First port of call for a question like this should be a search engine
http://en.wikipedia.org/wiki/Angstrom
Catch ya,
Dr. Dallas Warren
Drug Discovery Biology
Monash Institute of Pharmaceutical Sciences, Monash University
381 Royal Parade, Parkville VIC 3052
dallas.war...@monash.edu
+61 3 9
Dear Sir
I have to query as to how do we convert the paramaters in "nm" to Å
--. For example the RMSD and RMSF calculation gives result in "nm". I want
to convert
it to Å. I request you to kindly guide me with the process
Thanking You with Regards.
Arunima Shilpi
Ph. D Research Scholar(Cancer
What about OHN - the hydroxyl radical? I put two of them in the system to
understand the issue. Under DNA_chain_X, you clearly see nr=2 for OHN. If I
take one OHN out from pdb (means one DTMP, one OHN and water), I again get
nr=1 for OHN.
residue (2):
> residue[0]={name="DTMP", nr=1, ic=' '}
Peak can be higher, but if it is narrower the total area can still be less.
Remember it is an area under the curve. Additionally, that overall system /
box density that you are using may be different too, so that will make a
difference.
Catch ya,
Dr. Dallas Warren
Drug Discovery Biology
Mona
residue is a sub-field of moltype, so you are seeing that there is
indeed one SOL residue per water molecule, as expected. Look elsewhere
and you will see that there are 351 of those molecules recorded. The
same is true of the DNA chain, but since there's only one DNA chain,
the number of residues
Hi,
I am using v-4.5.5. I have a system of DNA nucleotide & *two* OH radicals
solvated in water.
The topology file has the following records in the end:
[ molecules ]
; Compound#mols
DNA_chain_X 1
SOL351
However, when I did gmxdump after running grompp, I s
Hi, Rajat-
We are working on ways to make the workshop materials available
online, either streaming or posted afterwards. The tutorials will
have online components as well. We were unable to obtain travel
funding for the conference this year, unfortunately!
> I would be willing to pay the whole
On 8/20/13 9:59 AM, Shima Arasteh wrote:
Hi,
I have a tpr-files.dat containing 5 tpr files as it:
4.tpr
5.tpr
6.tpr
7.tpr
8.tpr
Also the pullf-files.dat is in accordance with tpr-files.dat.
But when I run g_wham and visualize the histo output, I see only one curve and
not 4 curves which a
Hi,
I have a tpr-files.dat containing 5 tpr files as it:
4.tpr
5.tpr
6.tpr
7.tpr
8.tpr
Also the pullf-files.dat is in accordance with tpr-files.dat.
But when I run g_wham and visualize the histo output, I see only one curve and
not 4 curves which are expected to have appropriate overlaps! Wou
On 8/20/13 5:52 AM, grita wrote:
Dear Dwey & Justin,
I've not tried it yet and I've asked because in the 4.5.x GPU version of
Gromacs not all features were supported.
In my simulations I'm using the SD integrator and the Pull-Code.
Since both are supported in the current GPU version, I will
Dear Dwey & Justin,
I've not tried it yet and I've asked because in the 4.5.x GPU version of
Gromacs not all features were supported.
In my simulations I'm using the SD integrator and the Pull-Code.
Since both are supported in the current GPU version, I will try it on a
computer with a CUDA grap
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