| Literature DB >> 35786637 |
Chanmi Yeon1, Jeong Myo Im1, Minsung Kim1, Young Ro Kim2,3, Euiheon Chung1,4,5.
Abstract
Optical neuroimaging provides an effective neuroscience tool for multi-scale investigation of the neural structures and functions, ranging from molecular, cellular activities to the inter-regional connectivity assessment. Amongst experimental preparations, the implementation of an artificial window to the central nervous system (CNS) is primarily required for optical visualization of the CNS and associated brain activities through the opaque skin and bone. Either thinning down or removing portions of the skull or spine is necessary for unobstructed long-term in vivo observations, for which types of the cranial and spinal window and applied materials vary depending on the study objectives. As diversely useful, a window can be designed to accommodate other experimental methods such as electrophysiology or optogenetics. Moreover, auxiliary apparatuses would allow the recording in synchrony with behavior of large-scale brain connectivity signals across the CNS, such as olfactory bulb, cerebral cortex, cerebellum, and spinal cord. Such advancements in the cranial and spinal window have resulted in a paradigm shift in neuroscience, enabling in vivo investigation of the brain function and dysfunction at the microscopic, cellular level. This Review addresses the types and classifications of windows used in optical neuroimaging while describing how to perform in vivo studies using rodent models in combination with other experimental modalities during behavioral tests. The cranial and spinal window has enabled longitudinal examination of evolving neural mechanisms via in situ visualization of the brain. We expect transformable and multi-functional cranial and spinal windows to become commonplace in neuroscience laboratories, further facilitating advances in optical neuroimaging systems.Entities:
Keywords: Central nervous system; Craniotomy; Functional neuroimaging; Laboratory animal models; Neuroimaging; Optical imaging
Year: 2022 PMID: 35786637 PMCID: PMC9272117 DOI: 10.5607/en22015
Source DB: PubMed Journal: Exp Neurobiol ISSN: 1226-2560 Impact factor: 3.800
Fig. 1Region of interest (ROI)-based cranial and spinal window classification; (a) olfactory bulb window, (b) cerebral cortex window, (c) cerebellar window, and (d) spinal cord chamber window (SCCW). The CNS consists of the brain and the spinal cord. The cranial and spinal window is advantageous for observing the outer surface of the brain and the spinal cord. The cerebral cortex is the largest and the most accessible part of the cerebrum, where the motor and the sensory areas are located. The cranial and spinal window enables observing brain connectivity during a behavioral test in brain disease models combining neuroscience methods. The cranial and spinal window and behavioral apparatus are verified.
Fig. 2Types of the cranial and spinal window. (a) Open-skull cranial window, (b) sealed cranial window, (c) thinned-skull cranial window, (d) a plug type open-close window, (e) threaded retractable cranial window, (f) flexible PDMS-based accessible window, and (g) skull optical clearing window (SOCW). The cranial window thins down or removes a part of the skull and then takes proper steps for safe and long-term observation. The window structure, material, and size can be varied by the research objectives. Open skull preparation, sealed cranial window, and thinned-skull cranial window are the traditional forms of the cranial window. In contrast, variously modified forms have been developed, such as open-close, retractable and accessible windows, to combine with other neuroscience methodologies.
The cranial and spinal windows for optical neuroimaging in vivo
| Subject | Animal | Mouse | Mouse | Mouse | Mouse | Mouse | Mouse | Mouse | Mouse |
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| Species | Male B6CBAF1 or female Thy1.2YFP-H | YFP-H, CX3CR1-GFP, CX3CR1-GFP x YFP-H, Emx-1-cre, GFAP-GFP | Thy1-YFP-H and GFP-M (neuron) | Female transgenic C57BL/6 expressing GCaMP6s/f and GFP-m | C57BL/6 male | C57BL/6, Ai95(RCL-GCaMP6f)-D, NG2-CreERT2, Thy1-GCaMP6f | Sox9 cKO: Sox9fl/fl; CAG-CreER; Aldh1L1-EGFP | G7NG817, Thy1-EYFP-H | |
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| Anesthetization | Awake | Anesthetized with isoflurane | Anesthetized with isoflurane | Awake | Anesthetized with isoflurane | Awake | Anesthetized with isoflurane | Awake or anesthetized with isoflurane | |
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| Region of interest | Primary sensory cortical areas (S1HL[ | Spinal cord: vertebrae (T10-T12[ | CA1[ | Sensory and motor cortex | Primary sensory cortical areas (S1FL[ | Olfactory bulb | Olfactory bulb | Primary visual cortex (V1[ | |
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| Window | Window type | Open-close window (plug) | Open-close window (plug) | Modified sealed cranial window | Thinned-skull or intact skull window | Sealed cranial window | Sealed cranial window | Thinned-skull window | PEO-CYTOP[ |
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| Window size | ~4 mm in diameter | 5 mm in diameter | 0.84 mm in diameter | ~ 9×9 mm | 6 mm in diameter | 2~3 mm in diameter | > 8 mm in diameter | ||
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| Window material | Glass coverslip | Metal bars, glass coverslip | Glass capillary, glass coverslip, stainless steel screws | Glass coverslip, steel head bar | Anodized titanium | A titanium head-bar, glass coverslip | Glass coverslip | PEO-CYTOP nanosheet | |
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| Bonding material | N/A | Dental acrylic and cyanoacrylate | Dental acrylic, UV curing epoxy | Mixture of metabond and dental cement | Dental cement | Photopolymerizable dental cement | N/A | UV curable dental acrylic | |
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| Optical imaging | Imaging technique | 2PE-CaSDI | 2PEF | 1PEF and 2PEF | OISI | OISI, LSCI | 2PE-CaSDI | 2PE-CaSDI | 2PEF, 2PE-CaSDI |
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| Measuring frequency (temporal resolution) | (256 msec/frame) | N/A | 100 Hz (up to 1.2 kHz) | 30 Hz | 10 Hz/5 Hz (200 msec/ 400 msec) | (50~150 msec/frame) | 10~35 Hz | 1 Hz for EYFP, 30 Hz for GCaMP7, 3.8 Hz (CaSDI) | |
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| Measuring time | 4~5 min | N/A | Multiple sessions (30~60 min) | 30 sec or 11.5 and 5 min | 20 sec | N/A | 10 sec/trial | N/A | |
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| Objective lens | 40X/0.8 NA[ | 20X/1.0 NA water-immersion, 40X/0.8 NA, water-immersion, 4X/0.28 NA | 10X/0.25 NA, 20X/0.40 NA (1PEF) | Adjustable lens (f[ | 4X/0.10 NA | 60X/1.10NA, 40X/0.8NA | 20X/1.0 NA | 16X/0.80 NA water-immersion (cross-sectional imaging), 25X/1.10 NA water-immersion (deep in vivo imaging), 2X/0.20NA (CaSDI) | |
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| Test & Apparatus | Animal test | Spherical treadmill running training | Open field and runway assays | N/A | Automated self-head-fixation and visual-evoked cortical imaging | Somatosensory-evoked functional imaging | Synaptic activity triggers odor-specific OPC[ | Three compartment place preference assay | CaSDI in vast FOV, deep and wide-field imaging |
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| Behavior test apparatus | Air-supported free-floating Styrofoam ball | Plexiglass enclosure to enter a dark goal box at the end of the runway | N/A | Fully automated and self-initiated head-fixation system for functional imaging, yellow light flash stimulator | Electrical sensory stimulator | Sensory stimulation, running wheel with head fixed | A testing chamber, video with a behavior tracking camera (for odor discrimination) | N/A | |
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| Life supporting system | N/A | Rectal thermometer and feedback-controlled heating blanket at 37.5°C | Heating blanket | N/A | 37°C heating pad | 36.5~37°C heating pad, pneumogram transducer | Heating pad | Disposable heating pad | |
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| Ref. | Published year | 2007 | 2012 | 2011 | 2016 | 2016 | 2018 | 2021 | 2020, 2021 |
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| First author | Dombeck, D. A. | Farrar, M. J. | Barretto, R. P. J. | Murphy, T. H. | Cho, A. | Rungta, R. L. | Ung, K. | Takahashi, T. | |
The cranial and spinal window types were varied by the research objectives, animal condition and optical imaging methods.
aS1HL primary somatosensory hindlimb cortex; bT10-T12 tenth to twelfth thoracic vertebra; cCA1 the first region in the hippocampal circuit; dS1FL primary somatosensory forelimb cortex; eV1 primary visual cortex; fNA numerical aperture; gf focal length; hOPC oligodendrocyte precursor cell.
The advanced cranial and spinal windows applying to optical neuroimaging combined with other neurological research methods
| Subject | Animal | Mouse | Rat | Mouse | Mouse | Rat and mouse | Mouse |
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| Species | B6.Cg-Tg(Thy1-COP4/EYFP)18Gfng/J | Male Sprague Dawley rats | Thy1-GCaMP3, wild-type | VGAT-ChR2-EYFP BAC, Scnn1a-TG3-Cre x Ai32 | C57BL6, Cx3Cr1GFP+/− mice | Thy1-ChR2-YFP, GAD67-GFP10, wild-type ICR mice. | |
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| Anesthetization | Anesthetized with isoflurane | Anesthetized with isoflurane | Awake | Anesthetized with isoflurane (OISI), awake (2PE-CaSDI) | Anesthetized with isoflurane | Anesthetized with isoflurane | |
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| Region of interest | Primary sensory cortex (S1FL, S1HL), barrel cortex (S1BC[ | Somatosensory cortex | Somatosensory cortex | Barrel cortex (C2), somatosensory (S1), and frontal area (ALM[ | Somatosensory cortex | Barrel cortex | |
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| Window | Window type | Sealed cranial window | Partial open skull window | Sealed cranial window | Open-close window (plug) | Accessible window | Sealed cranial window |
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| Window size | 7 mm×8 mm bilateral, | 5 mm in diameter | 3~3.5 mm in diameter | 3 mm in diameter | 6 mm in diameter | ~ 4×4 mm | |
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| Window material | Glass coverslip | Glass coverslip | Glass coverslip | Glass coverslip | Glass coverslip, PDMS film | Glass coverslip, metal holding bar | |
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| Bonding material | Mixture of dental cement and polyacrylic glue | UV curable dental acrylic | Mixture of dental cement and polyacrylic glue | Optical curable glue, dental acrylic | Cyanoacrylate glue and a dental resin | Dental acrylic | |
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| Optical imaging | Imaging technique | VSDI | Vascular fluorescence imaging | 2PE-CaSDI, OISI | 2PE-CaSDI, OISI | 2PEF, OISI | 2PEF, 2PE-CaSDI, OISI |
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| Measuring frequency (temporal resolution) | 150 Hz (6.67 msec/frame) | N/A | 10 Hz | 7.8 Hz per plane (2PE-CaSDI) | 10 Hz (OISI) | 25~50 Hz (2PEF line scan), 10 Hz (CaSDI), 18 Hz (OISI) | |
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| Measuring time | 108 frames (~720 msec) | N/A | 6 min | 8 sec (2PE-CaSDI), 20 sec (OISI) | 5 min (2PEF), 20 sec (OISI) | N/A | |
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| Objective lens | 5X/0.15 NA, 20X/0.50 NA | N/A | N/A | 16x/0.8 NA | 25X/0.95 NA or 10X/0.22 NA (2PEF) | 4X/0.28 NA, 5X 0.16NA, 20X/0.5 NA | |
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| Test & Apparatus | Objectives | Comparison of sensory-evoked cortical maps with ChR2[ | N/A | Habituation-dishabituation olfactory test, smell recognition | Photoinhibition of barrel cortex during wall tracking | Electrical stimulation | Vascular and electrical responses to optogenetic photostimulation |
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| Combined methodology | Sensory stimulation, Optogenetic stimulation, electroencephalogram (EEG) | Micro-ECoG[ | Patch-clamp recordings evoked cortical activity | Optogenetic stimulation, sensory stimulation (whisker), extracellular electrophysiology | Hindpaw electrical stimulation | LFP[ | |
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| Additional apparatus | Piezoelectric device for sensory stimulator | N/A | Air-lifted mobile homecage | Tactile virtual reality system for head-fixed mice running on a spherical treadmill, movable walls for whisker stimulation, laser photostimulation system | Inserting 30-gauge needle electrodes, connected to a pulse isolator and pulse stimulator | Stimulation device | |
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| Life supporting system | 37°C heating pad | Pulse oximeter | N/A | 37°C heat blanket | 36.5~37.5°C heating pad | N/A | |
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| Ref. | Published year | 2012 | 2013 | 2014 | 2015 | 2016 | 2018 |
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| First author | Lim, D. H. | Schendel, A. A. | Kislin, M. | Sofroniew, N.J | Heo, C. | Thunemann, M. | |
This table shows the multi-functional cranial and spinal windows or special designed cranial and spinal windows to combine neuroimaging and other neuroscience methodologies such as EEG, ECoG, patch clamp or Optogenetic stimulation, simultaneously.
aS1BC primary somatosensory; aS1BC barrel cortex; bA1 primary auditory cortex; cALM anterior lateral motor cortex; dChR2 channelrhodopsin-2; eECoG electrocorticography; fLFP local field potential.
Fig. 3Examples of cranial and spinal window; (a) a sealed cranial windows (closed cranial window) (an original image), (b) a plug type open-close/retractable/accessible window (Reproduced with permission, Copyright 2014, Frontiers [84]), (c) a window with implanted micro-ECoG multi-channel electrode array and 12 holes (Reproduced with permission, Copyright 2013, Elsevier [114]), (d) a cranial window utilizing a gradient-index (GRIN) lens and endoscopy targeting hippocampus (Reproduced with permission, Copyright 2011, Springer Nature [68]), (e) a flexible PDMS-based accessible window (Reproduced with permission, Copyright 2016, Springer Nature [40]), (f) transparent graphene microelectrode arrays (Reproduced with permission, Copyright 2018, Springer Nature [108]), (g) modified open skull window with PEO-CYTOP fluoropolymer nanosheets (Reproduced with permission, Copyright 2020, Elsevier [87]), and (h) spinal cord chamber window (SCCW) (Reproduced with permission, Copyright 2012, Springer Nature [21]).