Thanks Mark, message noted:)
-Original Message-
From: gmx-users-boun...@gromacs.org
[mailto:gmx-users-boun...@gromacs.org] On Behalf Of Mark Abraham
Sent: Sunday, December 26, 2010 6:03 PM
To: Discussion list for GROMACS users
Subject: Re: [gmx-users] Replicating an experiment
On 26/12/20
Poojari, Chetan wrote:
Hi,
I am working on membrane protein.
In umbrella sampling tutorial...we saw the pulling of the peptide A away
from peptide B.
I want to pull the peptide deep into the hydrophobic core of the bilayer from
outside (solvent environment).
Please can someone suggest
Poojari, Chetan wrote:
Hi Mark,
I ran on 48 processors.the error is:
The X-size of the box (5.312040) times the triclinic skew factor (1.00)
is smaller than the number of DD cells (6) times the smallest allowed cell
size (0.885281)
I would say this further confirms Mark's suspicion
Hi Mark,
I ran on 48 processors.the error is:
The X-size of the box (5.312040) times the triclinic skew factor (1.00) is
smaller than the number of DD cells (6) times the smallest allowed cell size
(0.885281)
Kind regards,
chetan
From: gmx-us
On 26/12/2010 10:07 PM, gromacs564 wrote:
Hi all
I downloaded topolbuild1_3 from the GROMACS website,
and I run the command as follows:
"path: home/buct/topolbuild1_3 ??
# tar -xvf topolbuild1_3.tgz
#make -f Makefile ; (intel CPU) there were no a
On 27/12/2010 7:51 AM, Poojari, Chetan wrote:
Hi,
I am following umbrella sampling tutorial for my membrane protein system.
While running continuous pulling simulation (mdrun). under step five:
Generating Configurations of the tutorial. I get the below error.
The system ran initially but
On 27/12/2010 9:22 AM, WU Yanbin wrote:
Hi, Mark,
Thanks for the reply.
As suggested, I tried a "water in vacuum" case. Initially the water
droplet is a cubic 4nm-by-4nm-by-4nm water box, located in the middle
of the simulation box. Everywhere else is just vacuum. The simulation
box size is
Hi,
I am working on membrane protein.
In umbrella sampling tutorial...we saw the pulling of the peptide A away
from peptide B.
I want to pull the peptide deep into the hydrophobic core of the bilayer from
outside (solvent environment).
Please can someone suggest me how to go about this.
Hi,
To my earlier post on number of DD cells.i included -dds 0.6 and everything
seems to run fine.
Is this the possible solution to the error or is there other way to handle this
warning ?
Kind regards,
chetan.
---
Hi, Mark,
Thanks for the reply.
As suggested, I tried a "water in vacuum" case. Initially the water droplet
is a cubic 4nm-by-4nm-by-4nm water box, located in the middle of the
simulation box. Everywhere else is just vacuum. The simulation box size is
8nm by 8nm by 8nm. SPC/E model is used to des
Hi,
I am following umbrella sampling tutorial for my membrane protein system.
While running continuous pulling simulation (mdrun). under step five:
Generating Configurations of the tutorial. I get the below error.
The system ran initially but corrupted very soon with warning " The X-size of
>
> On Sun, Dec 26, 2010 at 12:28 AM, sreelakshmi ramesh <
> sree.laks...@research.iiit.ac.in> wrote:
>
>> Dear users,
>> I did nvt equil and after that npt equilbriation and i am
>> using parinello rahman as the barostat but the prob is even after 200 ps of
>> equil the avg pressu
Hi Xiaodu,
The fudgeLJ under defaults should be 1.0 for GLYCAM. I'm unable to check my
own files right now so can't compare. When you run grompp check in the
output that fudge is set to 1.0. So there will be no protein in your
simulation correct? I think there is a way to do mixed scaling in groma
Hi,
what is the standard deviation and drift? Are you sure this is a significant
difference to 1?
Roland
On Sun, Dec 26, 2010 at 12:28 AM, sreelakshmi ramesh <
sree.laks...@research.iiit.ac.in> wrote:
> Dear users,
> I did nvt equil and after that npt equilbriation and i am
> u
Hi all
I downloaded topolbuild1_3 from the GROMACS website,
and I run the command as follows:
"path: home/buct/topolbuild1_3 ”
# tar -xvf topolbuild1_3.tgz
#make -f Makefile ; (intel CPU) there were no any error messages.
then I wr
Hi all
I downloaded topolbuild1_3 from the GROMACS website,
and I run the command as follows:
"path: home/buct/topolbuild1_3 ”
# tar -xvf topolbuild1_3.tgz
#make -f Makefile ; (intel CPU) there were no any error messages.
then I wri
On 26/12/2010 4:37 AM, NG HUI WEN wrote:
Thank you David for your prompt and useful reply :) I am in fact simulating a
membrane protein.
It's good to know I can use the "generate-new-starting-velocity" method. But, do you mind
to elaborate a bit more what you mean by "if you simulate long eno
Hello Shikha
Replace NA+ with NA in your topol.top file.
It will solve the problem as it recognise NA for NA+.
Thanks
Yuvraj
IIIT Hyderabad
On Sun, Dec 26, 2010 at 12:26 PM, wrote:
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