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Spectrax led illuminator

Manufactured by Lumencor
Sourced in United States

The SpectraX LED illuminator is a high-performance light source designed for a variety of microscopy and imaging applications. It provides stable, uniform illumination across a wide range of wavelengths, enabling researchers to achieve high-quality, consistent results. The SpectraX offers multiple LED channels, allowing users to select the desired wavelength or combination of wavelengths to suit their specific experimental requirements.

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2 protocols using spectrax led illuminator

1

Fluorescence Imaging of Spore Germination

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Appropriate culture or spore suspension dilutions were placed on agarose pads containing the appropriate medium and supplemented with 1.5% LSL-LE 8200 agarose (Lonza, Basel, Switzerland) on a microscopy slide and covered with a cover glass attached to a 125 µL Gene Frame (Thermo Fisher Scientific, Waltham, MA, USA). TLFM was performed on a Ti-Eclipse inverted microscope (Nikon, Champigny-sur-Marne, France) equipped with a 60× Plan Apo λ oil objective, a TI-CT-E motorized condenser and a Nikon DS-Qi2 camera. GFP was imaged using a quad-edge dichroic (395/470/550/640 nm) and FITC single emission filters. A SpectraX LED illuminator (Lumencor, Beaverton, OR, USA) was used as a light source, using the 470/24 excitation filter. Temperature was controlled at 30 °C (for sporulation) or 37 °C (for germination) with an Okolab cage incubator (Okolab, Ottaviano, Italy). Images were acquired using NIS-Elements software (version 4.51, Nikon) and the resulting pictures were further handled with the open source software ImageJ (version 1.54d) [24 (link)].
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2

Single-Cell Imaging of Bacterial Growth

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Appropriate dilutions of cultures or spore suspensions were placed on agarose pads (MOPS medium supplemented with 1.5% LSL-LE 8200 agarose [Lonza, Basel, Switzerland] and 30 mM l-valine) on a microscopy slide and covered with a cover glass attached to a 125 μL Gene Frame (Thermo Fisher Scientific, Waltham, MA, USA). The process of making agarose pads has been previously described in more detail by De Jong et al. (55 (link)). Automated TLFM monitoring was performed on a widefield Ti-Eclipse inverted microscope (Nikon, Champigny-sur-Marne, France) equipped with a 60× Plan Apo λ oil objective, a TI-CT-E motorized condenser, and a Nikon DS-Qi2 camera. GFP was imaged using a quad-edge dichroic (395/470/550/640 nm) and a FITC single emission filter. A SpectraX LED illuminator (Lumencor, Beaverton, OR, USA) was used as light source, using the 470/24 excitation filter. Temperature was controlled at 37°C with an Okolab cage incubator (Okolab, Ottaviano, Italy). While phase contrast images were taken every 15 min, GFP was imaged every 30 min in order to avoid bleaching. Images were acquired using NIS-Elements software (Nikon), and the resulting pictures were further handled with the open source software ImageJ. During acquisition of fluorescent images, photobleaching was reduced by lowering the intensity of excitation light and prolonging time intervals between exposures.
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