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Summary
Abstract
Introduction
Protocol
Results
Discussion
Disclosures
Acknowledgements
Materials
References
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Neuroscience

Patch clamp di celle Starburst amacrine in un appartamento di montaggio Preparazione di Deafferentated mouse Retina

Published: October 13, 2016
doi:
10.3791/54608
, , ,
1Department of Ophthalmology,Baylor College of Medicine, 2Department of Neuroscience,Baylor College of Medicine, 3Department of Biochemistry and Molecular Biology,Baylor College of Medicine

Summary

Questo protocollo dimostra come eseguire cellula intera registrazione patch clamp su neuroni della retina da una preparazione TV a montare.

Abstract

La retina dei mammiferi è un tessuto stratificato composto da più tipi di neuroni. Per capire come i segnali visivi vengono elaborati all'interno della propria rete sinaptica intricata, registrazioni elettrofisiologiche sono spesso utilizzati per studiare le connessioni tra i singoli neuroni. Abbiamo ottimizzato una preparazione TV a monte per la registrazione patch clamp di neuroni geneticamente marcate sia in GCL (strato di cellule gangliari) e INL (strato nucleare interno) di retine di topo. Registrazione neuroni INL a Flat-monti è favorita rispetto fette perché le connessioni sia verticali e laterali sono conservati nella ex di configurazione, consentendo circuiti della retina con componenti di grandi dimensioni laterali da studiare. Abbiamo usato questa procedura per confrontare le risposte dei neuroni specchio-partnered in retine come i colinergici cellule amacrine starburst (ZSC).

Introduction

As an easily accessible part of the central nervous system, the retina has for decades been a useful model in neuroscience studies. Genetic marking of neurons has allowed detailed characterization of synaptic connections in the retina. With many methodologies available to examine function and morphology of retinal neurons, the patch clamp recording technique has been instrumental in our current understanding of vertically transmitted signals in the retina. These signals are originated from photon absorption in photoreceptors and sent to brain visual centers through spiking of retinal ganglion cells (RGCs). Despite a large body of knowledge accumulated thus far, neural diversity in vascularized mammalian retina remains unsolved and obstructs the full appreciation of retinal circuits that subserve normal vision. This is in part because most recordings were performed on retinal slices to trade lateral circuit integrity for access to more proximal retinal neurons1-3. To gain a comprehensive picture on how retina computes visual signals, it is thus desirable to record neurons in flat-mounts wherein lateral connections, large and small, may be better preserved.

When synaptic transmission from photoreceptors to bipolar cells is interrupted due to a defective metabotropic glutamate receptor 6 (mGluR6) signaling pathway in depolarizing bipolar cells4-6 or simply as the result of photoreceptor loss in degenerated retinas7-10, many RGCs exhibit oscillatory activities. These oscillations originate from multiple sources, however the one involving gap junction coupling between AII amacrine cells (AII-ACs) and depolarizing cone bipolar cells (DCBCs) has received the most attention and hence is best understood1,7,11. We have found another source, which persists under pharmacological blockade of the aforementioned AII-AC/DCBC network and drives oscillation of OFF-type SACs in RhoΔCTA and Nob mice with deafferentated retinas7,8,12. Here we detail our protocol of preparing retinal flat-mounts for INL neuron recording. This approach uses commercial mouse lines (Jax stock no. 006410 and 007905) to mark cholinergic retinal neurons by fluorescent protein (tdTomato) expression that is identifiable under a fluorescent microscope equipped with contrast enhancing optics. Some experimental results acquired through this approach have been previously reported4,5,7,13.

Protocol

l'approvazione etica – procedure che coinvolgono soggetti animali sono state condotte in conformità con le norme ei regolamenti del National Institutes of linee guida sanitarie per gli animali di ricerca, come approvato dalla cura degli animali istituzionale e usare comitato di Baylor College of Medicine. 1. esterno e delle soluzioni interne Utilizzare la soluzione di Ringer mammiferi durante la dissezione retina e la soluzione esterna nella successiva registrazione elettrofisiologica. Preparare …

Representative Results

Registrazioni rappresentativi di on e off-tipo ZSC da una retina deafferentated del mouse sono mostrati in figura 1. Le cellule colinergici sia in GCL e INL può essere attendibilmente identificate da tdTomato fluorescenza e mirati per la cellula intera registrazione patch clamp sotto DIC (Figura 1A) a rivelare l'oscillazione dei loro potenziali di membrana (in alto tracce) e le correnti sinaptiche che la determinano (tracce di fondo, figura …

Discussion

Molti laboratori hanno registrato dai neuroni GCL nella preparazione 15-18 TV a monte, ma le nostre procedure consentono la registrazione da neuroni INL. Con la presente sottolineare diversi passaggi che sono fondamentali per le registrazioni di routine di successo.

La freschezza e planarità della retina sono importanti per penetrare con una pipetta di registrazione. A questo proposito, il fermo attaccamento della retina alla membrana di nitrocellulosa perforato è fondamentale e…

Disclosures

The authors have nothing to disclose.

Acknowledgements

We thank Joung Jang and Xin Guan for technical assistance. We thank Dr. Rory McQuiston of Virginia Commonwealth University for setting up our first patch clamp rig and advices on experimental procedures. We thank Dr. Samuel Wu for suggestions on voltage clamp recording. The work is supported by NIH grants EY013811, EY022228 and a vision core grant EY002520. C-KC is the Alice R. McPherson Retina Research Foundation Endowed Chair at the Baylor College of Medicine.

Materials

Fixed-stage fluorescent microscope with DIC Olympus BX51-WI
Micromanipulators Sutter MP-225
Patch clamp amplifier A-M System AM2400
AD converter National Instrument NI-USB-6221
Heater controller Warner Instrument TC-324B
Inline heater Warner Instrument SC-20
Peristaltic pump Rainin Dynamax
pipette puller Sutter Instrument P-1000
Glass tube with filament King Precision Glass Customized
Stimulator A.M.P.I. Master-8
Biocytin Sigma B4261
NaCl Sigma S6191
KCl Sigma P5405
NaHCO3 Fisher BP328-1
Na2HPO4 Sigma S0876
NaH2PO4 Sigma S5011
CaCl2 Sigma C5670
MgSO4 Sigma M1880
D-glucose Sigma G6152
K-gluconate Sigma G4500
ATP-Mg Sigma A9187
Li-GTP Sigma G5884
EGTA Sigma E0396
HEPES Sigma H4034
KOH Sigma P5958
Cs-methanesulfonate Sigma C1426
CsOH Sigma 232041
Syringer filter Nalgene 171
1 ml syring Rainin 17013002
10 ul pipette tip Genesee Scientific 24-130RL
Streptavidin-488 ThermoFisher S-11223
10X PBS Lonza 17-517Q
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References

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Tags

Patch ClampStarburst Amacrine CellsFlat-mountDeafferentated Mouse RetinaRetinal NeurobiologyRetinal CircuitsWhole-cell RecordingNitrocellulose MembraneExternal SolutionCarbogenatedUpright Microscope

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Tu, H., Hsu, C., Chen, Y., Chen, C. Patch Clamp Recording of Starburst Amacrine Cells in a Flat-mount Preparation of Deafferentated Mouse Retina. J. Vis. Exp. (116), e54608, doi:10.3791/54608 (2016).
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