Whole-brain calcium imaging with cellular resolution in freely behaving
            <i>Caenorhabditis elegans</i>

Nguyen, Jeffrey P.; Shipley, Frederick B.; Linder, Ashley; Plummer, George S.; Liu, Mochi; Setru, Sagar; Shaevitz, Joshua W.; Leifer, Andrew M.

doi:10.1073/pnas.1507110112

Cited by 360 publications

(381 citation statements)

References 51 publications

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“…A similar approach to brainwide imaging in moving C. elegans using the same transgenic strain has recently been reported (22). Although both setups use customized spinning disk confocal microscopes, the strategies for tracking the moving neurons and analyzing behavioral and neural activity patterns are different.…”

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confidence: 99%

Pan-neuronal imaging in roaming Caenorhabditis elegans

Venkatachalam

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

215

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We present an imaging system for pan-neuronal recording in crawling Caenorhabditis elegans. A spinning disk confocal microscope, modified for automated tracking of the C. elegans head ganglia, simultaneously records the activity and position of ∼80 neurons that coexpress cytoplasmic calcium indicator GCaMP6s and nuclear localized red fluorescent protein at 10 volumes per second. We developed a behavioral analysis algorithm that maps the movements of the head ganglia to the animal's posture and locomotion. Image registration and analysis software automatically assigns an index to each nucleus and calculates the corresponding calcium signal. Neurons with highly stereotyped positions can be associated with unique indexes and subsequently identified using an atlas of the worm nervous system. To test our system, we analyzed the brainwide activity patterns of moving worms subjected to thermosensory inputs. We demonstrate that our setup is able to uncover representations of sensory input and motor output of individual neurons from brainwide dynamics. Our imaging setup and analysis pipeline should facilitate mapping circuits for sensory to motor transformation in transparent behaving animals such as C. elegans and Drosophila larva.C. elegans | Drosophila | calcium imaging | thermotaxis U nderstanding how brain dynamics creates behaviors requires quantifying the flow and transformation of sensory information to motor output in behaving animals. Optical imaging using genetically encoded calcium or voltage fluorescent probes offers a minimally invasive method to record neural activity in intact animals. The nematode Caenorhabditis elegans is particularly ideal for optical neurophysiology owing to its small size, optical transparency, compact nervous system, and ease of genetic manipulation. Imaging systems for tracking the activity of small numbers of neurons have been effective in determining their role during nematode locomotion and navigational behaviors like chemotaxis, thermotaxis, and the escape response (1-6).Recordings from large numbers of interconnected neurons are required to understand how neuronal ensembles carry out the systematic transformations of sensory input into motor patterns that build behavioral decisions.Several methods for fast 3D imaging of neural activity in a fixed imaging volume have been developed for different model organisms (7)(8)(9)(10)(11)(12)(13)(14). High-speed light sheet microscopy, light field microscopy, multifocus microscopy, and two-photon structured illumination microscopy have proved effective for rapidly recording large numbers of neurons in immobilized, intact, transparent animals like larval zebrafish and nematodes (15)(16)(17)(18)(19). However, these methods are problematic when attempting to track many neurons within the bending and moving body of a behaving animal. Panneuronal recording in moving animals poses higher demands on spatial and temporal resolution. Furthermore, extracting neuronal signals from recordings in a behaving animal requires an effective analysis pipel...

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confidence: 99%

Pan-neuronal imaging in roaming Caenorhabditis elegans

Venkatachalam

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

215

216

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“…Both CLSM and SDCM have been ground-breaking for imaging in vitro as well as in vivo; for instance, relatively thin model systems (Fig. 1C), such as tissue explants and organoids, or small organisms, such as Caenoerhabditis elegans (Nguyen et al, 2016) or zebrafish embryos (Kissa and Herbomel, 2010). Recent advances in CLSM have led to the development of the so-called Airyscan concept (Zeiss), whose detector array allows to efficiently collect the photons from the entire Airy diffraction image with confocal resolution owing to the intrinsic size of each detector.…”

Section: Optical Tweezers In Vivomentioning

confidence: 99%

“…Scale bar:10 µm. Adapted with permission from Nguyen et al, 2016. Middle: confocal laser scanning microscope (CLSM) used for long-term (>70 h) time-lapse imaging of zebrafish vasculature, highlighting the emergence of a hematopoietic stem cell in the ventral wall of the dorsal aorta (green).…”

Section: Shg Thg Carsmentioning

confidence: 99%

Seeing is believing: multi-scale spatio-temporal imaging towards in vivo cell biology

Follain

Mercier

Osmani

et al. 2016

Journal of Cell Science

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Life is driven by a set of biological events that are naturally dynamic and tightly orchestrated from the single molecule to entire organisms. Although biochemistry and molecular biology have been essential in deciphering signaling at a cellular and organismal level, biological imaging has been instrumental for unraveling life processes across multiple scales. Imaging methods have considerably improved over the past decades and now allow to grasp the inner workings of proteins, organelles, cells, organs and whole organisms. Not only do they allow us to visualize these events in their most-relevant context but also to accurately quantify underlying biomechanical features and, so, provide essential information for their understanding. In this Commentary, we review a palette of imaging (and biophysical) methods that are available to the scientific community for elucidating a wide array of biological events. We cover the most-recent developments in intravital imaging, light-sheet microscopy, superresolution imaging, and correlative light and electron microscopy. In addition, we illustrate how these technologies have led to important insights in cell biology, from the molecular to the whole-organism resolution. Altogether, this review offers a snapshot of the current and state-of-the-art imaging methods that will contribute to the understanding of life and disease.

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“…Recently developed optical recording methods based on calcium- and voltage-sensitive fluorescence can record a proxy for electrical activity of individual cells in intact C. elegans 7–18 ; however, compared to electrical recordings, optical measurements typically have a lower signal-to-noise ratio and reduced temporal resolution 19 . As a result, optical methods have yet to resolve individual action potentials (APs) or synaptic potentials in C. elegans 7–18 .…”

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confidence: 99%

“…As a result, optical methods have yet to resolve individual action potentials (APs) or synaptic potentials in C. elegans 7–18 .…”

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confidence: 99%

Scalable electrophysiology in intact small animals with nanoscale suspended electrode arrays

et al. 2017

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Electrical measurements from large populations of animals would help reveal fundamental properties of the nervous system and neurological diseases. Small invertebrates are ideal for these large-scale studies; however, patch-clamp electrophysiology in microscopic animals typically requires low-throughput and invasive dissections. To overcome these limitations, we present nano-SPEARs: suspended electrodes integrated into a scalable microfluidic device. Using this technology, we have made the first extracellular recordings of body-wall muscle electrophysiology inside an intact roundworm, Caenorhabditis elegans. We can also use nano-SPEARs to record from multiple animals in parallel and even from other species, such as Hydra littoralis. Furthermore, we use nano-SPEARs to establish the first electrophysiological phenotypes for C. elegans models for Amyotrophic Lateral Sclerosis and Parkinson’s disease, and show a partial rescue of the Parkinson’s phenotype through drug treatment. These results demonstrate that nano-SPEARs provide the core technology for microchips that enable scalable, in vivo studies of neurobiology and neurological diseases.

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Whole-brain calcium imaging with cellular resolution in freely behaving Caenorhabditis elegans

Cited by 360 publications

References 51 publications

Pan-neuronal imaging in roaming Caenorhabditis elegans

Pan-neuronal imaging in roaming Caenorhabditis elegans

Seeing is believing: multi-scale spatio-temporal imaging towards in vivo cell biology

Scalable electrophysiology in intact small animals with nanoscale suspended electrode arrays

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