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glacios_alignment

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glacios_alignment [2022/11/18 13:41] durandaglacios_alignment [2023/11/01 20:18] (current) – external edit 127.0.0.1
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 ==== Gain reference of the K2 camera ==== ==== Gain reference of the K2 camera ====
 This is done in Digital Micrograph (DM) on the K2 server. This is done in Digital Micrograph (DM) on the K2 server.
-  Go to an empty region on the sample +  Go to an empty region on the sample 
-  Go to high mag (e.g. 45000x) +  Go to high mag (e.g. 45000x) 
-  Insert 150µm C2 aperture +  Insert 150µm C2 aperture 
-  Go to spot size 2 +  Go to spot size 2 
-  Check on the FluScreen that beam is centered +  Check on the FluScreen that beam is centered 
-  Digital Micrograph > Camera > Prepare Gain Reference +  Digital Micrograph > Camera > Prepare Gain Reference 
-  Perform the gain in Linear mode first +  Perform the gain in Linear mode first 
-  Adjust Beam Intensity to match the number of count on the camera +  Adjust Beam Intensity to match the number of count on the camera 
-  Proceed to Counting mode +  Proceed to Counting mode 
-  Press 'Yes' to aquire the dark frame reference image (take twice 3 min 30) +  Press 'Yes' to aquire the dark frame reference image (take twice 3 min 30) 
-  At the end of the dark ref update, you will be prompt to lower the dose: insert 30µm C2 aperture, go to spot size 6, adjust C2 lens to 39.6%) +  At the end of the dark ref update, you will be prompt to lower the dose: insert 30µm C2 aperture, go to spot size 6, adjust C2 lens to 39.6%) 
-  Lift the Fluscreen and aquire Counting Gain Reference Image (you DON'T need to match the number given by DM)+  Lift the Fluscreen and aquire Counting Gain Reference Image (you DON'T need to match the number given by DM)
  
 ==== Direct alignment ==== ==== Direct alignment ====
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 ==== Objective Astigmatism / Coma-free alignment ==== ==== Objective Astigmatism / Coma-free alignment ====
-This is done in SerialEM. You need to have a sample inserted to do it. Re-use the calibration specimen or a carbon Quantifoil to do it (not a gold grid!)+This is done in SerialEM. You need to have a sample inserted to do it. Re-use the calibration specimen or a carbon Quantifoil (not a gold grid!). Use the Imaging state you will use for data collection (e.g. mag 45.000kx, spot 6, C2 aperture 30 µm, C2 lens 39.6%)
  
   - Insert and center Objective Aperture   - Insert and center Objective Aperture
glacios_alignment.1668778903.txt.gz · Last modified: (external edit)