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## page was renamed from e2tomo
= EMAN2 Tomography mini-Workflow Tutorial =

This version of the EMAN2 Tomography Pipeline tutorial is designed to run on well equipped laptops or standard workstations, unlike the [[EMAN2/e2tomo|full tutorial]] which requires a well-equipped tomography workstation. It should be possible to complete this tutorial in a reasonable time on a computer with 16 GB of ram and 4 cores, but resolution will be limited to ~15 A, not the subnanometer resolution provided by the main tutorial.

 * This tutorial is best suited for EMAN2 built after 09/27/2018. Not everything described in the tutorial was functioning yet in the 2.22 release.
 * This version of the tutorial is based on a subset of reduced sampling data from the same EMPIAR data set as the main tutorial. This should be downloaded from the EMAN2 website. The pixel size for this data is 3.93 A/pix.
= EMAN2 Tomography and Subtomogram/Subtilt Averaging Workflow Tutorial =
'''''Important note: Throughout the tutorial you will see a split between (small) and (large) instructions. The (small) tutorial is designed for laptops or basic desktops and can achieve ~12 Å resolution in a time compatible with live tutorial sessions. The (large) tutorial really requires a proper tomography workstation, but can achieve subnanometer resolution. Do not intermix (small) and (large) options below!'''''

 * This tutorial requires EMAN 2.91 at a minimum. The newer pipeline, which will become the primary pipeline in EMAN3, is also discussed. To use those instructions you should have a current EMAN2.99 snapshot version.
 * Some additional documentation for the newer pipeline for integrated subtomogram and subtilt refinement can be found in [[https://blake.bcm.edu/emanwiki/EMAN2/e2tomo_new|TomoNew]]
 * Documentation of some other recently developed tools can be found in [[https://blake.bcm.edu/emanwiki/EMAN2/e2tomo_more|TomoMore]].
 * To cite:
  * Chen, M., Bell, J.M., Shi, X. et al. A complete data processing workflow for cryo-ET and subtomogram averaging. Nat Methods 16, 1161–1168 (2019)
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 * This reduced version of the tutorial can be completed on a well equipped laptop or standard desktop workstation.
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  * 16 GB RAM
  * 4 cores @ >2 ghz
  * 40 gb free disk space
  * 16 GB RAM (small), 64 GB RAM (large)
  * 4 cores @ >2 ghz (small), 16 cores (large)
  * ~40 gb free disk space (small), ~100 gb free disk space, due to larger raw data (large)
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''Note: Any place in EMAN2 where you are requested to enter the number of threads to use, you should specify the number of '''cores''' your machine has. Computers are often advertised as 4 core/8 thread or 8 core/16 thread. Trying to run image processing using this advertised number of threads will usually make processing run slower, not faster. You may optionally increase the number of cores by ~25%, ie - on a 4 core machine, specifying 5 may give a 5-10% speedup over 4''
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 * Download the data from the [[http://eman2.org/Tutorials|EMAN2 Tutorials page]] The tutorial data comes from EMPIAR 10064, but only uses a subset of the data from the ''mixed CTEM'' tilt series.
 * (Large) The 4 fully sampled tilt series [[http://blake.bcm.edu/dl/tutorial_tomo_large.zip]]
 * (Small) 3/4 tilt series, downsampled by 2x for speed [[http://blake.bcm.edu/dl/tutorial_tomo_small.zip]]
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 * run '''[[http://blake.bcm.edu/emanwiki/EMAN2/Programs/e2projectmanager|e2projectmanager.py]]'''   * run '''[[http://blake.bcm.edu/emanwiki/EMAN2/Programs/e2projectmanager|e2projectmanager.py]]''':

{{{
e2projectmanager.py&
}}}
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 * You may use "Edit Project" from the Project menu to set default values for the project. While not required, it reduces later errors.  * You may use "Edit Project" from the Project menu to set default values for the project.
  * If you downloaded our prepared data set, it will already contain an ''info'' folder containing the project settings, so you should not need to change anything.
  * For this project use 300 kDa, 2.7 mm Cs, 300 keV and 3.93 (Small) or 1.97 (Large) A/pix.
  * The mass need not be precise, it is only used to keep isosurface values roughly self-consistent.
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{{attachment:e2pm.png|Project Manager|width=600}} {{attachment:e2pm.png|Project Manager|width="600"}}
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  * Select the 3 tilt series provided, and make sure '''importation''' says '''copy'''
  * In this step you should enter the correct A/pix for your data in the '''apix''' box. For this downsampled data, this is 3.93. For your own data, you need to know this number. In later steps you should be able to use -1 (default) for apix.
  * If your tilt series isn't a single stack file, but is many individual images instead, you will need to use '''Generate tiltseries''' to build an image stack. This is not necessary for the tutorial data.
  * ''Files'' -> select the 3 (Small) or 4 (Large) provided .hdf files
  * ''rawtlt, mdoc'' -> leave these blank
  * ''invert'' should not be selected
  * ''apix'' = 3.93 (Small) or 1.97 (Large), in later steps you can use -1, which tells it to use the known value
  * ''import_tiltseries'' = selected
  * ''importation'' = copy
  * ''compressbits'' = 5 (8 is fine as well, but will make file sizes slightly larger)
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 * It is critical that the filenames for your data not contain any spaces (replace with underscore) or periods (other than the final period used for the file extension). "__" (double underscore) is also reserved for describing modified versions of the same file, and should not be used in your original filenames.

== Tiltseries Alignment and Tomogram Reconstruction (10 min) ==
When working with your own data:

* It is critical that the filenames for your data not contain any spaces (replace with underscore) or periods (other than the final period used for the file extension).
 * {{{
"__"}}} (double underscore) is also reserved for describing modified versions of the same file, and should not be used in your image filenames.
 * If your tilt series isn't a single stack file, but is many individual images instead, you will need to use '''Generate tiltseries''' to build an image stack


== Tiltseries Alignment and Tomogram Reconstruction (~10 min Small) ==
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 * check ''alltiltseries''  * ''alltiltseries'' = selected
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 * check ''correctrot''  * ''correctrot'' = selected
 * ''tltax'' = -4.0
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 * ''clipz'' = 64
 * If you wish to look at the intermediate aligned tilt-series and other files, uncheck ''notmp'', but note that this will significantly increase disk requirements
  * This is not required for the remaining steps in the tutorial, but can be used to help understand how the tomogram alignment works. This requires significant additional disk space. You may consider doing this for only one tomogram.
  * In each ''tomorecon_XX'' folder
   * ''landmark_0X.txt'' has the location of the landmarks (which may be fiducials if present) in each iteration
   * ''samples_0X.hdf'' shows the top and side view of those landmarks
   * ''ptclali_0X.hdf'' has the trace of each landmark throughout the tilt series (they should stay at the center of image all the time if the alignment is good)
   * ''tomo_0X.hdf'' is the reconstruction after each iteration
 * ''clipz'' = 96
 * ''threads'' = number of physical cores on your machine, optionally *1.25.
 * ''notmp'' = checked by default. If you wish to look at the intermediate aligned tilt-series and other files, uncheck this, but note that this will significantly increase disk requirements
  * These files are not required for the remaining steps in the tutorial, but can be used to help understand how the tomogram alignment works. You may consider doing this for only one tomogram.
 * patchtrack = 2 (not really necessary for the tutorial, but shouldn't hurt. This is 3-D patchtracking, not the typical 2-D patchtracking)
 * extrapad = selected (this will make the tomogram reconstructions take a little longer, but look a bit nicer visually. No impact on the final subtomogram averages)
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{{attachment:tomorecon.png| Tomogram reconstruction |width=600}} If you opted to run without ''notmp'' on one or more tilt series:
 * You will see a ''tomorecon_XX'' folder for each tilt series, containing:
  * ''landmark_0X.txt'' has the location of the landmarks (which may be fiducials if present) in each iteration
  * ''samples_0X.hdf'' shows the top and side view of those landmarks
  * ''ptclali_0X.hdf'' has the trace of each landmark throughout the tilt series (they should stay at the center of image all the time if the alignment is good)
  * ''tomo_0X.hdf'' is the reconstruction after each iteration
 * Again, note that these files are not required by any downstream processing. If you have difficulty getting a particular tilt series to reconstruct, and the ''patchtrack=2'' option doesn't help, this may help debug the problem. However, if you do encounter problems, we would like to invite you to ask about it either publicly on the mailing list or privately to the developers.

{{attachment:tomorecon.png|Tomogram reconstruction|width="600"}}
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 * We strongly recommend reconstructing at most 5-10 tilt series to start. Then completing the handedness check in the next step before returning to this step and reconstructing the full set of tilt series! This will allow you to specify the correct ''tltax'' value.
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 * While the program can automatically compute the orientation of the tilt axis, it is better to fill in the correct value in ''tltax'' since there is a handedness ambiguity in the tomogram if determined automatically.
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 * The graphical interface only permits 1k or 2k reconstruction sizes. In our experience this is normally sufficient for segmentation or particle picking.  * The graphical interface only permits 1k or 2k reconstruction sizes. In our experience this is normally sufficient for segmentation or particle picking.
 * When the sample is thick, some grid-like tiling pattern can be seen in the reconstruction. Checking '''extrapad''' can largely reduce the artifacts. In versions after 2/3/2020, there is also a '''moretile''' option that further eliminates them. Note these artifacts will NOT impact the subtomogram averaging results because the particles are extracted in a separate process. Checking these options can make the reconstruction process more memory consuming, and up to 5 times slower.
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== CTF Estimation (<10 min) ==

For the tutorial tilt-series:
 * '''Subtomogram Averaging -> CTF Correction'''
 * check ''alltiltseries''
 * Double check the ''voltage'' and ''cs''
 * There is a new ''patchtrack'' option which may help with refinements that otherwise don't seem to be aligning well. Note that this is not conventional 2-D patchtracking, but a novel 3-D patchtracking routine. This acts as a preprocessing step if specified (2 is recommended).

== Handedness Check ==
EMAN2 will automatically locate the tilt axis in a tilt series if it is not provided, but there is a 180° ambiguity in this determination. An incorrect choice will lead to structures with the incorrect handedness, and may produce suboptimal CTF correction. In some data sets (not the tutorial) this may lead to particles with mixed handedness. Since we specified ''tltax'' above, this step isn't necessary for the tutorial, but you can run it to see what the results look like.

EMAN2 includes a novel procedure for resolving this ambiguity from a tilt series based on defocus estimates across the tilted images. The tutorial data set comes out correctly without running this check, but when working with your own data, this step is highly recommended. Once you know the correct tilt axis direction to use for a given microscope/camera, you shouldn't need to run this test on every data set, but it may not be a bad idea even then, as there are various possible configuration/software errors on the instrument which could potentially cause inconsistent results, particularly with a change of magnification.

For the tutorial tilt-series:

 * '''Subtomogram Averaging -> CTF Estimation'''
 * ''tiltseries'' = select any one tilt series
 * ''alltiltseries'' = not selected
 * ''voltage'' and ''cs'' (double check that values are correct)
 * ''dfrange'' = 1.0,4.0,0.02
 * ''checkhand'' = selected
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You will need to look at the console where you launched e2projectmanager to see the results of the test. It should look something like:

{{{
Average score: Current hand - 4.133, flipped hand - 3.290
Defocus std: Current hand - 0.110, flipped hand - 0.165
Current hand is better than the flipped hand in 86.4% tilt images
The handedness (--tltax=-4.1) seems to be correct. Rerun CTF estimation without the checkhand option to finish the process.
}}}
If you run this check on multiple images and it seems that they consistently indicate a flipped tilt axis/handedness, then you need to return to the previous step (Tomogram Reconstruction) and redo the reconstruction for all tomograms, with the correct tilt axis entered in the corresponding box. The same tilt axis should be used for all tilt series collected under the same conditions on the same instrument. The automatic value may vary a little among micrographs, just compute the approximate average or median value.

''Note: This method removes __almost__ all of the ambiguity about particle handedness. The one potential issue is that the MRC file format uses a non-conventional origin for images. If the data collection software doesn't take this into account, the images may be flipped when written to disk. The easiest way to check the software would be to collect 2 images of the same target and save them directly into different file formats, then checking (in EMAN2) whether the two images appear to have the same handedness''. If not, it is likely that the MRC files are incorrect.

== CTF Estimation (<5 min) ==
'''Do NOT forget this step!'''

This step will determine the defocus as a function of location for each tilt in each tilt series. This information is stored in the headers of particles as they are extracted from the tilt series, and used for CTF correction during subtomogram averaging. If you forget to do this, you will need to re-run the particle extraction step, which is quite time consuming.

For the tutorial tilt-series:

 * '''Subtomogram Averaging -> CTF Estimation'''
 * ''alltiltseries'' = selected, note that doing this will override anything present in the ''tiltseries'' field
 * ''dfrange'' = 1.0,4.0,0.02
 * ''' ''checkhand'' = not selected '''
 * Launch
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 * The first two options, ''dfrange'' and ''psrange'' indicate the defocus and phase shift range to search. They take the format of “start, end, step”, so “2, 5, .1” will search defocus from 2 to 5 um with a step size of 0.1. Units for phase shift is degrees.
* The first two options, ''dfrange'' and ''psrange'' indicate the defocus and phase shift range to search. It is critical that the actual defocus be within the search range (obviously). They take the format of “start, end, step”, so “2, 5, .1” will search defocus from 2 to 5 um with a step size of 0.1. Units for phase shift is degrees.
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Note that this program is only estimating CTF parameters, taking tilt into account. It is not performing any phase-flipping corrections on whole tomograms. CTF correction is performed later as a per-particle process. This process requires metadata determined during tilt-series alignment, so it cannot be used with tomograms reconstructed using other software packages.

== Tomogram reconstruction evaluation (optional) ==

{{attachment:tomo_evaluation.png| Tomogram evaluation |width=600}}
''Note: this program is only estimating CTF parameters, taking tilt into account. It is not performing any phase-flipping corrections on whole tomograms. CTF correction is performed later as a per-particle process. This process requires metadata determined during tilt-series alignment, so it cannot be used with tomograms reconstructed using other software packages.''

''Note: In >=2022 snapshots of EMAN2 it is possible after CTF correction to return to the 3-D reconstruction step and produce CTF corrected whole tomograms, but this does nothing useful when following the EMAN2 pipeline. If you wish to compare EMAN2 tomograms with other software doing CTF correction, this could potentially be useful''


== Tomogram reconstruction evaluation ==
{{attachment:tomo_evaluation.png|Tomogram evaluation|width="600"}}
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 * On the left is a list of tomograms in the project. The ''correctrot'' option often does not work well on tutorial tomo3. If you go through the tomograms you should see ribosomes spanning the plane of the image for all of the tomograms. If tomo3 shows only a narrow band containing ribosomes, return to the tomogram reconstruction step above, and re-run the process for only that tomogram (uncheck ''alltiltseries'', and select tiltseries/*tomo3.hdf. Also uncheck ''correctrot'').

 * On the left is a list of tomograms in the project.
  * Selecting a tomogram will show a thumbnail in the image pane on the right.
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  * ''loss'' is the average landmark uncertainty in nm. You should not try to compare this number to, for example, the fiducial alignment error in IMOD, as it is computed in a very different way. This number can be useful to detect specific tilt series within a project which have problems, but the absolute number is not a useful value to report/analyze. Even if this number is >5 nm, it is still quite possible to achieve a subnanometer resolution average.   * ''loss'' is the average landmark uncertainty in nm. You should not try to compare this number to, for example, the fiducial alignment error in IMOD, as it is computed in a completely different way. This number can be useful to identify specific tilt series within a project which aren't aligning as well as others, but the absolute number is not a useful value to report/analyze. Even if this number were >5 nm, it is still quite possible to achieve a subnanometer resolution subtomogram average.
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  * the ''show2d'' button displays the selected tomogram slice-wise.   * the ''show2d'' button displays the selected tomogram in a slice-wise view.
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   * Please note that most tomograms include some out-of-plane tilt (the actual rotation isn't a simple tilt along a single axis), which is taken into account during alignment. This may make it visually appear that the tilt series alignment is not as robust as it actually is. 
  * ''Boxer'' calls the 3D boxer
   * Please note that most tomograms include some out-of-plane tilt (the actual rotation isn't a simple tilt along a single axis), which is taken into account during alignment. This may make it visually appear that the tilt series alignment is not as robust as it actually is.
  * ''Boxer'' opens the 3D particle picker
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  * ''Tiltparams'' is a bit more complicated. It plots a point list with 6 columns and a number of rows corresponding to the images in the selected tilt series. These are the alignment parameters for the tilt series.    * ''Tiltparams'' is a bit more complicated. It plots a point list with 6 columns and a number of rows corresponding to the images in the selected tilt series. These are the alignment parameters for the tilt series.
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== Tomogram annotation (optional alternative to process below) ==

{{attachment:annotation.png| 2D particle picking |width=600}}

 * Since the tutorial data set is purified ribosomes, this step can be skipped for the tutorial data, and you can move on to template-based particle picking. For cells or other types of complex specimens, tomogram annotation can be used to produce locations of different types of objects.

This section is brief and is only an update to the more detailed tutorial: [[http://eman2.org/Programs/tomoseg| TomoSeg]]. Some directory structure and user interfaces have changed in the latest version to match new tomogram workflow as described here:
== Particle Picking Choices ==
There are 4 different tools you can use for particle picking in EMAN2 as of Feb 2022:

 1. A new deep-learning based 3-D picker. Not available in 2.91, must use a recent (2022+) snapshot.
 1. Abusing the deep-learning based segmentation tool for particle picking purposes
 1. Manual particle picking
 1. Template based picking (usually seeded with some manual picking results)

For live versions of this tutorial, we use the older manual+template based approach as it requires no specific hardware, and is a good learning experience, but the deep learning 3-D picker is a good choice for typical situations. For cellular tomograms, the annotation tool approach may still be a good choice.

=== New Deep-Learning 3-D Picker (recommended approach) ===
This is the easiest approach by far, and is basically a single step process, but is only available in recent (2022+) snapshots of EMAN2.
 * You should easily be able to select ~500 particles per tomogram, potentially more, but 500 is more than sufficient for the tutorial
 * For instructions, see: [[EMAN2/e2tomo_more#Automated_particle_selection|New automatic particle picking]]
 * When complete, skip ahead to the next major section '''Particle Extraction'''

=== Tomogram annotation (GPU recommended) ===
{{attachment:annotation.png|2D particle picking|width="600"}}

 * Since the tutorial data set is purified ribosomes, this step can be skipped for the tutorial data, and you can move on to template-based particle picking. For cells or other types of complex specimens, tomogram annotation can be used to more easily distinguish locations of different types of objects.

For a detailed description of how to use the annotation tool, see: [[http://eman2.org/Programs/tomoseg|TomoSeg]]

Here is a brief summary of the annotation-based approach:
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  * This step is not always necessary for tomograms reconstructed in EMAN2, but may slightly improve results.    * This step is not always necessary for tomograms reconstructed in EMAN2, but may slightly improve results.
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  * This is a newer interface than previously used for this step. Select a few "Good" (regions containing the feature of interest) and "Bad" (regions not containing the feature of interest) boxes.    * This is a newer interface than previously used for this step. Select a few "Good" (regions containing the feature of interest) and "Bad" (regions not containing the feature of interest) boxes.
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  * Input both the tomogram and its corresponding segmentation, and the particles coordinates will be written into the metadata file. 
  * Slightly tweaking the threshold parameters may yield better results. 
  * Input both the tomogram and its corresponding segmentation, and the particles coordinates will be written into the metadata file.
  * Slightly tweaking the threshold parameters may yield better results.
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== Particle picking (10-15 min) ==

{{attachment:ptclpicking.png| 3D particle picking |width=600}}

 * '''Subtomogram averaging -> Manual boxing''' Time above is to manually select 30-50 reference particles.
  * ''rename'' the set of boxes to "initribo". This will be used as the label in later stages.
  * Go through slices along z-axis using ''‘~’'' and ''‘1’'' on the keyboard
  * It will be much easier to locate particles if you adjust the ''Filt'' slider to ~70
  * left click and drag to place and reposition boxes in any of the 3 views
  * Hold down Shift when clicking to delete existing boxes.
  * Boxes are shown as circles, which vary in size depending on the Z distance from the center of the particle.
  * The interface supports different box types within a single tomogram. Each type has a label. Make sure the label is consistent if selecting the same feature in different tomograms.
  * The box size can be set in the main window at the left bottom corner, for this tutorial, use 32 for ribosomes (the unbinned box size is 128).

 * If you skipped the tomogram annotation step, we will pick a few particles here to generate an initial model, and use the initial model as a reference for template matching.
  * Select 30-50 particles from a tomogram, then close the boxer window.

 * If you have the particle coordinates from tomogram annotation above, you may still wish to do this step to delete any obviously bad particles.
  * While you can save 3D particles from the GUI, there is no need to do that here. When you are satisfied with the result, simply close the window.
  * You should have ~3000 particles from the 4 tomograms in the dataset.

== Particle extraction (2 min) ==

In this pipeline, the full 1k or 2k tomograms are used only as a reference to identify the location of the objects to be averaged. Now that we have particle locations, the software returns to the original tilt-series, extracts a per-particle tilt-series, and reconstructs each particle in 3-D independently.

For the tutorial tilt-series:
=== Manual particle picking (10-15 min) ===
{{attachment:ptclpicking.png|3D particle picking|width="600"}}

 * Time above is to manually select 30-50 reference particles.
 * You can launch the particle picker in two equivalent ways:
  * '''Subtomogram averaging -> Manual boxing''', select tomogram, Launch
  * '''Analysis and visualization -> Evaluate tomograms''' as above, press the "Boxer" button

 * two windows will appear ''Main Window'' and ''Options''. If you don't see ''Options'' it is probably hiding behind the main window.
 * in the ''Options'' window, ''rename'' the set of boxes to "initribo". This will be used as the label in later stages
 * The box size can be set in the main window at the left bottom corner, for this tutorial, use 32 for ribosomes (the unbinned box size is 128).
  * This is NOT the same as the size listed near the word ''erase'' in another window, which is the size of the eraser.
 * left click and drag to place and reposition boxes in any of the 3 views
 * Hold down Shift when clicking to delete existing boxes.
 * Boxes are shown as circles, which vary in size depending on the Z distance from the center of the particle.
 * If you accidentally include one or more particles with nearby gold fiducials or other high contrast artifacts, it may cause some issues with your generated model (do not do that).
 * Go through slices along z-axis using ''‘~’'' and ''‘1’'' on the keyboard, or using the slider in the lower right of the window
 * It may be easier to locate particles if you adjust the ''Filt'' slider to ~70, but it will slow things down
 * The interface supports different box types within a single tomogram. Each type has a label. Make sure the label is consistent if selecting the same feature in different tomograms.

 * If you skipped the tomogram annotation step, we will pick a few particles here to generate an initial model, and use the initial model as a reference for template matching.
 * Select 30-50 particles from one tomogram, then close the boxer window.
 * Do '''not''' use the ''Save'' button in the Options window or any of the menu items related to saving data. Those are available for special purposes. When you change the boxes, your changes are saved immediately and automatically. When you are done, simply close the main window.

 * If you did the previous optional annotation step above, you will be able to see the selected particles here, and if you like, manually update them.

== Particle extraction (~2 min (a few manual) - hours (a couple of thousand)) ==
Note that this step will be vastly different resource-wise if you are only extracting a few manually selected particles for purposes of later template matching or if you already selected hundreds of particles from each tomogram.

The reduced 1k x 1k (or 2k) tomograms are used only as a reference to identify the location of the objects to be averaged. Now that we have particle locations, the software returns to the original tilt-series, extracts a per-particle tilt-series, and reconstructs each particle in 3-D independently at full resolution. Since this is performing a full resolution reconstruction of each particle it is somewhat resource intensive.

For the tutorial tilt-series:
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  * set ''boxsz_unbin'' to 128. 
   * If you had the correct size in the previous step this may not be necessary, but it doesn't hurt.
  * enter the label you used when picking particles ("initribo" if you followed the instructions above)
  * Launch

 * '''Subtomogram Averaging -> Build Sets''' 
  * set ''boxsz_unbin'' to 128 (Small) or 256 (Large).
   * If you had the correct size in the previous step this should be the same as leaving the default -1
  * enter the label you used when picking particles ("initribo" if you manually boxed, "tomobox" if you used the deep learning picker)
  * ''threads'' =
value for your machine
  * Launch

 * '''Subtomogram Averaging -> Build Sets'''
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{{attachment:initial_model.png| Initial model generation | width=600}}

While intuitively it seems like (since the particles are already in 3-D) the concept of an "initial model" should not be necessary. Unfortunately, due to the missing wedge, and the low resolution of one individual particle (particularly from cells), it is actually critical to make a good starting average. Historically it has been challenging to get a good starting model, depending on the shape of the molecule. This new procedure based on stochastic gradient descent has proven to be quite robust, but it is difficult for the computer to tell when it has converged sufficiently. For this reason, the default behavior is to run much longer than is normally required, and have a human decide when it's "good enough" and terminate the process. If you use a small ''shrink'' value and let it run to completion, it can take some time to run. This is harmless, but unnecessary.

For the tutorial tilt-series:
While intuitively it seems like (since the particles are already in 3-D) the concept of an "initial model" should not be necessary. Unfortunately, due to the missing wedge, and the low resolution of one individual particle (particularly from cells), it is actually critical to make a good starting average. Historically it has been challenging to get a good starting model, depending on the shape of the molecule. This new procedure based on stochastic gradient descent has proven to be quite robust, but it is difficult for the computer to tell when it has converged sufficiently. For this reason, the default behavior is to run much longer than is normally required, and have a human decide when it's "good enough" and terminate the process. If you use a small ''shrink'' value and let it run to completion, it can take some time to run. This is harmless, but unnecessary. While the section below the solid line remains fully functional, a new program available since 2021 does a much more efficient job of making initial models.

=== New Initial Model Generator ===
{{attachment:initial_model.png|Initial model generation|width="600"}}

The new initial model generator was only added to e2projectmanager in Feb 2022, so if you have an older version, you may need to run it from the command-line. If it isn't available from the command-line either, you should probably update.

 * '''Subtomogram Averaging -> New initial model generator'''
  * ''particles'' = ''Browse'' for sets/initribo.lst (or whatever you called your set)
  * ''res'' = 50 This is a low resolution initial model. No reason to push it.
  * ''niter'' = 10 You may make this up to 100, and simply kill the job when the model seems good enough. 10 is fine for this tutorial, and often you can even stop after 3-5
  * ''shrink'' = 2 (Small) or 4 (Large)
  * ''parallel'' = thread:4 Replace this with the correct number of threads for your machine as above. If you have limited disk space on /tmp, you can also specify a temporary folder: thread:4:/home/username/tmp
  * ''Launch''

If you do not see ''New initial model generator'' in e2projectmanager, you can run it from the command line, replacing appropriate options:

{{{
e2spt_sgd_new.py sets/initribo.lst --res 50 --niter 10 --shrink 2 --parallel thread:4
}}}
The second program will produce output like:

{{{
Gathering metadata...
 69/69
iter 0, class 0:
17 jobs on 4 CPUs
iter 1, class 0:
17 jobs on 4 CPUs
iter 2, class 0:
17 jobs on 4 CPUs
}}}

Once it gets past 3-4 iterations, you can use the browser to look in ''sptsgd_00'', and double-click on ''output_cls0.hdf''. This file will change after each iteration completes. It contains the results of the most recent iteration. When you are satisfied with the quality of the initial model, you can kill it with the task manager in e2projectmanager.

For your own data:
 * If your particle has known ''symmetry'', specify that [[EMAN2/Symmetry]]
 * setting ''shrink'' to something in the range of 2-4 will make the runtime faster but, depending on the shape, could potentially cause problems.
 * using more than the minimal 30-50 particles is fine. If you have a very large set of selected particles, go ahead and use them all. This will not slow the process down at all, since it's stochastic.
 * it is critical that the full sampling box size of the extracted particles divided by ''shrink'' be divisible by 2. If not, the program will crash.

=== Old Initial Model Generator ===
This section is the older program, which is still functional, but not recommended. Skip this if you already used the new version above.

For the tutorial tilt-series:
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  * ''particles'' should be set to the sets/ribo.lst file you just created (whatever name you used).   * ''particles'' should be set to the sets/initribo.lst file you just created (or whatever name you used).
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  * The default ''niter'' of 5 is typically much more than is required    * The default ''niter'' of 5 is typically much more than is required
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== Template matching (5 min) ==

In this step, we will use the initial model you just produced as a template for finding all of the ribosomes in all 4 tomograms. If you completed the '''Tomogram Annotation''' step above, and have already extracted a full set of 1000+ particles, then you can skip this step, as we already have all of the particles.
== Template matching (ONLY if you manually boxed above) ==
If you manually boxed only a few particles in the steps above rather than using one of the semi-automated methods to pick the full 1000 - 3000 particles, then you will now need to use template matching to box out all of the particles. If you already have a set of 1000-3000 particles, skip ahead to '''New Integrated Refinement Program'''

Note that here, and everywhere else in the tomography pipeline, reconstructed particles have positive contrast (look white in projection) and tomograms/tilt series have negative contrast (look dark in projection). If you wish to use a reference volume from the PDB or somesuch, then it should have positive contrast as is normal in the single particle CryoEM field.
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  * browse to select ''tomograms''. Select all 3 tomograms.
  * set ''reference'' to the output.hdf file you produced in the previous step.
  * set ''label'' to "ribo"
  * set ''nptcl'' to 150 (the maximum number of particles per tomogram)
  * ''tomograms'' -> browse and select all 3 tomograms.
  * ''reference'' = the initial model you produced in the previous step
  * ''label'' = ribo
  * ''nptcl'' = 150
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  * Launch

 * when this finishes, you can use the same '''Manual Boxing''' tool you used before to look at the particles which were selected. You may wish to manually remove any bad particles it selected. For the tutorial data set or other tomograms of purified protein, this process should work pretty well. For cells you might wish to use the '''Tomogram Annotation''' method above.
  * ''vthr'' = 5
   * if using an older version of EMAN2, you may wish to use the default of 10, but with the current version, 10 may not find any particles and crash.
   * This threshold is in terms of the number of standard deviations above the mean. The definition was slightly different when the default was 10.
  * ''threads'' = the usual number
* Launch

 * Note: if you see an error, with some mention of zero, it is likely you forgot to reduce vthr to 5.
 * when this finishes,
you can use the same '''Manual Boxing''' tool you used before to look at the particles which were selected. You may wish to manually remove any bad particles it selected. For the tutorial data set or other tomograms of purified protein, this process should work pretty well.
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== Particle extraction (~15 min) ==

Again, if you already did '''Tomogram Annotation''' above, this step isn't necessary. It is only required if you just did '''Template Matching'''.

Since this involves several thousand particles instead of 30-50, it will take quite a lot longer to run. The actual time will depend partially on the speed of your storage.

For the tutorial tilt-series:
For your own data:
 * Frankly, in most cases the deep learning based picker will do a better job. For cells, you may consider the full Tomogram Annotation tool. This program works with highly downsampled tomograms and references for speed.
 * Picking a good ''vthr'' and a reasonable ''nptcl'' maximum may take a little trial and error. Test on 1-3 tomograms before the full run.

=== Particle extraction (ONLY if not done for full data above) ===
If you already extracted a complete set of particles (not just the few initial references) above, you don't need to repeat it again here.

Since this involves several hundred particles instead of 30-50, it will take quite a lot longer to run.

For the tutorial tilt-series:
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  * set ''boxsz_unbin'' to 128.
  * set ''label'' to "ribo"
  * Launch

 * '''Subtomogram Averaging -> Build Sets'''
  * ''boxsz_unbin'' = 128 (Small) or 256 (Large)
  * ''label'' = ribo
  * ''compressbits'' = 5
  * Launch

=== Build Sets (again) ===
It's harmless to repeat this, as it's almost instantaneous, and overwrites existing files.

 * '''Subtomogram Averaging -> Build Sets'''
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  * You can leave ''label'' blank. It will just regenerate all of the .lst files.
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== Subtomogram refinement (~1 hr/iteration) ==
{{attachment:refinement.png| 3D refinement | width=600}}
   * Generally just takes a few seconds. If you have a large project with hundreds of tomograms it will take a bit longer.

== New integrated refinement program ==
There is a new refinement program which implements both traditional subtomogram averaging and subtilt refinement in a single program. This is an alternative to the next two major sections (Subtomogram Refinement and Subtilt Refinement). The full tutorial on the new program is [[https://blake.bcm.edu/emanwiki/EMAN2/e2tomo_new|here]]. It was integrated into e2projectmanager in mid-2022, so make sure you have an up to date version.

=== Small (large below) ===
In the small tutorial will do this as 2 sequential refinement runs for efficiency, and to show how you can continue a refinement. The initial refinement should turn the initial model into something ribosome shaped, but at low resolution. The second refinement should get to ~12 Å resolution.

 * You may need to replace ''sets/ribo.lst'' with whatever you named your set.
 * Replace both ''4''s with the number of threads for your machine.
 * If you didn't use the "new" style initial model generation above, you may also need to alter --ref.

{{{
e2spt_refine_new.py --ptcls sets/ribo.lst --ref sptsgd_00/output_cls0.hdf --iters p,p,t --goldstandard --startres 50 --tophat local --parallel thread:4 --threads 4
}}}

When that's done, you should have a ''spt_00'' folder containing the results of the 3 iterations we requested. You may take a look at:
 * fsc_maskedtight_XX.txt - These are the masked gold-standard resolution curves after each iteration. Double click in the EMAN2 browser to plot them.
 * threed_XX.hdf - These are the 3D maps after each iteration. Again, double-click in the browser to visualize.

The 3rd map should look considerably more like a ribosome than the initial model (threed_00.hdf), but the resolution will still be limited. In the next run, we will do more subtilt refinement to push the resolution.

We could have done this all in a single run, but simply including the additional ''--iters'' letters except for one key addition. The ''--maxres 12'' argument indicates the highest resolution information to consider in the refinement. If this is not specified, it will be determined automatically based on the results of the previous iteration. This will make the iterations run faster, but it may make them progress towards the final resolution more slowly. So, we use the automatic method for 3 iterations to get the shape correct quickly, then in the second run, push the resolution.

 * note that ''--ref'' points at the final map from the previous run
 * ''--loadali2d'' and ''--loadali3d'' load the final alignment parameters from the first run. Note that aliptcls3d files are only produced for 'p' iterations.
 * ''--goldcontinue'' tells the refinement to continue with the even/odd pairs from the previous refinement, rather than phase randomizing the data at high resolution again
 * ''--maxres'' specifies the maximum resolution information to consider during alignment. If omitted, it uses an automatic scheme.
 * ''--tophat local'' enables local resolution measurement and filtration, it adds ~2 minutes per iteration. ''global'' will filter everything uniformly. ''e2help.py tophat''
{{{
e2spt_refine_new.py --ptcls sets/ribo.lst --ref spt_00/threed_03.hdf --loadali2d spt_00/aliptcls2d_03.lst --loadali3d spt_00/aliptcls3d_02.lst --goldcontinue --iters t,p,t,r,d --keep 0.95 --tophat local --parallel thread:4 --threads 4 --maxres 12
}}}

That's it. You hopefully have a ~12 Å resolution map. If you wish to try and push the resolution further, you can follow the Large version of the tutorial

Skip the next 2 sections about the old refinement. Other notes are below that.

=== Large ===

The Large data set should have 1000-3000 particles at full sampling, and should readily achieve ~6.5 Å resolution. This is really designed to run on a workstation, not a laptop.

 * In mid-2022+ versions, this is available from the project manager as '''New 3D Refinement''', you can enter the options from the command below if you prefer to run it that way.
 * You may need to replace ''sets/tomobox.lst'' with whatever you named your set.
 * --ref should point at whatever initial model you want to use
 * Replace both ''4''s with the number of threads for your machine.
 * Replace /home/username/tmp with a folder on a local hard-drive with a decent amount of free space (several GB at a minimum)

{{{
e2spt_refine_new.py --ptcls=sets/tomobox.lst --ref=sptsgd_00/output_cls0.hdf --startres=50.0 --goldstandard --sym=c1 --iters=p,p,p,t,t,t --keep=0.95 --tophat=global --parallel=thread:4:/home/username/tmp --threads=4 --m3dthread
}}}

If you like you could use the modified iters sequence: p,p,p,t,t,r,d,t but this will take considerably longer to run, and likely produce only very slightly improved results. This alternative includes in-plane rotational subtilt refinement and defocus refinement.

You can (and probably should) look at the results while the job is runing, you should have a ''spt_00'' folder containing the results each completed iteration. You may take a look at:
 * fsc_maskedtight_XX.txt - These are the masked gold-standard resolution curves after each iteration. Double click in the EMAN2 browser to plot them.
 * threed_XX.hdf - These are the 3D maps after each iteration. Again, double-click in the browser to visualize.

That's it. You hopefully have a ~6.5 Å resolution map when the job finishes, and it should get pretty close to that after 4-6 iterations.

Skip the next 2 sections about the old refinement. Other notes are below that.
== Old Subtomogram refinement (~1 hr/iteration) ==
{{attachment:refinement.png|3D refinement|width="600"}}
As an alternative to the new integrated tool above, the older pair of programs is still available. You shouldn't need to do both approaches. This step is similar to the "p" iterations above, though it uses an older algorithm.
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Results will gradually appear in spt_XX/
Feel free to look at intermediate results with the EMAN2 file browser as they appear.
Results will gradually appear in spt_XX/ Feel free to look at intermediate results with the EMAN2 file browser as they appear.
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== Subtilt refinement (~9 hr/iteration) ==

{{attachment:subtlt_dir.png| Subtilt refinement directory |width=600}}
== Old Subtilt refinement (~9 hr/iteration) ==
{{attachment:subtlt_dir.png|Subtilt refinement directory|width="600"}}
This is the second half of the old refinement strategy. It is conceptually similar to the t,p and r iterations in the newer integrated program above.
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{{attachment:refinement_evaluation.png| Refinement evaluation |width=600}}
This tool helps visualize and compare results from multiple subtomogram refinement runs. 
{{attachment:refinement_evaluation.png|Refinement evaluation|width="600"}} This tool helps visualize and compare results from multiple subtomogram refinement runs.
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  * In the GUI, you can look at all ''spt_XX'' or ''sptsgd_XX'' folders and compare the parameters which were used for each, as well as the resulting maps. 
  * Switch between folder types using the menu at top right. 
  * Columns can be sorted by clicking on the corresponding header. 
  * In the GUI, you can look at all ''spt_XX'' or ''sptsgd_XX'' folders and compare the parameters which were used for each, as well as the resulting maps.
  * Switch between folder types using the menu at top right.
  * Columns can be sorted by clicking on the corresponding header.
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  * ''!ShowBrowser'' will bring up the ''[[http://blake.bcm.edu/emanwiki/EMAN2/Programs/e2display|e2display.py]]'' browser in the folder of the selected row.    * ''!ShowBrowser'' will bring up the ''[[http://blake.bcm.edu/emanwiki/EMAN2/Programs/e2display|e2display.py]]'' browser in the folder of the selected row.

EMAN2 Tomography and Subtomogram/Subtilt Averaging Workflow Tutorial

Important note: Throughout the tutorial you will see a split between (small) and (large) instructions. The (small) tutorial is designed for laptops or basic desktops and can achieve ~12 Å resolution in a time compatible with live tutorial sessions. The (large) tutorial really requires a proper tomography workstation, but can achieve subnanometer resolution. Do not intermix (small) and (large) options below!

  • This tutorial requires EMAN 2.91 at a minimum. The newer pipeline, which will become the primary pipeline in EMAN3, is also discussed. To use those instructions you should have a current EMAN2.99 snapshot version.
  • Some additional documentation for the newer pipeline for integrated subtomogram and subtilt refinement can be found in TomoNew

  • Documentation of some other recently developed tools can be found in TomoMore.

  • To cite:
    • Chen, M., Bell, J.M., Shi, X. et al. A complete data processing workflow for cryo-ET and subtomogram averaging. Nat Methods 16, 1161–1168 (2019)

Computer Requirements

  • Minimum recommended configuration:
    • 16 GB RAM (small), 64 GB RAM (large)
    • 4 cores @ >2 ghz (small), 16 cores (large)

    • ~40 gb free disk space (small), ~100 gb free disk space, due to larger raw data (large)
    • a high performance disk (SSD or RAID) will significantly reduce runtimes

Note: Any place in EMAN2 where you are requested to enter the number of threads to use, you should specify the number of cores your machine has. Computers are often advertised as 4 core/8 thread or 8 core/16 thread. Trying to run image processing using this advertised number of threads will usually make processing run slower, not faster. You may optionally increase the number of cores by ~25%, ie - on a 4 core machine, specifying 5 may give a 5-10% speedup over 4

Download Data

The tutorial data comes from EMPIAR 10064, but only uses a subset of the data from the mixed CTEM tilt series.

Prepare input files (~2 minutes)

e2projectmanager.py&
  • Make sure any EMAN2 commands you run are executed from within this folder (not any subfolder)
  • You may use "Edit Project" from the Project menu to set default values for the project.
    • If you downloaded our prepared data set, it will already contain an info folder containing the project settings, so you should not need to change anything.

    • For this project use 300 kDa, 2.7 mm Cs, 300 keV and 3.93 (Small) or 1.97 (Large) A/pix.
    • The mass need not be precise, it is only used to keep isosurface values roughly self-consistent.
  • Make sure the workflow mode is set to "TOMO" not "SPR"

Project Manager

  • Raw Data -> Import tilt series

    • Files -> select the 3 (Small) or 4 (Large) provided .hdf files

    • rawtlt, mdoc -> leave these blank

    • invert should not be selected

    • apix = 3.93 (Small) or 1.97 (Large), in later steps you can use -1, which tells it to use the known value

    • import_tiltseries = selected

    • importation = copy

    • compressbits = 5 (8 is fine as well, but will make file sizes slightly larger)

    • Once the options are set, press Launch

When working with your own data:

  • It is critical that the filenames for your data not contain any spaces (replace with underscore) or periods (other than the final period used for the file extension).
  • "__" (double underscore) is also reserved for describing modified versions of the same file, and should not be used in your image filenames.

  • If your tilt series isn't a single stack file, but is many individual images instead, you will need to use Generate tiltseries to build an image stack

Tiltseries Alignment and Tomogram Reconstruction (~10 min Small)

Alignment of the tilt-series is performed iteratively in conjunction with tomogram reconstruction. Tomograms are not normally reconstructed at full resolution, generally limited to 1k x 1k or 2k x 2k, but the tilt-series are aligned at full resolution. For high resolution subtomogram averaging, the raw tilt-series data is used, based on coordinates from particle picking in the downsampled tomograms. On a typical workstation reconstruction takes about 4-5 minutes per tomogram.

For the tutorial tilt-series:

  • 3D Reconstruction -> Reconstruct Tomograms

  • alltiltseries = selected

    • alternatively you can select one or more tilt series from the tiltseries folder

  • correctrot = selected

  • tltax = -4.0

  • tltstep = 2

  • clipz = 96

  • threads = number of physical cores on your machine, optionally *1.25.

  • notmp = checked by default. If you wish to look at the intermediate aligned tilt-series and other files, uncheck this, but note that this will significantly increase disk requirements

    • These files are not required for the remaining steps in the tutorial, but can be used to help understand how the tomogram alignment works. You may consider doing this for only one tomogram.
  • patchtrack = 2 (not really necessary for the tutorial, but shouldn't hurt. This is 3-D patchtracking, not the typical 2-D patchtracking)
  • extrapad = selected (this will make the tomogram reconstructions take a little longer, but look a bit nicer visually. No impact on the final subtomogram averages)
  • Launch

If you opted to run without notmp on one or more tilt series:

  • You will see a tomorecon_XX folder for each tilt series, containing:

    • landmark_0X.txt has the location of the landmarks (which may be fiducials if present) in each iteration

    • samples_0X.hdf shows the top and side view of those landmarks

    • ptclali_0X.hdf has the trace of each landmark throughout the tilt series (they should stay at the center of image all the time if the alignment is good)

    • tomo_0X.hdf is the reconstruction after each iteration

  • Again, note that these files are not required by any downstream processing. If you have difficulty getting a particular tilt series to reconstruct, and the patchtrack=2 option doesn't help, this may help debug the problem. However, if you do encounter problems, we would like to invite you to ask about it either publicly on the mailing list or privately to the developers.

Tomogram reconstruction

When working with your own data:

  • We strongly recommend reconstructing at most 5-10 tilt series to start. Then completing the handedness check in the next step before returning to this step and reconstructing the full set of tilt series! This will allow you to specify the correct tltax value.

  • Either specify the correct tltstep if the tilt series is in order from one extreme to the other, or specify the name of a rawtlt file (as produced by serialem/IMOD).

  • In most cases, the default npk should be fine. If fiducials are present, it is not necessary to adjust this number to match the number of fiducials. The program will use any high contrast areas it finds as potential landmarks.

  • bytile should normally be selected, as it will normally produce better quality reconstructions at higher speed. If 2k or larger tomograms are created, memory consumption may be high, and you should check the program output for the anticipated RAM usage.

  • The graphical interface only permits 1k or 2k reconstruction sizes. In our experience this is normally sufficient for segmentation or particle picking.
  • When the sample is thick, some grid-like tiling pattern can be seen in the reconstruction. Checking extrapad can largely reduce the artifacts. In versions after 2/3/2020, there is also a moretile option that further eliminates them. Note these artifacts will NOT impact the subtomogram averaging results because the particles are extracted in a separate process. Checking these options can make the reconstruction process more memory consuming, and up to 5 times slower.

  • When the sample is thin (purified protein, not cells), it is useful to check correctrot to automatically position tomograms flat in ice

  • It can also be helpful with thin ice to specify a clipz value to generate thinner tomograms (perhaps 64 or 96 for a 1k tomogram).

  • There is a new patchtrack option which may help with refinements that otherwise don't seem to be aligning well. Note that this is not conventional 2-D patchtracking, but a novel 3-D patchtracking routine. This acts as a preprocessing step if specified (2 is recommended).

Handedness Check

EMAN2 will automatically locate the tilt axis in a tilt series if it is not provided, but there is a 180° ambiguity in this determination. An incorrect choice will lead to structures with the incorrect handedness, and may produce suboptimal CTF correction. In some data sets (not the tutorial) this may lead to particles with mixed handedness. Since we specified tltax above, this step isn't necessary for the tutorial, but you can run it to see what the results look like.

EMAN2 includes a novel procedure for resolving this ambiguity from a tilt series based on defocus estimates across the tilted images. The tutorial data set comes out correctly without running this check, but when working with your own data, this step is highly recommended. Once you know the correct tilt axis direction to use for a given microscope/camera, you shouldn't need to run this test on every data set, but it may not be a bad idea even then, as there are various possible configuration/software errors on the instrument which could potentially cause inconsistent results, particularly with a change of magnification.

For the tutorial tilt-series:

  • Subtomogram Averaging -> CTF Estimation

  • tiltseries = select any one tilt series

  • alltiltseries = not selected

  • voltage and cs (double check that values are correct)

  • dfrange = 1.0,4.0,0.02

  • checkhand = selected

  • Launch

You will need to look at the console where you launched e2projectmanager to see the results of the test. It should look something like:

Average score: Current hand - 4.133, flipped hand - 3.290
Defocus std: Current hand - 0.110, flipped hand - 0.165
Current hand is better than the flipped hand in 86.4% tilt images
The handedness (--tltax=-4.1) seems to be correct. Rerun CTF estimation without the checkhand option to finish the process.

If you run this check on multiple images and it seems that they consistently indicate a flipped tilt axis/handedness, then you need to return to the previous step (Tomogram Reconstruction) and redo the reconstruction for all tomograms, with the correct tilt axis entered in the corresponding box. The same tilt axis should be used for all tilt series collected under the same conditions on the same instrument. The automatic value may vary a little among micrographs, just compute the approximate average or median value.

Note: This method removes almost all of the ambiguity about particle handedness. The one potential issue is that the MRC file format uses a non-conventional origin for images. If the data collection software doesn't take this into account, the images may be flipped when written to disk. The easiest way to check the software would be to collect 2 images of the same target and save them directly into different file formats, then checking (in EMAN2) whether the two images appear to have the same handedness. If not, it is likely that the MRC files are incorrect.

CTF Estimation (<5 min)

Do NOT forget this step!

This step will determine the defocus as a function of location for each tilt in each tilt series. This information is stored in the headers of particles as they are extracted from the tilt series, and used for CTF correction during subtomogram averaging. If you forget to do this, you will need to re-run the particle extraction step, which is quite time consuming.

For the tutorial tilt-series:

  • Subtomogram Averaging -> CTF Estimation

  • alltiltseries = selected, note that doing this will override anything present in the tiltseries field

  • dfrange = 1.0,4.0,0.02

  • checkhand = not selected

  • Launch

When working with your own data:

  • The first two options, dfrange and psrange indicate the defocus and phase shift range to search. It is critical that the actual defocus be within the search range (obviously). They take the format of “start, end, step”, so “2, 5, .1” will search defocus from 2 to 5 um with a step size of 0.1. Units for phase shift is degrees.

  • For images taken with volta phase plate, we usually have dfrange of “0.2,2,0.1” and psrange of “60,120,2”.

Note: this program is only estimating CTF parameters, taking tilt into account. It is not performing any phase-flipping corrections on whole tomograms. CTF correction is performed later as a per-particle process. This process requires metadata determined during tilt-series alignment, so it cannot be used with tomograms reconstructed using other software packages.

Note: In >=2022 snapshots of EMAN2 it is possible after CTF correction to return to the 3-D reconstruction step and produce CTF corrected whole tomograms, but this does nothing useful when following the EMAN2 pipeline. If you wish to compare EMAN2 tomograms with other software doing CTF correction, this could potentially be useful

Tomogram reconstruction evaluation

Tomogram evaluation

Analysis and visualization -> Evaluate tomograms can be used to evaluate the quality of your tilt series alignments and tomogram reconstructions. This tool will show more information as you progress through the tutorial, but can be used already at this point to make various assessments of your tomograms. Note that some of this information may not be available if you had notmp checked during the reconstruction.

The correctrot option often does not work well on tutorial tomo3. If you go through the tomograms you should see ribosomes spanning the plane of the image for all of the tomograms. If tomo3 shows only a narrow band containing ribosomes, return to the tomogram reconstruction step above, and re-run the process for only that tomogram (uncheck alltiltseries, and select tiltseries/*tomo3.hdf. Also uncheck correctrot).

  • On the left is a list of tomograms in the project.
    • Selecting a tomogram will show a thumbnail in the image pane on the right.
    • Clicking the header of any column will sort the table by that attribute.
    • #box is the number of boxes in the tomogram

    • loss is the average landmark uncertainty in nm. You should not try to compare this number to, for example, the fiducial alignment error in IMOD, as it is computed in a completely different way. This number can be useful to identify specific tilt series within a project which aren't aligning as well as others, but the absolute number is not a useful value to report/analyze. Even if this number were >5 nm, it is still quite possible to achieve a subnanometer resolution subtomogram average.

    • defocus is the average defocus of the tilt series.

  • On the right
    • The image at the top is the central slice through the tomogram
    • the show2d button displays the selected tomogram in a slice-wise view.

    • ShowTilts shows the corresponding raw tilt series

      • Please note that most tomograms include some out-of-plane tilt (the actual rotation isn't a simple tilt along a single axis), which is taken into account during alignment. This may make it visually appear that the tilt series alignment is not as robust as it actually is.
    • Boxer opens the 3D particle picker

    • PlotLoss will plot the fiducial error for each tilt

    • PlotCtf plot the defocus and phase shift at the center of each tilt image

    • Tiltparams is a bit more complicated. It plots a point list with 6 columns and a number of rows corresponding to the images in the selected tilt series. These are the alignment parameters for the tilt series.

      • You can adjust X Col and Y Col in the plot control panel (middle click the plot). The columns represent:

        • 0 - tilt ID
        • 1 - translation along x
        • 2 - translation along y
        • 3 - tilt angle around y
        • 4 - tilt angle around x
        • 5 - tilt angle around z
    • The first panel below the buttons are the types of particles and how many of that type are in the project
    • The last box is reserved for comments for each tomogram. You can fill in any comments you have on a specific tomogram and it will be saved for future reference.

Particle Picking Choices

There are 4 different tools you can use for particle picking in EMAN2 as of Feb 2022:

  1. A new deep-learning based 3-D picker. Not available in 2.91, must use a recent (2022+) snapshot.
  2. Abusing the deep-learning based segmentation tool for particle picking purposes
  3. Manual particle picking
  4. Template based picking (usually seeded with some manual picking results)

For live versions of this tutorial, we use the older manual+template based approach as it requires no specific hardware, and is a good learning experience, but the deep learning 3-D picker is a good choice for typical situations. For cellular tomograms, the annotation tool approach may still be a good choice.

New Deep-Learning 3-D Picker (recommended approach)

This is the easiest approach by far, and is basically a single step process, but is only available in recent (2022+) snapshots of EMAN2.

  • You should easily be able to select ~500 particles per tomogram, potentially more, but 500 is more than sufficient for the tutorial
  • For instructions, see: New automatic particle picking

  • When complete, skip ahead to the next major section Particle Extraction

Tomogram annotation (GPU recommended)

2D particle picking

  • Since the tutorial data set is purified ribosomes, this step can be skipped for the tutorial data, and you can move on to template-based particle picking. For cells or other types of complex specimens, tomogram annotation can be used to more easily distinguish locations of different types of objects.

For a detailed description of how to use the annotation tool, see: TomoSeg

Here is a brief summary of the annotation-based approach:

  • Segmentation -> Preprocess tomogram

    • This step is not always necessary for tomograms reconstructed in EMAN2, but may slightly improve results.
  • Segmentation -> Box Training References

    • This is a newer interface than previously used for this step. Select a few "Good" (regions containing the feature of interest) and "Bad" (regions not containing the feature of interest) boxes.
    • "~" and "1" on the keyboard can be used to move along the Z axis.
    • The new interface permits different types of features to be identified in a single session and in the same tomogram.
    • If the different features of interest have very different scale, it is always better to keep the box size at 64, and instead rescale the tomogram. As long as the rescaling is done using EMAN2 utilities, the program will correctly keep track of the geometry relative to the original tomogram & tilt series.

    • if you are doing this with the tutorial data, you would only have 2 classes of particles "ribo_good" and "ribo_bad".
    • When pressing Save all visible particles (box checked next to the class name) will be saved

  • The rest of the annotation process remain unchanged from the original tutorial, except that now, all trained neural networks and training results are saved in the neuralnets folder, and all segmented maps are in the segmentations folder. You now only specify the label of the output file instead of the full file name.

  • Segmentation -> Find particles from segmentation to turn segmented maps into particle coordinates.

    • Input both the tomogram and its corresponding segmentation, and the particles coordinates will be written into the metadata file.
    • Slightly tweaking the threshold parameters may yield better results.
    • featurename will become the label of particles generated. Those particles can be viewed in the particle picking step and processed in the following protocols.

Manual particle picking (10-15 min)

3D particle picking

  • Time above is to manually select 30-50 reference particles.
  • You can launch the particle picker in two equivalent ways:
    • Subtomogram averaging -> Manual boxing, select tomogram, Launch

    • Analysis and visualization -> Evaluate tomograms as above, press the "Boxer" button

  • two windows will appear Main Window and Options. If you don't see Options it is probably hiding behind the main window.

  • in the Options window, rename the set of boxes to "initribo". This will be used as the label in later stages

  • The box size can be set in the main window at the left bottom corner, for this tutorial, use 32 for ribosomes (the unbinned box size is 128).
    • This is NOT the same as the size listed near the word erase in another window, which is the size of the eraser.

  • left click and drag to place and reposition boxes in any of the 3 views
  • Hold down Shift when clicking to delete existing boxes.
  • Boxes are shown as circles, which vary in size depending on the Z distance from the center of the particle.
  • If you accidentally include one or more particles with nearby gold fiducials or other high contrast artifacts, it may cause some issues with your generated model (do not do that).
  • Go through slices along z-axis using ‘~’ and ‘1’ on the keyboard, or using the slider in the lower right of the window

  • It may be easier to locate particles if you adjust the Filt slider to ~70, but it will slow things down

  • The interface supports different box types within a single tomogram. Each type has a label. Make sure the label is consistent if selecting the same feature in different tomograms.
  • If you skipped the tomogram annotation step, we will pick a few particles here to generate an initial model, and use the initial model as a reference for template matching.
  • Select 30-50 particles from one tomogram, then close the boxer window.
  • Do not use the Save button in the Options window or any of the menu items related to saving data. Those are available for special purposes. When you change the boxes, your changes are saved immediately and automatically. When you are done, simply close the main window.

  • If you did the previous optional annotation step above, you will be able to see the selected particles here, and if you like, manually update them.

Particle extraction (~2 min (a few manual) - hours (a couple of thousand))

Note that this step will be vastly different resource-wise if you are only extracting a few manually selected particles for purposes of later template matching or if you already selected hundreds of particles from each tomogram.

The reduced 1k x 1k (or 2k) tomograms are used only as a reference to identify the location of the objects to be averaged. Now that we have particle locations, the software returns to the original tilt-series, extracts a per-particle tilt-series, and reconstructs each particle in 3-D independently at full resolution. Since this is performing a full resolution reconstruction of each particle it is somewhat resource intensive.

For the tutorial tilt-series:

  • Subtomogram Averaging -> Extract Particles

    • check alltomograms

    • set boxsz_unbin to 128 (Small) or 256 (Large).

      • If you had the correct size in the previous step this should be the same as leaving the default -1
    • enter the label you used when picking particles ("initribo" if you manually boxed, "tomobox" if you used the deep learning picker)
    • threads = value for your machine

    • Launch
  • Subtomogram Averaging -> Build Sets

    • check allparticles

    • Launch
      • This will generate particle sets, which are virtual particle stacks that consist of particles with the same label from different tomograms.

For your own data

  • If the box size is correct when you select particles from the GUI, you can leave boxsz_unbin as -1, so the program will keep that box size (scaled to the original tilt series)

  • If your particles are deeply buried in other densities, using a bigger padtwod may help, but doing so may significantly increase the memory usage and slow down the process.

  • With CTF information present, it generally does not hurt to check wiener, which filters the 2D particles by SSNR before reconstructing them in 3D.

  • Specify a binning factor in shrink to produce downsampled particles if your memory/storage/CPU time is limited, but it will also limit the resolution you can achieve.

Initial model generation (10 - 60 min)

While intuitively it seems like (since the particles are already in 3-D) the concept of an "initial model" should not be necessary. Unfortunately, due to the missing wedge, and the low resolution of one individual particle (particularly from cells), it is actually critical to make a good starting average. Historically it has been challenging to get a good starting model, depending on the shape of the molecule. This new procedure based on stochastic gradient descent has proven to be quite robust, but it is difficult for the computer to tell when it has converged sufficiently. For this reason, the default behavior is to run much longer than is normally required, and have a human decide when it's "good enough" and terminate the process. If you use a small shrink value and let it run to completion, it can take some time to run. This is harmless, but unnecessary. While the section below the solid line remains fully functional, a new program available since 2021 does a much more efficient job of making initial models.

New Initial Model Generator

Initial model generation

The new initial model generator was only added to e2projectmanager in Feb 2022, so if you have an older version, you may need to run it from the command-line. If it isn't available from the command-line either, you should probably update.

  • Subtomogram Averaging -> New initial model generator

    • particles = Browse for sets/initribo.lst (or whatever you called your set)

    • res = 50 This is a low resolution initial model. No reason to push it.

    • niter = 10 You may make this up to 100, and simply kill the job when the model seems good enough. 10 is fine for this tutorial, and often you can even stop after 3-5

    • shrink = 2 (Small) or 4 (Large)

    • parallel = thread:4 Replace this with the correct number of threads for your machine as above. If you have limited disk space on /tmp, you can also specify a temporary folder: thread:4:/home/username/tmp

    • Launch

If you do not see New initial model generator in e2projectmanager, you can run it from the command line, replacing appropriate options:

e2spt_sgd_new.py sets/initribo.lst --res 50 --niter 10 --shrink 2 --parallel thread:4

The second program will produce output like:

Gathering metadata...
 69/69
iter 0, class 0:
17 jobs on 4 CPUs
iter 1, class 0:
17 jobs on 4 CPUs
iter 2, class 0:
17 jobs on 4 CPUs

Once it gets past 3-4 iterations, you can use the browser to look in sptsgd_00, and double-click on output_cls0.hdf. This file will change after each iteration completes. It contains the results of the most recent iteration. When you are satisfied with the quality of the initial model, you can kill it with the task manager in e2projectmanager.

For your own data:

  • If your particle has known symmetry, specify that EMAN2/Symmetry

  • setting shrink to something in the range of 2-4 will make the runtime faster but, depending on the shape, could potentially cause problems.

  • using more than the minimal 30-50 particles is fine. If you have a very large set of selected particles, go ahead and use them all. This will not slow the process down at all, since it's stochastic.
  • it is critical that the full sampling box size of the extracted particles divided by shrink be divisible by 2. If not, the program will crash.

Old Initial Model Generator

This section is the older program, which is still functional, but not recommended. Skip this if you already used the new version above.

For the tutorial tilt-series:

  • Subtomogram Averaging -> Generate Initial Model

    • particles should be set to the sets/initribo.lst file you just created (or whatever name you used).

    • set shrink to 2, 3 or 4

      • 2 will run slowly but will produce a more detailed initial model (not really necessary)
    • increasing batchsize will use more cores (if you have more than 12), and may cause it to converge to the correct answer in fewer iterations, but each iteration will not become faster.

    • The default niter of 5 is typically much more than is required

    • Launch
      • You can terminate the job as soon as sptsgd_00/output.hdf looks reasonable. If you display the progress monitor (4th icon on the right side of the project manager), you can easily kill the job when you're happy. Usually this will take about 10 minutes for the tutorial data.

For your own data:

  • If your particle has known symmetry, specify that EMAN2/Symmetry

  • The symmetry you specify will not be imposed on the map unless you also check applysym, but the map will be rotationally aligned so the symmetry axes are in the correct direction, which will make it easier to apply symmetry in later steps. We do not generally recommend checking this box in this step.

  • setting shrink to something in the range of 2-4 will make the runtime faster but, depending on the shape, could potentially cause problems.

  • using more than the minimal 30-50 particles is fine. If you have a very large set of selected particles, go ahead and use them all. This will not slow the process down at all, since it's stochastic.
  • it is critical that the full sampling box size of the extracted particles divided by shrink be divisible by 2. If not, the program will crash.

Template matching (ONLY if you manually boxed above)

If you manually boxed only a few particles in the steps above rather than using one of the semi-automated methods to pick the full 1000 - 3000 particles, then you will now need to use template matching to box out all of the particles. If you already have a set of 1000-3000 particles, skip ahead to New Integrated Refinement Program

Note that here, and everywhere else in the tomography pipeline, reconstructed particles have positive contrast (look white in projection) and tomograms/tilt series have negative contrast (look dark in projection). If you wish to use a reference volume from the PDB or somesuch, then it should have positive contrast as is normal in the single particle CryoEM field.

  • Subtomogram Averaging -> Reference Based Boxing

    • tomograms -> browse and select all 3 tomograms.

    • reference = the initial model you produced in the previous step

    • label = ribo

    • nptcl = 150

      • IMPORTANT NOTE: There are more particles than this in these images. We limit this to 150 from each tomogram so the tutorial runs faster. If you are unconcerned with speed, you can increase this number, but if you're doing that, you may consider running the full tutorial instead.

    • vthr = 5

      • if using an older version of EMAN2, you may wish to use the default of 10, but with the current version, 10 may not find any particles and crash.
      • This threshold is in terms of the number of standard deviations above the mean. The definition was slightly different when the default was 10.
    • threads = the usual number

    • Launch
  • Note: if you see an error, with some mention of zero, it is likely you forgot to reduce vthr to 5.
  • when this finishes, you can use the same Manual Boxing tool you used before to look at the particles which were selected. You may wish to manually remove any bad particles it selected. For the tutorial data set or other tomograms of purified protein, this process should work pretty well.

  • note that this process stores 3-D particle locations in the appropriate info/* files, but does not extract particles from the micrographs

For your own data:

  • Frankly, in most cases the deep learning based picker will do a better job. For cells, you may consider the full Tomogram Annotation tool. This program works with highly downsampled tomograms and references for speed.
  • Picking a good vthr and a reasonable nptcl maximum may take a little trial and error. Test on 1-3 tomograms before the full run.

Particle extraction (ONLY if not done for full data above)

If you already extracted a complete set of particles (not just the few initial references) above, you don't need to repeat it again here.

Since this involves several hundred particles instead of 30-50, it will take quite a lot longer to run.

For the tutorial tilt-series:

  • Subtomogram Averaging -> Extract Particles

    • check alltomograms

    • boxsz_unbin = 128 (Small) or 256 (Large)

    • label = ribo

    • compressbits = 5

    • Launch

Build Sets (again)

It's harmless to repeat this, as it's almost instantaneous, and overwrites existing files.

  • Subtomogram Averaging -> Build Sets

    • check allparticles

    • You can leave label blank. It will just regenerate all of the .lst files.

    • Launch
      • This will generate particle sets, which are virtual particle stacks that consist of particles with the same label from different tomograms.
      • Generally just takes a few seconds. If you have a large project with hundreds of tomograms it will take a bit longer.

New integrated refinement program

There is a new refinement program which implements both traditional subtomogram averaging and subtilt refinement in a single program. This is an alternative to the next two major sections (Subtomogram Refinement and Subtilt Refinement). The full tutorial on the new program is here. It was integrated into e2projectmanager in mid-2022, so make sure you have an up to date version.

Small (large below)

In the small tutorial will do this as 2 sequential refinement runs for efficiency, and to show how you can continue a refinement. The initial refinement should turn the initial model into something ribosome shaped, but at low resolution. The second refinement should get to ~12 Å resolution.

  • You may need to replace sets/ribo.lst with whatever you named your set.

  • Replace both 4s with the number of threads for your machine.

  • If you didn't use the "new" style initial model generation above, you may also need to alter --ref.

e2spt_refine_new.py --ptcls sets/ribo.lst --ref sptsgd_00/output_cls0.hdf --iters p,p,t --goldstandard --startres 50 --tophat local --parallel thread:4 --threads 4

When that's done, you should have a spt_00 folder containing the results of the 3 iterations we requested. You may take a look at:

  • fsc_maskedtight_XX.txt - These are the masked gold-standard resolution curves after each iteration. Double click in the EMAN2 browser to plot them.
  • threed_XX.hdf - These are the 3D maps after each iteration. Again, double-click in the browser to visualize.

The 3rd map should look considerably more like a ribosome than the initial model (threed_00.hdf), but the resolution will still be limited. In the next run, we will do more subtilt refinement to push the resolution.

We could have done this all in a single run, but simply including the additional --iters letters except for one key addition. The --maxres 12 argument indicates the highest resolution information to consider in the refinement. If this is not specified, it will be determined automatically based on the results of the previous iteration. This will make the iterations run faster, but it may make them progress towards the final resolution more slowly. So, we use the automatic method for 3 iterations to get the shape correct quickly, then in the second run, push the resolution.

  • note that --ref points at the final map from the previous run

  • --loadali2d and --loadali3d load the final alignment parameters from the first run. Note that aliptcls3d files are only produced for 'p' iterations.

  • --goldcontinue tells the refinement to continue with the even/odd pairs from the previous refinement, rather than phase randomizing the data at high resolution again

  • --maxres specifies the maximum resolution information to consider during alignment. If omitted, it uses an automatic scheme.

  • --tophat local enables local resolution measurement and filtration, it adds ~2 minutes per iteration. global will filter everything uniformly. e2help.py tophat

e2spt_refine_new.py --ptcls sets/ribo.lst --ref spt_00/threed_03.hdf --loadali2d spt_00/aliptcls2d_03.lst --loadali3d spt_00/aliptcls3d_02.lst --goldcontinue --iters t,p,t,r,d --keep 0.95 --tophat local --parallel thread:4 --threads 4 --maxres 12 

That's it. You hopefully have a ~12 Å resolution map. If you wish to try and push the resolution further, you can follow the Large version of the tutorial

Skip the next 2 sections about the old refinement. Other notes are below that.

Large

The Large data set should have 1000-3000 particles at full sampling, and should readily achieve ~6.5 Å resolution. This is really designed to run on a workstation, not a laptop.

  • In mid-2022+ versions, this is available from the project manager as New 3D Refinement, you can enter the options from the command below if you prefer to run it that way.

  • You may need to replace sets/tomobox.lst with whatever you named your set.

  • --ref should point at whatever initial model you want to use
  • Replace both 4s with the number of threads for your machine.

  • Replace /home/username/tmp with a folder on a local hard-drive with a decent amount of free space (several GB at a minimum)

e2spt_refine_new.py --ptcls=sets/tomobox.lst --ref=sptsgd_00/output_cls0.hdf --startres=50.0 --goldstandard --sym=c1 --iters=p,p,p,t,t,t --keep=0.95 --tophat=global --parallel=thread:4:/home/username/tmp --threads=4 --m3dthread

If you like you could use the modified iters sequence: p,p,p,t,t,r,d,t but this will take considerably longer to run, and likely produce only very slightly improved results. This alternative includes in-plane rotational subtilt refinement and defocus refinement.

You can (and probably should) look at the results while the job is runing, you should have a spt_00 folder containing the results each completed iteration. You may take a look at:

  • fsc_maskedtight_XX.txt - These are the masked gold-standard resolution curves after each iteration. Double click in the EMAN2 browser to plot them.
  • threed_XX.hdf - These are the 3D maps after each iteration. Again, double-click in the browser to visualize.

That's it. You hopefully have a ~6.5 Å resolution map when the job finishes, and it should get pretty close to that after 4-6 iterations.

Skip the next 2 sections about the old refinement. Other notes are below that.

Old Subtomogram refinement (~1 hr/iteration)

3D refinement As an alternative to the new integrated tool above, the older pair of programs is still available. You shouldn't need to do both approaches. This step is similar to the "p" iterations above, though it uses an older algorithm.

This step performs a conventional iterative subtomogram averaging using the full set of particles. Typically it will achieve resolutions in the 15-25 A range with a reasonable number of particles. As it involves 3-D alignment of the full set of particles multiple times, it takes a significant amount of compute time. Higher resolutions are achieved in the next stage after this (subtilt refinement).

For the tutorial tilt-series:

  • Subtomogram Averaging -> 3D Refinement

    • set particles to "sets/ribo.lst"

    • set reference to "output.hdf" from Initial Model Generation

    • set goldstandard to 30

    • set mass to 3000

    • set threads to the number of CPUs on your machine

    • Launch

Results will gradually appear in spt_XX/ Feel free to look at intermediate results with the EMAN2 file browser as they appear.

For your own data:

  • If your molecule has symmetry, you should specify it, but it's important that the alignment reference you provide has been properly aligned to the symmetry axes of whichever symmetry you specify.
  • localfilter will use e2fsc.py to compute a local resolution map after each iteration and filter the map accordingly. This is useful for molecules with significant variability.

  • If you suspect that a large fraction of your particles are "bad" in some way, you may wish to try reducing pkeep, which will hopefully exclude bad particles preferentially over "good" particles.

Old Subtilt refinement (~9 hr/iteration)

Subtilt refinement directory This is the second half of the old refinement strategy. It is conceptually similar to the t,p and r iterations in the newer integrated program above.

With the results of a good subtomogram alignment/average, we are now ready to switch to alignment of the individual particle images in each tilt, along with per-particle-per-tilt CTF correction and other refinements. This is effectively a hybrid of single particle analysis and subtomogram averaging, and can readily achieve subnanometer resolution IF the data is of sufficient quality. The tutorial data set is, but many cellular tomograms, for example, are not collected with high resolution in mind, and even with this sort of refinement will be unable to achieve resolutions better than 10-30 A, depending on the data. This process is completely automatic, based on all of the metadata collected up to this point. While it is possible to perform "subtomogram refinement" with subtomograms from any tomogram, Subtilt Refinement cannot operate properly unless all preceding steps occurred within EMAN2.

For the tutorial tilt series:

  • Subtomogram Averaging -> Sub-tilt Refinement

    • path should be set to the name of one of a "spt_XX" folder to use as a starting point for the refinement

    • iter can be -1 to use the last complete iteration in the "spt_XX" folder. Alternatively you can specify a specific iteration to use

    • parallel should be "thread:N" where N is the number of cores you wish to use on a single machine. This job can be run on a linux cluster if you like: EMAN2/Parallel.

    • threads should also be set to the number of cores to use on a single machine

    • Launch

For your own data:

  • niters is the number of iterations to run. The default of 4 should achieve convergence in most cases.

  • keep is the fraction of tilt images to use in the final map. This defaults to 0.5, meaning the worst 1/2 of the tilts for each particle will be discarded. This permits tilts which contain, for example, projections of fiducials or other strong densities, or with large amounts of motion to be automatically excluded in the final reconstruction.

  • maxalt specifies the maximum tilt angle to include from each particle. Most tilt series are collected such that the small tilt angles will have the least radiation damage, and very often high tilts suffer from more motion artifacts. If you enter, for example, "45" in this box then tilts <-45 and >45 will be discarded automatically. In most cases keep will already serve a similar purpose.

Congratulations! The final result of the tutorial will be found in "subtlt_00/". The final 3-D map will be "threed_04.hdf" with the default parameters. The final gold standard resolution curve will be "fsc_maskedtight_04.txt". The optional steps below are tools you can use to evaluate your results in more detail.

Refinement evaluation (optional)

Refinement evaluation This tool helps visualize and compare results from multiple subtomogram refinement runs.

  • Analysis and Visualization -> Evaluate SPT Refinements

    • In the GUI, you can look at all spt_XX or sptsgd_XX folders and compare the parameters which were used for each, as well as the resulting maps.

    • Switch between folder types using the menu at top right.
    • Columns can be sorted by clicking on the corresponding header.
    • Uncheck items in the list at bottom-right to hide corresponding columns
    • ShowBrowser will bring up the e2display.py browser in the folder of the selected row.

    • !PlotFSC will display the "tight" FSC curve over all iterations.

    • PlotParams will plot the Euler angle distribution and other alignment parameters

      • The 8 columns in the plot are:
        • 0 - az (EMAN convention Euler angle)
        • 1 - alt
        • 2 - phi
        • 3 - translation in X
        • 4 - Y
        • 5 - Z
        • 6 - alignment score
        • 7 - missing wedge coverage

EMAN2/e2TomoSmall (last edited 2024-07-14 21:59:58 by MuyuanChen)