Dear All,
I am planning to perform a QM/MM calculation of my protein system. Can
anybody suggest me whether gromacs-4.5.5 can be patched with any latest
version of CPMD? If not, then please suggest me some combination of the
gromacs-cpmd versions.
I came across this tutorial, but there, both groma
Dear All,
I am planning to perform a QM/MM calculation of my protein system. Can
anybody suggest me whether gromacs-4.5.5 can be patched with any latest
version of CPMD? If not, then please suggest me some combination of the
gromacs-cpmd versions.
I came across this tutorial, but there, both groma
k
On Thu, Aug 1, 2013 at 5:07 PM, Mark Abraham wrote:
> http://www.gromacs.org/Documentation/How-tos/Single-Point_Energy
>
> On Thu, Aug 1, 2013 at 7:03 AM, tarak karmakar
> wrote:
> > Dear All,
> >
> > Can anyone guide me how to perform the 'potential energy sc
Dear All,
Can anyone guide me how to perform the 'potential energy scan' for a
dihedral of a small molecule in gromacs?
Regrads,
Tarak
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gmx-users mailing listgmx-users@gromacs.org
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http://www.gromacs.org/Sup
raham wrote:
> Your call. Is that motion significant to what you are trying to report
> by your observation of the RMSD?
>
> Mark
>
> On Thu, Jun 27, 2013 at 9:03 AM, tarak karmakar
> wrote:
> > Dear All,
> >
> > While simulating a protein, I see the rmsd
Dear All,
While simulating a protein, I see the rmsd fluctuates around a mean of 0.6
nm. I carefully looked at the trajectory (VMD movie) and saw there are two
flexible terminii fluctuating with a very high amplitude contributing to
the high value of RMSD. Is it ok to report this problem with this
>
> On 6/4/13 12:51 PM, tarak karmakar wrote:
>
>> Yeah!
>> It is indeed a silly point to generate a velocity distribution at 0 K. (
>> Maxwell-Boltzmann will be in trouble)
>> After the warm up, now let say my protein is in 300 K, can't I generate a
>>
73529 ) during my production run?
Thanks,
Tarak
On Tue, Jun 4, 2013 at 10:10 PM, Justin Lemkul wrote:
>
>
> On 6/4/13 12:17 PM, tarak karmakar wrote:
>
>> Thanks Justin.
>> Sorry for not uploading the full .mdp. Here it is,
>>
>> ; 7.3.3 Run Control
I'm extremely sorry for copying the other '.mdp' file here. This is the
modified one I just created after seeing your reply. In the previous case I
didn't use 'continuation'.
On Tue, Jun 4, 2013 at 9:47 PM, tarak karmakar wrote:
> Thanks Justin.
> Sorry for
ngs of how ligand is interacting with
certain residues.
So, then should I use these different velocity generating seeds during the
warm up step?
Thanks,
Tarak
On Tue, Jun 4, 2013 at 5:46 PM, Justin Lemkul wrote:
>
>
> On 6/4/13 8:07 AM, tarak karmakar wrote:
>
>> Dear All,
&g
Dear All,
Although I have set gen_temp = 300, it is showing the initial temperature
445.7 K, generated at the very beginning of the run.
gen_vel = yes ; velocity generation
gen_temp= 300
gen_seed= 93873959697
Is it because of a bad geo
All these parameters are for Mg2+, forgot to mention.
On Fri, May 31, 2013 at 10:48 PM, tarak karmakar wrote:
> Dear All,
>
> I have a little confusion with the non-bonding parameters conversion from
> OPLS-AA to CHARMM in gromacs.
> If I see the ffnonbonded.itp in both the
Dear All,
I have a little confusion with the non-bonding parameters conversion from
OPLS-AA to CHARMM in gromacs.
If I see the ffnonbonded.itp in both the cases I get the following numbers
OPLS-GROMACS
Sigma = 0.1644471 nm
Epsilon = (0.875044*4.184) = 3.66118 kJ/mol
Dear All,
It seems the problem in the cut-off schemes while using charmm force
field in gromacs persists even in the latest gromacs-4.6.1 version.
Recently I have posted regarding this problem came in gromacs-4.5.5
version. If anybody has already tested this issue in the latest version,
please
his mail went to you twice. Facing lot of problems,
here, in mail delivery failure.
Thanks,
Tarak
On Fri, May 17, 2013 at 6:22 PM, tarak karmakar wrote:
> @ Justin and Mark,
>
> Do you have any idea about the rlist used by Bjelkmar et. al.
> 'Implementation of charmm in gromacs
y 17, 2013 at 5:42 PM, tarak karmakar wrote:
> I am extremely sorry for spaming the mail box. It was quite
> unintentionally. Believe me I was getting the following error every
> time while sending the mail.
>
> Final-Recipient: rfc822; jaanus.k...@eesti.ee
> Action: failed
>
...@eesti.ee
Tarak
-- Forwarded message --
From: tarak karmakar
To: Discussion list for GROMACS users
Cc:
Date: Fri, 17 May 2013 15:50:25 +0530
Subject: Re: [gmx-users] Inconsistent results in different clusters and cores
On Fri, May 17, 2013 at 5:36 PM, Mark Abraham wrote:
>
I have read the 'implementation of charmm in gromacs' by bjelkmar,
JCTC. There they have used following cut-offs
coulombtype=PME
rcoulomb=1.2
vdwtype=switch
rvdw=1.2
rvdw-switch=1.0
I am not sure about rlist.
Regards,
Tarak
On Fri, May 17, 2013 at 1:46 PM, tarak karmakar wrote:
Dear All,
I have read the 'implementation of charmm in gromacs' by bjelkmar,
JCTC. There they have used following cut-offs
coulombtype=PME
rcoulomb=1.2
vdwtype=switch
rvdw=1.2
rvdw-switch=1.0
If I use the same numbers with rlist=1.2 it is showing warning saying
rlist should be at lear 0.1 - 0.3 n
Dear All,
I'm using charmm force field for simulation of a protein ligand system.
I have read the paper "implementation of charmm in gromacs by Bjelkmar,
JCTC'
They have used the following set up
coulombtype = PME
rcoulomb= 1.2
vdwtype = switch
rvdw
Dear All,
I'm using charmm force field for simulation of a protein ligand system.
I have read the paper "implementation of charmm in gromacs by Bjelkmar,
JCTC'
They have used the following set up
coulombtype = PME
rcoulomb= 1.2
vdwtype = switch
rvdw
Dear All,
I'm using charmm force field for simulation of a protein ligand system.
I have read the paper "implementation of charmm in gromacs by Bjelkmar,
JCTC'
They have used the following set up
coulombtype = PME
rcoulomb= 1.2
vdwtype = switch
rvdw
Dear All,
I'm using charmm force field for simulation of a protein ligand system.
I have read the paper "implementation of charmm in gromacs by Bjelkmar,
JCTC'
They have used the following set up
coulombtype = PME
rcoulomb= 1.2
vdwtype = switch
rvdw
Dear All,
I'm using charmm force field for simulation of a protein ligand system.
I have read the paper "implementation of charmm in gromacs by Bjelkmar,
JCTC'
They have used the following set up
coulombtype = PME
rcoulomb= 1.2
vdwtype = switch
rvdw
Dear All,
I'm using charmm force field for simulation of a protein ligand system.
I have read the paper "implementation of charmm in gromacs by Bjelkmar,
JCTC'
They have used the following set up
coulombtype = PME
rcoulomb= 1.2
vdwtype = switch
rvdw
hanks,
Tarak
On Fri, May 17, 2013 at 1:34 PM, tarak karmakar wrote:
> What about Dispersion Correction ?
> But if I use this set of informations
>
> ; 7.3.3 Run Control
> integrator = md; md integrator
> tinit = 0
n Sun, May 12, 2013 at 11:57 PM, tarak karmakar wrote:
> Oh !
> Thanks a lot Justin. I'll rerun all my jobs with this corrected mdp.
> Restrains things I didn't follow properly, anyway I'll read about this.
>
>
> On Sun, May 12, 2013 at 11:27 PM, Justin Lemku
Dear All,
How do I incorporate the 1-4 scaling factor ( e.g., 1.0 for CHARMM and
0.833 in AMBER) in gromacs? Or, is it internally taken care of by gromacs
while specifying the -ff flag?
NAMD input file uses the following keyword
1-4scaling 1.0 (for charmm force field)
Thanks,
Tara
xas at Austin
> Department of Chemistry and Biochemistry
> The Webb Group
>
>
> On Mon, May 13, 2013 at 7:04 AM, tarak karmakar >wrote:
>
> > Dear All,
> >
> > I am running a simulation of ligand binding in a protein. Ligand is
> > mostly negative
Dear All,
I am running a simulation of ligand binding in a protein. Ligand is
mostly negatively charged, so as expected it should bind to the positive
region of the protein. To check the possible binding zone, I try to
calculate or rather visualize the electrostatic potential map of a protein
Oh !
Thanks a lot Justin. I'll rerun all my jobs with this corrected mdp.
Restrains things I didn't follow properly, anyway I'll read about this.
On Sun, May 12, 2013 at 11:27 PM, Justin Lemkul wrote:
>
>
> On 5/12/13 1:53 PM, tarak karmakar wrote:
>
>> Thank
lincs_warnangle = 30
On Sun, May 12, 2013 at 11:11 PM, Justin Lemkul wrote:
>
>
> On 5/12/13 1:34 PM, tarak karmakar wrote:
>
>> Thanks Justin for the Quick and Helpful reply.
>>
>> Yes. If I am right, the chaotic behavior of the simulations is
>
Remove all the hydrogens from the pdb file and then try to run pdb2gmx, I
hope it'll do fine.
Or you can also use -ignh option as suggested by Justin.
Tarak
On Fri, May 10, 2013 at 3:35 PM, Justin Lemkul wrote:
>
>
> On 5/10/13 5:16 AM, Jernej Zidar wrote:
>
>> Hi,
>>In CHARMM I generated
rote:
>
>
> On 5/12/13 1:17 PM, tarak karmakar wrote:
>
>> Dear All,
>>
>> I am simulating a protein in water to check the ligand movement
>> over a
>> time span. I haveminimized the system in STEEP and CG and after that
>> heated from
Dear All,
I am simulating a protein in water to check the ligand movement over a
time span. I haveminimized the system in STEEP and CG and after that
heated from 0K - 300K within a time span of 300 ps. Then, I performed the
NPT production runs. In two clusters I have got different results
g/Support/Mailing_Lists
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> * Can't post? Read http://www.grom
Dear All,
During a simulation of a protein with a ligand, I see the -NH3 of the
lysine side chain near the ligand is getting squeezed for a very short
time; N-H bonds are getting contracted and the angle are no longer within
tetrahedral normal http://lists.gromacs.org/pipermail/gmx-users/2010-Nov
Thanks Dr. Vitaly
Yeap !
>From that point of view I'm seeing the correct temperature drift and
it reaches nicely to 300 K after say, 300ps.
But is it a good integrator ( SD ) to perform this job ? Or, should I
opt for other, like Lep-frog or MD-VV with let say , Berendsen
thermostat?
Please expla
Thanks Justin
Yah! We can run steered MD or Umbrella Pulling ( sampling) for this
purpose. But one thing I am wondering that how to move the entire
complex. In my model there are no covalent bond ( bonding info)
between the metal and ligands. So how to select a particular point in
the complex to t
Dear All,
I have copied and patched the plumed script plumed_gromacs-4.5.5.sh,
given in the patches directory. But after doing that, while running
some umbrella sampling it's not printing the COLVAR file, only the
simple md is running there.
So, can anyone help me in this regard?
Thanks
--
Tarak
vmd protein.trr protein.gro
then go to the representation and then write 'all not water' with
cartoon representation, u will get the protein only.
Cheers,
Tarak
On Thu, Nov 22, 2012 at 12:58 PM, rama david wrote:
> Dear,
>-o MT.PnoH.xtc instad of xtc extenstion use pdb you will get pdb file
Hi,
I was also facing the same problem. If you check your pressure during
this NPT run, u can see that it got increased to a higher value. I had
posted the same problem few days back, u can follow the thread. It
seems MTTK is not stable enough and is not performing well in this
context. So I have
> Von: gmx-users-boun...@gromacs.org [mailto:gmx-users-
>> boun...@gromacs.org] Im Auftrag von tarak karmakar
>> Gesendet: Mittwoch, 21. November 2012 15:03
>> An: Discussion list for GROMACS users
>> Betreff: Re: [gmx-users] pressure_coupling
>>
>> Thanks for
tag, 20. November 2012 18:33
>> An: Discussion list for GROMACS users
>> Betreff: Re: [gmx-users] pressure_coupling
>>
>>
>>
>> On 11/20/12 12:29 PM, tarak karmakar wrote:
>> > Thanks Justin for the quick reply.
>> > Is there any problem with the algor
parameters ?
On Tue, Nov 20, 2012 at 10:10 PM, Justin Lemkul wrote:
>
>
> On 11/20/12 11:26 AM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> I want to keep the pressure at 1.0 bar during the NPT simulation. But
>> it is fluctuating around 130 bar. So can an
thanks a lot Justin
I'll try to follow this protocol.
On Sun, Nov 11, 2012 at 8:59 AM, Justin Lemkul wrote:
>
>
> On 11/10/12 10:27 PM, tarak karmakar wrote:
>>
>> Thanks Justin
>>
>> If I want to constrain all the bonds in the substrate molecule present
Thanks Justin
If I want to constrain all the bonds in the substrate molecule present
inside the enzyme cavity then along with SHAKE what I need to use ?
On Fri, Nov 9, 2012 at 5:47 PM, Justin Lemkul wrote:
>
>
> On 11/8/12 11:36 PM, tarak karmakar wrote:
>>
>> Thanks Ju
:
Double entries in block structure. Item 5247 is in blocks 1371 and 1370
Cannot make an unambiguous inverse block.
Please suggest me the exact protocol.
Thanks
On Fri, Nov 9, 2012 at 2:18 AM, Justin Lemkul wrote:
>
>
> On 11/8/12 1:07 PM, tarak karmakar wrote:
>>
>> Dea
I'm bit confused how to implement constraints algorithm for these
type of problem.
Thanks
On Wed, Nov 7, 2012 at 11:54 PM, Justin Lemkul wrote:
>
>
> On 11/7/12 10:46 AM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> As I am facing the following problem while
Dear All,
As I am facing the following problem while using SHAKE to constrain
some bonds, I have checked the mailing list but I think, this issue
has not been resolved. So if anyone knows the solution kindly inform
me.
Program mdrun, VERSION 4.5.5
Source code file: invblock.c, line: 79
Fatal err
, 2012 at 8:26 PM, Justin Lemkul wrote:
>
>
> On 10/12/12 10:39 AM, Dr. Vitaly Chaban wrote:
>>>
>>>
>>> On 10/12/12 2:42 AM, tarak karmakar wrote:
>>>>
>>>> Dear ALL,
>>>>
>>>> In my protein I need to constr
2 at 2:01 PM, Justin Lemkul wrote:
>>
>>
>> On 10/3/12 7:49 AM, tarak karmakar wrote:
>>>
>>> Thanks Justin,
>>> Actually if I would remove the proton from the tyrosine -OH and add
>>> the corresponding charge of the Hydrogen to the phenolic oxyge
kul wrote:
>
>
> On 10/3/12 6:00 AM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> Is it possible to deal a protein with tyrosyl radical in Molecular
>> Dynamics Simulation ?? If possible can you please provide me the
>> reference or literature where I can
Thanks Mark ,
I got it now :)
On Thu, Sep 20, 2012 at 3:06 PM, Mark Abraham wrote:
> On 20/09/2012 7:31 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
>>I need to plot a specific dihedral in my protein and I have to
>> see how it is changing with
thanks a lot Mark
On Thu, Sep 20, 2012 at 12:31 PM, Mark Abraham wrote:
> On 20/09/2012 4:21 PM, tarak karmakar wrote:
>>
>> Thanks Mark.
>> I was using the following command as I got it in the manual.
>> g_dist -f traj.xtc -s topol.tpr -n index.ndx -o dist.xvg
>
) and atom no. 879 (ligand atom) with respect to time)
On Thu, Sep 20, 2012 at 10:20 AM, Mark Abraham wrote:
> On 20/09/2012 2:05 PM, tarak karmakar wrote:
>>
>> Thanks Justin.
>>
>> But in my case I want to plot the distance between one atom in the
>> backb
;
> On 9/19/12 2:55 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> I want to calculate the distance between the nitrogen atom present in
>> the ligand and the H- attached to the backbone of the protein along a
>> long trajectory. So can anyone suggest me ho
Dear All,
I want to calculate the distance between the nitrogen atom present in
the ligand and the H- attached to the backbone of the protein along a
long trajectory. So can anyone suggest me how to consider these two
atoms to calculate and plot the distance along with the time ?
--
Tarak
--
gm
> On 17/09/2012 10:01 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> I want to have one of tyrosine residues in my protein to
>> be unprotonated. I am using amber force field for the simulation. But
>> in aminoacid.rtp there is no entry for the un
Dear All,
I want to have one of tyrosine residues in my protein to
be unprotonated. I am using amber force field for the simulation. But
in aminoacid.rtp there is no entry for the unprotonated one. So I am
adding it by myself in to the .rtp file. Now I am bit confused with
the charge
Thanks a lot Justin.
On Wed, Aug 29, 2012 at 11:57 PM, Justin Lemkul wrote:
>
>
> On 8/29/12 2:19 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> In my protein pdb file I am changing the protonation state of residue
>> and giving some other name to i
Dear All,
In my protein pdb file I am changing the protonation state of residue
and giving some other name to it . Now after creating the .gro file I
see that the residue present before the modified one has been
considered as the C-terminal and it is adding one extra oxygen atom to
it. I am givin
Dear All,
I am using AMBER94 force-field for my protein. In the original force
field paper the dihedral functional form has been given as (V/2)[ 1 +
cos(nPhi - gamma)] but in GROMACS(4.5.4) manual I see the (1/2)
factor is not there [ eq 4.62]. So is this internally handled in
GROMACS or should
Thanks a lot for the quick reply...probably I have
overlooked this point earlier
..now I'm getting it properly
On Thu, Aug 16, 2012 at 10:33 PM, Justin Lemkul wrote:
>
>
> On 8/16/12 12:57 PM, tarak karmakar wrote:
>>
>> Dear All,
>
Dear All,
In my simulation I want the temperature of the system to be reached at
300 K only after 3 ps. But after 3ps I see temperature became 402 K.
So am I doing any mistake in the '.mdp' file given below?
define= -DFLEXIBLE
constraints= h-bonds
integrator = sd
then why should I multiply by the
factor 180/pi ? Can you please make it clear, I gotta confused.
Thanks,
Tarak
On Tue, Aug 14, 2012 at 7:17 PM, David van der Spoel
wrote:
> On 2012-08-14 14:27, tarak karmakar wrote:
>>
>> Dear All,
>>
>> In the manual I see the unit of
sorry '-maxsol'
On Tue, Aug 14, 2012 at 11:24 AM, tarak karmakar wrote:
> Oh !!
> I got it it is not the -nmol but '-maxmol'
> thanks to both of u...:)
>
> On Tue, Aug 14, 2012 at 10:35 AM, Peter C. Lai wrote:
>> hmm. What happens if you try -max
Oh !!
I got it it is not the -nmol but '-maxmol'
thanks to both of u...:)
On Tue, Aug 14, 2012 at 10:35 AM, Peter C. Lai wrote:
> hmm. What happens if you try -maxsol instead of -nmol?
>
> On 2012-08-14 10:24:18AM +0530, tarak karmakar wrote:
>> This is the a
in the system before adding another 612?
>
> I don't know how VMD counts waters, but another way is to grep -c for SOL in
> the resulting gro file and divide by 3.
>
> On 2012-08-14 10:07:54AM +0530, tarak karmakar wrote:
>> Thanks for the quick reply, I have given thi
)Segments: 1
Info)Fragments: 669 Protein: 1 Nucleic: 0
On Tue, Aug 14, 2012 at 9:46 AM, Mark Abraham wrote:
> On 14/08/2012 2:02 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> Is there any way to add a specific number of water ( let say 650
>> water) molecul
Dear All,
Is there any way to add a specific number of water ( let say 650
water) molecules while dissolving the solute in a given box ?
Thanks,
Tarak
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*
Hi Mark,
I have used the following .mdp file for the run and got the excess
temperature for the system; it has reached the desired temp at around
150-155 ps. But I need to reach the temp at after 300 ps.
Thanks,
define = -DFLEXIBLE
constraints= h-bonds
integrator
Dear All,
I did the simmulated annealing for a protein where I wanted to
increase the temperature from 0 K to 300 K after 300 ps. But after the
simulation run I see the temp got increased up to 400 K and so.
So can anyone tell me whether I am doing any mistake ?
The .mdp file for the run is as fol
Dear All,
I am studying a molecule which is changing its conformation
during a reaction. So I want to calculate free energy for the
conformational change. I am planning to do Umbrella sampling for this
purpose. But what is the way to handle the dihedral angle as a
Collective Variable (C
Dear All,
I am studying a molecule which is changing its conformation
during a reaction. So I want to calculate free energy for the
conformational change. I am planning to do Umbrella sampling for this
purpose. But what is the way to handle the dihedral angle as a
Collective Variable (C
brium value. Is that
because my system is not minimized / equilibrated properly ?
Any suggestion ?
Thanks
On Mon, Jul 30, 2012 at 7:33 AM, Mark Abraham wrote:
> On 30/07/2012 3:39 AM, tarak karmakar wrote:
>>
>> Dear All,
>>
>> In my initial protein pdb structure I
see its not a big issue. Look at the atom types of the particular
RESIDUE in the pdb file and also have a look into the atom types
present in the rtp file. Now if these are matching properly then you
can choose any convenient name for that particular residue in the rtp
file. But the name of the par
Dear All,
In my initial protein pdb structure I have added some external ligand
molecules and as a result of that there are several short contacts.
So, well, I minimized the system and then got the 'prot_min.gro' file.
Now after the equilibration run, I plotted the RMSD of the resulting
trajectory
Dear All ,
I wanted to keep all the molecules other than water fixed [
positiion restraints]. So for that I have performed short NVT
[simulation with DEPOSRE] after minimization, but while seeing the
movie of the trajectory in VMD I see the protein backbone is moving.
So did I miss somethi
Dear All,
The protein with which I'm working with, contains Zn metal and it
has tetrahedral coordination site. There are HISTIDINE side chains
within distance ~ 2.3 to 2.4 . So my questions are as follows
(1) In that distance range there is no possibility to form a covalent
bond between Zn and
Dear All,
While running minimization I imposed the the condition for the
minimization as to be converged only at Fmax < 10 . But I got the
following
Stepsize too small, or no change in energy.
Converged to machine precision,
but not to the requested precision Fmax < 10
Double precision normally
ou are attempting to hold these
>>>> >> atoms
>>>> >>in
>>>> >>a straight line I would suggest that a type 2 virtual site might
>>>> >>(depending
>>>> >>on your system) be a better idea.
>>>
>>> >
>>> >
>>>
Indeed, a much better idea.
>
> Mark
>
>
>>
>> Richard
>>
>>
>> On 24/07/2012 07:21, "tarak karmakar" wrote:
>>
>>> Oh ! Thnaks
>>> I saw that table, the angle_restrain option is there but not constraints
>>> .
>>
many times but didn't get
proper clue; in one of those mails I saw someone has dealt with some
dummy atoms. I could not able to digest that logic.
On Tue, Jul 24, 2012 at 11:01 AM, Mark Abraham wrote:
> On 24/07/2012 3:21 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
&
Dear All,
I am constraining one angle in my protein sample by incorporating " [
constraints ]" block in topology file as
[ constraints ]
; index1 index2 index3 funct angle
6064 6063 6065 1 180.0
while doing that its showing the following error
Program grompp, VERSION 4.5.5
Sou
ees] maximum angle that
a bond can rotate before LINCS will complain
--
Tarak Karmakar
Molecular Simulation Lab.
Chemistry and Physics of Materials Unit
JNCASR
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* Only plain text messages are
Exactly so. But in the ffbonded.itp file there are two columns,
equilibrium bond length and Kb . So evenif I give zero then it won't
affect the bond .
Thanks a lot for the reply, it's working fine now .
On Mon, Jul 23, 2012 at 6:02 PM, Justin Lemkul wrote:
>
>
> On 7/23/12 8:31
Thanks for the reply.
But then what should I give as Kb [ bond stretching constant ] in the
ffbonded.itp file ? should I give 00.000 there or something else ???
On Mon, Jul 23, 2012 at 4:11 PM, Justin Lemkul wrote:
>
>
> On 7/23/12 2:39 AM, tarak karmakar wrote:
>>
>> Dear A
ogy for ions
#include "./amber94.ff/ions.itp"
[ system ]
; Name
Protein in water
[ molecules ]
; Compound#mols
Other_chain_A 1
SOL 622
--
Tarak Karmakar
Molecular Simulation Lab.
Chemistry and Physics of Materials Unit
JNCASR
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I need to have, prior
to the simulation.
Thanks in advance,
Tarak
--
Tarak Karmakar
Molecular Simulation Lab.
C.P.M.U
JNCASR
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particular pH ? [
Protein Calculator !! ]
Thanks in advance.
--
Tarak Karmakar
Molecular Simulation Lab.
Chemistry and Physics of Materials Unit
Jawaharlal Nehru Centre for Advanced Scientific Research
Jakkur P. O.
Bangalore - 560 064
Karnataka, INDIA
Ph. (lab) : +91-80-22082809
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sorry it's my mistake .
thanks a lot for the reply.
On Mon, Jul 9, 2012 at 10:55 PM, Justin A. Lemkul wrote:
>
>
> On 7/9/12 1:21 PM, tarak karmakar wrote:
>>
>> Oh !! nice work
>> Thanks a lot for the quick reply. But I'm very sorry to inform you
&
ibrary.wiley.com/doi/10.1002/anie.201202032/abstract
>
>
> hope it helps
>
>
>
> On 07/09/2012 12:21 PM, tarak karmakar wrote:
>>
>> Dear All,
>>
>>
>> Please suggest me any paper/article that contains force field
>> parameters for Mn 2+ .
>&
Dear All,
Please suggest me any paper/article that contains force field
parameters for Mn 2+ .
Thanks
--
Tarak Karmakar
Molecular Simulation Lab.
Chemistry and Physics of Materials Unit
Jawaharlal Nehru Centre for Advanced Scientific Research
Jakkur P. O.
Bangalore - 560 064
Karnataka, INDIA
be highly appreciated.*
* Thanks
Tarak
--
*Tarak Karmakar
Molecular Simulation Lab.
Chemistry and Physics of Materials Unit
Jawaharlal Nehru Centre for Advanced Scientific Research
Jakkur P. O.
Bangalore - 560 064
Karnataka, INDIA
Ph. (lab) : +91-80-22082809 *
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Thanks a lotnow it's working:)
On Fri, Jun 15, 2012 at 2:00 PM, Mark Abraham wrote:
> On 15/06/2012 6:21 PM, tarak karmakar wrote:
>
> Hi,
>
> Thanks for the reply.
> One thing, while giving the '-ff' flag it is asking for some string. So I
>
> On 15/06/2012 4:27 PM, tarak karmakar wrote:
>
> Dear All,
>
>
> In my protein pdb file I have changed some of the amino acid residue
> names. So accordingly I have changed corresponding residue names in force
> filed files and kept all the files [ modified and unmo
) aminoacids.rtp
3) ffnonbonded.itp
4) ffbonded.itp
5) spc.itp
6) ions.itp
now while giving the command
pdb2gmx -f prot.pdb -o prot.gro -p toplogy.top
how can I make use of all these force field files present in my current
working directory ?
Thanks in advance.
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*Tarak Karmakar
Molecular
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