fiber tracts clustered around midbrain #928
Replies: 4 comments 4 replies
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Hi @iliana-karipidis : If I had to guess something went wrong in the mapping stage. I would look at the file that has the suffix: "dwi_b0_in_MNI.nii.gz". I imagine it looks very wrong. If that is the case, there are two options here:
If you did that, I would suggest trying to run your pipeline without reference to the qsiprep mapping. I.e., take out this section from your config.
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Also, just to be sure: the sequences used are identical apart from the addition of a second shell? |
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I'll start by saying that I am not sure what is going on here, and I need to think about this more (maybe others have more ideas). What model are you using for tractography in the two-shell data? I don't think that mrtrix's standard CSD would work here because I don't think that it works out of the box on multi-shell data. Or maybe you are using the multi-shell multi-tissue tractography here? In addition, it looks like CSD fit to the two shells (which DIPY's implementation does do) doesn't work very well -- the APM is computed from the CSD coefficients. I don't think that I've ever seen an APM map with these very high-intensity spots. |
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On a bit more though, could you share your config file? I figure that can answer a few different questions that I have. |
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I am setting up a new DWI protocol and analyzing some pilot data (Philips scanner, 32 dirs, b=1,000 & 2,000, isotropic 2mm). Preprocessing was performed using qsiprep and qsirecon, output was reviewed and looks ok. The pyAFQ output looks incorrect, with all fiber tracts clustered around the midbrain. What went wrong?
This issue seems to be specific to this pilot data, processing single-shell data of another sequence (Philips scanner, 32 dirs, b=1,000, isotropic 2mm) worked well:
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