Re: [ccp4bb] AW: [ccp4bb] possible twinning issue in P4212 / I422
It helps to look at the output from the truncate step quite critically. First is there a non cryst translation of 1/2,1/2,1/2 indicated in the P4 2i2 data set? If so then the I centring at lower resolution might just be approximate.. If there is NC translation then other twinning statistics are distorted and I find the only semi-reliable one is the L test. But if you say there is no room for your protein with that translation and 4/mmm symmetry then there must be twinning or you have crystallised something else! Eleanor On 4 June 2014 08:48, herman.schreu...@sanofi.com wrote: Dear Bjørn, I guess the first step to enlightment is to recognize that we as mere mortals are not able to deduce the space group from diffraction data alone. All Aimless, XDS etc. can produce are educated guesses what the space group might be. Especially when twinning is involved, the crystal packing may not heed the rules and classifications that we humans try to impose. In many cases, one might have to go down to P1 and solve the structure in P1 to find out what the true space group is. Here are some comments to your questions: -the same protein under the same crystallization conditions and even in the same drop may produce crystals with very different crystal packings, even with the same unit cell, so your 4 and 7.5Å crystals may be different. -If there is no way to fit the protein in the asymmetric unit that is a very strong indication that you do have twinning. -There have been some discussions in the CCP4BB, but I do not believe that twinning can generate body centering. -You might be barking at the wrong tree and the twinning axis might be parallel to the 4-fold axis, or even generating the 4-fold. You may even have 4-fold twinning. -You may have pseudo body centering, which is perfect at low resolution, but breaks down at higher resolution. As a test, you could process your 4Å data only to 7.5Å and see what the statistics would look like. What I would do: If you have more crystals, collect data on them all, maybe there is one which is not or not perfectly twinned. If there is a model which could be used for molecular replacement: process the data in P4, I4, P222 and P1 and run molecular replacement with all possible space groups for both crystals. However, at 4Å with unclear twinning, solving your structure will be tough. Best, Herman -Ursprüngliche Nachricht- Von: CCP4 bulletin board [mailto:CCP4BB@JISCMAIL.AC.UK] Im Auftrag von Bjørn Panyella Pedersen Gesendet: Dienstag, 3. Juni 2014 21:01 An: CCP4BB@JISCMAIL.AC.UK Betreff: [ccp4bb] possible twinning issue in P4212 / I422 Dear All, I have a strange potential twinning issue that I cannot understand. I've searched high and low on all the internets to find an answer but have come up empty-handed, so I look to the wisdom of The Board to enlighten me. I have a 4'ish Å dataset that processes nicely in P 4 21 2 (#90). However intensity distributions indicate possible almost perfect twinning (eg. I^2/I^2 : 1.592 ). So I speculate that the real space group might be P 4 (#75). Recently we collected a new fairly low resolution (7.5Å) dataset, from the same type of crystals (same purification, same conditions). But the space group in XDS and aimless now comes out very clearly as either I422 (#97) or I4212 (#98) (screw-axis is unclear given the data). The unit-cell parameters are exactly the same as in sg #90, which btw. means that in the body-centered lattice there is no way the protein can fit in the asym. unit. So I guess what I don't understand is: Is it possible to go from a primitive lattice to a body-centered lattice by twinning. Is this just a low-resolution artifact? Or is this a P4 unitcell that can appear like P4212 or I422 depending on small variations (weak dehydration or similar). Has anyone experienced something similar? Am I missing a basic facet of how twinning works, or is something else at play here? Thanks for any insights or suggestions! All the best, /Bjørn -- Bjørn Panyella Pedersen Macromolecular Structure Group University of California, San Francisco
Re: [ccp4bb] AW: [ccp4bb] possible twinning issue in P4212 / I422
Dear All, Thanks for all the suggestions, on and off the board! Summary: Some have asked for the L-statistic in P 4 21 2: Mean |L| :0.397 (untwinned: 0.500; perfect twin: 0.375) All programs tried (xtriage, truncate, pointless) agree that the 4Å data is likely twinned P4 with an estimated twin-fraction ranging from 0.38 to 0.48. People seem to agree (as was my initial understanding) that twinning by itself cannot change a primitive lattice to a body-centered lattice. Thus this change in my low-resolution dataset must be caused by something else. Pseudo body centering has been suggested as the likely explanation for the primitive to body-centered lattice change in the low-resolution dataset. - As suggested, I have looked at the self-patterson for the 4Å dataset and see no peaks, at 1/2,1/2,1/2 or elsewhere. - As suggested, I have looked at the truncate output of the table Analysis of mean intensity by parity for reflection classes in the h+k+l column, but see no differences from h+k+l=2n to h+k+l=2n+1 in the 4Å dataset. - As suggested I have processed the 4Å data at 8Å to see if pseudo body centering was breaking down at higher resolution. At 8Å there was still not sign of pseudo body centering. Thus the 4Å data does not not support pseudo body centering, as far as I can tell. Some has suggested that the crystals are simply two different things. This might be, but since the low-resolution dataset has exactly the same unit-cell parameters as the 4Å dataset, it seems unlikely to me that the crystal packing is significantly different, or that the content of the crystals differ. It seem likely that both crystals contain the same thing in approx. the same type of packing. So no clear explanation for the observed behavior so far, but most likely the low resolution is obscuring the real problem in this particular instance. As is almost always the case, the way forward is to get more and better data to understand the problem. As one suggested offboard (tongue-in-cheek): Why not find crystals that are not twinned, probably with higher resolution? I will do that, and thanks again for your input! All the best, -Bjørn On 06/04/2014 03:09 AM, Eleanor Dodson wrote: It helps to look at the output from the truncate step quite critically. First is there a non cryst translation of 1/2,1/2,1/2 indicated in the P4 2i2 data set? If so then the I centring at lower resolution might just be approximate.. If there is NC translation then other twinning statistics are distorted and I find the only semi-reliable one is the L test. But if you say there is no room for your protein with that translation and 4/mmm symmetry then there must be twinning or you have crystallised something else! Eleanor On 4 June 2014 08:48, herman.schreu...@sanofi.com mailto:herman.schreu...@sanofi.com wrote: Dear Bjørn, I guess the first step to enlightment is to recognize that we as mere mortals are not able to deduce the space group from diffraction data alone. All Aimless, XDS etc. can produce are educated guesses what the space group might be. Especially when twinning is involved, the crystal packing may not heed the rules and classifications that we humans try to impose. In many cases, one might have to go down to P1 and solve the structure in P1 to find out what the true space group is. Here are some comments to your questions: -the same protein under the same crystallization conditions and even in the same drop may produce crystals with very different crystal packings, even with the same unit cell, so your 4 and 7.5Å crystals may be different. -If there is no way to fit the protein in the asymmetric unit that is a very strong indication that you do have twinning. -There have been some discussions in the CCP4BB, but I do not believe that twinning can generate body centering. -You might be barking at the wrong tree and the twinning axis might be parallel to the 4-fold axis, or even generating the 4-fold. You may even have 4-fold twinning. -You may have pseudo body centering, which is perfect at low resolution, but breaks down at higher resolution. As a test, you could process your 4Å data only to 7.5Å and see what the statistics would look like. What I would do: If you have more crystals, collect data on them all, maybe there is one which is not or not perfectly twinned. If there is a model which could be used for molecular replacement: process the data in P4, I4, P222 and P1 and run molecular replacement with all possible space groups for both crystals. However, at 4Å with unclear twinning, solving your structure will be tough. Best, Herman -Ursprüngliche Nachricht- Von: CCP4 bulletin board [mailto:CCP4BB@JISCMAIL.AC.UK mailto:CCP4BB@JISCMAIL.AC.UK] Im Auftrag von Bjørn Panyella Pedersen Gesendet: Dienstag, 3. Juni 2014 21:01 An:
[ccp4bb] ideal rms bond and rms angle
Dear all I request you to please tell me the ideal rms bond and rms angle for a perfectly refined structure..As we can see in order to have optimum R and Rfree we often adjust the weighing factor in Refmac so as the R and Rfree changes it brings changes in rms bond and rms angle as well..Does the quality of a structure depends upon the value of these rms deviation ? And what is the ideal value for these ? -- Regards Faisal School of Life Sciences JNU
Re: [ccp4bb] ideal rms bond and rms angle
Hi Faisal, There are no clearly defined targets for rmsd because it is the rms of values with different standard deviations. You should use rmsZ instead (reported by Refmac) because the deviations are on the same scale. For rmsZ, any value below 1.0 is fine if it gives you the best fit with the data. I would not recommend aiming for a specific value. HTH, Robbie -Original Message- From: CCP4 bulletin board [mailto:CCP4BB@JISCMAIL.AC.UK] On Behalf Of Faisal Tarique Sent: Wednesday, June 04, 2014 22:53 To: CCP4BB@JISCMAIL.AC.UK Subject: [ccp4bb] ideal rms bond and rms angle Dear all I request you to please tell me the ideal rms bond and rms angle for a perfectly refined structure..As we can see in order to have optimum R and Rfree we often adjust the weighing factor in Refmac so as the R and Rfree changes it brings changes in rms bond and rms angle as well..Does the quality of a structure depends upon the value of these rms deviation ? And what is the ideal value for these ? -- Regards Faisal School of Life Sciences JNU