Hi Phil,

Being young and impressionable, I only changed ZERR, and you are quiet right 
the result is the rigorous and expected error propagation of shelxl. Of course 
the more fun experiment would be in systematically changing various values in 
UNIT to watch the molecule distort.

Hope all is well,
jbb

Jeffrey B. Bonanno, Ph.D.
Department of Biochemistry
Albert Einstein College of Medicine
1300 Morris Park Avenue
Bronx, NY 10461
off. 718-430-2452 fax. 718-430-8565
email jeffrey.bona...@einsteinmed.org

From: Jeffrey, Philip D. <pjeff...@princeton.edu>
Sent: Wednesday, July 15, 2020 12:47 PM
To: CCP4BB@JISCMAIL.AC.UK; Jeffrey B Bonanno <jeffrey.bona...@einsteinmed.org>
Subject: Re: [ccp4bb] Quote source inquiry

CAUTION: This email comes from an external source; the attachments and/or links 
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:: took a working dataset and increased (only) the error on unit cell 
dimensions in the instruction file for the final round of full matrix :: least 
squares refinement in shelxl. Sure enough, the errors on the bonds and angles 
shot up. I was more careful

Question: did you change the unit cell dimensions (UNIT) or the reported 
standard error in the unit cell dimensions (ZERR) ?  If just the latter don't 
you think that the error propagation is just a factor of SHELXL converting from 
fractional to orthogonal coordinates to give you bond lengths and bond angles 
(i.e. the bonds and angles would be numerically the same, but the estimated 
error associated with them would be higher).  Did the e.s.d.'s of the actual 
coordinates in fractional space change ?

Phil Jeffrey
Princeton
________________________________
From: CCP4 bulletin board <CCP4BB@JISCMAIL.AC.UK<mailto:CCP4BB@JISCMAIL.AC.UK>> 
on behalf of Jeffrey B Bonanno 
<jeffrey.bona...@einsteinmed.org<mailto:jeffrey.bona...@einsteinmed.org>>
Sent: Wednesday, July 15, 2020 12:36 PM
To: CCP4BB@JISCMAIL.AC.UK<mailto:CCP4BB@JISCMAIL.AC.UK> 
<CCP4BB@JISCMAIL.AC.UK<mailto:CCP4BB@JISCMAIL.AC.UK>>
Subject: Re: [ccp4bb] Quote source inquiry

Hi Gerard and Bernhard,

As a postdoc in an unnamed small molecule lab, I was instructed by my lab head 
to get better unit cell estimates prior to data collection owing to error 
propagation from the uncertainty on cell dimensions through to the esd on 
atomic bond lengths and angles when refining in shelxl. To verify this (what, 
you believed everything your postdoc advisor told you?), I took a working 
dataset and increased (only) the error on unit cell dimensions in the 
instruction file for the final round of full matrix least squares refinement in 
shelxl. Sure enough, the errors on the bonds and angles shot up. I was more 
careful in determining the unit cell thereafter. That is, until, I became a 
macromolecular crystallographer...

After an inciteful (sp? lol) discussion with Wladek about cell dimensions, I 
was directed to read this paper:

Acta Crystallogr D Biol Crystallogr. 2015 Nov 1; 71(Pt 11): 2217-2226.

Have a look, it is interesting.

Having never followed up on these studies to see what happened to bonds and 
angles in proteins and their ligands when varying cell dimensions, I can't say 
with any confidence. However, I would guess that the quality of the refined 
ligand coordinates could only be as good as some combination of factors 
including but not limited to 1) the data (resolution, B factor, etc), 2) the 
actual occupancy of the ligand, and 3) the restraints employed.

jbb

Jeffrey B. Bonanno, Ph.D.
Department of Biochemistry
Albert Einstein College of Medicine
1300 Morris Park Avenue
Bronx, NY 10461
off. 718-430-2452 fax. 718-430-8565
email jeffrey.bona...@einsteinmed.org<mailto:jeffrey.bona...@einsteinmed.org>


-----Original Message-----
From: CCP4 bulletin board <CCP4BB@JISCMAIL.AC.UK<mailto:CCP4BB@JISCMAIL.AC.UK>> 
On Behalf Of Gerard DVD Kleywegt
Sent: Wednesday, July 15, 2020 11:49 AM
To: CCP4BB@JISCMAIL.AC.UK<mailto:CCP4BB@JISCMAIL.AC.UK>
Subject: Re: [ccp4bb] Quote source inquiry

Well, I've had this in my CSHL X-ray Course talk for many years.

In the attached 2007 Acta D paper it says (p 95): "Macromolecular X-ray 
crystallography is a notoriously poor method for determining the structure of 
small molecules that are bound to macromolecules [...]" and then goes on to 
explain why this is the case.

In the attached 2003 paper (pooling the wisdom of several of the usual 
suspects, including Eleanor) it says something similar (p 1057):

"Coordinates of molecules that have been determined in complex with 
macromolecules previously can of course also be retrieved from the PDB 
(Bernstein et al., 1977; Berman et al., 2000), HIC-Up (Kleywegt and Jones, 
1998), or CHEMPDB (Boutselakis et al., 2003). However, one should keep in mind 
that these coordinates are the result of refinement against comparatively
low-resolu- tion data where the small molecule constituted only a minute 
fraction of the total scattering matter. This makes these coordinates 
inherently much less accurate than those obtained from the CSD. In addition, 
the coordi- nates may contain errors due to the use of incorrect restraints.
Hence, such coordinate sets should only be used as a last resort, and only 
after verification that they are reliable. The latter can be facilitated by 
inspection of the electron density for the compound in question, for instance 
at the Uppsala Electron-Density Server (http:// fsrv1.bmc.uu.se/eds) (G.J.K.
et al., submitted)."

Happy to be confused with George though!

--Gerard (no, the other one)



On Tue, 14 Jul 2020, Bernhard Rupp wrote:

> Hi Fellows,
>
>
>
> afaicrimps (as far as I can recall in my progressing senility)
> someone once wrote/stated/cursed somewhere that "Macromolecular
> refinement is not a small molecule structure determination method".
>
>
>
> Any citable source - George Sheldrick might be a suspect.
>
>
>
> Thanks & best regards, BR
>
>
>
> ------------------------------------------------------
>
> Bernhard Rupp
>
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Best wishes,

--Gerard

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