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Troubles with Imaging - Troubleshooting » History » Revision 3

Revision 2 (Amber Herold, 04/27/2010 02:15 PM) → Revision 3/11 (Eric Hou, 06/24/2010 12:06 PM)

h1. Troubles with Imaging - Troubleshooting 

 




 * <link linkend="imageno">Empty Image</link> 


 * <link linkend="imageartifact">Image or FFT contains artifacts</link> 


 * <link linkend="cor_not_read">Reference image from other users not readable</link> 


 * <link linkend="beamshifttime">Beam shifts away from the imaging area over 
 time</link> 


 * <link linkend="beamshifttime">Beam shifts away from the imaging area after a large 
 defocus correction</link> 


 * <link linkend="beamshiftimage">Beam shifts away from the imaging area upon image shift 
 targeting</link> 


 * <link linkend="beamshiftstage">Beam shifts away from the imaging area upon stage shift 
 targeting in LM mode</link> 


 * <link linkend="apertureoff">Objective aperture is off-centered in LM when it is centered 
 in HM</link> 


 * <link linkend="specimenoverdose_gatan">The specimen appears over-dosed in the high 
 magnification images (while using a Gatan CCD)</link> 


 * <link linkend="specimenoverdose_gatan">Bright/Dark correction has no effect on the image 
 (while using a Gatan CCD)</link> 


 * <link linkend="badinput">Acquired image configuration is not what was 
 inputted</link> 


 * <link linkend="melt_beam_imprint">Exposure image has a circular focus 
 imprint</link> 


 * <link linkend="melt_beam_imprint">Image acquired at the wrong stage 
 position</link> 







 h2. Image is acquired but contains no real information 

 



 Commonly Why: 

 
 * Main screen at the scope is down 

 


 * Camera is not inserted (Gatan camera) 

 


 * Digital Micrograph program is not running (Gatan camera) 

 


 * Shutter switch box is set to CM, i.e., to collect film data only (Tietz 
 camera) 

 








 h2. Image is acquired but contains artifacts either in image or 
 in Fourier Transform 

 



 Commonly Why: 

 
 * Beam is partially covering the CCD. 

 


 * Scope viewing window is not covered and room light is on 

 


 * Dark/Bright images are not available or need to be reaquire. 

 


 * Bias level and quadrant correction may need to be reset (Digital Micrograph and 
 Gatan camera) 

 








 h2. Can not read reference images that were acquired by other 
 users 

 



 Commonly Why: You don't have permission to read their image files 

 




 Solution: 

 




 *    Have the person change the group or even world permission for reading the data 
 directory and the image files in it. 

 






 The person is not around when this happens: 

 


 Acquire your own reference images at the camera setting that needs the dark and bright 
 images. However, Leginon always look for the most recent calibration in the database by 
 anyone. Every user will have to do this everytime if the permission problem is not 
 solved. 

 







 h2. Beam shifts away from imaging area over time 

 



 Commonly Why: 

 
 * Residual lens hysteresis if you haven't allowed the scope to warm up for HM mode 
 after acquiring LM atlas. 

 


 * Focus correction has taken the absolute focus point far away from U-centric 
 focus. 

 h3. Solutions: 

 







 <title>Solutions:</title> 
 * Wait until the optics is stabilized 

 


 * Activate "Publish and wait for the reference target" in Exposure Node. This will 
 enable "Fix Beam" node to search for the beam in the desired range and shift the beam 
 to the best result. A reference target, normally an empty square, need to be selected 
 on the grid to use this function. See description in the node description chapter for 
 usage. 

 


 * Pause MSI and correct for residual beam shift 

 




 *    Pause before next hole or square by clicking Hole/Toolbar>Pause button 
 (Pause icon) or Square/Toolbar>Pause button (Pause icon), respectively. Which 
 one to pause depends on what is the next target. 

 


 *    Leginon/Presets Manager> When the acquisition sequence is stopped, send 
 the preset that has beam shift problem "To Scope" (ToScope icon). 

 


 *    Leginon/Navigation/Toolbar> Choose move type to be "Beam Shift" and make 
 sure "Use Camera Configuration" is unchecked in settings. 

 


 *    Leginon/Navigation> "Navigate"*(navigate icon) to center the beam. If 
 "Navigate" does not bring the beam in, manually shift the beam at the 
 microscope. Do not forget to lift the screen and cover the viewing area after 
 done. 

 


 *    Leginon/Presets Manager> save the new beam shift by retrieving it "From 
 Scope" (From Scope icon). 

 


 *    "Continue" data collection on next hole or square target by clicking 
 Hole/Toolbar> "Continue" button or Square/Toolbar> "Continue" button, 
 respectively. 

 *    "Navigate" 


 *"Navigate" means selecting the navigate tool on the top right of image 
 display and then single-left-clicking the location of the new center that is 
 translated by the given TEM Parameter. 

 






 * Reset the defocus=0 point back to U-centric focus. 

 


 * Leginon reset defocus after each defocus correction. Therefore, the point where 
 the user defines as defocus=0 may drift away from U-centric focus over time or after a 
 very large correction before it is reset to U-centric focus by z focus 
 correction. 

 




 *    Pause before next hole or square by clicking Hole/Toolbar>Pause button 
 (Pause icon) or Square/Toolbar>Pause button (Pause icon), respectively. Which 
 one to pause depends on what is the next target. 

 


 *    Leginon/Presets Manager> Send "hl" preset "To Scope" (ToScope 
 icon). 

 


 *    Leginon/Z Focus/Toolbar> Send stored U-centric focus to scope. 

 


 *    Leginon/Z Focus/Toolbar> Reset defocus to 0 

 


 *    Scope> U-center the stage if it is very out of focus. 

 


 *    Leginon/Presets Manager> Send the preset that showed bad beam shift "To 
 Scope" 

 


 *    Scope and Leginon/Presets Manager> Check the beam shift, make 
 correction, and then retrieve the correct value "From Scope" 

 


 *    Leginon/Drift Manager> Declare Drift (declare drift icon) to force 
 correction at next possible point in the process. 

 


 *    "Continue" data collection on next hole or square target by clicking 
 Hole/Toolbar> "Continue" button or Square/Toolbar> "Continue" button, 
 respectively. 

 













 h2. Beam shifts away from imaging area only when targeting 
 move type is image shift 

 



 Commonly Why: 

 
 * Image/Beam Shift calibration on the microscope is not optimal 

 


 * Defocus is very far from eucentric focus 

 h3. Solutions: 

 







 <title>Solutions:</title> 
 * Bad Image/Beam calibration 

 


 Follow instruction for performing the calibration for FEI Tecnai machines under 
 Alignments/Image HM-TEM(or LM)/Image-Beam calibration 

 


 *    Pause before next hole or square by clicking Hole/Toolbar>Pause button 
 (Pause icon) or Square/Toolbar>Pause button (Pause icon), respectively. Which 
 one to pause depends on what is the next target. If in queuing mode, pause at the 
 node that process the queue. 

 


 *    Scope> move to an unimportant area or pull the holder out enough to allow 
 the beam to go through. 

 


 *    Scope> reset defocus to eucentric height. 

 


 *    Scope> Follow instruction for performing the calibration for FEI Tecnai 
 machines under Alignments/Image HM-TEM(or LM)/Image-Beam calibration. 

 


 *    Leginon/Presets Manager> Cycle the presets a few times. The calibration 
 takes the scope to conditions outside the presets, and can cause strong hysteresis 
 if this step is not done. 

 


 *    Leginon> Follow the procedures for confirming and saving good image shift 
 at various presets. 

 


 *    "Continue" data collection on next hole or square target by clicking 
 Hole/Toolbar> "Continue" button or squares/Target Toolbar> "Continue" 
 button, respectively. 

 *    "Navigate" 


 *"Navigate" means selecting the navigate tool on the top right of image 
 display and then single-left-clicking the location of the new center that is 
 translated by the given TEM Parameter. 

 




 * Defocus far from eucentric focus 

 


 Image/Beam shift coupling worsens when the defocus is away from where it was 
 calibrated. If, after the above calibration, the problem remains during MSI 
 acquisition, additional focusing sequence should be added at lower magnification that 
 move the stage to close to eucentric height so that the image shift target is selected 
 on an image of a close-to-eucentric location. 

 


 *    Leginon/Z Focus/Focus Sequence> activate both Stage_Wobble and 
 Z_to_Encentric steps. 

 


 *    Leginon/Hole (or Subsquare) Targeting> selection a focus target if not 
 already done so when a newly acquired sq image comes in. 

 




 If the accuracy of moving stage to eucentric height by the focus sequences in "Z 
 Focus" is still not sufficient. Add another focus step performing the same task as 
 Z_to_Encentric step. Repeating beam-tilt based autofocusing often improve the accuracy 
 unless the calibration is off. 

 






 Still not working: You have chosen a target that requires too much image shift for an 
 independent image shift from beam shift. This is necessary when the lower mag targetting is 
 not good either because the preset image shifts are not aligned or the stage position 
 movement is not properly modeled. 

 


 Solution: For image shift problem see solution for "Target is consistently off in the 
 same direction and distance". For stage model problem, see "Modeled stage calibration" in 
 setup notes. 

 





 h2. Beam shifts away from imaging area when targeting move 
 type is stage movement 

 



 Commonly Why: 

 
 * U-center defocus not set to 0 in LM mode. 

 


 * LM alignment such as rotation center is way off. 

 





 Solution: Check and correct microscopic alignment error. Preset parameters checking and 
 reset may be necessary after the correction. 

 


 Comments: If the problem persist, the original stage matrix calibration may have been 
 performed with a bad alignment. The calibration should be redone with a well-aligned scope 
 in LM mode. 

 





 h2. Objective aperture appears off in "sq" preset when it is 
 centered in HM mode 

 



 Commonly Why: 

 
 * U-center defocus not set to 0 in LM mode. 

 


 * LM alignment such as image shift is way off. 

 





 Solution: Check and correct microscopic alignment error. Preset parameters checking and 
 reset may be necessary after the correction. 

 





 h2. The specimen appears over-dosed in the high 
 magnification images or the dark correction image has a high value (while using a Gatan 
 CCD) 

 



 This issue may occur when the shutter is incorrectly configured through Digital 
 Micrograph (the imaging software for the Gatan CCD that resides on the TEM computer) or 
 simply a bad dose calibration or too long an exposure time. To issue these 
 corrections: 

 




 *    Set the "shutter" to "Auto" on the external control box attached to the 
 TEM. 

 


 *    Open Digital Micrograph on the Microscope computer and go to the Camera Set-up 
 page. 

 




 *    Go to Configuration 

 


 *    Set the Primary Shutter to Pre-specimen 

 


 *    Set the Alternate Shutter to Post-specimen 

 


 *    Set the Default Primary Shutter to the Normally Closed position. 

 













 h2. The exposure image has a circular imprint of the beam 
 at the size of the preset used for melting the ice 

 



 This issue may occur when the main screen is left up during very long (such as over 30 
 sec) ice melting and at high HT. Leginon has a mechanism that put the screen down during ice 
 melting. It is caused by over-saturating the Phosphur layer on the CCD. If you see this 
 effect, the screen may have failed to lower. Please test it by observing the screen movement 
 with simulating target in any focuser node that has ice melt time set not to zero. Report 
 the problem back to the leginon team if you are sure it is not your scope's problem. 

 



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