{"Procedure":"
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  1. \n\t\t\tSet up timed mating with heterozygous animals. Dissect at a consistent time and collect >=2 homozygote embryos. Coordination with viability screen is at the centres discretion.
    2. \n\t\t
  2. \n\t\t\tScore embryos as live or dead if possible.
    3. \n\t\t
  3. \n\t\t\tAssess embryos according to Gross Morphology parameters.
    4. \n\t\t
  4. \n\t\t\tGenerate gross images of embryos (optional) with scored defects and control embryos.
    5. \n\t\t
  5. \n\t\t\tCollect tissue for genotyping
    6. \n\t\t
  6. \n\t\t\tProcess embryos for Histopathology, or other imaging (OPTIONAL - depending on center pipeline)
    7. \n\t\t
  7. \n\t\t\tScores will be shown per embryo and split by zygosity.
    8. \n\t
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\n\t\tIf capturing images please attempt to capture left, right, front, and back views of the embryo but if this is not possible left, right is sufficient. Feel free to take higher magnification views to show morphologies of interest.

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\n","Purpose":"
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\n\t\tTo assess visible morphological defects in E9.5 embryos from lethal strains

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\n","Experimental Design":"
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\n","Notes":"
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\n\t\tTam somite method for counting somites should be adopted:

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\n\t\tTam scoring system uses a forelimb range of 8 to 15 somite pairs resulting in E9.5 embryos ranging between 25 to 26 somite pairs.

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\n\t\tAll genotypes should be collected using validated assays.

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\n\t\tY chromosome assay required for X-linked lethal strains.

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\n\t\tEmbryos may be processed for Histopathology or 3D Imaging

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