subclass. We developed a data-driven clustering approach to classify them into multiple 47 morphological and projection types, suggesting that these neurons work in a targeted and 48coordinated manner to process cortical information. Imaging data and the new computational 49 reconstruction tools are publicly available to enable community-based efforts towards large-scale 50 full morphology reconstruction of neurons throughout the entire mouse brain. 51 52 53

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Section: Sparse Robust and Consistent Neuronal Labelingmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Brain-wide single neuron reconstruction reveals morphological diversity in molecularly defined striatal, thalamic, cortical and claustral neuron types

Peng

Xie

Liu

et al. 2019

Preprint

Self Cite

View full text Add to dashboard Cite

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“…Live-cell sampling in LAESI occurs on the millisecond timescale under ambient conditions,t hereby maintaining the cells in their native state until right before analysis. [130][131] This approach can be combined with capillary microsampling followed by ESI-MS analysis in ar apid and controlled fashion. [129] In situ sampling with probes,such as capillary microsampling,enables direct extraction of cell contents.…”

Section: Mitigating Perturbations Due To Samplingmentioning

confidence: 99%

Single‐Cell Mass Spectrometry Approaches to Explore Cellular Heterogeneity

2018

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Compositional diversity is a fundamental property in cell populations. Single-cell analysis promises new insight into this cellular heterogeneity on the genomic, transcriptomic, proteomic, and metabolomic levels. Mass spectrometry (MS) is a label-free technique that enables the multiplexed analysis of proteins, peptides, lipids, and metabolites in individual cells. The abundances of these molecular classes are correlated with the physiological states and environmental responses of the cells. In this Minireview, we discuss recent advances in single-cell MS techniques with an emphasis on sampling and ionization methods developed for volume-limited samples. Strategies for sample treatment, separation methods, and data analysis require special considerations for single cells. Ongoing analytical challenges include subcellular heterogeneity, non-normal statistical distributions of cellular properties, and the need for high-throughput, high molecular coverage and minimal perturbation.

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“…Zur Steigerung von experimentellem Durchsatz und Reproduzierbarkeit können das robotergesteuerte kapillare Mikrosampling und die automatisierte Laserablation untersucht werden. Beispielsweise wurden mit der robotergesteuerten Patch‐Clamp‐Technik spezifische Einzelneuronen anvisiert und ihre elektrophysiologischen Bedingungen gemessen . Diese Methode kann mit dem kapillaren Mikrosampling und anschließender ESI‐MS‐Analyse schnell und kontrolliert kombiniert werden.…”

Section: Vermindern Von Störungen Durch Die Probenentnahmeunclassified

Einzelzell‐Massenspektrometrie zur Untersuchung zellulärer Heterogenität

Zhang

Vertes

2018

Angewandte Chemie

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Die Diversität der Zusammensetzung ist eine fundamentale Eigenschaft von Zellpopulationen. Neue Einblicke in diese zelluläre Heterogenität auf Genom‐, Transkriptom‐, Proteom‐ und Metabolomniveau verspricht die Einzelzellanalyse. Die Massenspektrometrie (MS) ist ein markierungsfreies Verfahren, das die Multiplex‐Analyse von Proteinen, Peptiden, Lipiden und Metaboliten in Einzelzellen ermöglicht. Die Häufigkeiten dieser Verbindungsklassen werden mit den physiologischen Zuständen und den Reaktionen der Zellen auf Umgebungsänderungen korreliert. Dieser Kurzaufsatz beschreibt neue Fortschritte bei den Einzelzell‐MS‐Techniken mit dem Schwerpunkt auf Entnahme‐ und Ionisationsmethoden, die für volumenbegrenzte Proben entwickelt wurden. Bei Einzelzellen erfordern die Strategien zur Probenbehandlung, die Trennmethoden und die Datenanalyse besondere Überlegungen. Aktuelle analytische Herausforderungen betreffen unter anderem die subzelluläre Heterogenität, nicht normale statistische Verteilungen von Zelleigenschaften sowie die Notwendigkeit von Hochdurchsatzanwendungen, einem breiten Molekülspektrum und minimaler Störung.

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A robot for high yield electrophysiology and morphology of single neurons in vivo

Cited by 18 publications

References 43 publications

Brain-wide single neuron reconstruction reveals morphological diversity in molecularly defined striatal, thalamic, cortical and claustral neuron types

Brain-wide single neuron reconstruction reveals morphological diversity in molecularly defined striatal, thalamic, cortical and claustral neuron types

Single‐Cell Mass Spectrometry Approaches to Explore Cellular Heterogeneity

Einzelzell‐Massenspektrometrie zur Untersuchung zellulärer Heterogenität

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