İşitsel Yolu ve optogenetic Stimülasyon için Murin Dorsal Koklear Çekirdek Doğrudan Görselleştirme
Summary
The goal of this protocol is to outline a surgical approach to provide direct access to the dorsal cochlear nucleus in a murine model.
Abstract
Tutuklama veya işitme kaybı ters virüs aracılı gen transferi kullanımı soruşturma büyük ölçüde çevresel işitme sisteminin küme olmuştur. Birkaç çalışma, merkezi işitme sistemine gen transferi inceledik. işitsel yolun ikinci dereceden nöronları içeren beyin sapı dorsal koklear nükleus (DCN), gen transferi için potansiyel bir sitedir. Bu protokol, posterior fossa yaklaşımı ile kemirgen DCN doğrudan ve maksimal maruz kalma bir tekniktir gösterilmiştir. Bu yaklaşım, akut ya da hayatta kalma cerrahi sağlar. DCN doğrudan görselleştirme sonra, deney bir ana bilgisayar, bir mavi ışık lazer bağlanmış bir fiber optik ile koklear nükleus ve daha sonra stimülasyon içine opsins püskürtülmesi de dahil olmak üzere uygulanabilir. Böyle elektrik stimülasyonu ve nöral enjektör iz gibi diğer nörofizyoloji deneyler de mümkün bulunmaktadır. Visualiza düzeyiyon ve uyarılma süresi elde deneyler geniş bu yaklaşım uygulanamaz hale.
Introduction
Virus-mediated gene transfer to reverse hearing loss has largely been focused on the peripheral auditory system.1 Targeting the cochlea, investigators have examined a host of delivery routes, including osmotic minipump infusion2, vector-transgene complex-soaked Gelfoam®2 or gelatin sponge3, direct microinjection4; numerous gene transfer vectors, including adeno-associated viral vectors5,6, lentiviral vectors7, and cationic liposomes2; and the dissemination of gene transfer vectors beyond the target tissue2. Most recently, adeno-associated virus (AAV)-1 has been introduced in the cochlea in order to treat deafness in mice due to loss of vesicular glutamate transporter-3.8 Further, the application of optogenetics in peripheral auditory system has recently been described.9
Few studies, however, have examined gene transfer to the central auditory system. The dorsal cochlear nucleus (DCN) of the brainstem contain second order neurons of the auditory pathway. While gene transfer techniques in the cochlear nucleus (CN) may be utilized for a host of investigations, gene transfer of opsins, light-sensitive proteins, to the DCN may also be utilized to enable optogenetics-based experimental techniques. Following virus-mediated gene transfer delivery of an opsin, such as channelrhodopsin-2 (ChR2), the neurons of the DCN becomes sensitive to light stimuli. Optogenetic gene transfer has been previously attempted in several brainstem regions, including the rat retrotrapezoid nucleus, mouse locus coeruleus, monkey superior colliculus, and mouse ventral tegmental area.10-14
Recently, investigators have examined the use of optogenetics in the DCN.15,16 The DCN is the location of placement of auditory brainstem implants in humans, making it an attractive part of the auditory system to study for translational studies on auditory neuroprostheses. However, given the location of the DCN, surgical exposure is challenging. The technique described herein provides a protocol for maximal exposure of the DCN via posterior fossa approach to enable viral vector gene transfer and optogenetics-based experiments in a murine model. Previous studies used stereotactic microinjection into the DCN with channelrhodopsin-2.16 Stereotaxic injections, however, are potentially less accurate than injections made by direct visualization, especially in a nucleus as small and deep along the brainstem as the DCN. Transgenic mice expressing tissue specific proteins in the CN are also an attractive option and would obviate the need for gene transfer. Our protocol for exposure of the DCN would also work in transgenic mice as the DCN would need to be directly exposed for optical stimulation. This technique for surgical exposure of the DCN is adapted from previous protocols involving recordings from the auditory nerve and cochlear nucleus in mice and rat models.15,17-20
The overall goal of the protocol is to provide direct exposure to the CN to allow for gene transfer techniques. More specifically, the approach is compatible with both acute and survival surgery and the preparation can be repeated in the same animal for subsequent neurophysiological testing. The direct exposure of the DCN protocol has implications for optogenetics- and virus-mediated gene transfer-based experimentation in other nuclei of the brainstem.
Protocol
Representative Results
Discussion
Bu kağıt, merkezi işitme sisteminin manipülasyonu için fare modelinde DCN doğrudan görselleştirme tekniği anlatılmaktadır. Doğrudan görselleştirme özetlenen yaklaşım stereotaksik yaklaşımlar ana alternatif üzerinde önemli avantajlar sağlar. Stereotaksik yaklaşımlar doğrudan görselleştirme göze değil oysa Öncelikle, DCN doğrudan görselleştirme, beyin sapı sitenin hemen onay veriyor. Virüs-aracılı gen transferi durumunda olduğu gibi, inkübasyon sürelerini uzun süreli gerektirecek d…
Disclosures
The authors have nothing to disclose.
Acknowledgements
Finansman: Bu çalışma Vakfı Bertarelli hibe (DJL), bir MED-EL hibe (DJL) ve Sağlık Hibeler DC01089 bir National Institutes (MCB) tarafından desteklenmiştir.
Materials
| Name of the Material / Equipment | Company | Catalog Number |
| Stereotaxic holder | Stoelting | 51500 |
| Homeothermic blanket | Harvard | 507214 |
| Scalpel blade #11 | Fine Surgical Tools | 10011-00 |
| Iris scissor | Fine Surgical Tools | 14084-08 |
| 5 French suction | Symmetry Surgical | 2777914 |
| Dental Points | Henry Schein | 100-8170 |
| Bone rongeur | Fine Surgical Tools | 16020-14 |
| 10 µl Hamilton syringe | Hamilton | 7633-01 |
| 34 gauge, needle | Hamilton | 207434 |
| Rongeurs | Fine Surgical Tools | 16021-14 |
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