[Chimera-users] Fwd: Double coordinates for same residue

Francesco Pietra chiendarret at gmail.com
Thu Sep 15 10:10:57 PDT 2011


On Thu, Sep 15, 2011 at 6:23 PM, Elaine Meng <meng at cgl.ucsf.edu> wrote:
> Well, that is a more philosophical question that you will have to decide for yourself.
>
> There are also occupancy values (the column after the coordinates).  In many cases it is reasonable to just delete the alternate positions with the lower occupancies.  In your example A and B are equally strong (both 0.50), so one possibility is to just use one set and delete the others. For example, to delete all alternate locations B:
>
> delete @.b
>
> Another possibility is to make multiple models using the different locations.

If there are no criteria of preference, when many residues present
alternate atom locations, as in this case, the number of possible
combinations should deter anyone from going on. I would like to see
examples of classical MD carried out with proteins of such features.
If one is interested in ligand paths inside the protein, alternate
positions of side chains are not encouraging. 1.9A resolution is
excellent work, which might mean that this set of coordinates is not
what one can safely use for MD for that use, not to say if one is
interested in energies. Perhaps the collection of reflections was not
at low temp.
francesco

>
> A structure with alternate locations may often be quite high resolution and high quality, so my personal opinion is you wouldn't want to throw the whole structure away just because you aren't sure what to do with these data.
> Elaine
>
> On Sep 15, 2011, at 9:14 AM, Francesco Pietra wrote:
>
>> Addendum: I am aware about "alternate positions", what I don't know is
>> how to treat such a protein, or whether it should be better to abandon
>> modeling it. I have no idea which alternate position should be better
>> deleted.
>> francesco pietra
>>
>>
>> ---------- Forwarded message ----------
>> From: Francesco Pietra <chiendarret at gmail.com>
>> Date: Thu, Sep 15, 2011 at 5:31 PM
>> Subject: Double coordinates for same residue
>> To: chimera <chimera-users at cgl.ucsf.edu>
>>
>>
>> Hello:
>>
>> Surely a naive question: While beginning to treat a multichain,
>> engineered protein - downloaded from PDB web (1.94 A resolution) -
>> with Chimera, I noticed that many amino acids have such feature as GLU
>> 252 below. Same for many SER, ILE, HIS (two imidazole rings for the
>> same residue number)
>>
>> ATOM   2022  N   GLU A 252      15.171 -45.532  45.115  1.00 26.12           N
>> ATOM   2023  CA AGLU A 252      14.023 -44.631  45.214  0.50 26.30           C
>> ATOM   2024  CA BGLU A 252      14.048 -44.592  45.252  0.50 26.30           C
>> ATOM   2025  C   GLU A 252      13.983 -43.654  44.050  1.00 25.90           C
>> ATOM   2026  O   GLU A 252      12.894 -43.403  43.470  1.00 25.36           O
>> ATOM   2027  CB AGLU A 252      13.974 -43.909  46.559  0.50 26.93           C
>> ATOM   2028  CB BGLU A 252      14.170 -43.759  46.533  0.50 26.77           C
>> ATOM   2029  CG AGLU A 252      13.283 -44.741  47.629  0.50 29.02           C
>> ATOM   2030  CG BGLU A 252      12.874 -43.673  47.313  0.50 29.14           C
>> ATOM   2031  CD AGLU A 252      14.088 -45.948  48.051  0.50 33.10           C
>> ATOM   2032  CD BGLU A 252      12.806 -44.716  48.426  0.50 31.91           C
>> ATOM   2033  OE1AGLU A 252      13.481 -47.014  48.330  0.50 34.82           O
>> ATOM   2034  OE1BGLU A 252      13.394 -44.454  49.504  0.50 31.18           O
>> ATOM   2035  OE2AGLU A 252      15.333 -45.828  48.101  0.50 35.49           O
>> ATOM   2036  OE2BGLU A 252      12.162 -45.782  48.231  0.50 33.14           O
>> ATOM   2037  N   GLU A 253      15.141 -43.133  43.683  1.00 24.58           N
>> ATOM   2038  CA  GLU A 253      15.225 -42.212  42.559  1.00 25.11           C
>> ATOM   2039  C   GLU A 253      14.838 -42.941  41.242  1.00 23.83           C
>> ATOM   2040  O   GLU A 253      14.142 -42.383  40.374  1.00 23.54           O
>> ATOM   2041  CB  GLU A 253      16.637 -41.603  42.476  1.00 26.18           C
>> ATOM   2042  CG  GLU A 253      17.033 -40.722  43.697  1.00 30.81           C
>> ATOM   2043  CD  GLU A 253      17.635 -41.491  44.915  1.00 36.16           C
>> ATOM   2044  OE1 GLU A 253      17.540 -42.742  45.032  1.00 35.80           O
>> ATOM   2045  OE2 GLU A 253      18.198 -40.809  45.801  1.00 40.87           O
>>
>> About the protein:
>> SOURCE   2 ORGANISM_SCIENTIFIC: PSEUDOMONAS MENDOCINA;
>> SOURCE   3 ORGANISM_TAXID: 300;
>> SOURCE   4 GENE: TMOA;
>> SOURCE   5 EXPRESSION_SYSTEM: ESCHERICHIA COLI;
>> SOURCE   6 EXPRESSION_SYSTEM_TAXID: 562;
>> SOURCE   7 EXPRESSION_SYSTEM_STRAIN: BL21;
>> SOURCE   8 EXPRESSION_SYSTEM_VECTOR_TYPE: PLASMID;
>> SOURCE   9 EXPRESSION_SYSTEM_PLASMID: P58KABE;
>>
>> The said residue are not among those not located in the experiment.
>>
>> I am interested in channels, pores and so on in the protein, so that
>> the above issue is of most concern for me.
>>
>> Thanks for aid
>>
>> francesco pietra
>>
>> _______________________________________________
>> Chimera-users mailing list
>> Chimera-users at cgl.ucsf.edu
>> http://plato.cgl.ucsf.edu/mailman/listinfo/chimera-users
>>
>
>




More information about the Chimera-users mailing list