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3DNGPol

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@@ -26,7 +26,7 @@ The dimensions of each voxel are:
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  We provide both the [Real Nucleus Golgi Dataset](https://huggingface.co/datasets/Hemaxi/3DNGPol/tree/main/RealNucleusGolgiDataset) and the [Synthetic Nucleus Golgi Dataset](https://huggingface.co/datasets/Hemaxi/3DNGPol/tree/main/SyntheticNucleusGolgiDataset).
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- ## Experiments
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  All the retinas are from the GNrep mice (Barbacena et al. 2019, genesis). Tamoxifen was injected intraperitoneally (20μg/g) at two different time points at least 3 days before eyes were collected. Stainings were performed according to previously published protocols (Franco etl al., 2013, Development). Green fluorescence protein (GFP) and mCherry were used to label nuclei and Golgi, respectively. For analysis, a tile-scan spanning the retina was acquired on a Zeiss Cell Observer spinning disk confocal microscope, equipped with the Zen software and with a Plan-Apochromat 40×/1.4 Oil DIC M27 objective.
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  Knock-in mice were maintained at the Instituto de Medicina Molecular under standard husbandry conditions and national regulations. This study was conducted in accordance with European Union (EU) regulations and ethical approval was obtained from the Animal Ethics Committee of Instituto de Medicina Molecular (AWB\_2015\_10\_CF\_Polaridade).
 
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  We provide both the [Real Nucleus Golgi Dataset](https://huggingface.co/datasets/Hemaxi/3DNGPol/tree/main/RealNucleusGolgiDataset) and the [Synthetic Nucleus Golgi Dataset](https://huggingface.co/datasets/Hemaxi/3DNGPol/tree/main/SyntheticNucleusGolgiDataset).
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+ ## Image Acquistion Details
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  All the retinas are from the GNrep mice (Barbacena et al. 2019, genesis). Tamoxifen was injected intraperitoneally (20μg/g) at two different time points at least 3 days before eyes were collected. Stainings were performed according to previously published protocols (Franco etl al., 2013, Development). Green fluorescence protein (GFP) and mCherry were used to label nuclei and Golgi, respectively. For analysis, a tile-scan spanning the retina was acquired on a Zeiss Cell Observer spinning disk confocal microscope, equipped with the Zen software and with a Plan-Apochromat 40×/1.4 Oil DIC M27 objective.
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  Knock-in mice were maintained at the Instituto de Medicina Molecular under standard husbandry conditions and national regulations. This study was conducted in accordance with European Union (EU) regulations and ethical approval was obtained from the Animal Ethics Committee of Instituto de Medicina Molecular (AWB\_2015\_10\_CF\_Polaridade).