Processing CEST Data: Difference between revisions

Latest revision as of 15:30, 9 September 2024

Processing CEST Data

Have X11, nmrPipe, Python >=2.7, and ChemEx (from the Kay lab) installed
Open a c-shell with “csh” and navigate to the directory with your ser file
Open X11
In the terminal type “bruker”
Click “read parameters”
Switch the F1 and F2 axes
1. y should be real with N total and valid points
2. z should be the 15N dimension
3. zMODE Echo-Antiecho
4. yMODE Real
5. aq2D States
Save the script. It should look like the script that follows this protocol.
Add these lines:
1. xyz2pipe –in fid/test%03d.fid –z –ri2c
2. | pipe2xyz –out fids/UBQ%03d.fid –y –ov
3. /bin/rm –fr data/
Run the fid.com script you just saved.
Input file names and phase values into ftcpmg.com (follows this protocol) and run
Open test spectrum in nmrDraw
Pick peaks and save the peak list
Rename the peaks to their corresponding amino acid and residue #. Alternatively, create a peakList.txt with their IDs and run addA.py.
Run autoFit.tcl in the c-shell.
1. autoFit.tcl –specName fts/UBQ%03d.ft2 –inTab test.tab –series
Run extract_profiles_bru.py (follows)
1. ./extract_profiles_bru.py –tbl nlin.tab –par fq3list –out fit/
Make sure the .out files are named like “A#N-HN.out”
Then run ChemEx, check their tutorial

@@ Line 22: / Line 22: @@
 #	Open test spectrum in nmrDraw
 #	Pick peaks and save the peak list
-#	Rename the peaks to their corresponding amino acid and residue #. Alternatively, create a peakList.txt with their IDs and run [https://bionmr.unl.edu/files/misc/mediawikidownloads/CEST/caddA.py addA.py].
+#	Rename the peaks to their corresponding amino acid and residue #. Alternatively, create a peakList.txt with their IDs and run [https://bionmr.unl.edu/files/misc/mediawikidownloads/CEST/addA.py addA.py].
 #	Run [https://bionmr.unl.edu/files/misc/mediawikidownloads/CEST/autoFit.tcl autoFit.tcl] in the c-shell.
 ##autoFit.tcl –specName fts/UBQ%03d.ft2 –inTab test.tab –series