Hi
I recently processed a x-ray diffraction data set to 2.5 A for my protein complex. After data reduction with imosflm and Aimless, it turns out the Rmerge is 0.000 (see below). Also, the mean I/sigma I for innershell goes up to an abnormal value of 346.0
Could anyone shed some light on what has happened here?
Thanks in advance.
Low resolution limit 27.27 27.27 2.60
High resolution limit 2.50 9.01 2.50
Rmerge (within I+/I-) 0.000 0.000 0.000
Rmerge (all I+ and I-) 0.067 0.024 0.356
Rmeas (within I+/I-) 0.000 0.000 0.000
Rmeas (all I+ & I-) 0.094 0.034 0.503
Rpim (within I+/I-) 0.000 0.000 0.000
Rpim (all I+ & I-) 0.067 0.024 0.356
Rmerge in top intensity bin 0.000 - -
Total number of observations 17077 388 1887
Total number unique 11697 215 1375
Mean((I)/sd(I)) 35.7 376.0 2.2
Mn(I) half-set correlation CC(1/2) 0.990 0.996 0.688
R-merge = zero is fishy, unless you have a triclinic data set. One or two spots with high I/sigmaI may be ok. Your total number of observations is unduly high for a 2.5A data. How many resolution bins were chosen for the statistics. Default may be 10, but to see the range 9.01 to 2.5 A for last resolution bin does not sound normal. Please share cell parameters, distortion index values from indexing etc., to make further comments
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