Dear Justin
Thanks for your quick reply.
I was confused.
If I add #include "ffcntbon.itp" after #include "cnt.itp" in .top file,
my problem was solved and error was solved?
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Dear Justin
Thanks for your reply.
> In your previous setup, you were effectively trying to use CHARMM27 + some
> other
> force field related to the CNT. You can't do that.
Thus, Gromacs is not appropriate for systems containing cnt.
Is my deduction true?
In my case, peptid + cnt + water mole
Dear Justin
My cnt is infinite.
I obtained cnt.top by g_x2top and then modified cnt.top to cnt.itp.
For obtaining cnt.top, I used following files:
---
ffcnt.atp:
CA 12.01100 ; aromatic C
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Dear Justin
Very thanks for your reply.
I created a new topol.top file as below:
1) I used once default directive.
2) I put cnt.itp file in working directory.
3) I copied pr.top and renamed it to topol.top. I added #include "cnt.itp"
in the end of topol.top file. I modified [ molecules ] direc
Dear all
My system contains protein + cnt + water molecules.
I have summarized what I did below:
---
1) By pdb2gmx and charmm27 force field, I obtained pr.top for protein then
I converted it into pr.itp by deleting
Dear gromacs usres
I am doing simulation of lipid bilayer.
I did 2 steps: 1) energy minimization, 2) equilibration.
Before production run, I want to monitor dimensions of the simulation cell
to test the stability of the simulation.
On the other hands, I want to plot dimensions of the simulation
Dear Justin
Thanks for your reply.
Ok. You are right. There is no "time" during EM.
For example, if I use nstep = 10,000 and emstep = 0.01,
what means of Step size in this case, exactly?
Please give me more explanation.
Best wishes for you.
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Dear gromacs users
What is the reason of this point that
unit of the emstep (step size)is nm?
I think ps (unit of time) is more resonable.
If I am wrong, please give me explanation about this point.
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Dear gromacs users
Why should I install fftw before gromacs installation?
I want to know exact role of fftw in gromacs calculations.
Please guide me about that.
Best wishes
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Dear gromacs users
I want to use LAMBADA and InflateGRO2 to create a system containing
dopc lipid + cholesterol + drug.
When I use
~/lib/lambada/lambada_rc1/lambada -f1 drug.gro -f2 lipid_chol.gro
I encountered with
Illegal division by zero at /home/karami/lib/lambada/
lambada_rc1/lambada line
Dear Baptiste
Very thanks for your reply.
Unfortunately, I have not access to InflateGro2. I encountered with error.
If there are a script for InflateGro2 like InflateGro. please sent me perl
script related to InflateGro2.
Best wishes.
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Dear Justin
Thanks for your quick reply.
I want to study a system containing DOPC and cholesterol and drug.
I correctly prepared gro files and topology parameters for this system.
I did previous step (Step Two: Modify the Topology) without problem.
I have 2 problems.
1) After I use trjconv -
Dear Justin
I do your tutorial entitled " KALP15 in DPPC ".
In Step Three: Defining the Unit Cell & Adding Solvent,
You said "Use trjconv to remove periodicity ".
When I use trjconv -s em.tpr -f dppc128.gro -o dppc128_whole.gro -pbc mol
-ur compact,
gromacs tell me: Select group for output.
Wh
Hi all.
After using amber03 force field for protein-ligand simulation (pdb2gmx), I
encountered with following error:
Fatal error:
In the chosen force field there is no residue type for 'GLN' as a starting
terminus.
Ligand in my system is a single residue (GLN). There are [GLN], [NGLN] and
[CGLN]
Dear all
I have a question about g_analysis with option -ee.
What is difference between RMS fluctuations and error estimate obtained
from block averaging?
Best regards
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Dear Lina
Very thanks for your time and attention.
Initial command was : g_dist -f *.trr -s *.tpr -n *.ndx -o dist.xvg -dist 0.5
After running following command the problem was solved :
g_dist -f *.trr -s *.tpr -n *.ndx -o dist.xvg -dist 5
t: 17008 6773 NA 21881 NA 3.05534 (nm)
t: 17008 677
Dear Lina
There is not any things related to list of atoms on the terminal.
Best regards
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Pleas
Dear Lina
Thanks for your reply.
Without the -dist 0.5, I get the -o dist.xvg output, but I need list
of the all atoms in group 2 closer than dist to the center of mass of
group 1.
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Dear gromacs users
I read g_spatial tool of gromacs 4.5 manual. I have many questions.
There are in the manual:
USAGE:
1. Use make ndx to create a group containing the atoms around which
you want the SDF
2. trjconv -s a.tpr -f a.xtc -o b.xtc -center tric -ur compact -pbc none
3. trjconv -s a.tpr
Dear all
When I use g_dist -f *.trr -s *.tpr -n *.ndx -o dist.xvg -dist 0.5,
program was done without error, but it don't create output file
(dist.xvg) in the directory in which g_dist tool was run.
What is reason of this case?
Any help will highly appreciated.
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Dear Justin
thanks for your attention
I deleted posre.itp file which pdb2gmx was created (containing all solute).I
made a posre.itp (containing only protein) by genrestr.
now if I use define = -DPOSRES, gromacs use from my posre.itp. is it true?
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I want to use define = -DPOSRES_Protein_chain_A for step 1.
is it true?
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Dear Mark
thanks for your reply
you said "if pdb2gmx is able to treat the whole system in one pass, then it
will write such position restraint
files automatically"
in my system, what pdb2gmx includes are in below:
; Include forcefield parameters
#include "amber03.ff/forcefield.itp"
; Include c
Dear all
my system contains protein + ligand+ water molecules.
protein + ligand = solute
water molecules = solvent
I want to do minimization energy in 3 steps :
step 1) on protein only
step 2) on all solute (protein + ligand)
step 3) on all system
should I use position restrained minimizati
Dear gromacs users
in gromacs manual, there is [-a real 30 Cutoff angle (degrees, Acceptor -
Donor - Hydrogen)
-r real 0.35 Cutoff radius (nm, X - Acceptor, see next option)]
I think that in hb (D-H...A) distance of 0.35 nm = distance between D and A.
and angle of 30 = acceptor-donor–hydrogen an
Dear Ran
thanks for your reply.
Is psfgen a separately program?
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Dear gromacs users
I did simulation of protein-ligand by gromacs 4.0.7 with amber 03
forcefield.
I need to .psf and .dcd files. can I convert/obtain them?
any help will highly appreciated.
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Dear Justin
I used g_dist -f .xtc -s .tpr -n .ndx -o -lt -dist 1
but program give me only lifetime.xvg. there are no dist.xvg file. why?
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Dear Justin
are you sure g_dist -dist give me what I need. if so, how?
since, dist.xvg gives distance vs time and lifetime.xvg gives number of
contact vs time. while, I want number of water molecules (interfacial) to be
within 2.4 A distance from both the protein and the ligand during
simulation.
Dear Mark and gromacs users
thanks for your time and attention.
how to make selection.dat file? what should be in that?
please clarify this new tool more. how can I obtain what I need (number of
water molecules (interfacial) to be within
2.4 A distance from both the protein and the ligand durin
Dear all
my system includes protein, ligand and water.
I want to obtain number of water molecules (interfacial) to be within 2.4 A
distance from both the protein and the ligand during simulation. also, exact
numeration of each water being in interface between protein and ligand.
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Dear Justin
count = count of hydrogen bonds being in a certain distance (between
0-0.35) and angle (between 0-30)?
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Dear Justin
very thanks for your attention.
I have another question about g_hbond. in manual, -dist and -ang are distance
and angle distribution of all hydrogen bonds respectively. I want to know in
hbang and hbdist.xvg file, what is y-axis label?
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Dear Justin
I confused.
number of donors in donor.xvg file is 203. while, when use g_hbond: found
143 donors.
Select a group: 2
Selected 2: 'Protein_A'
Select a group: 3
Selected 3: 'Protein_B'
Checking for overlap in atoms between Protein_A and Protein_B
Calculating hydrogen bonds between Prote
Hi all
I want to know regarding 2nd and 3rd column of donor.xvg output about
g_hbond -don.
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Dear Justin
Header of file is as follow:
@title "Donor properties"
@xaxis label "Time (ps)"
@yaxis label "Number"
@TYPE xy
@ view 0.15, 0.15, 0.75, 0.85
@ legend on
@ legend box on
@ legend loctype view
@ legend 0.78, 0.8
@ legend length 2
@ s0 legend "Nbound"
@ s1
Dear gromacs users
my simulation time is 10 ns (1 ps), but, I want to use last 4ns for
analysis.
for example, if I use g_rms -b 6000 -e 1 -o rmsd.xvg, in xvg output
file, rmsd plotted versus time (from 6000 to 1 ps in horizontal axis).
while I want horizontal axis be from 0 to 4000 ps
Hi gmx users
Perhaps, this question be repetitive. I want to know using trjconv -pbc is
only a solution for visualization problem? Is there
feasibility to use old trajectory file (with out trjconv -pbc) for any kind
of analysis without any problem?
--
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Ph.D. student of BioPhysical
*Dear Justin*
**
*I read manual and specially g_hbond. but manual doesn't gime me information
about * residence time of water molecule and life time of hydrogen.
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htt
Hi gromacs users
I am beginner in gromacs. I did md simulation of a protein by gromacs and
now
I want to obtain residence time of water molecule and life time of hydrogen
bonds. Can I obtain both of them using gromacs?
please guide me by detail.
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Hi gromacs users
after simulation of protein-ligand, in analysis section, how to obtain
contact map for protein-ligand?
thanks in advance.
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Hi
how to obtain residence time of water molecule using md simulation and
gromacs?
What is the best way to do this? Please suggest.
-- atila
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