Re: [phenixbb] Phenix Xtriage label error

12 Apr 2016

      Hi Ryan,

Thank you very much!  Below are the summary of my pointless log after
"quick scale" from Imosflm (this time I force imosflm to choose P1 in the
integration and scale but pointless chose P31):

 $TEXT:Result: $$ $$

Summary data for        Project: New Crystal: New Dataset: New

                                           Overall  InnerShell  OuterShell

Low resolution limit                       82.13     82.13      2.49

High resolution limit                       2.40      8.98      2.40

Rmerge  (within I+/I-)                     0.075     0.033     0.851

Rmerge  (all I+ and I-)                    0.086     0.048     0.919

Rmeas (within I+/I-)                       0.089     0.039     1.007

Rmeas (all I+ & I-)                        0.093     0.052     0.996

Rpim (within I+/I-)                        0.047     0.021     0.534

Rpim (all I+ & I-)                         0.035     0.021     0.380

Rmerge in top intensity bin                0.031        -         -

Total number of observations              214291      4072     22139

Total number unique                        31247       617      3299

Mean((I)/sd(I))                             14.4      29.4       2.9

Mn(I) half-set correlation CC(1/2)         0.998     0.995     0.785

Completeness                               100.0      99.9      99.8

Multiplicity                                 6.9       6.6       6.7

*Anomalous completeness                      99.7      98.1      98.8*

*Anomalous multiplicity                       3.4       3.4       3.3*

*DelAnom correlation between half-sets      0.303     0.473     0.046*

*Mid-Slope of Anom Normal Probability       1.161       -         -  *

*Estimate of maximum resolution for significant anomalous signal =
3.97A, from CCanom >  0.15*

Estimates of resolution limits: overall

   from half-dataset correlation CC(1/2) >  0.30: limit =  2.40A  ==
maximum resolution

   from Mn(I/sd) >  1.50:                         limit =  2.40A  ==
maximum resolution

   from Mn(I/sd) >  2.00:                         limit =  2.40A  ==
maximum resolution

Estimates of resolution limits in reciprocal lattice directions:

  Along h k plane

   from half-dataset correlation CC(1/2) >  0.30: limit =  2.40A  ==
maximum resolution

   from Mn(I/sd) >  1.50:                         limit =  2.40A  ==
maximum resolution

  Along l axis

   from half-dataset correlation CC(1/2) >  0.30: limit =  2.40A  ==
maximum resolution

   from Mn(I/sd) >  1.50:                         limit =  2.40A  ==
maximum resolution

Anisotropic deltaB (i.e. range of principal components), A^2: 12.33

Average unit cell:   65.87   65.87  164.25   90.00   90.00  120.00

Space group: P 31

Average mosaicity:   0.58

Minimum and maximum SD correction factors: Fulls   1.07 104.68
Partials   1.18 134.50

Anomalous flag switched ON in input, strong anomalous signal found

$$

==============================================================

I do not know if this data set with such anomalous completeness and
multiplicity is enough for me to get phase information to

locate the Iodine, I do not have native dataset, and only have iodine
soaking dataset.

On Tue, Apr 12, 2016 at 11:53 AM, rspencer  wrote:
...
Hi Alex,
You need to look at you anomalous signal in the aimless.log output to see
if there was a detectable anomalous signal. You can also force iMosflm to
treat the dataset as having an anomalous signal so that it won’t merge your
intensities.
Soaking does not guarantee that you will have an anomalous signal in your
crystal and you may need to do a multiple crystals with increasing soak
time to get an anomalous signal. You can easily do this by soaking the
crystal and checking a few frames on your in-house source. Process the
frames and see if an anomalous signal is detected.
Good luck!
Ryan
*From:* [email protected] [mailto:
[email protected]] *On Behalf Of *Alex Lee
*Sent:* Tuesday, April 12, 2016 11:09 AM
*To:* [email protected]
*Subject:* [phenixbb] Phenix Xtriage label error
Dear Phenixbb members,
I have a data-set of a 8 kDa protein crystal around 2.5A resolution. The
protein crystal was soaked in potassium iodine before collecting data using
in-house beam (1.54A wavelength). As I expected some anomalous signal from
the iodine ion from the crystal, after I use Imosflm to index, integrate
and scale the data (space group P3). I got four output .mtz files:
pointless_XXX.mtz; aimless_xxx.mtz; ctruncate_xxx.mtz;
ctruncate_xxx-unique.mtz. After I check with viewHKL, I found the only
unmerged mtz data is pointless_XXX.mtz, the other three mtz files are
merged.
The next step I tried to use Phenix Xtriage (Linux version 1.10.1) to
check my mtz data for anomalous completeness, I thought in this step my mtz
should be unmerged type to see the anomalous signal, so I chose
"pointless_xxx.mtz" as Xtriage input, but for the data labels in the
Xtriage GUI panel, I can only have two choices of "I, SIGI, Merged" and
"IPR, SIGIPR, Merged", it seems I do not have a choice of an unmerged mtz
label. I decide to leave this choice blank by choosing data labels"---".
After I click "run", Xtriage gave an error "please select labels for input
data".
Any input on this issue?
Thanks in advance.