Spinsr confocal microscope

Manufactured by Olympus

The SpinSR confocal microscope is a high-performance imaging system designed for advanced microscopy applications. It utilizes spinning-disk confocal technology to provide high-speed, high-resolution imaging capabilities. The core function of the SpinSR is to capture detailed, optical sections of samples, enabling researchers to visualize and analyze intricate cellular and sub-cellular structures with precision.

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Lab products found in correlation

35 mm glass bottom dishes, by MatTek (1 mentions) Orca fusion camera, by Hamamatsu Photonics (1 mentions) Lysotracker green, by Thermo Fisher Scientific (1 mentions)

Close spelling variants of this product

Confocal microscope (790 citations) SpinSR (10 citations) SPINSR W1 SoRa Spinning Disk Confocal microscope (2 citations) IXplore SpinSR confocal microscope (2 citations)

2 protocols using spinsr confocal microscope

Live-cell Imaging Using Confocal Microscopy

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Cells were seeded into 35-mm glass bottom dishes (MatTek). Images stacks were acquired every 30 s using an Olympus SpinSR confocal microscope comprising Olympus IX83 stand, Olympus 60×1.5 NA UPLAPO objective lens, Yokogawa CSU-W1 scanhead, and Hamamatsu Orca Fusion camera. Images were acquired with a 2 × 2 camera bin, giving a pixel size of 108 nm. Laser excitation and emission filters for the GFP and RFP channels were 488 nm (ex) 525/50 nm (em) and 561 nm (ex) 617/73 nm (em), respectively. The image acquisition software was Olympus cellSens v4.1.

Cross J., Durgan J., McEwan D.G., Tayler M., Ryan K.M, & Florey O. (2023). Lysosome damage triggers direct ATG8 conjugation and ATG2 engagement via non-canonical autophagy. The Journal of Cell Biology, 222(12), e202303078.

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Intracellular Iron Quantification Using FeRhoNox-1

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Intracellular Fe²⁺ accumulation was assessed using the FeRhoNox-1 fluorescent probe (Maokang Biotechnology). HCC1954 cells were treated with DMSO or 10 μM ML-SI1 for 48 h. Subsequently, the cells were incubated at 37 °C for additional 30 min in culture medium containing 5 μM FeRhoNox-1 and 1 μM LysoTracker Green (Thermo Fisher Scientific). Prior to imaging, the cells were rinsed twice with warm-PBS. All images were captured using an Olympus SpinSR confocal microscope, employing lasers with wavelengths of 561 nm and 488 nm to excite FeRhoNox-1 and LysoTracker Green respectively.

Fan C., Wu H., Du X., Li C., Zeng W., Qu L, & Cang C. (2024). Inhibition of lysosomal TRPML1 channel eliminates breast cancer stem cells by triggering ferroptosis. Cell Death Discovery, 10, 256.

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