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Mz 16 1fa

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The Leica MZ 16 1FA is a stereomicroscope designed for laboratory use. It features a zoom range of 6.3x to 100x and a working distance of 63 mm to 40 mm. The microscope is equipped with a 1.0x FWD objective lens.

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Lab products found in correlation

C12fdg, by Thermo Fisher Scientific (2 mentions) Sa β gal staining kit, by Leica camera (2 mentions) Gallios flow cytometer, by Beckman Coulter (2 mentions) Dfc 480 color, by Leica camera (1 mentions) Cls 150x, by Leica camera (1 mentions)

3 protocols using mz 16 1fa

1

Senescence Assay for Primary Mouse Embryonic Fibroblasts

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Populations of primary MEFs (2 x 105 (link) per 10 cm dish) were counted by trypan blue exclusion every third day. SA-β-Gal staining was performed according to the manufactures instructions (Cell Signaling, SA-β-Gal staining kit (#9860)) and images were acquired with a stereomicroscope (Leica MZ 16 1FA). DAPI staining was used to identify nuclei.
For FACS-based determination of senescence, lysosomal alkalinization was induced by treating cells with 100 nM bafilomycin A1 for 1 h in fresh cell culture medium (2 ml per 35 mm dish) at 37 °C. 33 μl of 2 mM C12FDG (Thermofisher, ref. D2893) working solution was added to the cell culture medium to obtain a final concentration of 33 μM. After 1h of incubation, cells were washed, trypsinised and collected on a Gallios flow cytometer (Beckman Coulter) using Kaluza Acquisition software. Data were analysed with FlowJo software.
Glück S., Guey B., Gulen M.F., Wolter K., Kang T.W., Schmacke N.A., Bridgeman A., Rehwinkel J., Zender L, & Ablasser A. (2017). Innate immune sensing of cytosolic chromatin fragments through cGAS promotes senescence. Nature cell biology, 19(9), 1061-1070.
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2

Senescence Assay for Primary Mouse Embryonic Fibroblasts

Cited 1 time
Check if the same lab product or an alternative is used in the 5 most similar protocols
Populations of primary MEFs (2 x 105 (link) per 10 cm dish) were counted by trypan blue exclusion every third day. SA-β-Gal staining was performed according to the manufactures instructions (Cell Signaling, SA-β-Gal staining kit (#9860)) and images were acquired with a stereomicroscope (Leica MZ 16 1FA). DAPI staining was used to identify nuclei.
For FACS-based determination of senescence, lysosomal alkalinization was induced by treating cells with 100 nM bafilomycin A1 for 1 h in fresh cell culture medium (2 ml per 35 mm dish) at 37 °C. 33 μl of 2 mM C12FDG (Thermofisher, ref. D2893) working solution was added to the cell culture medium to obtain a final concentration of 33 μM. After 1h of incubation, cells were washed, trypsinised and collected on a Gallios flow cytometer (Beckman Coulter) using Kaluza Acquisition software. Data were analysed with FlowJo software.
Glück S., Guey B., Gulen M.F., Wolter K., Kang T.W., Schmacke N.A., Bridgeman A., Rehwinkel J., Zender L, & Ablasser A. (2017). Innate immune sensing of cytosolic chromatin fragments through cGAS promotes senescence. Nature cell biology, 19(9), 1061-1070.
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3

Gastruloid Transplantation: Hematopoiesis Analysis

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For transplantation, Gata6-Venus (CD45.2) Gastruloids at 168h were dissociated as described for FACs analysis. 10 weeks old, female, Bl6, CD45.1 recipient mice were lethally irradiated 24 hours before transplantation with a split dose of 2x 425cGy. 5x10 6 dissociated gastruloid cells were injected in the mice tail vein together with 2x10 4 competitor bone marrow cells isolated from Bl6, CD45.1/2 mice, in a total volume of 200 µl. Control mice received just 2x10 4 competitor bone marrow cells isolated from Bl6, CD45.1/2 mice, in a total volume of 200 µl.
Mice were euthanized 11 days after transplantation, and spleens were collected for analysis.
Whole spleen images were acquired with a Leica MZ16 1FA stereomicroscope equipped with Leica CLS 150X illumination and DFC480 color camera. All mice were purchased from Charles River Laboratories International and maintained at EPFL conventional animal facility, in microisolator cages, provided with food and water ad libitum. experiments were performed in compliance with the Swiss law after approval from the local and federal authorities (license VD2242.2).
Rossi G., Giger S., Hübscher T., & Lütolf M.P. (2021). Gastruloids asin vitromodels of embryonic blood development with spatial and temporal resolution.
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