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Ixon x3 du897

Manufactured by Oxford Instruments

The IXon X3 DU897 is a high-performance, back-illuminated, electron-multiplying CCD (EMCCD) camera designed for low-light imaging applications. It features a 1004 x 1002 pixel sensor with a 13 x 13 μm pixel size, providing a sensitive and efficient detection solution for a variety of scientific disciplines.

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2 protocols using ixon x3 du897

1

Live-cell Imaging of Cellular Dynamics

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Cells were seeded into glass bottom dishes (MatTek Corporation, P35G-1.5-14-C) and 12 hours later switched to culture medium containing 1% serum and transfected. Two days later, medium was changed to Leibovitz’s L-15 Medium (Gibco, 21083-027) and imaged on a Nikon Ti-E/B microscope equipped with a 100x, 1.49 NA oil-immersion TIRF objective, 1.5x tube lens, three 20mW diode lasers (488, 561, 640 nm) controlled via acousto-optical tunable filter (AOTF) (Agilent) and EMCCD detector (iXon X3 DU897, Andor). Time-lapse images were acquired with 488 nm excitation, 200 ms exposure at 5 or 2.5 frames per second in a humidified imaging chamber (Tokai Hit) at 37 °C. Kymographs were generated using the Multiple K ymograph plugin (J. Rietdorf and A. Seitz) for ImageJ (NIH).
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2

Visualizing Olfactory Neurons in Mice

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To express genes of interest, 10–20 µl of purified viral construct was intranasally administered to mice ranging between 10 and 40 days of age. Typically, viral delivery was repeated in three consecutive days. At 10 days post infection, mice were anesthetized with CO2, rapidly decapitated, and entire turbinates and septum were dissected and kept on ice in a Petri dish filled with freshly oxygenated carbogen-modified artificial cerebrospinal fluid (ACSF) that contained (in mM): 120 NaCl, 25 NaHCO3, 3 KCl, 1.25 Na2HPO4, 1 MgSO4, 1.8 CaCl2, 15 glucose, 305 mOsm (adjusted with sucrose), pH 7.4. For imaging, a small piece of the OE was mounted in the perfusion chamber (RC-23, Warner Instruments) with the apical surface facing down and analyzed on the Nikon TiE-PFS-A1R confocal microscope equipped with a 60× oil-immersion objective, using preset configuration for acquisition of GFP and mCherry fluorescence. Image acquisition settings were set to avoid pixel saturation and maintained equal when comparing WT control and INPP5E-KO tissue.
For total internal reflection fluorescence microscopy (TIRF) en face imaging, virally transduced mice were prepared as above. TIRF imaging was performed on a Nikon Eclipse Ti-E/B inverted microscope equipped with a 100× oil immersion CFI APO TIRF 1.49 NA and an EMCCD camera (iXon X3 DU897, Andor Technology).
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